METHOD OF TREATING A PATIENT SUFFERING FROM A SOLID TUMOUR
FIELD OF THE INVENTION
The present invention relates to the field of chemotherapy of neoplastic disorders and especially to medical treatment of solid tumours, malignant as well as non-malignant. In particular, the present invention relates to a method for delivering a chemotherapeutic agent via the vascular system to a solid tumour, while reducing delivery to non-tumour tissue.
BACKGROUND OF THE INVENTION
Over the last decades, the field of cancer chemotherapy has evolved so as to allow effective treatment of a large number of patients. However, a number of solid neoplasms are still associated with a high mortality rate in the patients suffering from such tumours.
One major problem in treatment with chemotherapeutic drugs is the fact that systemic administration of the chemotherapeutic drug results in severe adverse effects that are life- threatening to the patient. It is therefore often impossible to effectively eradicate the tumour cells, simply because the concentration over time of the chemotherapeutic drug is insufficient to effectively kill all tumour cells.
Another major problem is that certain tumours are inoperable - this is especially true for solid tumours of the central nervous system (CNS) where surgical intervention may be impossible - this is even true for solid tumours that are not malignant per se (since they do not invade neighbouring tissue or metastasize), but that are life-threatening simply due to their physical expansion in a very vulnerable environment.
Several ways of improving chemotherapy of such solid tumours are known in the art.
One method has been to exploit the so-called "magic bullet" principle, where the chemotherapeutic drug is coupled to a ligand for a receptor molecule overrepresented in the tumour tissue. The major problem of this technology is, that a large number of tumours do not express any suitable overrepresented receptor molecule.
In cases where it is possible to identify one single or very few solid tumours, it is known to administer the chemotherapeutic drug directly to the tumour, e.g. by direct injection of the chemotherapeutic agent into the tumour.
A variation of this technology consists in administering sustained release compositions and/or microspheres containing chemotherapeutic agents into the tumour, so as to ensure a prolonged exposure of the chemotherapeutic agent to the tumour cells. Such technology is disclosed in WO 01/10416, WO 02/051388, and EP 1 053 746 Bl.
A third approach has been to simply compromise the blood supply to the tumour by administering embolic agents to the vessels that supply the tumour with blood. Such technology is discloses in WO 01/66016, WO 01/68720, and WO 87/00062.
A refinement of this technology, known as "active embolisation" comprises use of embolising agents that at the same time function as carriers of anti-tumour drugs. Such technology is the focus of WO 01/72281.
A large number of patents and patent applications disclose microparticles that are useful as carriers of chemotherapeutic drugs. Such disclosures include US 6,447,796 and WO 01/72281.
However, there is still a need for improved delivery of chemotherapeutic drugs so as to render chemotherapy more effective.
OBJECT OF THE INVENTION
It is an object of the invention to provide for improved methods for treatment of solid tumours. It is a further object to provide for improved pharmaceutical compositions useful in therapy of patients suffering from solid tumours.
SUMMARY OF THE INVENTION
The vascular system
The present inventor has realised that it is possible to refine the known method of active embolisation by utilising micropartide carriers having a diametrical size that allows deposition in the pre-capillary environment whereby the distance of diffusion of a chemotherapeutic
drug becomes minimal. The effect obtained by using microparticles in this manner is that the microparticles are concentrated in the capillary compartment without being able to enter the afferent vessels that drain the tumour in question. On the other hand, it becomes possible to co-administer, or administer at a later stage, a different drug that e.g. protects surrounding non-tumour tissue from the damage exerted by the chemotherapeutic drug released from the microparticles.
Hence, in its broadest and most general scope, the present invention relates to a method of treating a patient suffering from a solid tumour, the method comprising administering, into at least one vessel that supplies the solid tumour with blood, microparticles loaded with a chemotherapeutical agent, said microparticles having a diametrical size that results in retention thereof in the tumour's arterioles, whereby the microparticles are allowed to release the chemotherapeutical agent to the surrounding tumour tissue while minimally compromising surrounding non-tumour tissue.
Another part of the invention relates to a pharmaceutical composition comprising 1) microparticles containing a chemotherapeutical agent and 2) particles of a larger mean diametrical size than the microparticles, said particles comprising a therapeutic agent different from a chemotherapeutical agent.
DETAILED DISCLOSURE OF THE INVENTION
In the following a number of terms will be defined in the context of the present invention and the present specification and claims.
