CA2248140C - Assay and reagents for quantifying hbnp - Google Patents
Assay and reagents for quantifying hbnp Download PDFInfo
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- CA2248140C CA2248140C CA002248140A CA2248140A CA2248140C CA 2248140 C CA2248140 C CA 2248140C CA 002248140 A CA002248140 A CA 002248140A CA 2248140 A CA2248140 A CA 2248140A CA 2248140 C CA2248140 C CA 2248140C
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- C07K14/435—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
- C07K14/575—Hormones
- C07K14/58—Atrial natriuretic factor complex; Atriopeptin; Atrial natriuretic peptide [ANP]; Cardionatrin; Cardiodilatin
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K16/00—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
- C07K16/18—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans
- C07K16/26—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against hormones ; against hormone releasing or inhibiting factors
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K2317/00—Immunoglobulins specific features
- C07K2317/30—Immunoglobulins specific features characterized by aspects of specificity or valency
- C07K2317/34—Identification of a linear epitope shorter than 20 amino acid residues or of a conformational epitope defined by amino acid residues
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- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S530/00—Chemistry: natural resins or derivatives; peptides or proteins; lignins or reaction products thereof
- Y10S530/827—Proteins from mammals or birds
- Y10S530/839—Nerves; brain
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- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S530/00—Chemistry: natural resins or derivatives; peptides or proteins; lignins or reaction products thereof
- Y10S530/827—Proteins from mammals or birds
- Y10S530/841—Muscles; heart
Abstract
The present invention provides reagents and assays for the quantification of hBNP in biological fluid samples such as plasma or serum. Antibodies are provided which are monospecific to epitopes comprising the amino acid sequences 5-13, 1-10 and 15-25 of hBNP. These antibodies, and peptide fragments containing these sequences, can be employed in the assays of the invention, which may be carried out in a sandwich format or a competition format.
Description
WO 97/32900 PCT/US97/03163 _ 1-0 ASSAY AND REAGENTS FOR QUANTIFYING hBNP
BACKGROUND OF THE INVENTION
I. Field of the Invention This invention relates to the field of immunoassays, more particularf to reagents and methods useful for the rapid and sensitive quantitication of the peptide hormone hBNP in a biological fluid such as plasma or serum.
II. Description of the Prior Art BNP is a cardiac derived peptide hornZOne that circulates in the blood and exerts potent 2~ cardiovascular and renal actions. BNP is structurally similar to two other cardiac peptides, atrial natriuretic peptide (ANP) and C-type natriuretic peptide (CNP}. Porcine BNP was isolated from pib brain (Sudoh et al., Nature 332:78-81, 1988) and, hence, was Given the name "brain natriuretic peptide". In man the cardiac ventricle is the primary site of BNP synthesis.
The sequence of human BNP (hBNP) was originally determined by the isolation and characterization of DNA clones from human genomic libraries (C1.S. Patent No.
S,I 14,923).
hBNP is synthesized, in vivo, as a 108 amino acid precursor that is enzymatically cleaved to yield the mature hBNP peptide. Mature hBNP consists of a 32 amino acid peptide containing a I 7 amino acid ring structure formed by two disulfide bonds (see Fig. 1 ).
Elevated expression of ventricular hBNP mRNA has been reported in congestive heart failure patients as compared to normal controls. Consistent with the increase in ventricular mass and expression of BNP mRNA, hBNP levels are elevated in patients with congestive heart failure and appear to correlate with disease severity. Plasma hBNP is also believed to provide a valuable predictive marker for heart disease. Elevated plasma hBNP has been reported in heart disease, following acute myocardial infarction and during symptomless or subclinical ventricular dysfunction (Mukoyama et al., J. Clin. Invest., 87:11402-14 / 2, 1991 ) (Motwani et al., Lancet, 34I :1109-1113, 1993) (Yoshibayashi et al., New Ena'J. Med., 327:434, 1992).
Reports from two major therapeutic trials, the SAVE trial (New EnQ. J. Med , 327:669-677, IS 1992) and the SOLVD trial (New EnQ. J. Med., 327:68-691, 1992) suggested that diagnosis arid appropriate treatment of patients with asymptomatic left ventricular dysfunction could significantly reduce the incidence of fatal and non-fatal cardiovascular events and related hospitalizations.
For use in a clinical laboratory setting, it would be hi;hly desirable to provide a diagnostic assay for hBNP which is sufficiently sensitive to measure clinically relevant titers of hBNP, sufficiently simple that it can be automated, requires a minimum amount of time to complete and preferably does not require the use of reagents having limited shelf lives. Normal levels of hBNP in plasma are quite low, on the order of 1 to 20 pg/mL.
Typically, 2~ radioimmunoassays are used to measure titers in this range, although the use of radioactive reagents requires special handling, adds steps to the assay and involves the use of material having limited shelf life. A radio immunoassay is commercially available for measuring hBNP, however, in addition to requiring the use of radioactive rea;ents, it is complex and cumbersome, requiring an extraction step, precipitation and several centrifugation steps, and takes several WO 97/32900 PCT/US97/03163 _ days to complete. European Patent Application No. 0 542 2~5 describes a radioimmunoassay for hBNP.
SUMMARY OF THE INVENTION
S
The present invention provides reagents and methods for the rapid and direct quantification of hBNP levels in biological fluids. The reagents and methods provided herein allow for the detection of hBNP titers at clinically relevant levels without the use of radioactive labelling (although radioactive labelling may be used, if desired). Moreover, they provide for the direct quantification of hBNP in plasma without the need for cumbersome extraction steps.
The reagents and methods provided herein lend themselves readily to the automated systems used to conduct blood tests on a large scale in commercial clinical laboratories.
In one embodiment of the invention, there are provided monospecific antibodies to selected peptide epitopes within the hBNP molecule. Preferably, these monospecific antibodies are monoclonal antibodies. The monospecific antibodies of the invention are selected from the group consisting of:
(a) an antibody that is monospecific to a peptide epitope comprisin; amino acids 5-13 of hBNP;
(b) an antibody that is monospecific to a peptide epitope comprising amino acids I-IO
of hBNP; and (c) an antibody that is monospecific to a peptide epitope comprising amino acids 15-25 of hBNP, or functionally active fragments thereof.
A preferred antibody of the invention is a monoclonal antibody that recognizes and binds the peptide epitope comprising amino acids 5-13 of hBNP.
In another embodiment of the invention, there is provided a method for quantifying the amount of hBNP in a biological fluid using the reagents of the invention in a sandwich type WO 97/32900 PCT/U597/03163 _ immunoassay. The immunoassay may employ any of numerous labelling techniques to label and quantify immune complexes, with enzymatic labelling being preferred. This method of the invention comprises the steps of:
(a) contacting a sample of the biological fluid with a first antibody selected from the group consisting of:
(i) an antibody that is monospecific for a peptide epitope comprising amino acids S-13 of hBNP;
(ii) an antibody that is monospecific for a peptide epitope comprising amino acids 1-10 of hBNP;
(iii) an antibody that is monospecitic for a peptide epitope comprising amino acids 1 S-2~ of hBNP;
(iv) an antibody that is monospecific for a peptide epitope comprising amino acids 27-32 of hBNP; and functionally active fragments of (i)-(iv), 1 ~ and a second antibody selected from the group consisting of:
(i) an antibody that is monospecific for a peptide epitope comprising amino acids 5-13 of hBNP;
(ii) an antibody that is monospecific for a peptide epitope comprising amino acids 1-10 of hBNP;
(iii) an antibody that is monospecifcc for a peptide epitope comprisin; amino acids 15-2~ of hBNP;
(iv) an antibody that is monospecific for a peptide epitope comprising amino acids 27-32 of hBNP;
(v) a high aff inity polyclonal antibody to hBNP; and functionally active tcagments of (i)-(v), under conditions which allow the formation of a first antibody-hBNP-second antibody complex, provided that if the first antibody is monospecific to hBNP 27-32, then the second antibody is not a polyclonal antibody;
(b) binding a quantifiable label to said second antibody, prior to, simultaneously with or after formation of the first antibody-hBNP-second antibody complex; and WO 97/32900 PCT/US97/03163 _ (c) deternZining the amount of hBNP in the sample by quantifying the label in the first antibody-hBNP-second antibody complex.
In other embodiments of the invention, there are provided methods for quantifying the amount of hBNP in a biological fluid using the reagents of the invention in competition type immunoassays. One such assay comprises the steps of:
(a) contacting a sample of the biological fluid with:
(i) an antibody that is monospecific for a peptide epitope comprising amino acids 5-13 of hBNP or a functionally active fragment thereof; and (ii) hBNP or a fragment thereof comprising amino acids S-13 of hBNP, having bound thereto a quantifiable label, under conditions that allow the formation of an antibody-hBNP complex; and (b) determining the amount of hBNP in the sample by quantifying the label in the antibody-hBNP complex.
1~
Another embodiment of the assay of the invention in a competition type format comprises the steps of:
(a) contacting a sample of the biolo;ical fluid with:
(i) an antibody that is monospecitic for a peptide epitope comprising amino acids 1-10 of hBNP or a functionally active twagment thereof; and (ii) hBNP or a fragment thereof comprising amino acids I-10 of hBNP, having bound thereto a quantifiable label, under conditions that allow the formation of an antibody-hBNP complex; and (b) determining the amount of hBNP in the sample by quantifying the label in the 2~ antibody-hBNP complex.
Another embodiment of the assay of the invention in a competition type format comprises the steps of:
(a) contacting a sample of the biological tluid with:
WO 97/32900 PCT/US97/03163 _ (i) an antibody that is monospecific for a peptide epitope comprising amino acids 15-25 of hBNP or a functionally active fragment thereof; and (ii) hBNP or a fragment thereof comprising amino acids I 5-25 of hBNP, having bound thereto a quantifiable label, S under conditions that allow the formation of an antibody-hBNP complex; and (b) determining the amount of hBNP in the sample by quantifying the label in the antibody-hBNP complex.
In the sandwich assays and the competition assays of the invention, the first antibody-hBNP-second antibody complex (in the case of a sandwich assay) or the antibody-hBNP
complex (in the case of a competition assay) will usually be separated from the remainder of the biological fluid sample prior to quantifying the label in the complex.
There are, however, known labelling techniques which allow for the direct measurement of labelled complex in the sample, i. e. without separating the complex from the sample, and such methods are considered 1 ~ to be within the scope of the invention. As merely exemplary of such methods, one can mention the scintillation proximity assay (Udenfciend, S. et al., Anal. Biochem., 161:494-500, 19$7) and the assay described in Mathis, G., Clin. Chem., 41:1391-1397, 199.
There are also provided by this invention fragments of hBNP which can be used as rea;ents in a_competition type assay of the invention.
In one embodiment, the hBNP tcagment of the invention has the formula X'-V-Q-G-S-G-C-P-G-R-X'-, (I) wherein X' is selected from the group consisting of hydroben, M-, K-M-, P-K-M- or S-P-K-M-WO 97/32900 PCTlUS97/03163 and X'- is selected from the group consisting of hydroxyl, -K, -K-M, -K-M-D; and -K-M-D-R.
In another embodiment, the hBNP fragment of the invention has the formula S-P-K-M-V-Q-G-S-G-C-X3, (II}
wherein X'' is selected from the group consisting of hydroxyl, -F and -F-G.
In another embodiment, the hBNP fragment of the invention has the formula X;-M-D-R-I-S-S-S-S-G-L-G-X5, (III) wherein X~ is selected from the group consisting of hydrogen, K-, R-K- and G-R-K-and XS is selected from the group consisting of hydroxyl, -C, -C-K, -C-K-V, -C-K-V-L,.
-C-K-V-L-R, -C-K-V-L-R-R and -C-K-V-L-R-R-H.
WO 97/32900 PCT/US97/03163 _ DESCRIPTION OF THE DRAWINGS
Fig. 1 is a representation of the amino acid sequence of the mature (32 amino acid) form of hBNP. Amino acids are represented by the standard single letter code and the solid line represents a disulfide bond between the two cysteine residues.
Fig. 2 represents the results of experiments conducted to determine the ability of rabbit polyclonal antisera raised to hBNP to bind various fragments of hBNP.
Fig. 3 represents the results of epitope mapping studies of three monoclonal antibodies designated MAb 201.3, MAb 106.3 and MAb 8.1.
Fig. 4 is a standard curve for a sandwich type enzyme linked immunosorbent assay using MAb 106.3 as the capture antibody and a polyclonal antibody #4024 as the second antibody.
Fig. 5 is a standard curve for a sandwich type enzyme linked immunosorbent assay using MAb 201.3 as the capture antibody and polyclonal antibody X4360 as the second antibody.
Fig. 6 is a standard curve for a sandwich type enzyme linked immunosorbent assay using MAb 106.3 as the capture antibody and a monospecific antibody against epitope 15-25 as the second antibody.
Fig. 7 is a standard curve for a sandwich type enzyme linked immunosorbent assay using MAb 201.3 as the capture antibody and a monospecitlc polyclonal antibody against epitope I S-25 as the second antibody.
WO 97/32900 PCT/US97I03163 _ Fig. 8 is a standard curve for a sandwich type immunosorbent assay using MAb 8.1 as the capture antibody and biotinylated MAb 106.3 as the second antibody in a monoclonal:rnonoclonal sandwich.
Fig. 9 is a standard curve for a sandwich type immunosorbent assay using MAb 20I .3 as a capture antibody and biotinylated MAb 8.1 as a second antibody in a monoclonal:monoclonal sandwich.
Fig. 10 is a standard curve for a competition type enzyme linked immunosorbent assay using MAb 106.3 as the antibody.
Fig. 11 presents the results obtained using a competition type enzyme linked immunosorbent assay to quantify hBNP levels in the plasma of normal control subjects and subjects with congestive heart disease.
DETAILED DESCRIPTION AND PREFERRED EMBODIMENTS OF THE INVENTION
I. Antibodies of the Invention This invention provides highly sensitive reagents which allow for the rapid, simple and accurate quantification of hBNP at clinically relevant titers in biological fluids such as plasma or serum. In particular, we have identified three previously unidentified highly immunogenic epitopes within the hBNP molecule and produced antibodies monospecific to these regions.
When an antibody is referred to herein as being ''monospecific" to an epitope, it is meant that the antibody is capable of binding a sequence of amino acids within hBNP
containing the an>ino acids comprising the epitope, but is incapable of binding to a sequence of amino acids within hBNP that does not contain the amino acids comprising the epitope. The monospecific antibodies ofthe invention are preferably, thou;h not necessarily. monoclonal antibodies.
WO 97/32900 PCT/US97t03163 _ The three epitopes recognized by the monospecific antibodies of the invention comprise amino acids 1-10, 5-13 and 15-25 of hBNP.
Monoclonal antibodies of the invention can be produced by hybridoma cells prepared according to known procedures, e.g. Kohler, G. and Milstein, C., Nature, 256:495, 1975. In General, mice are immunized with an immunogenic conjugate of hBNP and a suitable partner, such as bovine serum albumin. Periodic booster injections are administered until good antibody titers are achieved. Spleen cells from the immunized mice are then fused with myeloma cells according to known procedures (i.e. Galfre et al.,Nature, 266:550, 1977) to produce hybridoma cells. Supernatants from the hybridoma cell cultures are screened for reactivity to hBNP.
