WO1996022532A1 - Immunoassay method and reagent involving suspendible carbon labelled bioaffine particles - Google Patents

Immunoassay method and reagent involving suspendible carbon labelled bioaffine particles Download PDF

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Publication number
WO1996022532A1
WO1996022532A1 PCT/SE1996/000042 SE9600042W WO9622532A1 WO 1996022532 A1 WO1996022532 A1 WO 1996022532A1 SE 9600042 W SE9600042 W SE 9600042W WO 9622532 A1 WO9622532 A1 WO 9622532A1
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WIPO (PCT)
Prior art keywords
particles
analyte
ige
carbon
zone
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Application number
PCT/SE1996/000042
Other languages
French (fr)
Inventor
Maria LÖNNBERG
Jan Carlsson
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Pharmacia Ab
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Filing date
Publication date
Application filed by Pharmacia Ab filed Critical Pharmacia Ab
Priority to AU45928/96A priority Critical patent/AU4592896A/en
Priority to JP8522207A priority patent/JPH11505603A/en
Priority to EP96901591A priority patent/EP0804733A1/en
Publication of WO1996022532A1 publication Critical patent/WO1996022532A1/en

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    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/53Immunoassay; Biospecific binding assay; Materials therefor
    • G01N33/558Immunoassay; Biospecific binding assay; Materials therefor using diffusion or migration of antigen or antibody
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/53Immunoassay; Biospecific binding assay; Materials therefor
    • G01N33/543Immunoassay; Biospecific binding assay; Materials therefor with an insoluble carrier for immobilising immunochemicals
    • G01N33/54366Apparatus specially adapted for solid-phase testing
    • G01N33/54386Analytical elements
    • G01N33/54387Immunochromatographic test strips
    • G01N33/54388Immunochromatographic test strips based on lateral flow
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/58Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving labelled substances
    • G01N33/585Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving labelled substances with a particulate label, e.g. coloured latex