A "solid tumour" is in the present context meant to denote a malignant or non-malignant tumour having a defined localisation and a defined blood supply. Malignant tumours belonging to the class of solid tumours include, but are not limited to, carcinomas, adenocarcinomas, sarcomas (including liposarcomas, fibrosarcomas, chondrosarcomas, osteosarcomas, leiomyosarcomas, rhabdomyosarcomas), gliomas, neuroblastomas, medullablastomas, malignant melanoma, neurofibrosarcoma, and choriocarcinoma. Non- malignant tumours of interest in the present invention are especially of neuro-ectodermal origin and comprise, but are not limited to, ganglioneuromas, meningioma, schwannomas, and neurofibromas.
"Microparticles" are intended to mean particles that have a mean diametrical size in the range from 1 to 1000 μm. It will be understood by the skilled reader, that the microparticles used according to the present invention are sufficiently large to prevent them from entering
the capillary space, since that would entail their subsequent entering the venous system and hence a dissemination of the chemotherapeutic drug. Microparticles can in principle have many forms, but are normally grouped into microspheres and microcapsules, where the latter are substantially hollow, sphere-shaped particles that can carry a substance in the hollow space, whereas "microspheres" are denote solid spherical microparticles, optionally having open cavities.
When stating that microparticles or particles are "loaded" with a substance (such as a chemotherapeutical agent or any other drug) it is intended that the substance is contained in or otherwise bound to the micropartide, and that the microparticles can release the drug to the surrounding environment.
A "chemotherapeutical agent" is broadly intended to mean any chemical substance that is useful in chemotherapy of solid tumours. As such, the term embraces antimetabolites, immune modulators, cytotoxic agents, antibiotic derivatives, nitrogen mustard derivatives, antiangiogenic agents, receptor antagonists, receptor ligands, stimulators, and any combinations thereof.
An "arteriole" is an arterial vessel having a diameter of less than 100 μm, having a wall including from 1 to 3 layers of circularly arranged smooth muscle cells. Arterioles i.a. serve the function of regulating the blood flow to the capillaries in a tissue by changing the diameter of their lumen.
When referring to the "diametrical size" of the microparticles is meant their diametrical size in situ, i.e. after administration and deposition in the arterioles.
The present invention presents a number of improvements to the known technology of active embolisation as this is e.g. described in WO 01/72281 and much earlier in e.g. US 4,536,387. By selecting microparticles having a very well-defined size which ensures deposition of the microparticles in the arterioles, the localisation of the released chemotherapeutic drug becomes optimized from a therapeutic point of view. Very high concentrations of chemotherapeutic agent can be accomplished in the tumour tissue while preserving the function of arteries supplying surrounding tissue, thus rendering possible the co- administration or subsequent administration of drugs that rescues non-tumour tissue from the effects of the chemotherapeutic agent.
The solid tumours that are targets for the present technology are typically malignant or non- malignant tumours of the CNS (especially the brain), prostate, breast, colon, lung, kidney, bladder, liver, bone, head, neck, stomach, larynx, esophagus, cervix, rectum, uterus, skin,
endometrium, pancreas or testis. It is preferred that the tumours are primary tumours with only one single feeding artery or a few feeding arteries. It is especially preferred to utilise the present invention for treatment of tumours in the brain.
The present, invention utilises methods well-established in the art for administering the microparticles to the tumour. The art has described various suitable catheter devices for localised interarterial administration of pharmaceutical compositions - typically such an administration is performed using a catheter that can be positioned correctly by the assistance of real time X-ray visualiszation (or alternatively by using ultrasound or NMR imaging in real time), meaning that the catheter or alternative injection device must be one that can be visualised by one of these methods.
According to the present invention, it is preferred that the microparticles are in the form of microspheres (beads) or (most preferred) microcapsules. Depending on the particular solid tumour to be treated, it is of interest to effect an acute release of drug into the tumour tissue or to effect a sustained release. Further, these two modes of administration may conveniently be combined.
In order to effect a sustained release, any of the methods known to the person skilled in the art for preparing a sustained release of a drug may be utilised. The microparticles may be coated with concentric layers of materials that are degraded over time so as to result in a gradual release of the chemotherapeutic agent loaded therein, the microparticles may themselves be degraded over time to release the drug bound thereto, or the microparticles may carry a composition of matter that slowly releases the chemotherapeutic drug over time. Suitable examples of sustained release microspheres are disclosed in US 4,536,387, WO 92/05866 (which also discloses a method for preparing microparticles of a well-defined size), WO 01/35932 and in many others.