Hybridomas testing positive are recloned and their supernatants retested for reactivity. Using this procedure, as described in more detail below, we obtained hybridoma cell line 106.3, which secretes monoclonal antibodies that specifically recognize the hBNP fragment 5-13, hybridoma cell Line 201.3, which secretes monoclonal antibodies that specifically recognize the hBNP
I ~ ti-agment I-10 and hybridoma cell line 8.1, which secretes monoclonal antibodies that specifically recognize the hBNP fragment 27-32.
Once a highly immunogenic epitope has been identified, non-monoclonal monospecific antibodies can be produced from polyclonal antisera. Polyclonal antisera is produced according to known techniques. A suitable animal, such as a rabbit, is immunized with an immunoaenic conjugate of hBNP and a suitable partner. Periodic booster injections are administered until good antibody titers are achieved. By testing the antisera thus obtained for immunoreactivity against various peptide fcagments of hBNP, desirable epitopes are identified.
Using this procedure, we identified the peptide fragment hBNP 15-25 as a highly immunogenic epitope 2~ of hBNP. Monospecific antibodies to the identified epitope can be obtained by affinity purification of polycLonal serum on an affinity column in which a peptide fragment including only. that epitope and none of the other epitopes identified in the epitope mapping is bound to a solid support. Using this general procedure, as described in more detail below, we produced non-monoclonal monospecific antibodies that specifically reco~nize the hBNP
fragment 15-25.
WO 97/32900 PCT/US97/03163 _ It will be recognized, however, that monoclonal antibodies to this epitope can also be produced using known procedures.
Functionally active fragments of the monospecific antibodies of the invention can also S be used in assays for hBNP. A functional fragment is one that retains the immunologic specificity of the antibody, although avidity and/or affinity may not be quantitatively identical.
Included in the functionally active fragments are such immunoglobulin fragments as Fab, F(ab')Z and Fab'. The tcagments can be produced by known methods such as by enzymatic cleavage of the monospecific antibodies (see, e.g., Mariani, M. et nl., Mol.
Immunol., 28:69-77, 1991; Ishikawa, E. et al., J. Immunoassay, 4:209-327, 1983).
II. Peptide Fragments of hBNP Useful in Immunoassays In order to conduct an immunoassay in a competition type format, it is necessary to 1 ~ employ a labelled peptide which is capable of competing with hBNP in the biological fluid sample being assayed for binding to the antibody employed in the assay. The labelled peptide can be labelled hBNP 1-32. Using the monospecific antibodies of this invention, however, it is not necessary to employ intact hBNP 1-32 as the competing reagent. Rather, novel hBNP
peptide fragments of the formulae I-III, above, can be used. In formulae I-III, amino acids are represented by their standard single-letter abbreviations. An indication that X~ or X' is hydrogen means that it represents the amino-terminus of the peptide fragment.
An indication that X-', X' or X' is hydroxyl means that it represents the carboxy-terminus of the peptide fragment.
2~ In particular, peptide fragments of formula I, which contain amino acids S-13 of the hBNP sequence, can be used as reagents to compete with hBNP in the test sample for binding to an antibody of the invention that is monospecitic to the epitope comprising amino acids 5-13.
Peptide fragments of formula I in which X' is S-P-K-M- can be used as reagents in a competition assay employing an antibody of the invention that is monospecitic to the epitope comprising amino acids 1-10.
Peptide fragments of formula II, which contain amino acids 1-10 of hBNP, can be used as reagents to compete with hBNP in the test sample for binding to an antibody of the invention that is monospecific to the epitope comprising amino acids 1-10.
Peptide fragments of formula III, which contain amino acids 1 S-25 of hBNP, can be employed as reagents to compete with hBNP in the test sample for binding to an antibody of the invention that is monospecific to the epitope comprising amino acids 15-25.
Additionally, one can employ, for the same purposes, peptides corresponding to the peptides of formulae I-III in which all of the amino acids have been substituted by the corresponding D-amino acids (referred to hereafter as the "D-amino acid isomers") or one can employ retro-inverso-isomers or partially modified retro-inverso-isomers of the peptides of formulae I-III. Retro-inverso-isomers are isomers in which the direction of the sequence is reversed and the chiralit5r of each amino acid residue is inverted. Partially modified retro-inverso-isomers are isomers in which only some of the peptide bonds are reversed and the chirality of the amino acid residues in the reversed portion is inverted.
Retro-inverso-isomers and partially modified retro-inverso-isomers are described by Chorev, M. and Goodman, M., TIBTECH, Vol. 13:438-444, 1995. These isomers have been shown to be imrnunologically cross-reactive with their parent peptides.
The peptide fragments of the invention can be prepared by methods known to those skilled in the art such as, for example, solid phase peptide synthesis using the procedure of Merrifield e1 al., (Proc. Natl. Acad. Sci. USA, 92:3449-343, 1955). The retro-inverso derivatives can be prepared by the procedure of Briand et al., J. Biol. Chem., 270:20686-20691, 1995.
III. Immunoassays of the Invention The reagents of the invention can be used to carry out immunoassays to quantify hBNP
levels in biological fluids such as plasma, serum and whole blood. The assays can be carried WO 97132900 PCT/US97/03163 _ out either in a sandwich type format or in a competition format. When measuring hBNP levels in blood, the biological fluid is preferably plasma or serum, which can be prepared from whole blood using known procedures.
In a sandwich type assay, two different antibodies are employed to separate and quantify the hBNP in the biological fluid sample. The two antibodies bind to the hBNP, thereby forming an immune complex, or sandwich. Generally, one of the antibodies is used to capture the hBNP
in the sample and a second antibody is used to bind a quantifiable label to the sandwich.
Preferably, the antibodies chosen to carry out the sandwich type assay are selected such that the - first antibody which is brought into contact with the hBNP-containing sample does not bind all or part of the epitope recognized by the second antibody, thereby significantly interfering with the ability of the second antibody to bind hBNP. Consequently, if a sandwich type format is chosen, one preferably should not employ an antibody monospecific for hBNP 5-13 in combination with an antibody monospecific for hBNP 1-10 inasmuch as the epitopes 1 S recognized by these antibodies overlap. We have found, however, that an excellent assay can be effected using a monospecific antibody as the first antibody brought into contact with the hBNP-containing sample and a high affinity polyclonal antibody for hBNPI-32 as the second antibody. In particular, we have produced a sandwich ripe assay which is sensitive in the range of clinically relevant hBNP titers using a monoclonal antibody which recognizes the epitope hBNP 5-13 as a capture antibody and a rabbit polyclonaE antibody to hBNP as the second antibody (see Examples 9 and 10).
The fluid sample can be contacted with the first antibody and the second antibody simultaneously or sequentially. In a preferred embodiment of the sandwich assay of the 2~ invention, the hBNP-containing biological fluid sample is first brought into contact with a first antibody which is monospecific for a particular epitope under conditions which allow the formation of an antibody-hBNP complex. Preferably, the first antibody is bound to a solid support to facilitate the ultimate separation of the sandwich complex from the fluid sample. The solid supports that can be used are well known to those skilled in the art and can be, for example, polymeric materials in the form of wells, tubes or beads. The antibody can be bound WO 97/32900 PCT/US97/03163 _ to the solid support by adsorption or by covalent bonding using a chemical coupling agent, provided the coupling agent employed does not interfere with the ability of the antibody to bind hBNP. The polymeric support materials can be derivatized to allow reactivity with various functional groups on the antibody. Typically used coupling agents include malefic anhydride, N-hydroxysuccinimide and 1-ethyl-3-(3-dimethylaminopropyl)carbodiimide. In a sandwich type assay, the antibody is normally employed in amounts substantially in molar excess of the maximum amount of hBNP expected to be in the sample. Preferably, there are employed from about 0.01 nM to about 1.0 nM of antibody per mL, of undiluted plasma. In practice, one may dilute the biological fluid sample in an appropriate physiologic buffer in order to achieve an acceptable molar ratio of antibody to hBNP.
After the hBNP-containing sample has been brought into contact with the first monospecific antibody, the sample is incubated to allow the formation of a first antibody-hBNP
complex. Generally, incubation is carried out at or near physiologic pH, e.g.
pH b.0 to pH 8.0 1~ at a temperature from about 4°C to about 37°C. Incubation time is at least about 2 minutes, although incubation can be carried out for as long as 18 hours.
The first antibod~~-hBNP complex is contacted with the second antibody under conditions which allow formation of a first antibody-hBNP-second antibody complex.
Typically, this entails incubation under conditions similar to those outlined above for the formation of the first antibody-hBNP complex. A quantifiable label is bound to the second antibody prior to, simultaneously with or after formation of the first antibody-hBNP-second antibody complex Any of the known labels conventionally used in immunoassays may be employed. These may be, for example, radioactive labels, such as ''-$I, enzymatic labels such as horseradish peroxidase or alkaline phosphatase, chemiluminescent labels such as acridinium esters, bioluminescent labels, fluorescent labels, thermometric labels, immuno-polylnerase chain reaction labels or others. For a review of some of the more sensitive labels that can be employed in the assays ofthe invention, see Kricka, L.J., Clin. Chem., 40(3):347-3~7, 1994 and Kricka, L.J., Clin. Biochem., 26:325-331, 1993. The Label can be bound to the antibody directly or through a coupling agent. For example, in the.case of horseradish peroxidase, the second WO 97/32900 PCT/US97/03163 _ antibody can be bound to biotin, using known techniques. Following formation of the first antibody-hBNP-second antibody complex, the complex can be contacted with avidin-horseradish peroxidase, which is tightly bound by the biotin on the second antibody. An alternative method of binding the label to the second antibody involves contacting the first antibody-hBNP-second antibody complex with an antibody which recognizes and binds the F
region of the second antibody and which has the label bound thereto. Other methods of binding label to the second antibody will be readily apparent to those skilled in the art.
In a preferred embodiment, the first antibody-hBNP-second antibody complex is separated from the remainder of the biological fluid sample prior to quantification of the label.
When the first antibody is bound to solid support, such as a well or a bead, separation is accomplished simply by removing the fluid from contact with the solid support.
For example, the first antibody bound to a solid support may be incubated with the hBNP-containing sample to form a first antibody-hBNP complex and the fluid sample may then be removed from contact with the solid support prior to contacting the first antibody-hBNP complex with the second antibody. Alternatively, the first antibody bound to a solid support may be simultaneously contacted with the hBNP-containing sample and the second antibody to form a first antibody-hBNP-second antibody complex, followed by removal of the biological fluid from contact with the solid support.
After formation of labelled antibody-hBNP-second antibody complex and separation of the complex from the remainder of the biological fluid sample, the amount of label in the complex is quantified using known methods. For example, in the case of an enzymatic label, the labelled complex is reacted with a substrate for the label, giving a quantifiable reaction such as the development of color. Where the enzymatic label is horseradish peroxidase, for example, the labelled complex is reacted with tetramethylbenzidine (TMB), giving a reaction which can be quantified by measuring the development of color. Where the (abet is a radioactive label, the label is quantified using a scintillation counter. Numerous other methods are well known for quantifying the various t5rpes of labels that can be employed in the assays of the inventions.
BACKGROUND OF THE INVENTION
I. Field of the Invention This invention relates to the field of immunoassays, more particularf to reagents and methods useful for the rapid and sensitive quantitication of the peptide hormone hBNP in a biological fluid such as plasma or serum.
II. Description of the Prior Art BNP is a cardiac derived peptide hornZOne that circulates in the blood and exerts potent 2~ cardiovascular and renal actions. BNP is structurally similar to two other cardiac peptides, atrial natriuretic peptide (ANP) and C-type natriuretic peptide (CNP}. Porcine BNP was isolated from pib brain (Sudoh et al., Nature 332:78-81, 1988) and, hence, was Given the name "brain natriuretic peptide". In man the cardiac ventricle is the primary site of BNP synthesis.
The sequence of human BNP (hBNP) was originally determined by the isolation and characterization of DNA clones from human genomic libraries (C1.S. Patent No.
S,I 14,923).
hBNP is synthesized, in vivo, as a 108 amino acid precursor that is enzymatically cleaved to yield the mature hBNP peptide. Mature hBNP consists of a 32 amino acid peptide containing a I 7 amino acid ring structure formed by two disulfide bonds (see Fig. 1 ).
Elevated expression of ventricular hBNP mRNA has been reported in congestive heart failure patients as compared to normal controls. Consistent with the increase in ventricular mass and expression of BNP mRNA, hBNP levels are elevated in patients with congestive heart failure and appear to correlate with disease severity. Plasma hBNP is also believed to provide a valuable predictive marker for heart disease. Elevated plasma hBNP has been reported in heart disease, following acute myocardial infarction and during symptomless or subclinical ventricular dysfunction (Mukoyama et al., J. Clin. Invest., 87:11402-14 / 2, 1991 ) (Motwani et al., Lancet, 34I :1109-1113, 1993) (Yoshibayashi et al., New Ena'J. Med., 327:434, 1992).
Reports from two major therapeutic trials, the SAVE trial (New EnQ. J. Med , 327:669-677, IS 1992) and the SOLVD trial (New EnQ. J. Med., 327:68-691, 1992) suggested that diagnosis arid appropriate treatment of patients with asymptomatic left ventricular dysfunction could significantly reduce the incidence of fatal and non-fatal cardiovascular events and related hospitalizations.
For use in a clinical laboratory setting, it would be hi;hly desirable to provide a diagnostic assay for hBNP which is sufficiently sensitive to measure clinically relevant titers of hBNP, sufficiently simple that it can be automated, requires a minimum amount of time to complete and preferably does not require the use of reagents having limited shelf lives. Normal levels of hBNP in plasma are quite low, on the order of 1 to 20 pg/mL.
Typically, 2~ radioimmunoassays are used to measure titers in this range, although the use of radioactive reagents requires special handling, adds steps to the assay and involves the use of material having limited shelf life. A radio immunoassay is commercially available for measuring hBNP, however, in addition to requiring the use of radioactive rea;ents, it is complex and cumbersome, requiring an extraction step, precipitation and several centrifugation steps, and takes several WO 97/32900 PCT/US97/03163 _ days to complete. European Patent Application No. 0 542 2~5 describes a radioimmunoassay for hBNP.
SUMMARY OF THE INVENTION
S
The present invention provides reagents and methods for the rapid and direct quantification of hBNP levels in biological fluids. The reagents and methods provided herein allow for the detection of hBNP titers at clinically relevant levels without the use of radioactive labelling (although radioactive labelling may be used, if desired). Moreover, they provide for the direct quantification of hBNP in plasma without the need for cumbersome extraction steps.
The reagents and methods provided herein lend themselves readily to the automated systems used to conduct blood tests on a large scale in commercial clinical laboratories.