Definitions

  • the analysis is concerned with determining the analyte content of a sample either qualitatively or quantatively with the aid of its bioaffine counterpart, by forming a complex between the counterpart and the analyte.
  • a bioaffine reactant R x
  • the analyte concentration of the sample can then be determined from the amount of complex-bound and/or non-complex-bound labelled reactant (R ⁇ and R 1 " respectively) .
  • the invention uses suspendible carbon particles as a label.
  • bioaffinity When the bioaffinity relates to antibodies and antigens/hapt- ens, one speaks about immunoassays or immunochemical assaying. When the bioaffinity concerns complementary oligo/ polynucleotides, one speaks about hybridization methods.
  • the invention is adapted particularly to immunoassays.
  • Particles are important in this context. According to known techniques, these particles will primarily have colloidal dimensions - be in the form of sols (i.e. normally 1-200 run and spherical and monodispersed) .
  • Well- known particulate label groups are metal particles, non-metal particles (e.g. Si0 2 and carbon, latex and killed erythrocytes and bacteria) .
  • labels that can be shown indirectly such as individual members of bioaffine pairs, e.g. biotin or (strept)avidin, hapten or antibodies, class-specific determinants in antibodies, etc.
  • the indirectly detectable labels are often determined or assayed with the aid of their bioaffine counterparts labeled with labels that can be detected directly or indirectly.
  • heterogenous and homogenous methods describe whether or not labelled reactants (R ) present in the complex are separated from non- complex-bound reactants (R ⁇ ') prior to assaying labelled reactants.
  • Competitive methods utilize analyte analogs which compete with analytes in binding to a deficiency of reactants that have biospecific affinity to both the analyte and the analyte analog.
  • Analyte analogs may be analytes that are labelled with or bound to an insoluble phase (solid phase) in the analysis medium.
  • non-competitive methods are so-called sandwich methods in which the analyte is complexed between two or more reactants that exhibit biospecific affinity to mutually spaced epitopes on the analyte.
  • India Ink is ink/drawing ink based on stably suspended carbon black (sol) (Hackhs Chemical Dictionary, 4th Ed., Ed. Julius Grant, McGraw-Hill Book Company, page 346) .
  • EP 321,008 HBT Holland Biotechnology
  • the patent emphasizes that the particles shall be in the form of sols, meaning that particles which are able to settle to form a sediment are not present in the particle preparations used.
  • the patent makes particular mention to the production of sols by enclosing non-metallic colloidal primary particles in an inert hydrophilic envelope or by coupling reactants directly to the naked particle.
  • sensitivity increases with increasing particle sizes, provided that the particle preparations used are monodispersed particles in sol form.
  • the object of the present invention is to improve and simplify analysis methods of the kind defined in the introduction with the use of carbon particles as label groups.
  • FIGURE 1 This illustrates an embodiment of the invention (test strip) for determining total IgE with the aid of a sandwich test using solid-phase bound anti-IgE antibodies (R 2 ) bound in a detection zone (Z j ) , labelled anti-IgE antibodies (R : ) and a control zone (Z 4 ) containing solid-phase bound anti-IgG antibodies (in our case anti-mouse IgG because R x is a mouse monoclonal) .
  • the sample application zone (Z 3 ) is located in the lower part of the strip and the reagent R x is mixed with sample prior to its application to the strip at zone Z 3 .
  • Transport zones (Z 2 ' and Z 2 " and Z 2 '") are located between the sample application zone (Z 3 ) and the detection zone Z ) , between the detection zone ( Z x ) and the control zone (Z 4 ) and between the control zone and a sucking body, respectively. That part of the strip which remains above the control zone may be understood as being a further transport zone (Z 2 ''').
  • the arrow indicates the direction of flow in the strip.
  • the reactants can be replaced as discussed below for different types of analytes. By replacing the solid-phase bound antibody R 2 for an antigen/hapten, the test will measure antigen/hapten-specific IgE (see the following examples) .
  • the invention is based on the discovery that carbon particles of non-colloidal dimensions, preferably polydispersed and/or of irregular shape, function as labels and can even have a beneficial effect on the aforesaid analysis methods. Irregular particles have a greater surface/volume ratio per particle than spherical particles and thus give greater response or sensitivity to the analyses in which they are used as labels.
  • One aspect of the invention includes methods of the kind defined in the introduction. These methods generally include
  • the amount of particle-labelled reactant bound (R ⁇ ') or non-bound (Rx”) to the complex is determined qualitatively or quantitatively, wherein
  • the determined quantity is taken as a measure of the presence or amount, respectively, of the amount of analyte in the sample.
  • sensitivity increases with the amount o particles that can settle in accordance with the precedin paragraph.
  • the amount of particles that ar able to settle is often > 0.1%, such as > 1%, preferably > 50%, with an upper limit of 100% (all percentages being w/ percentages, alternatively measured in accordance with th method described under the heading "Sensitivity as a functiono of the amount of settleable particles" in the experimental par of this document.
  • the carbon particles have a weighted mean particl size of > 0.05 ⁇ m, preferably in the range of 0.2-5 ⁇ an more preferably in the range of 0.2-1 ⁇ ;
  • the top value of the particle distribution gives a diamete which is > 0.1 ⁇ , preferably a diameter in the range o 0.2-5 ⁇ m and more preferably in the range of 0.2-1 ⁇ m;
  • > 1%, such as > 10% or > 50%, with an upper limit of 100% of the particles, is > 0.1 ⁇ m and preferably lies in the range of 0.2-5 ⁇ m, and more preferably in the range of 0.2- 1 ⁇ m.
  • Suitable particle sizes and percentages of settleable particles will vary in accordance with the test method applied, analyte, affinity and specificity of the bioaffine reagent used.
  • the main rule is that, compared to a higher analyte concentration, a lower analyte concentration will demand a greater portion of particles that are > 200 n .
  • low- concentration analytes ⁇ 10 "10 M
  • FFF disk Centrifuge Photodensedimentometer
  • Tests carried out hitherto have been effected with commercially available carbon-particle preparations in the form of primary aggregates of primary carbon nodules (primary particles) stably linked together, most likely covalently.
  • the size of the nodules varies from carbon quality to carbon quality, but is normally in the range of 5-250 nm, with preference for 20-100 nm.
  • the number of primary nodules contained in each primar aggregate also varies, and is 4-200 with regard to the most usable qualities, with preference to 6-75.
  • stabl linked together is meant that the aggregates will not disintegrate under the conditions normally applicable to biospecific affinity reactions.
  • the configuration of the primary aggregates may also vary from an elongated, branche configuration to more compact structures.
  • the primary aggregates may, in turn, be secondarily aggregated to form larger units .
  • these secondary aggregates are stable against disintegration, they can be used in the inventive analysis method provided that their sizes have no deleterious effect on the method applied.
  • a number of potentially usable carbon qualities which fulfil the aforesaid definitions are commercially available from Degussa (Germany) and other manufacturers.
  • Examples are carbon black, which is the collective name for furnace black, channel black, lamp black and acetylene black.
  • the carbon content of these materials is usually from 85% and more, terminating at a content immediately beneath 100% (99.999%) (w/w) .
  • the manufacturers have lowered the carbon content from 99-100% down to 85-99.9% (w/w) , by oxidative treatment of carbon black, among others. Oxidatively-treated forms of the carbon particles concerned have been found particularly usable in the inventive method, due to improved suspendibility when preparing the carbon-labelled reactant R x .
  • the aforesaid carbon particles may be enclosed in polymeric envelopes and/or may carry bioaffine reactants or other groups that are able to take part in hydrophobic interactions, ion- binding, dipole, dipole-binding, etc.
  • One or more particles may be enclosed in one and the same polymeric envelope or casing.
  • Bioaffine reactants R x may be bound adsorptively directly t the naked aggregates or via an envelope in accordance with the previous paragraph. In this latter case, the possibility of covalent bonding is obvious and covalent bonding directly to the naked aggregates is also potentially feasible. Bioaffine reactants are best adsorbed on the carbon particles that are in suspended form.
  • the labelled bioaffine reactant is exogenous to the sample, and normally also exogenous to the individual/organism/source from which the sample derives.
  • sample pretreatments are a) sample dilution, b) sample concentration, c) analyte enrichment (e.g. removing disturbing substances) , d) pH-adjustment or adjustment by the use of other means, e) forming complexes between the analyte and a bioaffine counterpart, f) analyte modifications other than complex formation according to e) , and so on.
  • Points e) and f) above imply that the analyte in steps i-iii refers to an analyte that is a modified version of the analyte in the original sample. All pretreatment processes are carried out so that the amount of analyte in the original sample and the amount of modified analyte in the pretreated sample will be unequivocally related to one another.
  • Analysis conditions such as temperature, concentration, pH, sequence of additions of reactants and selection of reactants to be added are analogous with the conditions previously applied in respect of other labels used in assays which employ biospecific affinity reactions (immunochemical assaying, hybridizing methods, etc.).
  • the assay medium is normally water, optionally mixed with water-miscible solvents.
  • the temperature is in the range of 0- 40°C and the pH in the range of 4-10.
  • the temperature will preferably lie in the range of 0-100°C.
  • heterogenous methodology i.e. a technique in which labelled reactant R l ' included in the complex is separated physically from labelled reactant R 1 " which is not included in the complex, prior to assaying one or both of said reactants.
  • said reactants are separated by using a phase (matrix) which is insoluble in the assay medium and which has a bioaffine reactant bound thereto, to achieve selective partition of the complex-bound labelled reactant to the matrix before separation takes place.
  • the insoluble phase (the matrix) used in heterogenous variants of the invention may have the form of a strip, plate, porous continuous matrix (monolith) , hydrophilic particles, preferably porous particles, membranes, diaphragms, etc.
  • the prerequisites for separating, assaying and correlating analytes as a function of labelled reactants are the same as those applicable in known techniques, with the exception of being adapted to the fact that according to the invention, the label group consists of particles.
  • the heterogenous method according to the invention considered most practical at present utilizes porous matrices, either in the form of particle-packed beds or in the form of monoliths (self-coherent matrices) .
  • Monolith-type matrices may be given the form of test strips or membranes which include a detection zone (Z x ) for the detection of formed complexes.
  • the test strip or membrane will also normally include one or more zones (e.g. Z 2 ' and Z 2 ") for the transportation of sample, reactant (e.g. R , washing solution, etc., to and/or from respective detection zones, and a sample application zone (Z 3 ) , and optionally further zones Z 4 , Z 5 , etc.
  • the transport zone Z 2 ' lies between the sample application zone and the detection zone.
  • the zones need not necessarily be comprised of the same material. For instance, it is often practical to choose material with regard to the function of the zone. See below.
  • the detection zone Z x contains a bioaffine reactant (R 2 ) which is stably bound to the matrix and which is capable of capturing labelled reactant R x in a quantity which is a function of the analyte content of the sample.
  • R 2 bioaffine reactant
  • the detection zone will blacken. Blackening of the detection zone can be shown both quantatively and qualita ⁇ tively, in several ways, preferably visually although perhaps more preferably, and more reliably, through the medium of computer-based picture or image analysis in accordance with Amerongen, et al (J. Biotechnol. 30 (1983), pp. 185-189, and Clin. Chim. Acta 229 (1994), pp. 67-75).
  • the stably bound reactant R 2 and the labelled reactant R x are both directed against the analyte (sandwich test) ;
  • the bioaffine reactant R 2 stably anchored to the detection zone is directed against epitopes present in both analyte and reactant R x (R x is an analyte analog) (competitive test) .
  • R 2 being stably anchored in the detection zone is meant to imply that R 2 will not be eluated by the various assay-buffers that pass through.
  • the reactant R 2 is anchored in a conventional manner, i.e. covalently bound or bound via adsorption (normally via hydrophobic forces) .
  • the simplest heterogenous variant of the invention using a porous matrix in the form of a packed particle bed or in the form of a monolith has only one detection zone Z 1 , this zone also functioning as a sample application zone.
  • Reagent e.g. R x
  • washing solution are applied directly to the detection zone and leave the matrix immediately after having passed through said zone.
  • the detection zone is in contact with one or two transport zones (Z 2 ' and Z 2 ") for transportation to and from the detection zone respectively.
  • Z 2 " is preferably highly absorbent so as to facilitate liquid transportation.
  • the reactant R x can be contacted with the detection zone in a number of different ways. It is generally preferred to bring reactant R x into contact (incubated) with analyte so that they are able to wander into the detection zone (Z x ) together. One variant is to pre-incubate/mix the sample with reactant R x prior to its application to the sample application zone. Reactant R j may also be pre-dispensed in the transport zone Z 2 ' or in the sample application zone Z 3 , so that R j is transported together with analyte to the detection zone Z x .
  • Conceivable alternatives include pre-dispensing the reactant R x in the detection zone Z x or in a zone which is separated physically from the hitherto mentioned zones, or is applied directly to the detection zone Zj subsequent to having bound the analyte thereto.