To effect a rapid release it is e.g. possible to utilise loaded microcapsules, where the chemotherapeutic agent is present in the lumen of the microparticles. One possibility is then that the wall of the microcapsule includes "weak spots" that are degraded after the microcapsules have been delivered so as to allow rapid release of the chemotherapeutic agent - the degradation may be spontaneous, or, preferably, it may be the result of a subsequent injection of a substance that induces the degradation of the microcapsule wall (i.e. by injection of an enzyme that specifically digests the material in the "weak spots"). Alternatively, the microcapsule can be made of e.g. amorphous silica that after deposition is subjected to a ultrasonic or electromagnetic shock wave that breaks the microcapsule wall. The skilled person will know how to apply such a shock wave and the precise amplitude and frequency to use.
Alternatively, the chemotherapeutic agent can be delivered in the microparticles in a substantially inert pro-form that requires activation before the antitumour effect is brought about. Any one of a multitude of methods can be used: The chemotherapeutic agent may be bound to the particles by a chemical bond that requires the action of an enzyme or other catalyst that has to be administered; the chemotherapeutic agent may be one that has to be activated by means of radiation, enzymatic cleavage or other enzymatic action. The intention is therefore the same as when using microcapsules that are rendered leaky via external control, namely to ensure that the therapy is instigated after correct administration.
Further, whether or not rapid and/or sustained release is desired, it is of interest to be able to control the commencement of the release or of the therapeutic effect. For instance, after introduction of the microparticles containing the chemotherapeutic drug, it is of interest to verify that the microparticles have in fact been localised in all the desired compartments in the tumour. This particular embodiment can be rendered possible by encapsulating the chemotherapeutic agent in microcapules that can be visualised by means of X-rays, ultrasound or NMR imaging (e.g. by incorporating a radioopague substance in the microcapsule wall or together with the chemotherapeutic agent). After administration, the localisation is checked, i.a. in order to verify that the microcapsules are not disseminated into other tissue or for some reason have entered the venous system. When confirmation has been obtained, the release can be effected, cf. above.
It is of course also possible to combine the use of rapid and sustained release, either by co- administering microparticles destined for rapid release of drug with microparticles destine for sustained release, but also by combining these two modes of action into one single micropartide species. Further, the chemotherapeutic agent released rapidly may be the same or different from the drug undergoing sustained release.
At any rate, if a sustained release is desired, it is of interest to effect such a sustained release for a prolonged period of time, e.g. for at least 5 days, at least 10 days, at least 15 days, at least 20 days, and even at least 25 days such as up to 30 days.
The microparticles may be biodegradable or non-biodegradable. Suitable materials for microparticles are disclosed in WO 01/72281, US 6,447,796, WO 00/57852 and the references cited therein.
Suitable biodegradable materials are selected from the group consisting of a biodegradable polymers such as a polysaccharides, polyamino acids, biodegradable polyurethanes, poly(phosphorester) biodegradable polymers, polymers and copolymers of glycolic acid and
lactic acid, poly(dioxanone), poly(trimethylene carbonate)copolymers, and poly(α-caprolactone) homopolymers and copolymers.
Preferred non-biodegradable materials are selected from the group consisting of amorphous silica, carbon, a metal, a ceramic material, and a non-biodegradable polymer.
One particular interesting embodiment of the present invention utilises amorphous silica as the material of which the microparticles are made. WO 00/09652 discloses a convenient method for preparing amorphous silica microcapsules of well-defined size that are completely inert before they are rendered leaky by e.g. Shockwave exposure. Even though WO 00/09652 describes mainly cosmetic applications of the technology, it can without any problems be utilised for preparing drug-containing microparticles of the desired size.
Needless to say that it is preferred that the materials, biodegradable or not, are preferably biocompatible, meaning that the particles in their own right are not responsible for any adverse effects due to immunological or toxic reactions.
The diametrical size of the microparticles in situ (i.e. after administration) are preferably in the range between 10 and 100 μm, such as between 11 and 90 μm, preferably between 12 and 80 μm, and most preferred between 15 and 40 μm. This latter size range ensures that the microparticles are confined exclusively to the arterioles upon administration.