In one embodiment of the invention, there are provided monospecific antibodies to selected peptide epitopes within the hBNP molecule. Preferably, these monospecific antibodies are monoclonal antibodies. The monospecific antibodies of the invention are selected from the group consisting of:
(a) an antibody that is monospecific to a peptide epitope comprisin; amino acids 5-13 of hBNP;
(b) an antibody that is monospecific to a peptide epitope comprising amino acids I-IO
of hBNP; and (c) an antibody that is monospecific to a peptide epitope comprising amino acids 15-25 of hBNP, or functionally active fragments thereof.
A preferred antibody of the invention is a monoclonal antibody that recognizes and binds the peptide epitope comprising amino acids 5-13 of hBNP.
In another embodiment of the invention, there is provided a method for quantifying the amount of hBNP in a biological fluid using the reagents of the invention in a sandwich type WO 97/32900 PCT/U597/03163 _ immunoassay. The immunoassay may employ any of numerous labelling techniques to label and quantify immune complexes, with enzymatic labelling being preferred. This method of the invention comprises the steps of:
(a) contacting a sample of the biological fluid with a first antibody selected from the group consisting of:
(i) an antibody that is monospecific for a peptide epitope comprising amino acids S-13 of hBNP;
(ii) an antibody that is monospecific for a peptide epitope comprising amino acids 1-10 of hBNP;
(iii) an antibody that is monospecitic for a peptide epitope comprising amino acids 1 S-2~ of hBNP;
(iv) an antibody that is monospecific for a peptide epitope comprising amino acids 27-32 of hBNP; and functionally active fragments of (i)-(iv), 1 ~ and a second antibody selected from the group consisting of:
(i) an antibody that is monospecific for a peptide epitope comprising amino acids 5-13 of hBNP;
(ii) an antibody that is monospecific for a peptide epitope comprising amino acids 1-10 of hBNP;
(iii) an antibody that is monospecifcc for a peptide epitope comprisin; amino acids 15-2~ of hBNP;
(iv) an antibody that is monospecific for a peptide epitope comprising amino acids 27-32 of hBNP;
(v) a high aff inity polyclonal antibody to hBNP; and functionally active tcagments of (i)-(v), under conditions which allow the formation of a first antibody-hBNP-second antibody complex, provided that if the first antibody is monospecific to hBNP 27-32, then the second antibody is not a polyclonal antibody;
(b) binding a quantifiable label to said second antibody, prior to, simultaneously with or after formation of the first antibody-hBNP-second antibody complex; and WO 97/32900 PCT/US97/03163 _ (c) deternZining the amount of hBNP in the sample by quantifying the label in the first antibody-hBNP-second antibody complex.
In other embodiments of the invention, there are provided methods for quantifying the amount of hBNP in a biological fluid using the reagents of the invention in competition type immunoassays. One such assay comprises the steps of:
(a) contacting a sample of the biological fluid with:
(i) an antibody that is monospecific for a peptide epitope comprising amino acids 5-13 of hBNP or a functionally active fragment thereof; and (ii) hBNP or a fragment thereof comprising amino acids S-13 of hBNP, having bound thereto a quantifiable label, under conditions that allow the formation of an antibody-hBNP complex; and (b) determining the amount of hBNP in the sample by quantifying the label in the antibody-hBNP complex.
1~
Another embodiment of the assay of the invention in a competition type format comprises the steps of:
(a) contacting a sample of the biolo;ical fluid with:
(i) an antibody that is monospecitic for a peptide epitope comprising amino acids 1-10 of hBNP or a functionally active twagment thereof; and (ii) hBNP or a fragment thereof comprising amino acids I-10 of hBNP, having bound thereto a quantifiable label, under conditions that allow the formation of an antibody-hBNP complex; and (b) determining the amount of hBNP in the sample by quantifying the label in the 2~ antibody-hBNP complex.
Another embodiment of the assay of the invention in a competition type format comprises the steps of:
(a) contacting a sample of the biological tluid with:
WO 97/32900 PCT/US97/03163 _ (i) an antibody that is monospecific for a peptide epitope comprising amino acids 15-25 of hBNP or a functionally active fragment thereof; and (ii) hBNP or a fragment thereof comprising amino acids I 5-25 of hBNP, having bound thereto a quantifiable label, S under conditions that allow the formation of an antibody-hBNP complex; and (b) determining the amount of hBNP in the sample by quantifying the label in the antibody-hBNP complex.
In the sandwich assays and the competition assays of the invention, the first antibody-hBNP-second antibody complex (in the case of a sandwich assay) or the antibody-hBNP
complex (in the case of a competition assay) will usually be separated from the remainder of the biological fluid sample prior to quantifying the label in the complex.
There are, however, known labelling techniques which allow for the direct measurement of labelled complex in the sample, i. e. without separating the complex from the sample, and such methods are considered 1 ~ to be within the scope of the invention. As merely exemplary of such methods, one can mention the scintillation proximity assay (Udenfciend, S. et al., Anal. Biochem., 161:494-500, 19$7) and the assay described in Mathis, G., Clin. Chem., 41:1391-1397, 199.
There are also provided by this invention fragments of hBNP which can be used as rea;ents in a_competition type assay of the invention.
In one embodiment, the hBNP tcagment of the invention has the formula X'-V-Q-G-S-G-C-P-G-R-X'-, (I) wherein X' is selected from the group consisting of hydroben, M-, K-M-, P-K-M- or S-P-K-M-WO 97/32900 PCTlUS97/03163 and X'- is selected from the group consisting of hydroxyl, -K, -K-M, -K-M-D; and -K-M-D-R.
In another embodiment, the hBNP fragment of the invention has the formula S-P-K-M-V-Q-G-S-G-C-X3, (II}
wherein X'' is selected from the group consisting of hydroxyl, -F and -F-G.
In another embodiment, the hBNP fragment of the invention has the formula X;-M-D-R-I-S-S-S-S-G-L-G-X5, (III) wherein X~ is selected from the group consisting of hydrogen, K-, R-K- and G-R-K-and XS is selected from the group consisting of hydroxyl, -C, -C-K, -C-K-V, -C-K-V-L,.
-C-K-V-L-R, -C-K-V-L-R-R and -C-K-V-L-R-R-H.
WO 97/32900 PCT/US97/03163 _ DESCRIPTION OF THE DRAWINGS
Fig. 1 is a representation of the amino acid sequence of the mature (32 amino acid) form of hBNP. Amino acids are represented by the standard single letter code and the solid line represents a disulfide bond between the two cysteine residues.
Fig. 2 represents the results of experiments conducted to determine the ability of rabbit polyclonal antisera raised to hBNP to bind various fragments of hBNP.
Fig. 3 represents the results of epitope mapping studies of three monoclonal antibodies designated MAb 201.3, MAb 106.3 and MAb 8.1.
Fig. 4 is a standard curve for a sandwich type enzyme linked immunosorbent assay using MAb 106.3 as the capture antibody and a polyclonal antibody #4024 as the second antibody.
Fig. 5 is a standard curve for a sandwich type enzyme linked immunosorbent assay using MAb 201.3 as the capture antibody and polyclonal antibody X4360 as the second antibody.
Fig. 6 is a standard curve for a sandwich type enzyme linked immunosorbent assay using MAb 106.3 as the capture antibody and a monospecific antibody against epitope 15-25 as the second antibody.
Fig. 7 is a standard curve for a sandwich type enzyme linked immunosorbent assay using MAb 201.3 as the capture antibody and a monospecitlc polyclonal antibody against epitope I S-25 as the second antibody.
WO 97/32900 PCT/US97I03163 _ Fig. 8 is a standard curve for a sandwich type immunosorbent assay using MAb 8.1 as the capture antibody and biotinylated MAb 106.3 as the second antibody in a monoclonal:rnonoclonal sandwich.
Fig. 9 is a standard curve for a sandwich type immunosorbent assay using MAb 20I .3 as a capture antibody and biotinylated MAb 8.1 as a second antibody in a monoclonal:monoclonal sandwich.
Fig. 10 is a standard curve for a competition type enzyme linked immunosorbent assay using MAb 106.3 as the antibody.
Fig. 11 presents the results obtained using a competition type enzyme linked immunosorbent assay to quantify hBNP levels in the plasma of normal control subjects and subjects with congestive heart disease.
DETAILED DESCRIPTION AND PREFERRED EMBODIMENTS OF THE INVENTION
I. Antibodies of the Invention This invention provides highly sensitive reagents which allow for the rapid, simple and accurate quantification of hBNP at clinically relevant titers in biological fluids such as plasma or serum. In particular, we have identified three previously unidentified highly immunogenic epitopes within the hBNP molecule and produced antibodies monospecific to these regions.
When an antibody is referred to herein as being ''monospecific" to an epitope, it is meant that the antibody is capable of binding a sequence of amino acids within hBNP
containing the an>ino acids comprising the epitope, but is incapable of binding to a sequence of amino acids within hBNP that does not contain the amino acids comprising the epitope. The monospecific antibodies ofthe invention are preferably, thou;h not necessarily. monoclonal antibodies.
WO 97/32900 PCT/US97t03163 _ The three epitopes recognized by the monospecific antibodies of the invention comprise amino acids 1-10, 5-13 and 15-25 of hBNP.
Monoclonal antibodies of the invention can be produced by hybridoma cells prepared according to known procedures, e.g. Kohler, G. and Milstein, C., Nature, 256:495, 1975. In General, mice are immunized with an immunogenic conjugate of hBNP and a suitable partner, such as bovine serum albumin. Periodic booster injections are administered until good antibody titers are achieved. Spleen cells from the immunized mice are then fused with myeloma cells according to known procedures (i.e. Galfre et al.,Nature, 266:550, 1977) to produce hybridoma cells. Supernatants from the hybridoma cell cultures are screened for reactivity to hBNP.
Hybridomas testing positive are recloned and their supernatants retested for reactivity. Using this procedure, as described in more detail below, we obtained hybridoma cell line 106.3, which secretes monoclonal antibodies that specifically recognize the hBNP fragment 5-13, hybridoma cell Line 201.3, which secretes monoclonal antibodies that specifically recognize the hBNP
I ~ ti-agment I-10 and hybridoma cell line 8.1, which secretes monoclonal antibodies that specifically recognize the hBNP fragment 27-32.
Once a highly immunogenic epitope has been identified, non-monoclonal monospecific antibodies can be produced from polyclonal antisera. Polyclonal antisera is produced according to known techniques. A suitable animal, such as a rabbit, is immunized with an immunoaenic conjugate of hBNP and a suitable partner. Periodic booster injections are administered until good antibody titers are achieved. By testing the antisera thus obtained for immunoreactivity against various peptide fcagments of hBNP, desirable epitopes are identified.
Using this procedure, we identified the peptide fragment hBNP 15-25 as a highly immunogenic epitope 2~ of hBNP. Monospecific antibodies to the identified epitope can be obtained by affinity purification of polycLonal serum on an affinity column in which a peptide fragment including only. that epitope and none of the other epitopes identified in the epitope mapping is bound to a solid support. Using this general procedure, as described in more detail below, we produced non-monoclonal monospecific antibodies that specifically reco~nize the hBNP
fragment 15-25.
WO 97/32900 PCT/US97/03163 _ It will be recognized, however, that monoclonal antibodies to this epitope can also be produced using known procedures.
Functionally active fragments of the monospecific antibodies of the invention can also S be used in assays for hBNP. A functional fragment is one that retains the immunologic specificity of the antibody, although avidity and/or affinity may not be quantitatively identical.
Included in the functionally active fragments are such immunoglobulin fragments as Fab, F(ab')Z and Fab'. The tcagments can be produced by known methods such as by enzymatic cleavage of the monospecific antibodies (see, e.g., Mariani, M. et nl., Mol.
Immunol., 28:69-77, 1991; Ishikawa, E. et al., J. Immunoassay, 4:209-327, 1983).
II. Peptide Fragments of hBNP Useful in Immunoassays In order to conduct an immunoassay in a competition type format, it is necessary to 1 ~ employ a labelled peptide which is capable of competing with hBNP in the biological fluid sample being assayed for binding to the antibody employed in the assay. The labelled peptide can be labelled hBNP 1-32. Using the monospecific antibodies of this invention, however, it is not necessary to employ intact hBNP 1-32 as the competing reagent. Rather, novel hBNP
peptide fragments of the formulae I-III, above, can be used. In formulae I-III, amino acids are represented by their standard single-letter abbreviations. An indication that X~ or X' is hydrogen means that it represents the amino-terminus of the peptide fragment.
An indication that X-', X' or X' is hydroxyl means that it represents the carboxy-terminus of the peptide fragment.
2~ In particular, peptide fragments of formula I, which contain amino acids S-13 of the hBNP sequence, can be used as reagents to compete with hBNP in the test sample for binding to an antibody of the invention that is monospecitic to the epitope comprising amino acids 5-13.
Peptide fragments of formula I in which X' is S-P-K-M- can be used as reagents in a competition assay employing an antibody of the invention that is monospecitic to the epitope comprising amino acids 1-10.
Peptide fragments of formula II, which contain amino acids 1-10 of hBNP, can be used as reagents to compete with hBNP in the test sample for binding to an antibody of the invention that is monospecific to the epitope comprising amino acids 1-10.
Peptide fragments of formula III, which contain amino acids 1 S-25 of hBNP, can be employed as reagents to compete with hBNP in the test sample for binding to an antibody of the invention that is monospecific to the epitope comprising amino acids 15-25.
Additionally, one can employ, for the same purposes, peptides corresponding to the peptides of formulae I-III in which all of the amino acids have been substituted by the corresponding D-amino acids (referred to hereafter as the "D-amino acid isomers") or one can employ retro-inverso-isomers or partially modified retro-inverso-isomers of the peptides of formulae I-III. Retro-inverso-isomers are isomers in which the direction of the sequence is reversed and the chiralit5r of each amino acid residue is inverted. Partially modified retro-inverso-isomers are isomers in which only some of the peptide bonds are reversed and the chirality of the amino acid residues in the reversed portion is inverted.
Retro-inverso-isomers and partially modified retro-inverso-isomers are described by Chorev, M. and Goodman, M., TIBTECH, Vol. 13:438-444, 1995. These isomers have been shown to be imrnunologically cross-reactive with their parent peptides.
The peptide fragments of the invention can be prepared by methods known to those skilled in the art such as, for example, solid phase peptide synthesis using the procedure of Merrifield e1 al., (Proc. Natl. Acad. Sci. USA, 92:3449-343, 1955). The retro-inverso derivatives can be prepared by the procedure of Briand et al., J. Biol. Chem., 270:20686-20691, 1995.
III. Immunoassays of the Invention The reagents of the invention can be used to carry out immunoassays to quantify hBNP
levels in biological fluids such as plasma, serum and whole blood. The assays can be carried WO 97132900 PCT/US97/03163 _ out either in a sandwich type format or in a competition format. When measuring hBNP levels in blood, the biological fluid is preferably plasma or serum, which can be prepared from whole blood using known procedures.