  • the biospecific reactants R 2 which is stably linked to the detection zone is not capable of binding directly to the analyte. It may then be neccessary to preincubate, e.g. the sample or the detection zone Z or the transportation zone Z 2 ', with a bifunctional affinity reagent that is capable of creating a link between the analyte and R 2 .
  • the sample can be transported from different zones to the detection zone by capillary forces when the matrix is initially dry to a substantial extent.
  • a suction body may be included in the vicinity of the transport zone Z 2 ' (transportation from detection zone) .
  • Transportation can also be effected with the aid of an electric field.
  • the sample application zone is located at a higher level than the detection zone, transportation can be effected with the aid of hydrostatic pressure, particularly in the case of porous matrices in the form of membranes .
  • Washing of the detection zone after applying different reagents will often require a surplus liquid absorption capacity in a position downstream of the detection zone. This can be achieved by increasing the volume of the transport zone Z 2 " or by placing a highly absorbent matrix in liquid-flow contact therewith.
  • the sample application zone Z 3 often has the form of a porous matrix which possesses good water retention properties and, at the same time, is well capable of releasing water to the transport zone Z 2 ' during the analysis process .
  • the matrix may be sufficiently hydrophilic to permit the transportation of liquid.
  • the matrix shall have a porosity which will enable the carbon particles to wander from the sample application zone to the detection zone.
  • the pore size shall be greater than the size of the carbon particles.
  • the pore size will preferably lie in the range of 0.4-100 ⁇ m, in order to obtain an acceptable function of hydrophilic matrices.
  • Nylon, nitrocellulose and cellulose were used in the detection zone. Nylon and cellulose have been used for reactants R 2 that are anchored covalently, and nitrocellulose has been used for reactants R 2 that have been anchored adsorptively.
  • the material used in the sample application zone was the same as the material used in the transport zone, optionally in combination with a cellulose filter and/or fiberglass filter as a liquid reservoir.
  • Particle size, porosity and hydrophobicity can be optimized with respect to one another by simple experimentation in ready manner. See the experimental part.
  • the most preferred embodiment geometrically in the case o porous matrices is a test strip in which the sample applicatio zone, transport zone and detection zone are placed laterall after one another, with the possibility of liqui transportation therebetween.
  • th control zone contains a bioaffine reactant which binds to R 1( the control zone will be blackened in response to negativ samples (and also in response to positive samples) , therewit providing a function control .
  • the matrix will preferably be white in colour, even though pale nuances of other colours which provide good contrasts wit black carbon particles are acceptable.
  • R x and R 2 may b antibodies that are directed against physically spaced epitope on the analyte, which is an antigen or a hapten having at leas two epitopes.
  • This technique is used to determine primaril high molecular weight, bio-organic molecules, such as proteins, e.g. Ig of a given class (IgA, IgD, IgE, IgG and IgM) .
  • one of R x and R 2 is an antigen/hapte and the other is an antibody directed against a class-specific determinant (IgA, IgD, IgE, IgG and IgM) .
  • R x is an analyte analog and R 2 is an antibody directed against both the analyte and the analyte analog.
  • This technique is primarily directed towards low-molecular bio-organic molecules and can be used to assay high molecular weight proteins, such as IgE.
  • the inventive method has been developed primarily for assaying serum/plasma levels levels of total-IgE and allergen-specific IgE for the purpose of allergy diagnosis, and corresponding methods in relation to other Ig classes.
  • the ranges of IgE concentration in this type of use was 10 "10 - 10 "7 M total IgE/1 serum and 10 "12 - 10 "9 M allergen-specific IgE/1 serum respectively (i.e. both total IgE and allergen-specific IgE are low-concentration analytes) .
  • antibody as used here includes intact antibodies and antigen-binding antibody fragments.
  • antigen as used here includes the antigen as such, hapten and antigen fragments that exhibit antibody-binding activity.
  • Another aspect of the invention is an immunoreagent which is labelled with particles and chosen from the group comprising IgE, anti-IgE antibody and allergen, including IgE-binding epitopes thereof.
  • This aspect is characterized in that the particles are carbon particles.
  • the particles are defined in the same way as those used in the inventive method.
  • the invention can be used in clinical diagnosis (including therapy monitoring processes) , to which the aforesaid particle ranges are directly applicable and in many cases necessary.
  • Typical samples are: Cerebro Spinal fluid (CSF) , saliva, lachrymal fluid, urine, blood (plasma and serum) , etc.
  • Diagnostic areas of particular interest are assays in which an analyte is assayed in order to follow up a treatment (monitoring) and to diagnose various inflammatory conditions, such as asthma, and allergy-related conditions, and prolonged alcohol over-consumption.
  • relevant analytes are antigen/allergen-specific antibodies of different classes (particularly IgA, IgD, IgE, IgG and IgM) , total levels of respective Ig classes, eosinophilic cationic protein (ECP) , eosinophilic protein X (EPX) , myeloperoxidase (MPO) , human neutrophilic lipocalin (HNL) , lysozyme, tryptase, interleukins (IL-5, IL-6, IL-8), hyaluronic acid (HA), osteocalcin, etc.
  • ECP eosinophilic cationic protein
  • EPX eosinophilic protein X
  • MPO
  • CDT carbohydrate deficient transferrins
  • asialotransferrin and disialotransferrin are important analytes. This does not mean, of course, that the inventive method cannot also be applied in the diagnosis of other illnesses, such as cancer, hormonal disorders, etc.
  • the invention can also be applied in conjunction with quality controls in the production of substances which exhibit biospecific affinity.
  • concentrations are often much higher and completely different requirements are placed on sensitivity and specificity.
  • the demand placed on the carbon particles is also correspondingly lower, meaning that suspendibility will often suffice.
  • This applies, inter alia, to IgE, anti-IgE antibodies, allergen and allergen epitopes ( haptens deriving from allergens) which bind to antibodies (particularly to IgE) and other earlier mentioned analytes and antibodies directed thereagainst.
  • the invention can also be applied in environmental analyses, for instance for determining the presence of allergens in ambient air. Allergens normally derive from pollen, mites, cats, etc., and often have a protein structure.
  • the invention has primarily been developed for measuring low- concentration analytes by which are meant analytes that are measured in a range extending wholly or partly below 10" 10 , i.e. concentrations within 1-I0xl0 ⁇ 10 belong to the low- concentration range.
  • concentrations within 1-I0xl0 ⁇ 10 belong to the low- concentration range.
  • This ranges refer to the concentrations of the analyte as it is present in its natural environment (CSF, plasma, serum, whole blood, urine, lachrymal fluid, saliva etc) .
  • Carbon suspension (mother liquor) : About 500 mg of carbon particles were suspended in 50 ml of a 5 mM borate buffer at pH 8.5 and sonicated for thirty minutes. Prior to the adsorption of protein on the carbon particles, the suspension was diluted to 1 mg/ml and sonicated for a further three minutes. The carbon quality used will be apparent from the following description of respective tests.
  • borate buffer 0.1 M, pH 8.5, containing 1% BSA and 0.05% NaN 3 , with intermediate centrifugation at 16,000 x g.
  • the sediment was diluted with borate buffer (0.1 M, pH 8.5, 1% BSA, 0.05% NaN 3 ) to a carbon content of 500 ⁇ g/ml .
  • the quantities used were adapted so that the anti-IgE antibody concentration was 25-50 ⁇ g/ml in the final solution.
  • the centrifugation times varied with different types of carbons.
  • Test strip 1 A nitrocellulose membrane (Schleicher and Schuell, Germany, 8 ⁇ m) was laid against a stiff pre-gummed polyester sheet. An anti-IgE antibody solution was then sprayed onto the sheet in a line (detection zone) parallel with one side of the sheet, and an anti-Fc mouse IgG antibody solution was sprayed onto the sheet in a line (control zone) parallel with and well-spaced from the first line. The membrane was allowed to dry and was then clipped into strips measuring 0.8 cm x 4 cm (with the antibody lines parallel with the short ends of the strips) .
  • a filter paper (Whatman cellulose 17 CHr, England, measuring 0.8 cm x 0.8 cm (sample application zone)) was placed at the short end of the strip (at the bottom of the strip) on the same side as the detection zone.
  • a suction filter (Whatman cellulose 17 CHr, 2 cm x 2 cm) was placed at the other end of the strip (at the top of the strip) .
  • the control zone was omitted in certain tests. The precise measurements varied slightly from case to case.
  • Test strip 2 was analogous with test strip 1 with the exception that the detection zone was comprised of a strip of cellulose paper (3 mm in width) to which mite allergen was covalently bound (CNBr coupling) , the strip was clipped from a mite disc (dl allergen disc) , Kabi Pharmacia Diagnostics AB, Sweden) . The nitrocellulose membrane had been cut-off in the position of the detection zone, and the mite strip gummed to the test strip with opposite ends overlapping (membrane on top and mite strip beneath in the lower part of the detection zone (the part facing in the flow direction)) and vice versa in the upper part.
  • the detection zone was comprised of a strip of cellulose paper (3 mm in width) to which mite allergen was covalently bound (CNBr coupling)
  • the strip was clipped from a mite disc (dl allergen disc) , Kabi Pharmacia Diagnostics AB, Sweden) .
  • the nitrocellulose membrane had been cut-off in the position of the detection zone
  • Test strip 3 A nylon membrane. Anti-IgE antibodies, birch allergens or casein were bound covalently in the detection zone.
  • Mite-specific IgE 38 ⁇ l of a positive human serum containing
  • Casein-specific IgE 45 ⁇ l of a positive human serum (RAS positive with regard to casein) was diluted with normal huma serum to 20 kU/1 of casein-specific IgE per litre or of a blan sample (human serum ⁇ 0.35 kU IgE/1) and mixed with 7.5 ⁇ l (5 g carbon) of a suspension of carbon particles into which casei had been adsorbed in accordance with the aforegoing, and the applied directly to the sample application zone on test stri 1. Subsequent to absorption of the sample into the zone, a was was initiated in the same manner as that for total IgE. Th positive sample resulted in unequivocal blackening of th detection zone. No blackening was observed in the case of th blank sample.
  • Aggregate labelled anti-IgE antibodies Tests were carried ou with 125 -anti-IgE antibodies labelled in accordance with th Chloramine T-method. The labelled antibody was then adsorbed o carbon particles (sp 100 (Degussa, Germany) in accordance wit the above method. Mother liquors were stored in a refrigerato at +4°C and all of the particles were found to have settle after two calendar days. Suspensions containing adsorbe antibodies were centrifuged at different G numbers, to obtai fractions of different sizes (in the form of pellets an supernatants) .
  • Respective pellets were re-suspended and allowed to settle a room temperature over a period of eleven calendar days Supernatants were also allowed to settle under the sam conditions. The radioactivity of the sediments was determine and taken as a measurement of the portion/percentage o settleable particles in respective fractions. The results ar set forth in Table 1 below.
  • Signal strength as a function of carbon aggregate sizes The procedure applied was in accordance with standard protocol for lateral immunoassay chromatography.
  • the samples used were IgE- standards (0.5-50 kU IgE/1, 6% BSA, 50 mM phosphate buffer, pH 7.5, 0.05% NaN 3 ) . Because the low measuring range is the range of most interest when testing allergen-specific IgE, the signal strength was compared at 0.5 kU IgE/1. The signal strength was converted to relative measurement values (signal strength:mean signal).
  • the fractions were divided into three groups: supernatants (3 in number) , non-centrifuged suspensions (2 in number) and pellets, sediment (3 in number) . The results are set forth in Table 1.
  • the signal strength wa compared at 0.5-1 kU/1 with a plurality of carbon sorts.
  • the measured values were converted to relative values (signal strength:mean signal) .
  • the carbon sorts were divided into three groups with 6-7 carbon sorts in each group, depending on the function of the low IgE values in the assay.
  • the tendency of the carbon particles on which anti-IgE antibodies had been adsorbed to settle (+4°C for a month) from the suspension was taken as a measurement of aggregate size. A suspension from which all carbon particles had settled to provide a complete sediment was given the value of 4+, whereas a suspension which resulted in no sediment was given the value 0+.
  • Table II The results are set forth in Table II below.
  • the test protocol was the same as that used for total IgE.
  • Two analysis series were carried out with the same amount of carbon of two different carbon sorts (sp 4 and sp 100 respectively) .
  • the IgE contents of the samples were 1, 5, 20 and 100 kU/1.
  • Standard curves for respective carbon sorts show that sp 100 gives a higher signal than sp 4 in the case of low IgE concentrations, but that on a molar basis sp 4 carried more reagent, resulting in a higher signal at higher concentrations
  • the tendency of larger particles/aggregates to produce stronge signals was also observed when corresponding comparisons were made on different membranes.
  • Sp 100 produces with:
  • the diameter of aggregate sizes for sp 100 and sp 4 were determined by:
  • Weighted mean values are 200 nm for sp 100 and 85 nm for sp 4.
  • Anti-IgE (Pharmacia Diagnostics, Uppsala, Sweden) had previously been adsorbed in a thin line (1x5 mm) 2 cm from the application end (detection zone) .
  • a sucking cellulose pad (5x15 mm Whatha cellulose 17 Chr) was placed at the top of the nitro-cellulose membrane, downstream the adsorbed anti-IgE.
  • Casein had previously been adsorbed in a thin line (1x5 mm, detection zone) 2 cm from the application end.
  • a sucking cellulose pad (5x15 mm Whatham cellulose 17 Chr) was placed at the top of the nitro-cellulose membrane, downstream the adsorbed casein.