The chemotherapeutic agent used in the invention can be any substance that is useful in effecting killing of tumour cells by local administration as taught herein, but is preferably selected from carboplatin, mitomycin C, 5-fluorouracil, pirarubicin, cisplatin, carmustine, paclitaxel, doxorubicin, adiramycin, lomustine, teniposide, etoposide, 06-benzylguanine, vincristine, vinblastine, vinorelbine, gemcitabine, cyclophosphamide, temasolamide, 4-HC, methotrexate, and any combination thereof. Most preferred are carboplatin, mitomycin C, 5- fluorouracil, and pirarubicin.
It should be noted that an alternative embodiment of the present invention where inert microcapsules such as those of amorphous silica are used will be to load the microcapsules with a radiotherapeutic agent that has a short half-life. This would mean that a local radiation is not spread to the rest of the body when scavenger cells at some stage are clearing the microcapsules from the site of introduction. One particular advantageous version of this embodiment is the use of a radiotherapeutic agent that emits alpha radiation, because the amorphous silica will effectivel prevent harmful radiation from entering the surrounding tissue before the capsules are rendered leaky.
As indicated above, the present invention also contemplates that the chemotherapeutical action in the solid tumour tissue be combined with co-administration of other drugs that primarily serve as protection of surrounding tissue. Even though it is believed that the presently claimed invention will result in a highly focussed localised action of the chemotherapeutical agent, it is expected that some adverse effects are observed in the neighboring tissue.
For instance, when tumour tissue degrades, it is inevitable that an inflammatory process is instigated, and it is not uncommon that the inflammatory process in its own right is capable of inducing destruction in surrounding tissue, a so-called "innocent bystander" effect. However, since the present invention does not compromise the arterial bloodflow as such but only affects the arterioles of the solid tumour, it is possible to administer, either at the same time (co-administration) or at a later stage (e.g. merely as a second stage of the administration of the invention), therapeutic agents that will help to protect the surrounding tissue from these effects.
Therefore, an embodiment of the invention comprises co-administration or later administration to the patient of at least one therapeutic agent. It is preferred that this therapeutic agent is comprised in particles (e.g. as microparticles) in order to ensure correct deposition of the therapeutic agent, but in the event that the microparticles used in the method of the invention have been effective in occluding the arterioles, a systemic administration of an anti-inflammatory drug would be sufficient.
In preferred embodiments, this therapeutic drug is comprised in particles having a different mean diametrical size than the particles that comprise the at least one therapeutic agent; normally the microparticles (with the chemotherapeutic agent) have a smaller mean diametrical size than the particles comprising the at least one therapeutic agent, meaning that administration of both the microparticles and the larger particles will result in a different distribution of the drug effects, the therapeutic agent being deposited upstream of the chemotherapeutic agent. In preferred embodiments, these larger particles are of such a size and structure, that they do not compromise the blood flow, meaning that tissue supplied down-stream is still supplied with blood.
The larger particles are thus preferably retained in the supplying blood vessels relative to their mean diametrical size, thereby giving rise to delivery of the therapeutic agent to the peritumoural tissue from vessels of a defined size. And, since the microparticles containing the chemotherapeutic agent may be capable of stopping the blood-flow to the tumour tissue, no limitation is imposed on the antitumour effect of the chemotherapeutic agent.
The at least one therapeutic agent is preferably an anti-inflammatory drug (e.g. an NSAID or a corticosteroid or analogue thereof) and a drug inhibiting cell death.
Simultaneous administration of the two set of particles may be problematic, because the particles carrying the larger may block delivery to the tumour of the microparticles. Therefore, it may be advantageous to deliver the larger particles at a later stage, but alternatively, a catheter containing both set of particles may have the microparticles in the distal end so that these are administered first, followed directly by administration of the larger particles.
Another part of the invention pertains to a pharmaceutical composition that includes 1) microparticles containing a chemotherapeutical agent and 2) particles of a larger mean diametrical size than the microparticles, said particles comprising a therapeutic agent different from a chemotherapeutical agent. The microparticles and the chemotherapeutic agent are preferably as discussed above and the same is true for the therapeutic agent and the larger particles.
The invention also pertains to a catheter for injection of a micropartide preparation, said catheter comprising, in the distal (delivering) end microparticles having a smaller mean diametrical size than particles that are present in the proximal (opposite end) of the catheter. Thus, the catheter comprises 1) microparticles and 2) particles of a larger mean diametrical size than the microparticles, wherein the microparticles are predominantly situated in the distal end of the cathether and wherein the particles are predominantly situated in the proximal end of the catheter, whereby administration of the microparticles and particles from the catheter results in administration of the microparticles prior to administration of the particles. The microparticles and the particles as well as their respective contents and functionality are as disclosed above.