In a sandwich type assay, two different antibodies are employed to separate and quantify the hBNP in the biological fluid sample. The two antibodies bind to the hBNP, thereby forming an immune complex, or sandwich. Generally, one of the antibodies is used to capture the hBNP
in the sample and a second antibody is used to bind a quantifiable label to the sandwich.
Preferably, the antibodies chosen to carry out the sandwich type assay are selected such that the - first antibody which is brought into contact with the hBNP-containing sample does not bind all or part of the epitope recognized by the second antibody, thereby significantly interfering with the ability of the second antibody to bind hBNP. Consequently, if a sandwich type format is chosen, one preferably should not employ an antibody monospecific for hBNP 5-13 in combination with an antibody monospecific for hBNP 1-10 inasmuch as the epitopes 1 S recognized by these antibodies overlap. We have found, however, that an excellent assay can be effected using a monospecific antibody as the first antibody brought into contact with the hBNP-containing sample and a high affinity polyclonal antibody for hBNPI-32 as the second antibody. In particular, we have produced a sandwich ripe assay which is sensitive in the range of clinically relevant hBNP titers using a monoclonal antibody which recognizes the epitope hBNP 5-13 as a capture antibody and a rabbit polyclonaE antibody to hBNP as the second antibody (see Examples 9 and 10).
The fluid sample can be contacted with the first antibody and the second antibody simultaneously or sequentially. In a preferred embodiment of the sandwich assay of the 2~ invention, the hBNP-containing biological fluid sample is first brought into contact with a first antibody which is monospecific for a particular epitope under conditions which allow the formation of an antibody-hBNP complex. Preferably, the first antibody is bound to a solid support to facilitate the ultimate separation of the sandwich complex from the fluid sample. The solid supports that can be used are well known to those skilled in the art and can be, for example, polymeric materials in the form of wells, tubes or beads. The antibody can be bound WO 97/32900 PCT/US97/03163 _ to the solid support by adsorption or by covalent bonding using a chemical coupling agent, provided the coupling agent employed does not interfere with the ability of the antibody to bind hBNP. The polymeric support materials can be derivatized to allow reactivity with various functional groups on the antibody. Typically used coupling agents include malefic anhydride, N-hydroxysuccinimide and 1-ethyl-3-(3-dimethylaminopropyl)carbodiimide. In a sandwich type assay, the antibody is normally employed in amounts substantially in molar excess of the maximum amount of hBNP expected to be in the sample. Preferably, there are employed from about 0.01 nM to about 1.0 nM of antibody per mL, of undiluted plasma. In practice, one may dilute the biological fluid sample in an appropriate physiologic buffer in order to achieve an acceptable molar ratio of antibody to hBNP.
After the hBNP-containing sample has been brought into contact with the first monospecific antibody, the sample is incubated to allow the formation of a first antibody-hBNP
complex. Generally, incubation is carried out at or near physiologic pH, e.g.
pH b.0 to pH 8.0 1~ at a temperature from about 4°C to about 37°C. Incubation time is at least about 2 minutes, although incubation can be carried out for as long as 18 hours.
The first antibod~~-hBNP complex is contacted with the second antibody under conditions which allow formation of a first antibody-hBNP-second antibody complex.
Typically, this entails incubation under conditions similar to those outlined above for the formation of the first antibody-hBNP complex. A quantifiable label is bound to the second antibody prior to, simultaneously with or after formation of the first antibody-hBNP-second antibody complex Any of the known labels conventionally used in immunoassays may be employed. These may be, for example, radioactive labels, such as ''-$I, enzymatic labels such as horseradish peroxidase or alkaline phosphatase, chemiluminescent labels such as acridinium esters, bioluminescent labels, fluorescent labels, thermometric labels, immuno-polylnerase chain reaction labels or others. For a review of some of the more sensitive labels that can be employed in the assays ofthe invention, see Kricka, L.J., Clin. Chem., 40(3):347-3~7, 1994 and Kricka, L.J., Clin. Biochem., 26:325-331, 1993. The Label can be bound to the antibody directly or through a coupling agent. For example, in the.case of horseradish peroxidase, the second WO 97/32900 PCT/US97/03163 _ antibody can be bound to biotin, using known techniques. Following formation of the first antibody-hBNP-second antibody complex, the complex can be contacted with avidin-horseradish peroxidase, which is tightly bound by the biotin on the second antibody. An alternative method of binding the label to the second antibody involves contacting the first antibody-hBNP-second antibody complex with an antibody which recognizes and binds the F
region of the second antibody and which has the label bound thereto. Other methods of binding label to the second antibody will be readily apparent to those skilled in the art.
In a preferred embodiment, the first antibody-hBNP-second antibody complex is separated from the remainder of the biological fluid sample prior to quantification of the label.
When the first antibody is bound to solid support, such as a well or a bead, separation is accomplished simply by removing the fluid from contact with the solid support.
For example, the first antibody bound to a solid support may be incubated with the hBNP-containing sample to form a first antibody-hBNP complex and the fluid sample may then be removed from contact with the solid support prior to contacting the first antibody-hBNP complex with the second antibody. Alternatively, the first antibody bound to a solid support may be simultaneously contacted with the hBNP-containing sample and the second antibody to form a first antibody-hBNP-second antibody complex, followed by removal of the biological fluid from contact with the solid support.
After formation of labelled antibody-hBNP-second antibody complex and separation of the complex from the remainder of the biological fluid sample, the amount of label in the complex is quantified using known methods. For example, in the case of an enzymatic label, the labelled complex is reacted with a substrate for the label, giving a quantifiable reaction such as the development of color. Where the enzymatic label is horseradish peroxidase, for example, the labelled complex is reacted with tetramethylbenzidine (TMB), giving a reaction which can be quantified by measuring the development of color. Where the (abet is a radioactive label, the label is quantified using a scintillation counter. Numerous other methods are well known for quantifying the various t5rpes of labels that can be employed in the assays of the inventions.
3() When the amount of label in the complex has been quantified, the concentration of hBNP in the biological fluid sample is determined by use of a standard curve which has been generated using serial dilutions of hBNP of known concentration.
The assay of the invention can also be earned out in a competition format. In this format, an aliquot of labelled hBNP or a suitable fragment thereof of known concentration is used to compete with the hBNP in the biological fluid for binding to hBNP
monospecific antibody. In the competition assay, immobilized antibody can be simultaneously or sequentially contacted with the biological fluid sample and the labelled hBNP or hBNP
fragment. The labelled hBNP or hBNP fragment, the fluid sample and the antibody are incubated under I 0 conditions similar to those indicated above in the description of the sandwich type assay. There are thus formed two species of antibody-hBNP complex, one being labelled and the other being unlabelled. The amount of label in the antibody-hBNP complex is quantified.
The concentration of hBNP in the biological fluid sample can then be determined by comparing the quantity of label in the antibody-hBNP complex to a standard curve generated using serial 1 S dilutions of hBNP of known concentration. Preferably, the antibody-hBNP
complex is separated from the remainder of the biological fluid sample prior to quantification of the label in the complex.
The labels which may be employed in the competition format include those previously 20 indicated to be useful in a sandwich type assay. The label is covalently bound to the hBNP or hBNP fragment using known techniques. Commonly used techniques include the use of heterobifunctional crosslinking reagents which react with primary amines, sulfhydryls or carboxyl groups. For example, succinimidyl 4-(N-maleimidomethyl)cyclohexane-I-carboxylate can be used to bind glucose oxidase, horseradish peroxidase, ~3-galactosidase or alkaline 2~ phosphatase to peptides containing free sulfhydryl groups. Biotin can be conjugated to free sulfhydryl groups using BMCC, to carboxyl groups using biotin hydrazide or to amino groups using N-hydroxysuccinimide. Separation of the antibody-hBNP complex can conveniently be accomplished by binding the antibody to a solid support, such as those previously mentioned in connection with the sandwich assay format. The antibody-hBNP complex is then WO 97/32900 PCT/US97/03163 _ conveniently separated by removing the remainder of the biological fluid sample from contact with the solid support.
The labelled peptide which is used to compete with hBNP in the sample for binding to the monospecific antibody can be intact hBNP 1-32 or any peptide fragment thereof, providing the fragment contains at least that sequence of amino acids corresponding to the epitope recognized by the monospecific antibody. Thus, when the antibody employed is monospecific to the epitope comprising amino acids 1-10 of hBNP, the labelled peptide fragment can be any fragment containing at Least amino acids 1-10, including, but not limited to the peptides of -formula II and peptides of formula I in which X~ is S-P-K-M-. When the antibody employed is monospecific to the epitope comprising amino acids S-13 of hBNP, the labelled peptide fragment can be any fragment containing at least amino acids 5-13, including, but not limited to the peptides of formula I. When the antibody employed is monospecific to the epitope comprising amino acids 1 ~-2~ of hBNP, the labelled peptide fragment can be any fragment containing at least amino acids 15-2~, including, but not limited to the peptides of formula III.
IV. Examples The following examples are intended to further illustrate the practice of the invention and are not to be construed as limiting the scope of the invention in any way.
Preparation of BNP Coniugates for Antibody Production hBNP 1-32 and the fragments hBNP 1-10 and hBNP 26-32 were prepared by solid phase 2~ synthesis. These peptides were coupled to bovine serum albumin (BSA) carrier protein through a carbodiimide coupling procedure or by using the heterobifunctional cross-linking regent N-maleimido-L-aminocaproyl ester of 1-hydroxysuccinimide-2-nitro-4-benzenesulfonic acid (mal-sac-HNSA) according to the method of Aldwin and Nitecki (Anal. Biochem., 164:494-~U1, 1987). BSA (1 mg) was reacted with 0.5 mg of the mal-sac-HNSA cross-linker in 250 pL
of phosphate buttered saline (PBS) pH 7.~ for 40 minutes at room temperature.
The activated BSA was purified over a G-25 Sephadexcolumn with O.1M phosphate buffer pH 6.0 and combined with approximately 1 mg of the cysteine containing peptides hBNP 1-10 (SPKMVQGSGC) and hBNP 26-32 (CKVLRRH). The mixture was reacted for 4 hours at room temperature and dialyzed overnight against PBS at 4°C. A
successful conjugation was indicated by the presence of a protein in an area corresponding to 75 Kd to 90 Kd on a 12%
polyacrylamide gel.
BNP 1-32 BSA conjugates were prepared by dissolving approximately 1 mg BNP in 450 pL of 1 mM HCl and adding 2.8 mg of 1-ethyl-3-(3-dimethylaminopropylkarbodiimide (EDAC). The mixture was reacted for 30 minutes on ice and added to 1.47 mg BSA
in 300 pL
of 5 mM NaOH. After 4 hours at room temperature, the solution was dialyzed against PBS at 4°C.
hBNP 1-32 conjugates for preparation of rabbit polyclonal antibodies were prepared by 1 ~ mixing 100 ug of methylated BSA (MeBSA) with 100 pg hBNP 1-32 in 100 pL
PBS, pH 7.4.
2. Immun~,~ations For production of monoclonal antibodies, mice were immunized with peptide conjugate emulsions prepared using RIBI Adjuvant System (RIBI Immunochemical Research Inc.).
About 700 pg of Synthetic Trehalose Dicorynomycolate and about 650 pg of Monophosphoryl Lipid A from S. minnesota 8595 dissolved in 4:1 chloroform:methanol were dried in a small.
glass homogenizer. Sixty p.L squalene was added and mixed into a paste. The peptide conjugate was then added, with continuous stirring, and an additional 1.5 mL
0.2% Tween 80 2~ in water was added with stirring to generate a final emulsion containing approximately 1 mg/mL of protein. The emulsion was stored at 4°C until use. Female Balb/c mice (4 to 6 weeks old) were injected intraperitoneally with approximately 12~ to 150 pg of the peptide conjugate. Mice were boosted with intraperitoneal injections once every three weeks until good titers were established. Mice received a final boost four days prior to spleen cell fusions.
For production of polyclonal antibodies rabbits were immunized with the hBNP 1-MeBSA conjugates. Emulsions were prepared by mixing thoroughly 100 ~tL of the peptide conjugate with 200 pL of Freund's Complete Adjuvant (FCA) or Freund's Incomplete Adjuvant (FIA). Three hundred pL of the FCA emulsion was injected into the inguinal lymph nodes .following the method of Mojsov et al. (J. Biol. Chem., 261:11880-11889).
Peptide emulsified in FIA was used for additional boosts at weeks 2 and 3. Animals were tested and bled out when titers were sufficient. Polyclonal antibodies from two animals, identified as #4024 and#4360, were employed in several of the assays described below.
3. Spleen Cell Fusions Spleen cells were fused with the myeloma partner FOX-NY (ATCC CRL-1732) according to a method modified from Galfre et al., Nature, 266:550, 1977.
Spleens were removed aseptically and single cell suspensions were prepared in serum free medium by homogenization in a 7 mL, glass homogenizer. The spleen cells were washed twice prior to mixing with the myeloma partner cells. The FOX-NY:myelorna cells were harvested at log phase growth , washed and combined with the spleen cells in a 5:1 spleen:myelorna) ratio. The cells were centrifuged, medium was removed and the cell pellet was loosened by tapping. One mL of 50% polyethylene glycol (PEG) was added and stirred Gently at 37°C for approximately 2 minutes. The cells were slowly diluted with 10 mL of serum free medium, centrifuged at 400 x g and resuspended in hybridoma selection medium: RPMI-1640 hybridoma medium, lOmM Hepes, 20% fetal bovine serum, 50 U/mL penicillin, 50 p.g/mL
streptomycin, 75 pM
adenine, 0.8 pM aminopterin and 16 pM thymidine. The cells were transferred to a T-1 SO
culture flask and incubated overnight prior to plating in 96-well plates (about 105 cells per well).
Cultures were maintained at 37°C, 7% CO, in a humidified incubator.
Cells were re-fed 6 days after fusion and conditioned medium was assayed for antibodies at day 10.
4. Screening and Selection Hybridoma supernatants were tested for reactivity to hBNP 1-32 or various hBNp peptides by a standard ELISA method. Peptides, 0.1-0.5 p.g/I00 pL/well in PBS, were adsorbed to microtiter plates overnight at 4°C. Wells were washed with PBS/Tween (PBS containing 0.05% Tween-20) and blocked with 0.1% gelatin 1 hour at 37°C. Undiluted hybridoma supernatants (100 pL/well) were added to the peptide-coated wells for 2 hours at 37°C. Wells were washed and incubated with a goat anti-mouse IgG horseradish peroxidase conjugate diluted in PBS/Tween/ovalbumin (0.1 % ovalbumin in PBS/Tween) for 2 additional hours.
Another wash was followed by addition of the substrate {0.5 mg/mL O-phenyienediamine, 0.012% hydrogen peroxide in 100 mM citric phosphate buffer pH 5.0). The color reaction was stopped with 5 M sulfuric acid and absorbance read at 490 nm. An O.D. value greater than twice background was considered a positive response.