Abstract

An analysis method comprises establishing the presence of an analyte in a sample by forming a complex between the analyte and its bioaffine counterpart and a suspendible bioaffine reactant (R1) which is labelled with carbon particles and incorporated in the complex in an amount related to the amount of analyte in the sample. The method is characterized in that a measurable part of the particles are able to settle. An immunoreagent labelled with particles and chosen from the group IgE, anti-IgE antibody, or allergen including IgE-reactive epitopes thereof characterized in that the particles are carbon particles.

Description

Immunoassay method and reagent involving suspendible carbon labeled bioaffine particles
TECHNICAL FIELD AND KNOWN TECHNIQUES
The analysis is concerned with determining the analyte content of a sample either qualitatively or quantatively with the aid of its bioaffine counterpart, by forming a complex between the counterpart and the analyte. In order to determine the analyte, there is used a bioaffine reactant (Rx) which is labelled with a group that can be shown analytically (= label) and which is incorporated in the complex. The analyte concentration of the sample can then be determined from the amount of complex-bound and/or non-complex-bound labelled reactant (R^ and R1 " respectively) .
The invention uses suspendible carbon particles as a label.
When the bioaffinity relates to antibodies and antigens/hapt- ens, one speaks about immunoassays or immunochemical assaying. When the bioaffinity concerns complementary oligo/ polynucleotides, one speaks about hybridization methods.
The invention is adapted particularly to immunoassays.
Many labels used in analysis processes based on biospecific affinity are known to the art. Particles are important in this context. According to known techniques, these particles will primarily have colloidal dimensions - be in the form of sols (i.e. normally 1-200 run and spherical and monodispersed) . Well- known particulate label groups are metal particles, non-metal particles (e.g. Si02 and carbon, latex and killed erythrocytes and bacteria) . Particular mention can also be made to labels that can be shown indirectly, such as individual members of bioaffine pairs, e.g. biotin or (strept)avidin, hapten or antibodies, class-specific determinants in antibodies, etc. The indirectly detectable labels are often determined or assayed with the aid of their bioaffine counterparts labeled with labels that can be detected directly or indirectly.
Various methodologies are available in this regard depending on when, where and how an analysis is carried out and the material to be analyzed. Examples of typical methods are:
a. Heterogenous and homogenous methods. The terms heterogenous and homogenous describe whether or not labelled reactants (R ) present in the complex are separated from non- complex-bound reactants (R^') prior to assaying labelled reactants.
b. Competitive (inhibitions) and non-competitive methods. Competitive methods utilize analyte analogs which compete with analytes in binding to a deficiency of reactants that have biospecific affinity to both the analyte and the analyte analog. Analyte analogs may be analytes that are labelled with or bound to an insoluble phase (solid phase) in the analysis medium. Examples of non-competitive methods are so-called sandwich methods in which the analyte is complexed between two or more reactants that exhibit biospecific affinity to mutually spaced epitopes on the analyte.
c. Agglutination tests which involve clumping together of colloidal particles that are coated with a reactant which takes part in the aforementioned complex forming process.
d. Immunohistochemical methods.
e. Methods involving precipitation/insolubilizing processes using a reactant which selectively insolubilizes the complex bound or non-complex-bound labelled reactant, either via biospecific affinity (e.g. DASP) , ion-bonding, hydrophobic interactions, covalent bonding, etc.
The aforesaid methods have been carried out in more or less homogenous solutions, on test strips, porous matrices, in test tubes, microtiter wells, on flat surfaces, etc. Known techniques relating to the use of carbon particles as labels and test strips for iπr unoche ical assays with the aid of particle-labelled immunore gents.
A. Waller et al, Laboratory Animal 11 (1977) 93-97, describes immunochemical assaying in which serum samples are treated with India Ink followed by contacting the sample with antigen from Encephalitosoon cuniculi. India Ink is ink/drawing ink based on stably suspended carbon black (sol) (Hackhs Chemical Dictionary, 4th Ed., Ed. Julius Grant, McGraw-Hill Book Company, page 346) .
B. EP 321,008 (HBT Holland Biotechnology) relates to an immunochemical method that uses colloidal, monodispersed non-metallic particles (carbon particles are mentioned) bound to an analyte or to the bioaffine counterpart of the analyte. The patent emphasizes that the particles shall be in the form of sols, meaning that particles which are able to settle to form a sediment are not present in the particle preparations used. The patent makes particular mention to the production of sols by enclosing non-metallic colloidal primary particles in an inert hydrophilic envelope or by coupling reactants directly to the naked particle. The patent mentions that sensitivity increases with increasing particle sizes, provided that the particle preparations used are monodispersed particles in sol form.
C. Amerongen, et al (J. Biotechnol. 30 (1983) 185-189 and Clin. Chim. Acta 229 (1994) 67-75) relates to immunochem¬ ical assaying with the use of carbon particles in sol form as labels. The sol used is produced in accordance with EP 321,008. Neither Amerongen, et al, nor EP 321,008 discloses anything with regard to source, characteristics or manufacture of the carbon particles that are said to be suitable for use. The technique using carbon particles is applied to test strips and quantitative analysis is effected with computer-based image analysis. As in the case of EP 321,008, emphasis is made of the importance of the particle preparations being in sol form.
D. Diverse. U.S. 4,318,707 (Syva) describes homogenous immunochemical assaying with the use of fluorescent- labelled reactants in combination with sound-adsorbing particles (e.g. sol) with bioaffine reactants bound thereto. GB 2,005,019 describes charcoal as an antigen carrier in heterogenous immunochemical assaying processes.
E. During the priority year the Swedish Patent Office has carried out an International Type Search. The report cites GB 2,239,314 that in general terms describes immunoassays employing as the labels carbon particles similar to the ones used in our experimental part, and EP 239,318 and WO 8911102 that discuss various types of particles among which charcoal is included.
OBJECTS OF THE INVENTION
The object of the present invention is to improve and simplify analysis methods of the kind defined in the introduction with the use of carbon particles as label groups.
FIGURE 1 This illustrates an embodiment of the invention (test strip) for determining total IgE with the aid of a sandwich test using solid-phase bound anti-IgE antibodies (R2) bound in a detection zone (Zj) , labelled anti-IgE antibodies (R:) and a control zone (Z4) containing solid-phase bound anti-IgG antibodies (in our case anti-mouse IgG because Rx is a mouse monoclonal) . The sample application zone (Z3) is located in the lower part of the strip and the reagent Rx is mixed with sample prior to its application to the strip at zone Z3. Transport zones (Z2' and Z2" and Z2'") are located between the sample application zone (Z3) and the detection zone Z ) , between the detection zone ( Zx ) and the control zone (Z4) and between the control zone and a sucking body, respectively. That part of the strip which remains above the control zone may be understood as being a further transport zone (Z2'''). The arrow indicates the direction of flow in the strip. The reactants can be replaced as discussed below for different types of analytes. By replacing the solid-phase bound antibody R2 for an antigen/hapten, the test will measure antigen/hapten-specific IgE (see the following examples) .
THE INVENTION
The invention is based on the discovery that carbon particles of non-colloidal dimensions, preferably polydispersed and/or of irregular shape, function as labels and can even have a beneficial effect on the aforesaid analysis methods. Irregular particles have a greater surface/volume ratio per particle than spherical particles and thus give greater response or sensitivity to the analyses in which they are used as labels.
One aspect of the invention includes methods of the kind defined in the introduction. These methods generally include
i. contacting a sample that contains an analyte, possibly a pretreated sample/analyte, with a suspendible bioaffine reactant (R labelled with carbon particles, under conditions which permit the formation of a bioaffine complex in which Rj is present in an amount corresponding to a qualitative or quantitative measurement of the analyte concentration of the sample, whereafter
ii. the amount of particle-labelled reactant bound (Rα') or non-bound (Rx") to the complex is determined qualitatively or quantitatively, wherein
iii . the determined quantity is taken as a measure of the presence or amount, respectively, of the amount of analyte in the sample.
The inventive method is characterized in that a measurable quantity of the carbon particles is so great that the particles
(in the form of particle-labelled bioaffine reactant (Rj) ) settle in an assay buffer at +4°C over a period of seven calendar days. Whether or not a suspension fulfils thi condition can be decided by visual determination after havin allowed the suspension to stand under the aforesaid conditions
According to the results disclosed in the experimental portio of this document, sensitivity increases with the amount o particles that can settle in accordance with the precedin paragraph. This means that the amount of particles that ar able to settle is often > 0.1%, such as > 1%, preferably > 50%, with an upper limit of 100% (all percentages being w/ percentages, alternatively measured in accordance with th method described under the heading "Sensitivity as a functio of the amount of settleable particles" in the experimental par of this document.
In preparing the particles concerned, it is particularl preferred
a. that the carbon particles have a weighted mean particl size of > 0.05 μm, preferably in the range of 0.2-5 μ an more preferably in the range of 0.2-1 μ ; and
b. that > 1%, such as > 50%, with an upper limit of 100%, o the particles will lie in the range of 0.2-5 μ , preferabl in the range of 0.2-1 μm.
The aforesaid sizes are measured with the aid of a Dis Centrifuge Photosedimentometer using instruments from Brook haven Corporation, U.S.A.
When measuring in accordance with "Flow-Field-Flow-Fraction ation" (= FFF) - (Jengthun Li, et al, Size Analysis of a Bloc Copolymer-Coated Polystyrene Latex, ACS Symposium Series No. 472, Particle Size Distribution 2, Chapter 16, pp. 246-26 (1991) American Chemical Society) corresponding preferred size are
a. the top value of the particle distribution gives a diamete which is > 0.1 μ , preferably a diameter in the range o 0.2-5 μm and more preferably in the range of 0.2-1 μm; and
b. > 1%, such as > 10% or > 50%, with an upper limit of 100% of the particles, is > 0.1 μm and preferably lies in the range of 0.2-5 μm, and more preferably in the range of 0.2- 1 μm.
Suitable particle sizes and percentages of settleable particles will vary in accordance with the test method applied, analyte, affinity and specificity of the bioaffine reagent used. The main rule is that, compared to a higher analyte concentration, a lower analyte concentration will demand a greater portion of particles that are > 200 n . Among other things, low- concentration analytes (< 10"10 M) normally require particle preparations in which > 50% of the carbon particles lie in the range 0.2-1 μm (measured in accordance with FFF) (corresponding limits of particle sizes measured in accordance with "Disk Centrifuge Photodensedimentometer" are > 25% of the particles are greater than 0.2-1 μm) . In the case of high-concentration analytes (> 10"10 M) , it is necessary to reduce the signal strength and to increase the quantity of reagent, which means, among other things, that the portion of particles > 0.2 μm is advantageously lowered to a level approaching the lowest percentages (alternatively one lowers the mean particle size (Disk Centrifuge Photosedimentometer) or the top mean value
(FFF) . Analyte concentrations > 10"7 M, these concentrations are normally measured by other means.
The subject matter of the preceding paragraph is related primarily to lateral immunoassay chromatography, although the person skilled in this art will be able to adapt the points discussed to suit other methods that employ biospecific affinity reactions, by reasoning in a corresponding manner. See also the experimental part.
Tests carried out hitherto have been effected with commercially available carbon-particle preparations in the form of primary aggregates of primary carbon nodules (primary particles) stably linked together, most likely covalently. The size of the nodules varies from carbon quality to carbon quality, but is normally in the range of 5-250 nm, with preference for 20-100 nm. The number of primary nodules contained in each primar aggregate also varies, and is 4-200 with regard to the most usable qualities, with preference to 6-75. By the term "stabl linked together" is meant that the aggregates will not disintegrate under the conditions normally applicable to biospecific affinity reactions. The configuration of the primary aggregates may also vary from an elongated, branche configuration to more compact structures.
The primary aggregates may, in turn, be secondarily aggregated to form larger units . When these secondary aggregates are stable against disintegration, they can be used in the inventive analysis method provided that their sizes have no deleterious effect on the method applied.
A number of potentially usable carbon qualities (aggregates consisting of covalently bound primary nodules) which fulfil the aforesaid definitions are commercially available from Degussa (Germany) and other manufacturers. Examples are carbon black, which is the collective name for furnace black, channel black, lamp black and acetylene black. The carbon content of these materials is usually from 85% and more, terminating at a content immediately beneath 100% (99.999%) (w/w) . The manufacturers have lowered the carbon content from 99-100% down to 85-99.9% (w/w) , by oxidative treatment of carbon black, among others. Oxidatively-treated forms of the carbon particles concerned have been found particularly usable in the inventive method, due to improved suspendibility when preparing the carbon-labelled reactant Rx .
The aforesaid carbon particles may be enclosed in polymeric envelopes and/or may carry bioaffine reactants or other groups that are able to take part in hydrophobic interactions, ion- binding, dipole, dipole-binding, etc. One or more particles ma be enclosed in one and the same polymeric envelope or casing.
Bioaffine reactants Rx may be bound adsorptively directly t the naked aggregates or via an envelope in accordance with the previous paragraph. In this latter case, the possibility of covalent bonding is obvious and covalent bonding directly to the naked aggregates is also potentially feasible. Bioaffine reactants are best adsorbed on the carbon particles that are in suspended form.
According to preferred embodiments, the labelled bioaffine reactant is exogenous to the sample, and normally also exogenous to the individual/organism/source from which the sample derives.
Examples of sample pretreatments are a) sample dilution, b) sample concentration, c) analyte enrichment (e.g. removing disturbing substances) , d) pH-adjustment or adjustment by the use of other means, e) forming complexes between the analyte and a bioaffine counterpart, f) analyte modifications other than complex formation according to e) , and so on. Points e) and f) above imply that the analyte in steps i-iii refers to an analyte that is a modified version of the analyte in the original sample. All pretreatment processes are carried out so that the amount of analyte in the original sample and the amount of modified analyte in the pretreated sample will be unequivocally related to one another.
Analysis conditions, such as temperature, concentration, pH, sequence of additions of reactants and selection of reactants to be added are analogous with the conditions previously applied in respect of other labels used in assays which employ biospecific affinity reactions (immunochemical assaying, hybridizing methods, etc.). The assay medium is normally water, optionally mixed with water-miscible solvents. In the case of immunochemical reactions, the temperature is in the range of 0- 40°C and the pH in the range of 4-10. In the case of reactions that involve hybridization between complementary oligo/poly- nucleotides, the temperature will preferably lie in the range of 0-100°C. EMBODIMENTS PREFERRED IN PRACTICE
Heterogenous methodology
The most practical embodiments of the invention employ heterogenous methodology, i.e. a technique in which labelled reactant Rl ' included in the complex is separated physically from labelled reactant R1 " which is not included in the complex, prior to assaying one or both of said reactants. In the majority of cases, said reactants are separated by using a phase (matrix) which is insoluble in the assay medium and which has a bioaffine reactant bound thereto, to achieve selective partition of the complex-bound labelled reactant to the matrix before separation takes place.
The insoluble phase (the matrix) used in heterogenous variants of the invention may have the form of a strip, plate, porous continuous matrix (monolith) , hydrophilic particles, preferably porous particles, membranes, diaphragms, etc.
The prerequisites for separating, assaying and correlating analytes as a function of labelled reactants are the same as those applicable in known techniques, with the exception of being adapted to the fact that according to the invention, the label group consists of particles.
Porous matrices - test strips and other iinmunochromatographic techniques
The heterogenous method according to the invention considered most practical at present utilizes porous matrices, either in the form of particle-packed beds or in the form of monoliths (self-coherent matrices) .
Monolith-type matrices may be given the form of test strips or membranes which include a detection zone (Zx) for the detection of formed complexes. The test strip or membrane will also normally include one or more zones (e.g. Z2' and Z2") for the transportation of sample, reactant (e.g. R , washing solution, etc., to and/or from respective detection zones, and a sample application zone (Z3) , and optionally further zones Z4 , Z5, etc. The transport zone Z2' lies between the sample application zone and the detection zone.
The zones need not necessarily be comprised of the same material. For instance, it is often practical to choose material with regard to the function of the zone. See below.
The detection zone Zx contains a bioaffine reactant (R2) which is stably bound to the matrix and which is capable of capturing labelled reactant Rx in a quantity which is a function of the analyte content of the sample. When analyte is present in the sample, the detection zone will blacken. Blackening of the detection zone can be shown both quantatively and qualita¬ tively, in several ways, preferably visually although perhaps more preferably, and more reliably, through the medium of computer-based picture or image analysis in accordance with Amerongen, et al (J. Biotechnol. 30 (1983), pp. 185-189, and Clin. Chim. Acta 229 (1994), pp. 67-75).
In the simplest cases,
a. the stably bound reactant R2 and the labelled reactant Rx are both directed against the analyte (sandwich test) ; or
b. the bioaffine reactant R2 stably anchored to the detection zone is directed against epitopes present in both analyte and reactant Rx (Rx is an analyte analog) (competitive test) .
The reference to R2 being stably anchored in the detection zone is meant to imply that R2 will not be eluated by the various assay-buffers that pass through. The reactant R2 is anchored in a conventional manner, i.e. covalently bound or bound via adsorption (normally via hydrophobic forces) .
The simplest heterogenous variant of the invention using a porous matrix in the form of a packed particle bed or in the form of a monolith, has only one detection zone Z1 , this zone also functioning as a sample application zone. Reagent (e.g. Rx) and washing solution are applied directly to the detection zone and leave the matrix immediately after having passed through said zone.
In a simple further development, the detection zone is in contact with one or two transport zones (Z2' and Z2") for transportation to and from the detection zone respectively. Z2" is preferably highly absorbent so as to facilitate liquid transportation. When a transport zone Z2' is present, the sample application zone Z3 will be juxtaposed thereto.
The reactant Rx can be contacted with the detection zone in a number of different ways. It is generally preferred to bring reactant Rx into contact (incubated) with analyte so that they are able to wander into the detection zone (Zx) together. One variant is to pre-incubate/mix the sample with reactant Rx prior to its application to the sample application zone. Reactant Rj may also be pre-dispensed in the transport zone Z2 ' or in the sample application zone Z3, so that Rj is transported together with analyte to the detection zone Zx. Conceivable alternatives include pre-dispensing the reactant Rx in the detection zone Zx or in a zone which is separated physically from the hitherto mentioned zones, or is applied directly to the detection zone Zj subsequent to having bound the analyte thereto.
In some variants of the invention, the biospecific reactants R2, which is stably linked to the detection zone is not capable of binding directly to the analyte. It may then be neccessary to preincubate, e.g. the sample or the detection zone Z or the transportation zone Z2', with a bifunctional affinity reagent that is capable of creating a link between the analyte and R2.
The sample can be transported from different zones to the detection zone by capillary forces when the matrix is initially dry to a substantial extent. Alternatively, a suction body may be included in the vicinity of the transport zone Z2' (transportation from detection zone) . Transportation can also be effected with the aid of an electric field. When the sample application zone is located at a higher level than the detection zone, transportation can be effected with the aid of hydrostatic pressure, particularly in the case of porous matrices in the form of membranes .
Washing of the detection zone after applying different reagents will often require a surplus liquid absorption capacity in a position downstream of the detection zone. This can be achieved by increasing the volume of the transport zone Z2" or by placing a highly absorbent matrix in liquid-flow contact therewith.
The sample application zone Z3 often has the form of a porous matrix which possesses good water retention properties and, at the same time, is well capable of releasing water to the transport zone Z2 ' during the analysis process . The matrix may be sufficiently hydrophilic to permit the transportation of liquid. The matrix shall have a porosity which will enable the carbon particles to wander from the sample application zone to the detection zone. By way of a guide line, it can be said that the pore size shall be greater than the size of the carbon particles. The pore size will preferably lie in the range of 0.4-100 μm, in order to obtain an acceptable function of hydrophilic matrices.
At the priority date of this publication, we were successful in testing porous nylon matrices and porous nitrocellulose matrices in the transport zone. Nylon, nitrocellulose and cellulose (paper) were used in the detection zone. Nylon and cellulose have been used for reactants R2 that are anchored covalently, and nitrocellulose has been used for reactants R2 that have been anchored adsorptively. The material used in the sample application zone was the same as the material used in the transport zone, optionally in combination with a cellulose filter and/or fiberglass filter as a liquid reservoir.
Particle size, porosity and hydrophobicity can be optimized with respect to one another by simple experimentation in ready manner. See the experimental part.