1 ~ Hybridomas testing positive were recloned by limiting dilution and their supernatants retested for specific reactivity. Hybridoma and secretory stability were established by measuring growth and antibody production characteristics over several passages. This process resulted in the establishment of hybridoma cell line 106.3 and MAb 106.3, which specifically recognizes the hBNP peptide ti-agment S-13, hybridoma cell line 201.3 and MAb 201.3, which specifically recognizes the hBNP peptide fragment 1-10 and hybridoma cell line 8.1 and MAb 8. I , which specitlcally recognizes the hBNP peptide tcagment 27-32.
Hybridoma cell line 106.3 was deposited at the American Type Culture Collection, Rockville, Md. on February 14, 1996 and has accession no. HB 12044. Hybridoma cell line 201.3 was deposited at the American Type Culture Collection, Rockville, Md. on February 14, 1996 and has accession no.
2~ HB 12045. Hybridoma cell line 8.1 was deposited at the American Type Culture Collection, Rockville, Md. on February 21, 1996 and has the accession no. HB 12050.
The assay of the invention can also be earned out in a competition format. In this format, an aliquot of labelled hBNP or a suitable fragment thereof of known concentration is used to compete with the hBNP in the biological fluid for binding to hBNP
monospecific antibody. In the competition assay, immobilized antibody can be simultaneously or sequentially contacted with the biological fluid sample and the labelled hBNP or hBNP
fragment. The labelled hBNP or hBNP fragment, the fluid sample and the antibody are incubated under I 0 conditions similar to those indicated above in the description of the sandwich type assay. There are thus formed two species of antibody-hBNP complex, one being labelled and the other being unlabelled. The amount of label in the antibody-hBNP complex is quantified.
The concentration of hBNP in the biological fluid sample can then be determined by comparing the quantity of label in the antibody-hBNP complex to a standard curve generated using serial 1 S dilutions of hBNP of known concentration. Preferably, the antibody-hBNP
complex is separated from the remainder of the biological fluid sample prior to quantification of the label in the complex.
The labels which may be employed in the competition format include those previously 20 indicated to be useful in a sandwich type assay. The label is covalently bound to the hBNP or hBNP fragment using known techniques. Commonly used techniques include the use of heterobifunctional crosslinking reagents which react with primary amines, sulfhydryls or carboxyl groups. For example, succinimidyl 4-(N-maleimidomethyl)cyclohexane-I-carboxylate can be used to bind glucose oxidase, horseradish peroxidase, ~3-galactosidase or alkaline 2~ phosphatase to peptides containing free sulfhydryl groups. Biotin can be conjugated to free sulfhydryl groups using BMCC, to carboxyl groups using biotin hydrazide or to amino groups using N-hydroxysuccinimide. Separation of the antibody-hBNP complex can conveniently be accomplished by binding the antibody to a solid support, such as those previously mentioned in connection with the sandwich assay format. The antibody-hBNP complex is then WO 97/32900 PCT/US97/03163 _ conveniently separated by removing the remainder of the biological fluid sample from contact with the solid support.
The labelled peptide which is used to compete with hBNP in the sample for binding to the monospecific antibody can be intact hBNP 1-32 or any peptide fragment thereof, providing the fragment contains at least that sequence of amino acids corresponding to the epitope recognized by the monospecific antibody. Thus, when the antibody employed is monospecific to the epitope comprising amino acids 1-10 of hBNP, the labelled peptide fragment can be any fragment containing at Least amino acids 1-10, including, but not limited to the peptides of -formula II and peptides of formula I in which X~ is S-P-K-M-. When the antibody employed is monospecific to the epitope comprising amino acids S-13 of hBNP, the labelled peptide fragment can be any fragment containing at least amino acids 5-13, including, but not limited to the peptides of formula I. When the antibody employed is monospecific to the epitope comprising amino acids 1 ~-2~ of hBNP, the labelled peptide fragment can be any fragment containing at least amino acids 15-2~, including, but not limited to the peptides of formula III.
IV. Examples The following examples are intended to further illustrate the practice of the invention and are not to be construed as limiting the scope of the invention in any way.
Preparation of BNP Coniugates for Antibody Production hBNP 1-32 and the fragments hBNP 1-10 and hBNP 26-32 were prepared by solid phase 2~ synthesis. These peptides were coupled to bovine serum albumin (BSA) carrier protein through a carbodiimide coupling procedure or by using the heterobifunctional cross-linking regent N-maleimido-L-aminocaproyl ester of 1-hydroxysuccinimide-2-nitro-4-benzenesulfonic acid (mal-sac-HNSA) according to the method of Aldwin and Nitecki (Anal. Biochem., 164:494-~U1, 1987). BSA (1 mg) was reacted with 0.5 mg of the mal-sac-HNSA cross-linker in 250 pL
of phosphate buttered saline (PBS) pH 7.~ for 40 minutes at room temperature.
The activated BSA was purified over a G-25 Sephadexcolumn with O.1M phosphate buffer pH 6.0 and combined with approximately 1 mg of the cysteine containing peptides hBNP 1-10 (SPKMVQGSGC) and hBNP 26-32 (CKVLRRH). The mixture was reacted for 4 hours at room temperature and dialyzed overnight against PBS at 4°C. A
successful conjugation was indicated by the presence of a protein in an area corresponding to 75 Kd to 90 Kd on a 12%
polyacrylamide gel.
BNP 1-32 BSA conjugates were prepared by dissolving approximately 1 mg BNP in 450 pL of 1 mM HCl and adding 2.8 mg of 1-ethyl-3-(3-dimethylaminopropylkarbodiimide (EDAC). The mixture was reacted for 30 minutes on ice and added to 1.47 mg BSA
in 300 pL
of 5 mM NaOH. After 4 hours at room temperature, the solution was dialyzed against PBS at 4°C.
hBNP 1-32 conjugates for preparation of rabbit polyclonal antibodies were prepared by 1 ~ mixing 100 ug of methylated BSA (MeBSA) with 100 pg hBNP 1-32 in 100 pL
PBS, pH 7.4.
2. Immun~,~ations For production of monoclonal antibodies, mice were immunized with peptide conjugate emulsions prepared using RIBI Adjuvant System (RIBI Immunochemical Research Inc.).
About 700 pg of Synthetic Trehalose Dicorynomycolate and about 650 pg of Monophosphoryl Lipid A from S. minnesota 8595 dissolved in 4:1 chloroform:methanol were dried in a small.
glass homogenizer. Sixty p.L squalene was added and mixed into a paste. The peptide conjugate was then added, with continuous stirring, and an additional 1.5 mL
0.2% Tween 80 2~ in water was added with stirring to generate a final emulsion containing approximately 1 mg/mL of protein. The emulsion was stored at 4°C until use. Female Balb/c mice (4 to 6 weeks old) were injected intraperitoneally with approximately 12~ to 150 pg of the peptide conjugate. Mice were boosted with intraperitoneal injections once every three weeks until good titers were established. Mice received a final boost four days prior to spleen cell fusions.
For production of polyclonal antibodies rabbits were immunized with the hBNP 1-MeBSA conjugates. Emulsions were prepared by mixing thoroughly 100 ~tL of the peptide conjugate with 200 pL of Freund's Complete Adjuvant (FCA) or Freund's Incomplete Adjuvant (FIA). Three hundred pL of the FCA emulsion was injected into the inguinal lymph nodes .following the method of Mojsov et al. (J. Biol. Chem., 261:11880-11889).
Peptide emulsified in FIA was used for additional boosts at weeks 2 and 3. Animals were tested and bled out when titers were sufficient. Polyclonal antibodies from two animals, identified as #4024 and#4360, were employed in several of the assays described below.
3. Spleen Cell Fusions Spleen cells were fused with the myeloma partner FOX-NY (ATCC CRL-1732) according to a method modified from Galfre et al., Nature, 266:550, 1977.
Spleens were removed aseptically and single cell suspensions were prepared in serum free medium by homogenization in a 7 mL, glass homogenizer. The spleen cells were washed twice prior to mixing with the myeloma partner cells. The FOX-NY:myelorna cells were harvested at log phase growth , washed and combined with the spleen cells in a 5:1 spleen:myelorna) ratio. The cells were centrifuged, medium was removed and the cell pellet was loosened by tapping. One mL of 50% polyethylene glycol (PEG) was added and stirred Gently at 37°C for approximately 2 minutes. The cells were slowly diluted with 10 mL of serum free medium, centrifuged at 400 x g and resuspended in hybridoma selection medium: RPMI-1640 hybridoma medium, lOmM Hepes, 20% fetal bovine serum, 50 U/mL penicillin, 50 p.g/mL
streptomycin, 75 pM
adenine, 0.8 pM aminopterin and 16 pM thymidine. The cells were transferred to a T-1 SO
culture flask and incubated overnight prior to plating in 96-well plates (about 105 cells per well).
Cultures were maintained at 37°C, 7% CO, in a humidified incubator.
Cells were re-fed 6 days after fusion and conditioned medium was assayed for antibodies at day 10.
4. Screening and Selection Hybridoma supernatants were tested for reactivity to hBNP 1-32 or various hBNp peptides by a standard ELISA method. Peptides, 0.1-0.5 p.g/I00 pL/well in PBS, were adsorbed to microtiter plates overnight at 4°C. Wells were washed with PBS/Tween (PBS containing 0.05% Tween-20) and blocked with 0.1% gelatin 1 hour at 37°C. Undiluted hybridoma supernatants (100 pL/well) were added to the peptide-coated wells for 2 hours at 37°C. Wells were washed and incubated with a goat anti-mouse IgG horseradish peroxidase conjugate diluted in PBS/Tween/ovalbumin (0.1 % ovalbumin in PBS/Tween) for 2 additional hours.
Another wash was followed by addition of the substrate {0.5 mg/mL O-phenyienediamine, 0.012% hydrogen peroxide in 100 mM citric phosphate buffer pH 5.0). The color reaction was stopped with 5 M sulfuric acid and absorbance read at 490 nm. An O.D. value greater than twice background was considered a positive response.
1 ~ Hybridomas testing positive were recloned by limiting dilution and their supernatants retested for specific reactivity. Hybridoma and secretory stability were established by measuring growth and antibody production characteristics over several passages. This process resulted in the establishment of hybridoma cell line 106.3 and MAb 106.3, which specifically recognizes the hBNP peptide ti-agment S-13, hybridoma cell line 201.3 and MAb 201.3, which specifically recognizes the hBNP peptide fragment 1-10 and hybridoma cell line 8.1 and MAb 8. I , which specitlcally recognizes the hBNP peptide tcagment 27-32.
Hybridoma cell line 106.3 was deposited at the American Type Culture Collection, Rockville, Md. on February 14, 1996 and has accession no. HB 12044. Hybridoma cell line 201.3 was deposited at the American Type Culture Collection, Rockville, Md. on February 14, 1996 and has accession no.
2~ HB 12045. Hybridoma cell line 8.1 was deposited at the American Type Culture Collection, Rockville, Md. on February 21, 1996 and has the accession no. HB 12050.
5. C~~~cte,-'Lzation of Antibodies A microtiter plate ELISA was used to identify the class/subclass of the monoclonal _ antibodies. Mouse antibody was added to micratiter plates precoated with hBNP. Subclass specific second antibodies conjugated to horseradish peroxidase were added to detect the bound murine monoclonal antibody. Several washes followed by the addition of TMB
substrate gave specific subclass reactivities for the three monoclonals. MAb 106.3 was determined to be an IgGtx antibody, MAb 201.3 was determined to belong to subclass IgCn.x and MAb 8.1 was determined to belong to subclass IgGtx.
Rabbit polyclonal antibody was tested for reactivity to hBNP 1-32 as well as to a variety of hBNP fragments. Microtiter plates were coated with 100 ng of the various peptides/well in 200 pL of 0.1 M bicarbonate buffer, pH 8-9. The plates were blocked with 0.1%
gelatin for 30 minutes at 37°C. Rabbit serum was diluted 1:1000 followed by 5 three-fold dilutions in a 1 ~ Tris/Tween/BSA buffer (O.OSM Tris, pH 7.5, 0.15 M NaCI, 1% BSA, 0.1% Tween-20). One hundred microliters of the antibody dilution series were added to the microtiter wells and incubated at 4°C for 2 hours. A wash with Tris/Tween/BSA buffer was followed by a 1 hour incubation with goat anti-rabbit horseradish peroxidase. The wells were washed with buffer 4 times and 200 pL TMB substrate was added. Following a 30 to 45 minute incubation the reaction was stopped with 2.5 M sulfuric acid and the O.D. was read at 450 nnt. Reactivity with the various peptides is presented in Fig. 2. The rabbit antiserum demonstrated specific reactivities with four hBNP peptide fragments, 1-10, 5-13, 15-25 and 27-32, as well as strong reactivity to hBNP 1-32.
2~ 6. Antibody Production and Purification Hybridoma cells were seeded in roller bottles at a concentration of 300,000 cellslmL in RPMI 1640 tissue culture medium supplemented with ~% Fetal Clone (Hyclone) and grown to a density of approximately 1 x 106 cells/mL. The medium was replaced with serum free Hybridoma SFM medium and incubation was continued for an additional 3 to 5 days. Cells were separated from the culture medium by centrifugation at 400 x g and the medium was clarified by filtration through a 0.2 p filter. The medium was applied to a Prosep Protein-A
affinity column (Bioprocessing Inc.) that had been previously equilibrated with binding buffer at pH 8.6 (1 M glycine, 0.15 M NaCI). After application of the culture medium was completed . __ the column was washed with binding buffer until OD readings monitored at 280 nM returned to baseline levels. Antibody was eluted using 100 mM citric acid pH 3.0, concentrated to .
approximately 1 mg/rnL in a Centriprep 10 concentrator and dialyzed overnight at 4°C against PBS, pH 7.5. Rabbit antiserum was cleared of lipid prior to column purification of polyclonal IgG. Each 1.5 parts of serum was mixed with 1 part of SeroClea~'~''Reagent (Calbiochem), vortexed for approximately 1 minute and centrifuged to separate lipid and aqueous phases. The cleared serum was then loaded directly onto the column with a perfusion pump and purified in the same manner as the tissue culture supernatant fluid.
Rabbit antibody monospecific to the hBNP epitope comprising amino acids 15-25 was isolated from the polyclonal IgG using a diaminodipropylamine affinity column (DADPA) to which the synthetic hBNP fragment 15-27 was immobilized. The DADPA gel was prepared for coupling by washing with 5 mL water followed by 5 mL 0.1 MES buffer (2-(N-morpholino)ethanesulfonic acid), 0.9% NaCI, pH 4.7. hBNP I ~-27 (2 mg) was dissolved in 2 mL of MES buffer and mixed with the gel. EDC (1-ethyl-3-(3-dimethylarninopropyl)carbodiimide) dissolved in MES buffer was added to the gel and incubated with stirring for 3 hours at room temperature. The column was washed several times with I M NaCI to remove unbound peptide and blocked with 0.1% ovalbumin. Prior to application of the rabbit IaG, the column was washed with 5 column volumes of PBS, pH 7.5.
The rabbit IgG was cycled through the column 5 times followed by 5 washes with PBS buffer.