The most preferred embodiment geometrically in the case o porous matrices is a test strip in which the sample applicatio zone, transport zone and detection zone are placed laterall after one another, with the possibility of liqui transportation therebetween. In the case of embodiments i which surplus labelled reactant Rj is transported from th detection zone Zx into a transport zone Z2", it may b advantageous to place downstream of the detection zone control zone ( Zt ) , through which Rx is forced to pass. When th control zone contains a bioaffine reactant which binds to R1( the control zone will be blackened in response to negativ samples (and also in response to positive samples) , therewit providing a function control .
The matrix will preferably be white in colour, even though pale nuances of other colours which provide good contrasts wit black carbon particles are acceptable.
For a more detailed description of the construction of test strips and the choice of material connected therewith, reference is made, inter alia, to WO 8808534 (Unilever), U.S. 5,120,643 (Abbott Labs), U.S. 4,954,452 (Abbott Labs), Amerongen, et al (J. Biotechnol. 30 (1983), pp. 185-189, Clin. Chim. Acta 229 (1994), pp. 67-75), and others, which also deal with the use of label groups in the form of colloidal particles.
Particularly preferred heterogenous techniques
According to heterogenous sandwich techniques, Rx and R2 may b antibodies that are directed against physically spaced epitope on the analyte, which is an antigen or a hapten having at leas two epitopes. This technique is used to determine primaril high molecular weight, bio-organic molecules, such as proteins, e.g. Ig of a given class (IgA, IgD, IgE, IgG and IgM) . I another sandwich variant, one of Rx and R2 is an antigen/hapte and the other is an antibody directed against a class-specific determinant (IgA, IgD, IgE, IgG and IgM) . This latter variant measures antigen-specific antibodies of a given class (analyte) . When R, is an anti-IgE antibody and R2 is the antigen, there is obtained a PAST-type RAST-test (allergy test; PAST = particle Allergy Sorbent Test) . Sandwich techniques can provide a very high degree of sensitivity and are therefore particularly suited for low-concentration analytes.
In the most preferred competitive technique, Rx is an analyte analog and R2 is an antibody directed against both the analyte and the analyte analog. This technique is primarily directed towards low-molecular bio-organic molecules and can be used to assay high molecular weight proteins, such as IgE.
The inventive method has been developed primarily for assaying serum/plasma levels levels of total-IgE and allergen-specific IgE for the purpose of allergy diagnosis, and corresponding methods in relation to other Ig classes. At the priority date of this publication, the ranges of IgE concentration in this type of use was 10"10 - 10"7 M total IgE/1 serum and 10"12 - 10"9 M allergen-specific IgE/1 serum respectively (i.e. both total IgE and allergen-specific IgE are low-concentration analytes) .
The term antibody as used here includes intact antibodies and antigen-binding antibody fragments. The term antigen as used here includes the antigen as such, hapten and antigen fragments that exhibit antibody-binding activity.
OTHER ASPECTS OF THE INVENTION
Another aspect of the invention is an immunoreagent which is labelled with particles and chosen from the group comprising IgE, anti-IgE antibody and allergen, including IgE-binding epitopes thereof. This aspect is characterized in that the particles are carbon particles. In the case of preferred embodiments, the particles are defined in the same way as those used in the inventive method. THE FIELD OF USE OF THE INVENTION
The invention can be used in clinical diagnosis (including therapy monitoring processes) , to which the aforesaid particle ranges are directly applicable and in many cases necessary. Typical samples are: Cerebro Spinal fluid (CSF) , saliva, lachrymal fluid, urine, blood (plasma and serum) , etc.
Diagnostic areas of particular interest are assays in which an analyte is assayed in order to follow up a treatment (monitoring) and to diagnose various inflammatory conditions, such as asthma, and allergy-related conditions, and prolonged alcohol over-consumption. Examples of relevant analytes are antigen/allergen-specific antibodies of different classes (particularly IgA, IgD, IgE, IgG and IgM) , total levels of respective Ig classes, eosinophilic cationic protein (ECP) , eosinophilic protein X (EPX) , myeloperoxidase (MPO) , human neutrophilic lipocalin (HNL) , lysozyme, tryptase, interleukins (IL-5, IL-6, IL-8), hyaluronic acid (HA), osteocalcin, etc. For alcohol over-consumption carbohydrate deficient transferrins (CDT; particularly asialotransferrin and disialotransferrin) are important analytes. This does not mean, of course, that the inventive method cannot also be applied in the diagnosis of other illnesses, such as cancer, hormonal disorders, etc.
The invention can also be applied in conjunction with quality controls in the production of substances which exhibit biospecific affinity. In this latter context the concentrations are often much higher and completely different requirements are placed on sensitivity and specificity. The demand placed on the carbon particles is also correspondingly lower, meaning that suspendibility will often suffice. This applies, inter alia, to IgE, anti-IgE antibodies, allergen and allergen epitopes (= haptens deriving from allergens) which bind to antibodies (particularly to IgE) and other earlier mentioned analytes and antibodies directed thereagainst.
The invention can also be applied in environmental analyses, for instance for determining the presence of allergens in ambient air. Allergens normally derive from pollen, mites, cats, etc., and often have a protein structure.
The invention has primarily been developed for measuring low- concentration analytes by which are meant analytes that are measured in a range extending wholly or partly below 10"10, i.e. concentrations within 1-I0xl0~10 belong to the low- concentration range. This ranges refer to the concentrations of the analyte as it is present in its natural environment (CSF, plasma, serum, whole blood, urine, lachrymal fluid, saliva etc) .
The invention will now be illustrated in more detail with the aid of a number of non-limiting examples. The invention is defined in the following Claims.
EXPERIMENTAL PART
THE PREPARATION OF LABELLED REAGENTS
Carbon suspension (mother liquor) : About 500 mg of carbon particles were suspended in 50 ml of a 5 mM borate buffer at pH 8.5 and sonicated for thirty minutes. Prior to the adsorption of protein on the carbon particles, the suspension was diluted to 1 mg/ml and sonicated for a further three minutes. The carbon quality used will be apparent from the following description of respective tests.
Labelling of anti-IgE antibodies with carbon particles (aggre- gate) : A determined number of micrograms of mother liquor according to the above (X μg carbon; see respective applica¬ tions) and 50 μg of anti-IgE antibodies (in 5 mM borate buffer, pH 8.5) were diluted with 5 mM borate buffer pH of 8.5 to a final volume of 1 ml. The solution was allowed to stand for three hours at room temperature, after which 10 mg of bovine serum albumin (BSA) were added for each milliliter and the mixture was allowed to incubate for a further thirty minutes. The mixture was then washed three times with 0.1 M borate buffer, pH 8.5, containing 1% BSA and 0.05% NaN3, with intermediate centrifugation at 16,000 x g. Upon completion of the last wash, the sediment was diluted with borate buffer (0.1 M, pH 8.5, 1% BSA, 0.05% NaN3) to a carbon content of 500 μ g/ml .
The quantities used were adapted so that the anti-IgE antibody concentration was 25-50 μg/ml in the final solution. The centrifugation times varied with different types of carbons.
Labelling of casein with carbon particles (aggregate) : Mother liquor containing 250 μg carbon (sp 100, Degussa) and 100 μg casein was diluted to a final volume of 1 ml with 5 mM borate buffer, pH 8.5. Labelling of anti-IgE antibodies was analogous in other respects.
MANUFACTURE OF TEST STRIPS
Test strip 1: A nitrocellulose membrane (Schleicher and Schuell, Germany, 8 μm) was laid against a stiff pre-gummed polyester sheet. An anti-IgE antibody solution was then sprayed onto the sheet in a line (detection zone) parallel with one side of the sheet, and an anti-Fc mouse IgG antibody solution was sprayed onto the sheet in a line (control zone) parallel with and well-spaced from the first line. The membrane was allowed to dry and was then clipped into strips measuring 0.8 cm x 4 cm (with the antibody lines parallel with the short ends of the strips) . A filter paper (Whatman cellulose 17 CHr, England, measuring 0.8 cm x 0.8 cm (sample application zone)) was placed at the short end of the strip (at the bottom of the strip) on the same side as the detection zone. A suction filter (Whatman cellulose 17 CHr, 2 cm x 2 cm) was placed at the other end of the strip (at the top of the strip) . The control zone was omitted in certain tests. The precise measurements varied slightly from case to case.
Test strip 2: Test strip 2 was analogous with test strip 1 with the exception that the detection zone was comprised of a strip of cellulose paper (3 mm in width) to which mite allergen was covalently bound (CNBr coupling) , the strip was clipped from a mite disc (dl allergen disc) , Kabi Pharmacia Diagnostics AB, Sweden) . The nitrocellulose membrane had been cut-off in the position of the detection zone, and the mite strip gummed to the test strip with opposite ends overlapping (membrane on top and mite strip beneath in the lower part of the detection zone (the part facing in the flow direction)) and vice versa in the upper part.
Test strip 3: A nylon membrane. Anti-IgE antibodies, birch allergens or casein were bound covalently in the detection zone.
STANDARD PROTOCOL FOR LATERAL IMMUNOASSAY CHROMATOGRAPHY
Total IgE: 30-80 μl of a mixture of three parts standard solution/sample (varying contents of IgE in 6% BSA, 50 mM phosphate buffer, pH 7.5, 0.05% NaN3) and part of a carbon suspension (about 0.1 μg carbon/μl) onto which anti-IgE antibodies had been adsorbed in accordance with the aforegoing (X = 390 μg carbon, sp 100 (Degussa) ) was applied to the sample application zone on test strip 1 and transportation towards the detection zone was initiated. A fibre glass filter wetted in buffer (1% BSA in 0.1 M borate, pH 89.5, 0.05% NaN3) was then placed in the sample application zone. A dark band could be detected in the detection zone for IgE-containing samples within ten minutes. The signal was easily distinguishable from results obtained with samples that did not contain IgE.
Blackening of the strip was measured with a video camera
(Kappa, CF 8/1) mounted on a zoom microscope (Askania MZM-1) and calculated in a picture analysis program.
Mite-specific IgE: 38 μl of a positive human serum containing
125 kU/1 of mite-specific IgE or blank sample (normal human serum < 0.35 kU IgE/1) were mixed with 12 μl of suspended carbon particles (2.3 μg carbon) on whose surfaces anti-IgE had been adsorbed in accordance with the aforegoing (X = 250 μg carbon Pr 150T (Degussa) ) and applied directly to the sample application zone on the test strip 2. A wash was then initiated, by applying 40 μl 0.1 M borate (containing 1% BSA, 0.05% NaN3, pH 8.5) followed by a further wash with 20 μl o the same borate buffer, which now also contained 0.1% Tween 20. The positive sample resulted in clear blacking of th detection zone. No blacking was obtained with the blank sample
Casein-specific IgE: 45 μl of a positive human serum (RAS positive with regard to casein) was diluted with normal huma serum to 20 kU/1 of casein-specific IgE per litre or of a blan sample (human serum < 0.35 kU IgE/1) and mixed with 7.5 μl (5 g carbon) of a suspension of carbon particles into which casei had been adsorbed in accordance with the aforegoing, and the applied directly to the sample application zone on test stri 1. Subsequent to absorption of the sample into the zone, a was was initiated in the same manner as that for total IgE. Th positive sample resulted in unequivocal blackening of th detection zone. No blackening was observed in the case of th blank sample.
SENSITIVITY AS A FUNCTION OF THE AMOUNT OF SETTLEABLE PARTICLE (AGGREGATES)
Aggregate labelled anti-IgE antibodies: Tests were carried ou with 125-anti-IgE antibodies labelled in accordance with th Chloramine T-method. The labelled antibody was then adsorbed o carbon particles (sp 100 (Degussa, Germany) in accordance wit the above method. Mother liquors were stored in a refrigerato at +4°C and all of the particles were found to have settle after two calendar days. Suspensions containing adsorbe antibodies were centrifuged at different G numbers, to obtai fractions of different sizes (in the form of pellets an supernatants) .
Percentage of settleable particles in respective fractions:
Respective pellets were re-suspended and allowed to settle a room temperature over a period of eleven calendar days Supernatants were also allowed to settle under the sam conditions. The radioactivity of the sediments was determine and taken as a measurement of the portion/percentage o settleable particles in respective fractions. The results ar set forth in Table 1 below.
Ability to wander in a membrane (pore size 8 μm) : Re-suspended sediment, supernatant, or non-centrifuged suspension was placed in the sample application zone of test strip 1 and allowed to wander towards the detection zone. A certain degree of blackening remained in the sample application zone, due to the fact that some carbon particles fastened in the zone. The extent of the radioactivity remaining in the sample application zone was taken as a measurement of the particles that were unable to wander. The results are set forth in Table 1.
Signal strength as a function of carbon aggregate sizes: The procedure applied was in accordance with standard protocol for lateral immunoassay chromatography. The samples used were IgE- standards (0.5-50 kU IgE/1, 6% BSA, 50 mM phosphate buffer, pH 7.5, 0.05% NaN3) . Because the low measuring range is the range of most interest when testing allergen-specific IgE, the signal strength was compared at 0.5 kU IgE/1. The signal strength was converted to relative measurement values (signal strength:mean signal). The fractions were divided into three groups: supernatants (3 in number) , non-centrifuged suspensions (2 in number) and pellets, sediment (3 in number) . The results are set forth in Table 1.
Table 1. Signal strength as a function of aggregate size measured in terms of settleability. Carbon quality, sp 100 (Degussa) .
Relative
Fraction % sediment start zone signal
11 cal. days %-carbon strength for remaining 0.5 kU IgE/1
Supernatant 17 3.6 0.59
Non-fractionated 44 7.1 1.20
Pellets 52 14.4 1.20
In summary, it was found that: 1. The fraction (pellets) having the smallest particle size
(supernatants) gave a weak signal with low IgE levels.
2. Non-centrifuged suspensions which settled (> 95%) whe stored in an assay buffer (0.1 M borate buffer, 1% BSA,
0.05% NaN3, pH 8.5) at +4°C to +8°C for two calendar day gave a better test than the fractions which were enriche with regard to particles having lower settling tendencies.
3. Fractions containing large particles (pellets, sediment) were equally as sensitive as non-fractionated suspension of the same carbon sorts, due to the fact that the majo part of the increase in sediment remained in the sampl application zone.
SIGNAL STRENGTH DEPENDENCY ON DIFFERENT CARBON QUALITIES
About twenty different types of carbon black (Degussa) , particularly channel black and furnace black and certai particular black-types were tested with regard to th adsorption of IgG (125I-anti-IgE antibody) and their function i tests (lateral immunoassay chromatography) . We found i impossible to produce suspensions from several of the carbo blacks used. This problem was solved in many cases, b sonicating carbon mixed with antibodies, although certain type of carbon still produced suspensions which were less ideal . Th method for total-IgE in accordance with the aforegoing was use as standard protocol for lateral immunoassay chromatography. The samples used were IgE standards, containing 0.5-125 k IgE/1.
All carbon sorts tested gave a positive signal in the regio over 5 kU IgE/1, although only a small percentage gave a stron signal in the low measuring range. The degree of blackening wa correlated to the IgE level for all carbon sorts. The contro zone was blackened with all the carbon sorts studied.
Because the lower part of the IgE range is of most interes when testing allergen-specific IgE, the signal strength wa compared at 0.5-1 kU/1 with a plurality of carbon sorts. The measured values were converted to relative values (signal strength:mean signal) . The carbon sorts were divided into three groups with 6-7 carbon sorts in each group, depending on the function of the low IgE values in the assay. The tendency of the carbon particles on which anti-IgE antibodies had been adsorbed to settle (+4°C for a month) from the suspension was taken as a measurement of aggregate size. A suspension from which all carbon particles had settled to provide a complete sediment was given the value of 4+, whereas a suspension which resulted in no sediment was given the value 0+. The results are set forth in Table II below.
Grouping Settling tendency Relative assay response (low IgE)
Best 3.4+ 1.7
Mean 2.8+ 1.1
Worst 2.0+ 0.5
In summary/ we found that:
1. All carbon sorts adsorbed anti-IgE antibodies (125I-anti-IgE antibodies) .
2. In the case of lateral immunoassay chromatography, the carbon sorts exhibited clearly different performances - a higher settling tendency resulted in increased test sensitivity.
Comparison tests at sp 100 and sp 4 (Degussa)
The test protocol was the same as that used for total IgE. Two analysis series were carried out with the same amount of carbon of two different carbon sorts (sp 4 and sp 100 respectively) . The IgE contents of the samples were 1, 5, 20 and 100 kU/1. Standard curves for respective carbon sorts show that sp 100 gives a higher signal than sp 4 in the case of low IgE concentrations, but that on a molar basis sp 4 carried more reagent, resulting in a higher signal at higher concentrations The tendency of larger particles/aggregates to produce stronge signals was also observed when corresponding comparisons wer made on different membranes. Sp 100 produces with:
0.5 kU/1 IgE a signal which is 2.6 times higher than th signal produced with sp 4.
1.0 kU/1 IgE a signal which is 2.4 times higher than th signal produced with sp 4.
5.0 kU/1 IgE a signal which is 1.7 times higher than th signal produced with sp 4.
20 kU/1 IgE a signal which is 1.3 times higher than th signal produced with sp 4.
DETERMINING THE SIZE OF CARBON PARTICLES (PRIMARY AGGREGATES)
The diameter of aggregate sizes for sp 100 and sp 4 (Degussa) were determined by:
Flow-Field-Flow-Fractionation (= FFF. : (Jengthun Li, e al, Size Analysis of a Block Copolymer-Coated Polystyren Latex, ACS Symposium Series No. 472, Particle Siz Distribution 2, Chapter 16, pp. 247-262 (1991) America Chemical Society) . The diameter of carbon sp 100 and sp (Degussa) was determined. The peak value of the particl distribution gives a diameter of 280 nm for sp 100 and diameter of 140 nm for sp 4. The results are set forth i Table III below:
Particle size < 100 nm 100-200 nm > 200 nm
sp 100 5% 18% 77% sp 4 18% 48% 34%
Disk Centrifuge Photosedimentometer [= DCP. : The measurin processes were carried out with instruments from Brookhave Corp., U.S.A. The results are set forth in Table IV below: Particle size < 100 nm 100-200 nm > 200 nm sp 100 30 28% 42% sp 4 70 28% 2%
Weighted mean values are 200 nm for sp 100 and 85 nm for sp 4.
Carbon particle sizes were measured indirectly in terms of their ability to settle, and directly by FFF and DCP. FFF and DCP are analysis methods which focus on different aspects of particle geometry. The results obtained (Tables III and IV) illustrate differences that are a consequence of the particles being irregular and non-spherical with complicated geometry.
EXPERIMENTAL RESULTS OBTAINED DURING THE PRIORITY YEAR. During the priority year, the performance of the test strip mode of the invention has been improved. Our recent findings support that, at least with respect to sandwich heterogenous techniques, it is preferred to use as immune reagents antibodies in the form of fragments lacking the Fc-portion. This is at least applicable to labelled reactant Rα. With respect to the order of addition, the sequential mode is preferred, i.e. a mode which is arranged so that the analyte/sample and the labelled reactant Rx is transported through at least a part of the transportation zone (Z2') in this order. Preferentially this means that they are added separately to the strip, for instance at different times to the application zones (example 1 below, sample before R:) or more preferably at different locations in the transportation zone between the application zone and the detection zone (example 2 below, Rj to an early segment of the transportation zone Z2' after addition of sample to the application zone) .
1. Total IgE, sequential mode.
30 μl IgE in buffer (different IgE concentrations in 6% BSA, 50 mM phosphate buffer pH 7.5, 0.05 % Na 3) was applied on one end (the liquid application zone) of a polyester supported nitro¬ cellulose membrane (8 μm, Whatham, UK) with the dimensions 5x30 mm. The membrane carried a glued thin polyester strip about 7 mm downstream from the application zone to prevent spreading of the applied liquid on the membrane surface.
Anti-IgE (Pharmacia Diagnostics, Uppsala, Sweden) had previously been adsorbed in a thin line (1x5 mm) 2 cm from the application end (detection zone) . A sucking cellulose pad (5x15 mm Whatha cellulose 17 Chr) was placed at the top of the nitro-cellulose membrane, downstream the adsorbed anti-IgE.
When the sample had migrated into the membrane, 30 μl of a washing buffer (1% BSA, 0.05% bovine gamma globulin, 0.1 M borate buffer pH 8.5, 0.9% NaCl, 10% sucrose, 0.05% Na β ) was applied on the application zone. After this washing step, 30 μl of carbon-labelled anti-IgE fab'2 (anti-IgE fab'2 labelled in analogy with previous examples from 6 μg sp 100 + 0.6 μg anti- IgE fab'2 in washing buffer) was placed on the application zone. After adsorption of this suspension a final washing step was performed by applying a cellulose pad, containing 0.1 ml of washing buffer (see above), on the liquid application zone. 10 minutes after the sample application, a black band became gradually visible on the reaction zone 2 cm downstream from the liquid application zone. The intensity of the band was related to the amount of IgE in the applied sample. The intensity was measured with a CCD camera mounted on a zoom microscope and calculated with a computer image program.
Table V
IgE kU/1 CCD units
0 364
0.13 600
0.25 771
0.5 1189
2.0 3131
5.0 5444
20 8211
50 8790
200 9314
500 9736
2000 10341 2. Allergen (casein) specific IgE in human plasma, sequential mode.
30 μl patient sample (diluted in a negative plasma, see table below) was applied on one end (the liquid application zone) of a polyester supported nitro-cellulose membrane (8 μm, Whatham, UK) with the dimensions 5x30 mm. The application was done via a filtering membrane (Cytosep 1661, Gelman, USA) mounted on top of the nitro-cellulose membrane. The membrane carried two glued thin polyester strips glued to the nitro-cellulose membrane about 7 and 13 mm, respectively, downstream from the application zone to prevent spreading of the applied liquid on the membrane surface.
Casein had previously been adsorbed in a thin line (1x5 mm, detection zone) 2 cm from the application end. A sucking cellulose pad (5x15 mm Whatham cellulose 17 Chr) was placed at the top of the nitro-cellulose membrane, downstream the adsorbed casein.
When the sample had migrated into the membrane, 30 μl of a washing buffer (1 % BSA, 0.05 % bovine gamma globulin, 0.1 M phosphate buffer pH 7.5, 0.9 % NaCl, 10 % sucrose, 0.05 % NaNβ) was applied on the application zone. After this washing step, 30 μl of carbon-labelled anti-IgE fab'2 (labelling in analogy with previous examples from 6 μg sp 100 + 0.6 μg anti-IgE fab'2 in washing buffer) was placed on the zone between the polyester strips immediately followed by application of 30 μl of washing buffer on the application zone. 15 minutes after sample application, a black band became gradually visible in the detection zone located 2 cm downstream from the liquid application zone. The intensity of the band was related to the amount of casein-specific IgE in applied sample. The intensity was measured with a CCD camera mounted on a zoom microscope and calculated with a computer image program. Table VI
Casein specific IgE CCD units kUA/l
Negative plasma 320
0.55 622
1.1 957
4,5 2064
45 6573
The results presented in tables V and VI illustrate that concentrations at least as low as 10~12 can be measured.
The order of additions secured that the analyte had passed the application segment for carbon-labelled anti-IgE fab'2 (Rx) before addition of carbon-labelled anti-IgE fab'2 (R was added. It further prevented transport of carbon-labelled anti- IgE fab'2 (R:) into the application zone.