The antibodies bound to hBNP I 5-27 were eluted with 0.1 M glycine HCI, pH
2.5, brought to pH 7.5 with 2 M Tris buffer and concentrated in a Centriprep I 0.
_ 22 WO 97/32900 PCT/LTS97/03163 _ 7. Preparation of Biotinvlated MAbs 106.3. 201.3 and 8.1 The monoclonal antibodies were dialyzed against 0.1 M sodium borate buffer, pH
8.8 and brought to a final concentration of 1 to 3 mg/mL. Amino-hexanoyl-biotin-N-hydroxysuccinimide was prepared in dimethyl sulfoxide at a concentration of 10 mglmL and added to the antibodies at a ratio of 200 pg of the biotin ester/mg MAb.
Conjugation was carried out at room temperature for 4 hours. Uncoupled material was removed from the conjugated antibody by dialysis against phosphate buffered saline.
8. ~itope Analysis hBNP epitopes reacting with MAb 201.3, MAb 106.3 and MAb 8.I were determined using an inhibition ELISA. hBNP biotinylated with a single biotin at the N-terminal amino acid during solid phase synthesis was used as the indicator for competition studies with MAb 106.3 and MAb 8.1. hBNP biotinylated at the two cysteine residues, 10 and 26, was prepared by coupling with the sulfl~ydryl reactive biotinylation reagent Biotin-BN1CC.
This reagent was necessary to complete the inhibition studies with MAb 201.3.
Microtiter plates were coated with goat anti-mouse IgG (F~ specific) (0.5 pg/100 pL/well in bicarbonate buffer, pH 9 for 2 hours at 37°C).
Wells were washed four times with wash buffer (0.0~ M Tris, pH 7.5, 0.15 M NaCI, 0.05% Tween-20).
Purified monoclonal antibodies 106.3, 201.3 and 8.1 were diluted in assay buffer (0.0~
M Tris, pH 7.5, 0.1 S M NaCI, 0.1 % Tween-20 and 1 % BSA) and 180 pg/100 pL/well was incubated for 2 hours at room temperature. The wells were washed with wash buffer. Various different hBNP peptide fragments were mixed in assay buffer with biotinylated hBNP 1-32 at a molar ratio of 100:1 peptide fca~ment:biotin-hBNP, added to the microtiter wells and incubated for 1.5 hours at 4°C. Wells were washed once with wash buffer, streptavidin-horseradish peroxidase was added in 100 ~L assay buffer and incubated for 20 minutes at 4°C. Plates were washed 4 times with wash buffer and 200 uL TMB substrate was added and incubated for WO 97/32900 PCT/US97/03163 _ 30 minutes at room temperature. Color development was stopped with 2.5 M
sulfuric acid and O.D. values were read at 4~0 nm.
Results of the epitope analysis for MAb 106.3, MAb 201.3 and MAb 8.1 are presented in Fig. 3. The binding of biotin-hBNP 1-32 was significantly inhibited by the hBNP fragments specifically reactive with the monoclonal antibodies. For MAb 106.3, the smallest hBNP
fragment capable of producing an inhibition comparable to full length hBNP 1-32 was the peptide fragment hBNP 5-13. For MAb 201.3, the smallest hBNP peptide fragment producing an inhibition comparable to that seen with hBNP 1-32 was the hBNP fragment hBNP 1-10. For MAb 8.1, the smallest hBNP peptide fragment producing an inhibition comparable to that seen with hBNP I-32 was the fragment hBNP 27-32. Thus, hBNP fragments 1-10, 5-13 and 27-32 represent the hBNP epitopes specifically recognized by MAb 201.3, MAb 106.3 and MAb 8.1, respectively. This data also indicates that appropriate hBNP fragments, when used in a competition assay with the appropriate antibody, can provide an alternative reagent to the full lens h hBNP probe as an indicator of inhibition.
9. Assav for hBNP Usin~ MAb106.3 in a Monoclonal:Polvclonai Sandwich Microtiter plates were coated with MAb 106.3 at 100 ng/200 pL/well in bicarbonate buffer, pH 9 and allowed to adsorb for 2 hours at 37°C. hBNP was diluted in assay buffer at 12.8 ng/mL and 2-fold serial dilutions were prepared to produce a standard curve ranging down to 12.5 pg/mL. Buffer was removed from the plates and 100 p.L aliquots of the hBNP dilution series were added to the wells. Plates were incubated overnight at 4°C, washed once with wash buffer and incubated with 200 pL of a 1:2,500 dilution of rabbit antiserum containing polyclonal antibodies to hBNP. Plates were incubated for 2 hours at 37°C, washed 4 times with wash buffer and 200 pL/well goat anti-rabbit horseradish peroxidase was added.
Incubation was continued at 37°C for an additional 2 hours. Plates were washed 4 times with wash buffer, 200 pL TMB substrate was added and incubation was continued for ~ to 30 minutes. Color development was stopped with 100 pL of 2.5 M sulfuric acid and O.D. was measured at WO 97/32900 PCT/US97/03163 _ 450 nm. A standard curve was prepared by plotting O.D. versus pg/well hBNP.
The standard curve is presented in Fig. 4.
10. Assav for hBNP Using MAb 201.3 in a Monoclonal:Polyclonal Sandwich Plates were coated overnight at 4°C with 400 ng/well MAb 201.3 in bicarbonate buffer.
Plates were washed with wash buffer and blocked with assay buffer for 1 hour at room temperature. hBNP was diluted in assay buffer at a concentration of 10 ng/mL
and 4-fold serial dilutions were prepared to produce a standard curve ranging down to 10 pg/mL.
Plates were emptied and 100 pL aliquots of the dilution series were added to the wells.
Incubation was continued at room temperature for 2 hours. The plates were washed once with wash buffer.
Rabbit antiserum containing polyclonal antibodies to hBNP was diluted 1:1,000 in assay buffer, 100 ~tL was added to the wells and incubated at room temperature for 2 hours.
After three washes with wash buffer, 100 ~tL/well goat anti-rabbit horseradish peroxidase was added and incubation was continued at room temperature for 1 hour. Plates were washed 3 times with wash buffer, TMB substrate was added and color was allowed to continue for 20 minutes. The reaction was stopped with 100 pL of 2.5 M sulfuric acid and O.D. was measured at 450 nm.
The standard curve produced from these serial dilutions of hBNP is presented in Fig. ~.
11. Sandwich Assav Usin7 IylAb 106.3 and Monos~ecitic Polvclonal Reco~nizin~
hBNP 1 S-25 Microtiter plates were coated with MAb 106.3 at 100 ng/100 pLlwell in bicarbonate buffer, pH 9 overnight at 4°C. hBNP was diluted in assay buffer to 10 ng/mL and 2-fold serial dilutions were used to prepare a standard curve ranging down to 10 pg/mL,.
Plates were washed and blocked for 1 hour with assay buffer. One hundred microliter aliquots of the hBNP dilution series were added to the wells and incubated at room temperature for 2 hours.
The wells were washed 4 times with wash buffer and 100 pL of a 1:50 dilution of rabbit IgG
monospecific for hBNP 1 ~-25 were added. The plates were incubated for 2 hours, washed 4 times with wash butter and 200 p.L/well of goat anti-rabbit horseradish peroxidase was added.
Incubation was WO 97/32900 PCT/US97/03163 _ continued for 30 minutes. Plates were washed 4 times with wash buffer, 200 pL
TMB substrate was added and color was allowed to develop for 10 minutes. Color development was stopped with 100 pL of 2.5 M sulfuric acid and O.D. was measured at 450 nm. A standard curve was prepared by plotting O.D. versus pg/well hBNP. The standard curve is presented in Fig. 6.
S
12. Sandwich Assav Using MAb 201.3 and Monos ecific Polvclonal RecoQnizina hBNP 15-25 Microtiter plates were coated with MAb 201.3 at 400 ng/100 pL/weIl in bicarbonate buffer, pH 9 overnight at 4°C. hBNP was diluted in assay buffer to 10 ng/mL and 2-fold serial dilutions were used to prepare a standard curve ranging dow to 10 pg/mL.
Plates were washed and blocked for 1 hour with assay buffer. One hundred microliter aliquots of the hBNP dilution series were added to the wells and incubated at room temperature for 2 hours.
The wells were washed 4 times with wash buffer and 100 uL of a 1:50 dilution of rabbit IgG
monospecific for 1 S hBNP 15-25 were added. The plates were incubated for 2 hours at room temperature, washed 4 times with wash buffer and 200 pL/well goat anti-rabbit horseradish peroxidase was added.
Incubation was continued for 30 minutes. Plates were washed 4 times with wash buffer, TMB
substrate was added and color was allowed to develop for 10 minutes. Color development was stopped with 100 pL of 2.~ M sulfuric acid and O.D. was measured at 450 nm. A
standard curve was prepared by plotting O.D. versus pg/well hBNP. The standard curve is presented in Fig. 7.
13. Sandwich Assav for hBNP Usin~ MAb 8.1 and MAb 106.3 2~ Microtiter plate wells were coated overnight at 4°C with 100 ng/well MAb 8.1 in 200 uL bicarbonate buffer. 'Veils were washed with wash buffer and blocked far 1 hour at 4°C.
hBNP was diluted in assay buffer to 10 ng/mL and 2-fold standard dilutions were prepared to produce a standard curve ran~in~ down to approximately l0 pg/mL,. Buffer was removed from the wells and 100 uL aliquots of the hBNP standard dilution series and 100 p.L
of assay buffer containing 10 ng of biotinylated IvIAb 106.3 were added. Plates were incubated at 4°C for WO 97/32900 PCT/US97/03163 _ 1.5 hours. Plates were washed three times with wash buffer and 200 p.L of a 1:3,000 dilution of streptavidin-horseradish peroxidase was added to each well. Incubation was continued for an additional hour at 4°C. Wells were washed four times with wash buffer, 200 p.L TMB
substrate was added and incubation was continued for S to 30 minutes at room temperature.
Color development was stopped with 100 pL of 2.5 M sulfuric acid and O.D. was measured at 450 nm. A standard curve was prepared by plotting O.D. versus pg/well hBNP.
The standard curve is presented in Fig. 8.
14. Sandwich Assav for hBNP Using MAb 201.3 and MAb 8.1 Microtiter plate wells were coated overnight at 4°C with 400 ng/well MAb 201.3 in 200 pL bicarbonate buffer. Wells were washed three times with wash buffer and blocked for I hour. hBNP was diluted in assay buffer to 100 ng/mL and 10 ng/mL and serial 4-fold dilutions were prepared to produce a standard curve ranging down to approximately 10 pglmL.
Buffer was removed from the wells and 100 pL aliquots of the hBNP standard dilution series were added. Incubation was carried out at room temperature for I .5 hours.
Plates were washed three times with wash buffer and 100 pL of assay buffer containing 10 ng of biotinylated MAb 8.1 was added to each well. Incubation was continued for an additional 1.5 hours at room temperature. Wells were washed three times with wash buffer and 100 pL of a 1:3,000 dilution of streptavidin-horseradish peroxidase was added to each well. Incubation was continued for an additional hour at room temperature. Wells were washed three times with wash buffer.
TMB substrate (200 pL) was added and incubated at room temperature for S to 30 minutes.
Color development was stopped with 100 p.L of 2.5 M sulfuric acid and O.D. was measured at 450 nm. A standard curve was prepared by plotting O.D. versus pj/well hBNP.
The standard 2~ curve is presented in Fig. 9.
I ~. Competition .'ISSaV Using MAb 106.3 Rea<'ents used in this assay included NIAb 106.3, biotinylated hBNP 1-32 competing rea;ent and a plasma diluent capable of controlling patient sample interference. Plasma diluent WO 97/32900 PCT/US97/03163 _ can be prepared from pooled human plasma or pooled human serum. Preparation from plasma involves inducement of clotting by addition of 2 mg/mL calcium chloride, incubation at room temperature to promote clotting and degrade endogenous hBNP, dialysis using 15,000 MW
cutoff dialysis tubing against 0.001 M phosphate buffer containing 0.15 M
NaCI, removal of S clotted material, addition of EDTA at a concentration of 1.5 mg/mL and filtration through a 0.2 p filter. Because of the susceptibility of hBNP to proteolytic degradation, it is important to add a protease inhibitor such as 4-(2-aminoethyl)-benzenesulfonyl fluoride, HCl (1 mM to the plasma diluent and assay buffer). Microtiter plates were prepared by adding 200 pL/well of goat anti-murine antibody (F~ specific, approximately 0.5 ug/well) in bicarbonate buffer, pH 9 and incubating for 2 hours at 37°C. Plates were washed 4 times with wash buffer.
MAb 106.3 was diluted in assay buffer and 100 pL (90 pg/well) was added to the microtiter wells. Incubation was continued for 2 hours at room temperature. Plates were emptied and 200 pL/well assay buffer was added. hBNP 1-32 was diluted directly in the plasma diluent using two-fold dilutions to produce a standard curve ranging from 320 pg/mL, to S pg/mL. One I S hundred microliter samples were added to wells containing 200 pL assay buffer, plates were covered and incubated overnight at 2-8°C on an orbital shaker. Plasma samples from patients were generally diluted at least 1:2 in plasma diluent before they were added to the wells. For patients with high levels of hBNP all further sample dilutions were prepared in plasma diluent.
Following the overnight incubation, the wells were emptied and washed once with 200 pL wash buffer. Biotin-hBNP was diluted in assay buffer and 200 uL/well (12p pg/well) was added.
Incubation was carried out for 1 hour at 1-8°C on an orbital shaker.
The contents were removed from the wells, 200 uL streptavidin-horseradish peroxidase was added and incubation was continued for 30 minutes at 2-8°C. The plate was washed 4-S times with 200 pL/well wash buffer and 200 pL TMB mas added. Incubation was continued at room temperature for 30 minutes to 1 hour. Color development was stopped by adding 100 pL 2.5 M
sulfuric acid to the wells and O.D. measurements were made at 450 nm. O.D. values were converted to BBo values and a standard curve was prepared by plotting BB~ versus pg/mL hBNP.
The standard curve is shown in Fi;. 10. The standard curve provides a workin~ range of s 10 to 200 pg/mL.
hBNP levels in patient samples were determined by extrapolation from the standard curve.
WO 97/32900 PCT/US97/03163 _ Plasma hBNP levels deternlined for 15 control subjects and 15 patients with congestive heart disease are provided in Fig. 11.
substrate gave specific subclass reactivities for the three monoclonals. MAb 106.3 was determined to be an IgGtx antibody, MAb 201.3 was determined to belong to subclass IgCn.x and MAb 8.1 was determined to belong to subclass IgGtx.