Claims

1. An analysis method wherein the presence of an analyte in a sample is established by forming a complex between the analyte and its bioaffine counterpart and a suspendible bioaffine reactant (R which is labelled with carbon particles and incorporated in the complex in an amount related to the amount of analyte in the sample, characterized in that a measurable percentage of the particles are able to settle from the suspension.
2. A method according to Claim 1, characterized in that the particles have the form of stable primary particle aggregates.
3. A method according to any one of Claims 1-2, characterized in that each aggregate contains between 4-200 primary particles.
4. A method according to any one of Claims 2-3, characterized in that the primary particles have a size in the range of 5-250 nm, preferably in the range of 20-100 nm.
5. A method according to any one of Claims 1-4, characterized in that the carbon particles are carbon black.
6. A method according to any one of Claims 1-5, characterized in that the carbon particles are chosen from the group furnace black, channel black, lamp black and acetylene black.
7. A method according to any one of Claims 1-6, characterized in that the carbon particles are treated oxidatively prior to binding the particles to Rx.
8. A method according to any one of Claims 1-7, characterized in that the carbon content of the particles is 85-99.99% (w/w).
9. A method according to any one of Claims 1-8, characterized by using a porous matrix which includes a sample application zone (Z3) , a detection zone (Zx) and a transport zone (Z2') located therebetween for transporting analyte and liquid to the detection zone ( Z- ) , wherein the method includes the steps of
1) applying the analyte to the sample application zone (Z3) and allowing the analyte to wander to the detection zone (Z , said detection zone containing a stably anchored bioaffine reactant R2 capable of binding the analyte; and thereafter
2) establishing the specific presence of analyte bound in the detection zone, with the aid of the reactant R in the form of blackening said zone.
10. A method according to Claim 9, characterized in that the labelled reactant Rx and the analyte are incubated with one another prior to wandering into the detection zone.
11. A method according to any one of Claims 8-10, character¬ ized in that Rx is an antibody directed against the analyte, and R2 is an antigen, or vice versa, and the analyte is an antigen-specific antibody.
12. A method according to Claim 11, characterized in that Rj is a class-specific antibody selected from the group anti-IgA, anti-IgD, anti-IgE, anti-IgG and anti-IgM antibody, particularly anti-IgE antibody.
13. A method according to any one of Claims 8-9, characterized in that Rx and R2 are antibodies directed against physically spaced epitopes on the analyte; and in that the analyte is a multi-epitopic antigen, wherein preferably Rx and R2 are anti- IgE antibodies and the analyte is IgE.
14. A method according to any one of Claims 8-12, character¬ ized in that the porous matrix is continuous and has the form of a test strip on which the zones are arranged laterally.
15. An immunoreagent labelled with particles and chosen from the group IgE, anti-IgE antibody, or allergen including IgE- reactive epitopes thereof, characterized in that the particles are carbon particles .
16. An immunoreagent according to the preceding Claims, characterized in that the particles are defined in the same way as that defined in Claims 1-7.
PCT/SE1996/000042 1995-01-20 1996-01-18 Immunoassay method and reagent involving suspendible carbon labelled bioaffine particles WO1996022532A1 (en)

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SE9500184A SE9500184D0 (en) 1995-01-20 1995-01-20 Assay method utilizing biospecific affinity reactions and labeled reactant as well as reagents to be used in preferred embodiment

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WO1998032019A1 (en) * 1997-01-14 1998-07-23 Akzo Nobel N.V. Device for detecting an analyte and an analytical method
WO1998052044A1 (en) * 1997-05-15 1998-11-19 Clinical Diagnostic Chemicals Limited Immunoassay apparatus for diagnosis
WO1998053321A1 (en) * 1997-05-21 1998-11-26 Merck Patent Gmbh STRIP TEST FOR DIAGNOSING ALLERGIES $i(IN-VITRO)
WO1999060402A1 (en) * 1998-04-30 1999-11-25 Pharmacia & Upjohn Diagnostics Ab Ligand binding assay and kit with a separation zone for disturbing analytes
WO2000036418A1 (en) * 1998-12-11 2000-06-22 Axis-Shield Asa Dipstick for carbohydrate-free transferrin assay
JP2002509253A (en) * 1997-12-30 2002-03-26 ファルマシア・アンド・アップジョン・ディアグノスティクス・アクチエボラーグ Analytical method using particles and test kit for performing this method
US6916666B1 (en) 1997-12-30 2005-07-12 Pharmacia Diagnostics Ag Method using a new calibrator and a device and test kit including the calibrator
WO2007067680A2 (en) * 2005-12-05 2007-06-14 Guava Technologies Particle-based analyte characterization
US20110076698A1 (en) * 2008-06-10 2011-03-31 Intec Products, Inc. (Xiamen) method of quickly determining human abo/rh/mn blood type and a test kit thereof

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WO1998032019A1 (en) * 1997-01-14 1998-07-23 Akzo Nobel N.V. Device for detecting an analyte and an analytical method
WO1998052044A1 (en) * 1997-05-15 1998-11-19 Clinical Diagnostic Chemicals Limited Immunoassay apparatus for diagnosis
WO1998053321A1 (en) * 1997-05-21 1998-11-26 Merck Patent Gmbh STRIP TEST FOR DIAGNOSING ALLERGIES $i(IN-VITRO)
US6916666B1 (en) 1997-12-30 2005-07-12 Pharmacia Diagnostics Ag Method using a new calibrator and a device and test kit including the calibrator
US7405084B1 (en) 1997-12-30 2008-07-29 Phadia Ab Analytical method using particles and test kit for performing the method
JP2002509253A (en) * 1997-12-30 2002-03-26 ファルマシア・アンド・アップジョン・ディアグノスティクス・アクチエボラーグ Analytical method using particles and test kit for performing this method
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WO2000036418A1 (en) * 1998-12-11 2000-06-22 Axis-Shield Asa Dipstick for carbohydrate-free transferrin assay
WO2007067680A2 (en) * 2005-12-05 2007-06-14 Guava Technologies Particle-based analyte characterization
WO2007067680A3 (en) * 2005-12-05 2007-08-23 Guava Technologies Particle-based analyte characterization
US20110076698A1 (en) * 2008-06-10 2011-03-31 Intec Products, Inc. (Xiamen) method of quickly determining human abo/rh/mn blood type and a test kit thereof

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EP0804733A1 (en) 1997-11-05
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CA2210794A1 (en) 1996-07-25

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