Rabbit polyclonal antibody was tested for reactivity to hBNP 1-32 as well as to a variety of hBNP fragments. Microtiter plates were coated with 100 ng of the various peptides/well in 200 pL of 0.1 M bicarbonate buffer, pH 8-9. The plates were blocked with 0.1%
gelatin for 30 minutes at 37°C. Rabbit serum was diluted 1:1000 followed by 5 three-fold dilutions in a 1 ~ Tris/Tween/BSA buffer (O.OSM Tris, pH 7.5, 0.15 M NaCI, 1% BSA, 0.1% Tween-20). One hundred microliters of the antibody dilution series were added to the microtiter wells and incubated at 4°C for 2 hours. A wash with Tris/Tween/BSA buffer was followed by a 1 hour incubation with goat anti-rabbit horseradish peroxidase. The wells were washed with buffer 4 times and 200 pL TMB substrate was added. Following a 30 to 45 minute incubation the reaction was stopped with 2.5 M sulfuric acid and the O.D. was read at 450 nnt. Reactivity with the various peptides is presented in Fig. 2. The rabbit antiserum demonstrated specific reactivities with four hBNP peptide fragments, 1-10, 5-13, 15-25 and 27-32, as well as strong reactivity to hBNP 1-32.
2~ 6. Antibody Production and Purification Hybridoma cells were seeded in roller bottles at a concentration of 300,000 cellslmL in RPMI 1640 tissue culture medium supplemented with ~% Fetal Clone (Hyclone) and grown to a density of approximately 1 x 106 cells/mL. The medium was replaced with serum free Hybridoma SFM medium and incubation was continued for an additional 3 to 5 days. Cells were separated from the culture medium by centrifugation at 400 x g and the medium was clarified by filtration through a 0.2 p filter. The medium was applied to a Prosep Protein-A
affinity column (Bioprocessing Inc.) that had been previously equilibrated with binding buffer at pH 8.6 (1 M glycine, 0.15 M NaCI). After application of the culture medium was completed . __ the column was washed with binding buffer until OD readings monitored at 280 nM returned to baseline levels. Antibody was eluted using 100 mM citric acid pH 3.0, concentrated to .
approximately 1 mg/rnL in a Centriprep 10 concentrator and dialyzed overnight at 4°C against PBS, pH 7.5. Rabbit antiserum was cleared of lipid prior to column purification of polyclonal IgG. Each 1.5 parts of serum was mixed with 1 part of SeroClea~'~''Reagent (Calbiochem), vortexed for approximately 1 minute and centrifuged to separate lipid and aqueous phases. The cleared serum was then loaded directly onto the column with a perfusion pump and purified in the same manner as the tissue culture supernatant fluid.
Rabbit antibody monospecific to the hBNP epitope comprising amino acids 15-25 was isolated from the polyclonal IgG using a diaminodipropylamine affinity column (DADPA) to which the synthetic hBNP fragment 15-27 was immobilized. The DADPA gel was prepared for coupling by washing with 5 mL water followed by 5 mL 0.1 MES buffer (2-(N-morpholino)ethanesulfonic acid), 0.9% NaCI, pH 4.7. hBNP I ~-27 (2 mg) was dissolved in 2 mL of MES buffer and mixed with the gel. EDC (1-ethyl-3-(3-dimethylarninopropyl)carbodiimide) dissolved in MES buffer was added to the gel and incubated with stirring for 3 hours at room temperature. The column was washed several times with I M NaCI to remove unbound peptide and blocked with 0.1% ovalbumin. Prior to application of the rabbit IaG, the column was washed with 5 column volumes of PBS, pH 7.5.
The rabbit IgG was cycled through the column 5 times followed by 5 washes with PBS buffer.
The antibodies bound to hBNP I 5-27 were eluted with 0.1 M glycine HCI, pH
2.5, brought to pH 7.5 with 2 M Tris buffer and concentrated in a Centriprep I 0.
_ 22 WO 97/32900 PCT/LTS97/03163 _ 7. Preparation of Biotinvlated MAbs 106.3. 201.3 and 8.1 The monoclonal antibodies were dialyzed against 0.1 M sodium borate buffer, pH
8.8 and brought to a final concentration of 1 to 3 mg/mL. Amino-hexanoyl-biotin-N-hydroxysuccinimide was prepared in dimethyl sulfoxide at a concentration of 10 mglmL and added to the antibodies at a ratio of 200 pg of the biotin ester/mg MAb.
Conjugation was carried out at room temperature for 4 hours. Uncoupled material was removed from the conjugated antibody by dialysis against phosphate buffered saline.
8. ~itope Analysis hBNP epitopes reacting with MAb 201.3, MAb 106.3 and MAb 8.I were determined using an inhibition ELISA. hBNP biotinylated with a single biotin at the N-terminal amino acid during solid phase synthesis was used as the indicator for competition studies with MAb 106.3 and MAb 8.1. hBNP biotinylated at the two cysteine residues, 10 and 26, was prepared by coupling with the sulfl~ydryl reactive biotinylation reagent Biotin-BN1CC.
This reagent was necessary to complete the inhibition studies with MAb 201.3.
Microtiter plates were coated with goat anti-mouse IgG (F~ specific) (0.5 pg/100 pL/well in bicarbonate buffer, pH 9 for 2 hours at 37°C).
Wells were washed four times with wash buffer (0.0~ M Tris, pH 7.5, 0.15 M NaCI, 0.05% Tween-20).
Purified monoclonal antibodies 106.3, 201.3 and 8.1 were diluted in assay buffer (0.0~
M Tris, pH 7.5, 0.1 S M NaCI, 0.1 % Tween-20 and 1 % BSA) and 180 pg/100 pL/well was incubated for 2 hours at room temperature. The wells were washed with wash buffer. Various different hBNP peptide fragments were mixed in assay buffer with biotinylated hBNP 1-32 at a molar ratio of 100:1 peptide fca~ment:biotin-hBNP, added to the microtiter wells and incubated for 1.5 hours at 4°C. Wells were washed once with wash buffer, streptavidin-horseradish peroxidase was added in 100 ~L assay buffer and incubated for 20 minutes at 4°C. Plates were washed 4 times with wash buffer and 200 uL TMB substrate was added and incubated for WO 97/32900 PCT/US97/03163 _ 30 minutes at room temperature. Color development was stopped with 2.5 M
sulfuric acid and O.D. values were read at 4~0 nm.
Results of the epitope analysis for MAb 106.3, MAb 201.3 and MAb 8.1 are presented in Fig. 3. The binding of biotin-hBNP 1-32 was significantly inhibited by the hBNP fragments specifically reactive with the monoclonal antibodies. For MAb 106.3, the smallest hBNP
fragment capable of producing an inhibition comparable to full length hBNP 1-32 was the peptide fragment hBNP 5-13. For MAb 201.3, the smallest hBNP peptide fragment producing an inhibition comparable to that seen with hBNP 1-32 was the hBNP fragment hBNP 1-10. For MAb 8.1, the smallest hBNP peptide fragment producing an inhibition comparable to that seen with hBNP I-32 was the fragment hBNP 27-32. Thus, hBNP fragments 1-10, 5-13 and 27-32 represent the hBNP epitopes specifically recognized by MAb 201.3, MAb 106.3 and MAb 8.1, respectively. This data also indicates that appropriate hBNP fragments, when used in a competition assay with the appropriate antibody, can provide an alternative reagent to the full lens h hBNP probe as an indicator of inhibition.
9. Assav for hBNP Usin~ MAb106.3 in a Monoclonal:Polvclonai Sandwich Microtiter plates were coated with MAb 106.3 at 100 ng/200 pL/well in bicarbonate buffer, pH 9 and allowed to adsorb for 2 hours at 37°C. hBNP was diluted in assay buffer at 12.8 ng/mL and 2-fold serial dilutions were prepared to produce a standard curve ranging down to 12.5 pg/mL. Buffer was removed from the plates and 100 p.L aliquots of the hBNP dilution series were added to the wells. Plates were incubated overnight at 4°C, washed once with wash buffer and incubated with 200 pL of a 1:2,500 dilution of rabbit antiserum containing polyclonal antibodies to hBNP. Plates were incubated for 2 hours at 37°C, washed 4 times with wash buffer and 200 pL/well goat anti-rabbit horseradish peroxidase was added.
Incubation was continued at 37°C for an additional 2 hours. Plates were washed 4 times with wash buffer, 200 pL TMB substrate was added and incubation was continued for ~ to 30 minutes. Color development was stopped with 100 pL of 2.5 M sulfuric acid and O.D. was measured at WO 97/32900 PCT/US97/03163 _ 450 nm. A standard curve was prepared by plotting O.D. versus pg/well hBNP.
The standard curve is presented in Fig. 4.
10. Assav for hBNP Using MAb 201.3 in a Monoclonal:Polyclonal Sandwich Plates were coated overnight at 4°C with 400 ng/well MAb 201.3 in bicarbonate buffer.
Plates were washed with wash buffer and blocked with assay buffer for 1 hour at room temperature. hBNP was diluted in assay buffer at a concentration of 10 ng/mL
and 4-fold serial dilutions were prepared to produce a standard curve ranging down to 10 pg/mL.
Plates were emptied and 100 pL aliquots of the dilution series were added to the wells.
Incubation was continued at room temperature for 2 hours. The plates were washed once with wash buffer.
Rabbit antiserum containing polyclonal antibodies to hBNP was diluted 1:1,000 in assay buffer, 100 ~tL was added to the wells and incubated at room temperature for 2 hours.
After three washes with wash buffer, 100 ~tL/well goat anti-rabbit horseradish peroxidase was added and incubation was continued at room temperature for 1 hour. Plates were washed 3 times with wash buffer, TMB substrate was added and color was allowed to continue for 20 minutes. The reaction was stopped with 100 pL of 2.5 M sulfuric acid and O.D. was measured at 450 nm.
The standard curve produced from these serial dilutions of hBNP is presented in Fig. ~.
11. Sandwich Assav Usin7 IylAb 106.3 and Monos~ecitic Polvclonal Reco~nizin~
hBNP 1 S-25 Microtiter plates were coated with MAb 106.3 at 100 ng/100 pLlwell in bicarbonate buffer, pH 9 overnight at 4°C. hBNP was diluted in assay buffer to 10 ng/mL and 2-fold serial dilutions were used to prepare a standard curve ranging down to 10 pg/mL,.
Plates were washed and blocked for 1 hour with assay buffer. One hundred microliter aliquots of the hBNP dilution series were added to the wells and incubated at room temperature for 2 hours.
The wells were washed 4 times with wash buffer and 100 pL of a 1:50 dilution of rabbit IgG
monospecific for hBNP 1 ~-25 were added. The plates were incubated for 2 hours, washed 4 times with wash butter and 200 p.L/well of goat anti-rabbit horseradish peroxidase was added.
Incubation was WO 97/32900 PCT/US97/03163 _ continued for 30 minutes. Plates were washed 4 times with wash buffer, 200 pL
TMB substrate was added and color was allowed to develop for 10 minutes. Color development was stopped with 100 pL of 2.5 M sulfuric acid and O.D. was measured at 450 nm. A standard curve was prepared by plotting O.D. versus pg/well hBNP. The standard curve is presented in Fig. 6.
S
12. Sandwich Assav Using MAb 201.3 and Monos ecific Polvclonal RecoQnizina hBNP 15-25 Microtiter plates were coated with MAb 201.3 at 400 ng/100 pL/weIl in bicarbonate buffer, pH 9 overnight at 4°C. hBNP was diluted in assay buffer to 10 ng/mL and 2-fold serial dilutions were used to prepare a standard curve ranging dow to 10 pg/mL.
Plates were washed and blocked for 1 hour with assay buffer. One hundred microliter aliquots of the hBNP dilution series were added to the wells and incubated at room temperature for 2 hours.
The wells were washed 4 times with wash buffer and 100 uL of a 1:50 dilution of rabbit IgG
monospecific for 1 S hBNP 15-25 were added. The plates were incubated for 2 hours at room temperature, washed 4 times with wash buffer and 200 pL/well goat anti-rabbit horseradish peroxidase was added.
Incubation was continued for 30 minutes. Plates were washed 4 times with wash buffer, TMB
substrate was added and color was allowed to develop for 10 minutes. Color development was stopped with 100 pL of 2.~ M sulfuric acid and O.D. was measured at 450 nm. A
standard curve was prepared by plotting O.D. versus pg/well hBNP. The standard curve is presented in Fig. 7.
13. Sandwich Assav for hBNP Usin~ MAb 8.1 and MAb 106.3 2~ Microtiter plate wells were coated overnight at 4°C with 100 ng/well MAb 8.1 in 200 uL bicarbonate buffer. 'Veils were washed with wash buffer and blocked far 1 hour at 4°C.
hBNP was diluted in assay buffer to 10 ng/mL and 2-fold standard dilutions were prepared to produce a standard curve ran~in~ down to approximately l0 pg/mL,. Buffer was removed from the wells and 100 uL aliquots of the hBNP standard dilution series and 100 p.L
of assay buffer containing 10 ng of biotinylated IvIAb 106.3 were added. Plates were incubated at 4°C for WO 97/32900 PCT/US97/03163 _ 1.5 hours. Plates were washed three times with wash buffer and 200 p.L of a 1:3,000 dilution of streptavidin-horseradish peroxidase was added to each well. Incubation was continued for an additional hour at 4°C. Wells were washed four times with wash buffer, 200 p.L TMB
substrate was added and incubation was continued for S to 30 minutes at room temperature.
Color development was stopped with 100 pL of 2.5 M sulfuric acid and O.D. was measured at 450 nm. A standard curve was prepared by plotting O.D. versus pg/well hBNP.
The standard curve is presented in Fig. 8.
14. Sandwich Assav for hBNP Using MAb 201.3 and MAb 8.1 Microtiter plate wells were coated overnight at 4°C with 400 ng/well MAb 201.3 in 200 pL bicarbonate buffer. Wells were washed three times with wash buffer and blocked for I hour. hBNP was diluted in assay buffer to 100 ng/mL and 10 ng/mL and serial 4-fold dilutions were prepared to produce a standard curve ranging down to approximately 10 pglmL.
Buffer was removed from the wells and 100 pL aliquots of the hBNP standard dilution series were added. Incubation was carried out at room temperature for I .5 hours.
Plates were washed three times with wash buffer and 100 pL of assay buffer containing 10 ng of biotinylated MAb 8.1 was added to each well. Incubation was continued for an additional 1.5 hours at room temperature. Wells were washed three times with wash buffer and 100 pL of a 1:3,000 dilution of streptavidin-horseradish peroxidase was added to each well. Incubation was continued for an additional hour at room temperature. Wells were washed three times with wash buffer.
TMB substrate (200 pL) was added and incubated at room temperature for S to 30 minutes.
Color development was stopped with 100 p.L of 2.5 M sulfuric acid and O.D. was measured at 450 nm. A standard curve was prepared by plotting O.D. versus pj/well hBNP.
The standard 2~ curve is presented in Fig. 9.
I ~. Competition .'ISSaV Using MAb 106.3 Rea<'ents used in this assay included NIAb 106.3, biotinylated hBNP 1-32 competing rea;ent and a plasma diluent capable of controlling patient sample interference. Plasma diluent WO 97/32900 PCT/US97/03163 _ can be prepared from pooled human plasma or pooled human serum. Preparation from plasma involves inducement of clotting by addition of 2 mg/mL calcium chloride, incubation at room temperature to promote clotting and degrade endogenous hBNP, dialysis using 15,000 MW
cutoff dialysis tubing against 0.001 M phosphate buffer containing 0.15 M
NaCI, removal of S clotted material, addition of EDTA at a concentration of 1.5 mg/mL and filtration through a 0.2 p filter. Because of the susceptibility of hBNP to proteolytic degradation, it is important to add a protease inhibitor such as 4-(2-aminoethyl)-benzenesulfonyl fluoride, HCl (1 mM to the plasma diluent and assay buffer). Microtiter plates were prepared by adding 200 pL/well of goat anti-murine antibody (F~ specific, approximately 0.5 ug/well) in bicarbonate buffer, pH 9 and incubating for 2 hours at 37°C. Plates were washed 4 times with wash buffer.
MAb 106.3 was diluted in assay buffer and 100 pL (90 pg/well) was added to the microtiter wells. Incubation was continued for 2 hours at room temperature. Plates were emptied and 200 pL/well assay buffer was added. hBNP 1-32 was diluted directly in the plasma diluent using two-fold dilutions to produce a standard curve ranging from 320 pg/mL, to S pg/mL. One I S hundred microliter samples were added to wells containing 200 pL assay buffer, plates were covered and incubated overnight at 2-8°C on an orbital shaker. Plasma samples from patients were generally diluted at least 1:2 in plasma diluent before they were added to the wells. For patients with high levels of hBNP all further sample dilutions were prepared in plasma diluent.
Following the overnight incubation, the wells were emptied and washed once with 200 pL wash buffer. Biotin-hBNP was diluted in assay buffer and 200 uL/well (12p pg/well) was added.
Incubation was carried out for 1 hour at 1-8°C on an orbital shaker.
The contents were removed from the wells, 200 uL streptavidin-horseradish peroxidase was added and incubation was continued for 30 minutes at 2-8°C. The plate was washed 4-S times with 200 pL/well wash buffer and 200 pL TMB mas added. Incubation was continued at room temperature for 30 minutes to 1 hour. Color development was stopped by adding 100 pL 2.5 M
sulfuric acid to the wells and O.D. measurements were made at 450 nm. O.D. values were converted to BBo values and a standard curve was prepared by plotting BB~ versus pg/mL hBNP.
The standard curve is shown in Fi;. 10. The standard curve provides a workin~ range of s 10 to 200 pg/mL.
hBNP levels in patient samples were determined by extrapolation from the standard curve.
WO 97/32900 PCT/US97/03163 _ Plasma hBNP levels deternlined for 15 control subjects and 15 patients with congestive heart disease are provided in Fig. 11.
Claims (30)
1. An antibody or a functionally active fragment thereof that is monospecific for a peptide epitope comprising amino acids 5-13 of human brain natriuretic peptide (hBNP) as set out in Figure 1.
2. An antibody or a functionally active fragment thereof of claim 1 which is a monoclonal antibody.
3. An antibody or a functionally active fragment thereof of claim 2 which is produced by hybridoma cell line 106.3, ATCC HB 12044.
4. An antibody or a functionally active fragment thereof that is monospecific for a peptide epitope comprising amino acids 1-10 of human brain natriuretic peptide (hBNP) as set out in Figure 1.
5. An antibody or a functionally active fragment thereof of claim 4 which is a monoclonal antibody.
6. An antibody or a functionally active fragment thereof of claim 5 which is produced by hybridoma cell line 201.3, ATCC HB 12045.
7. An antibody or a functionally active fragment thereof which is monospecific for a peptide epitope comprising amino acids 15-25 of human brain natriuretic peptide (hBNP) as set out in Figure 1.
8. A method of quantifying human brain natriuretic peptide (hBNP) in a biological fluid which method comprises forming a labeled first antibody-hBNP-second antibody complex said complex consisting of:
(a) a first antibody selected from the group consisting of:
(i) an antibody or a functionally active fragment thereof that is monospecifically reactive with an hBNP fragment comprising amino acids 5-13 of hBNP as set out in Figure 1;
(ii) an antibody or a functionally active fragment thereof that is monospecifically reactive with an hBNP fragment comprising amino acids 1-10 of hBNP as set out in Figure 1;
(iii) an antibody or a functionally active fragment thereof that is monospecifically reactive with an hBNP fragment comprising amino acids 15-25 of hBNP as set out in Figure 1;
(b) any hBNP contained in said biological fluid; and (c) a second antibody or a functionally active fragment thereof immunoreactive with hBNP; wherein at least one of said first and second antibody comprises at least one label; and determining the amount of hBNP in the sample by quantifying the label in said complex.
(a) a first antibody selected from the group consisting of:
(i) an antibody or a functionally active fragment thereof that is monospecifically reactive with an hBNP fragment comprising amino acids 5-13 of hBNP as set out in Figure 1;
(ii) an antibody or a functionally active fragment thereof that is monospecifically reactive with an hBNP fragment comprising amino acids 1-10 of hBNP as set out in Figure 1;
(iii) an antibody or a functionally active fragment thereof that is monospecifically reactive with an hBNP fragment comprising amino acids 15-25 of hBNP as set out in Figure 1;
(b) any hBNP contained in said biological fluid; and (c) a second antibody or a functionally active fragment thereof immunoreactive with hBNP; wherein at least one of said first and second antibody comprises at least one label; and determining the amount of hBNP in the sample by quantifying the label in said complex.
9. The method of claim 8 further comprising the step of separating the first antibody-hBNP-second antibody complex from the remainder of the biological fluid sample prior to quantifying the label in the first antibody-hBNP-second antibody complex.
10. The method of claim 8 wherein the label is selected from the group consisting of radioactive labels, enzymatic labels, fluorescent labels, thermometric labels and immuno-polymerase chain reaction labels.
11. The method of claim 10 wherein the label is an enzymatic label.
12. The method of claim 11 wherein the label is horseradish peroxidase.
13. The method of claim 8 wherein the quantifiable label is bound to the first or second antibody after formation of the first antibody-hBNP-second antibody complex.
14. The method of claim 13 wherein the first or second antibody is labeled after formation of the first antibody-hBNP-second antibody complex by contacting the complex with a labeled antibody that binds to the first or second antibody without displacing the first or second antibody from the complex.
15. The method of claim 9 wherein separation of the first antibody-hBNP-second antibody complex from the remainder of the biological fluid sample is effected by binding the first or second antibody to a solid support and removing the remainder of the biological fluid sample from contact with said solid support after formation of the first antibody-hBNP-second antibody complex.
16. The method of claim 8 wherein the biological fluid is plasma.
17. The method of claim 8 wherein the first antibody is a monoclonal antibody.
18. The method of claim 17 wherein the first antibody is a monoclonal antibody that recognizes a peptide epitope comprising amino acids 5-13 of hBNP as set out in Figure 1.
19. A method of quantifying the amount of human brain natriuretic peptide (hBNP)in a biological fluid which comprises:
(a) contacting a sample of the biological fluid with:
(i) an antibody or functional fragment thereof according to any one of claims 1-6 or 7; and (ii) hBNP or a fragment thereof comprising the peptide epitope which the antibody or functional fragment thereof is monospecific, having bound thereto a quantifiable label, under conditions that allow the formation of an antibody-hBNP
complex; and (b) determining the amount of hBNP in the sample by quantifying the label in the antibody-hBNP complex.
(a) contacting a sample of the biological fluid with:
(i) an antibody or functional fragment thereof according to any one of claims 1-6 or 7; and (ii) hBNP or a fragment thereof comprising the peptide epitope which the antibody or functional fragment thereof is monospecific, having bound thereto a quantifiable label, under conditions that allow the formation of an antibody-hBNP
complex; and (b) determining the amount of hBNP in the sample by quantifying the label in the antibody-hBNP complex.
20. The method of claim 19 further comprising the step of separating the antibody-hBNP complex from the remainder of the biological fluid sample prior to quantifying the label in the antibody-hBNP complex.
21. The method of claim 20 wherein separation of the antibody-hBNP complex from the remainder of the biological fluid sample is effected by binding the antibody to a solid support and removing the biological fluid sample from contact with the solid sup port after formation of the antibody-hBNP complex.
22. The method of claim 19 wherein the antibody is a monoclonal antibody.
23. The method of claim 19, wherein the antibody is an antibody that is monospecifically reactive with a peptide epitope comprising amino acids 1-10 of hBNP as set out in Figure 1.
24. The method of claim 19, wherein the antibody is an antibody that is monospecifically reactive with a peptide epitope comprising amino acids 15-25 of hBNP as set out in Figure 1.
25. A peptide fragment of hBNP, useful as a reagent in an immunoassay for quantifying hBNP, having the formula X1-V-Q-G-S-G-C-F-G-R-X2, wherein X1 is selected from the group consisting of hydrogen, M-, K-M-, P-K-M- or S-P-K-M-and X2 is selected from the group consisting of hydroxyl, -K, -K-M, -K-M-D and -K-M-D-R, or the retro-inverso isomers, partial retro-inverso isomers or D-amino acid isomers thereof.
26. A peptide fragment of claim 25 having a quantifiable label bound thereto.
27. A peptide fragment of hBNP, useful as a reagent in an immunoassay for quantifying hBNP, having the formula S-P-K-M-V-Q-G-S-G-C-X3, wherein X3 is selected from the group consisting of hydroxyl, -F and -F-G, or the retro-inverso-isomers, partial retro-inverso-isomers or D-amino acid isomers thereof.
28. A peptide fragment of claim 27 having a quantifiable label bound thereto.
29. A peptide fragment of hBNP, useful as a reagent in an immunoassay for quantifying hBNP, having the formula X4-M-D-R-I-S-S-S-S-G-L-G-X5, wherein X4 is selected from the group consisting of hydrogen, K-R-K- and G-R-K-and X5 is selected from the group consisting of hydroxyl, -C, -C-K, -C-K-V, -C-K-V-L,.
-C-K-V-L-R, -C-K-V-L-R-R and -C-K-V-L-R-R-H, or the retro-inverso-isomers, partial retro-inverso-isomers or D-amino acid isomers thereof.
-C-K-V-L-R, -C-K-V-L-R-R and -C-K-V-L-R-R-H, or the retro-inverso-isomers, partial retro-inverso-isomers or D-amino acid isomers thereof.
30. A peptide fragment of claim 29 having a quantifiable label bound thereto.
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| US61017296A | 1996-03-04 | 1996-03-04 | |
| US08/610,172 | 1996-03-04 | ||
| PCT/US1997/003163 WO1997032900A1 (en) | 1996-03-04 | 1997-03-04 | ASSAY AND REAGENTS FOR QUANTIFYING hBNP |
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| CA2248140A1 CA2248140A1 (en) | 1997-09-12 |
| CA2248140C true CA2248140C (en) | 2005-02-01 |
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| EP (3) | EP1557431B1 (en) |
| JP (3) | JP4049816B2 (en) |
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| PT (2) | PT2292662E (en) |
| WO (1) | WO1997032900A1 (en) |
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| US6117644A (en) * | 1998-06-04 | 2000-09-12 | Ottawa Heart Institute Research Corporation | Predicting and detecting cardiac allograft rejection |
| GB9827348D0 (en) * | 1998-12-12 | 1999-02-03 | Univ Leicester | Natriuretic peptide |
| AU5043900A (en) * | 1999-05-24 | 2000-12-12 | Mayo Foundation For Medical Education And Research | Adenovirus vectors encoding brain natriuretic peptide |
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| ES2380367T3 (en) * | 2000-12-05 | 2012-05-11 | Alexion Pharmaceuticals, Inc. | Rationally designed antibodies |
| US7396917B2 (en) | 2000-12-05 | 2008-07-08 | Alexion Pharmaceuticals, Inc. | Rationally designed antibodies |
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| US20040176914A1 (en) * | 2001-04-13 | 2004-09-09 | Biosite Incorporated | Methods and compositions for measuring biologically active natriuretic peptides and for improving their therapeutic potential |
| US20030219734A1 (en) * | 2001-04-13 | 2003-11-27 | Biosite Incorporated | Polypeptides related to natriuretic peptides and methods of their identification and use |
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| US5114923A (en) | 1988-05-31 | 1992-05-19 | California Biotechnology Inc. | Recombinant techniques for production of novel natriuretic and vasodilator peptides |
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| GB9211686D0 (en) * | 1992-06-03 | 1992-07-15 | Medisinsk Innovation A S | Chemical compounds |
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1997
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- 1997-03-04 EP EP05007745A patent/EP1557431B1/en not_active Expired - Lifetime
- 1997-03-04 AT AT97907946T patent/ATE297950T1/en active
- 1997-03-04 DK DK97907946T patent/DK0914344T3/en active
- 1997-03-04 EP EP10013178.8A patent/EP2292662B1/en not_active Expired - Lifetime
- 1997-03-04 DK DK10013178.8T patent/DK2292662T3/en active
- 1997-03-04 PT PT100131788T patent/PT2292662E/en unknown
- 1997-03-04 JP JP53184497A patent/JP4049816B2/en not_active Expired - Lifetime
- 1997-03-04 EP EP97907946A patent/EP0914344B8/en not_active Expired - Lifetime
- 1997-03-04 ES ES97907946T patent/ES2243979T3/en not_active Expired - Lifetime
- 1997-03-04 PT PT97907946T patent/PT914344E/en unknown
- 1997-03-04 DE DE69733560T patent/DE69733560T2/en not_active Expired - Lifetime
- 1997-03-04 WO PCT/US1997/003163 patent/WO1997032900A1/en active IP Right Grant
- 1997-03-04 ZA ZA9701864A patent/ZA971864B/en unknown
- 1997-03-04 AU AU19815/97A patent/AU1981597A/en not_active Abandoned
- 1997-10-01 US US08/942,332 patent/US6124430A/en not_active Expired - Lifetime
- 1997-10-01 US US08/942,456 patent/US6162902A/en not_active Expired - Lifetime
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2000
- 2000-02-23 US US09/510,721 patent/US6376207B1/en not_active Expired - Lifetime
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- 2006-01-17 HK HK06100788.0A patent/HK1078096A1/en not_active IP Right Cessation
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- 2007-02-07 JP JP2007028622A patent/JP2007169293A/en not_active Withdrawn
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| ATE297950T1 (en) | 2005-07-15 |
| JP2000507094A (en) | 2000-06-13 |
| JP2007169293A (en) | 2007-07-05 |
| EP2292662A2 (en) | 2011-03-09 |
| ZA971864B (en) | 1997-12-18 |
| EP0914344B8 (en) | 2005-08-10 |
| EP2292662A3 (en) | 2011-07-13 |
| PT2292662E (en) | 2014-07-16 |
| PT914344E (en) | 2005-10-31 |
| JP2011102318A (en) | 2011-05-26 |
| WO1997032900A1 (en) | 1997-09-12 |
| EP2292662B1 (en) | 2014-04-23 |
| EP0914344A1 (en) | 1999-05-12 |
| US6376207B1 (en) | 2002-04-23 |
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