The invention relates to systems and methods for delivering a therapeutic agent to a selected site in a subject. These systems and methods allow for precise placement of selected amounts, e.g., very small amounts, of a therapeutic agent at a predetermined site in a subject with minimal trauma to the subject. In addition, if the therapeutic agent to be delivered to the subject includes cells or tissue, the systems and methods of the invention provide for increased survival of the cells or tissue in the subject. The systems and methods of the invention can also be used to remove, with great precision and minimal trauma to a subject, selected substances, cells, and/or tissues from a selected site in a subject. One area in which use of the systems and methods of the invention is particularly relevant is in cell and/or tissue, e.g., neural cell and/or neural tissue, transplantation.
Neural transplantation holds promise as a method of reconstituting cell populations, supplementing levels of certain brain chemicals, and reestablishing neural circuitry. Presently, one main technique or a variation thereof is used for transplanting neural tissue. See e.g., Kordower, J. H. et al. (1995) N. Engl. J. Med. 332(17):1118-1124; Freeman, T. et al. (1995) Annals Neural. 38(3):379-388; Widner, H. et al. (1992) N. Engl. J. Med. 327(22):1556-1563. This technique employs a cell or tissue delivery device which includes a stereotaxic needle with a blunt end and a tip diameter from about 0.9 to about 1.5 mm. The cells or tissue to be transplanted are loaded into this needle, the needle is advanced toward the transplant site, and the cells or tissue are released from the needle at the site. Using this needle, multiple grafts can be placed along a straight path. However, if one wishes to graft at a site which is not along this path, the needle must be removed and reinserted along a new path. Reinsertion of this needle causes additional trauma to the tissue in the path of the needle. Typically, it is desirable to make multiple grafts along different paths. In such a case, the needle is generally removed and reinserted into the subject from about six to about eight times per side of the brain, increasing trauma to the brain tissues with each new penetration.
In addition to the simple injection needles described above, other instruments have been described for transplantation of tissue into the brain. See U.S. Pat. Nos. 5,006,122 and 5,004,457. U.S. Pat. No. 5,006,122 discloses a brain tissue transplantation method utilizing a cannula within a cannula assembly. The first cannula is a large bore cannula which is fixed to a stereotaxic holding apparatus and which is advanced into the brain to the transplant site. The second cannula, which carries donor tissue and a stylet which is used to expel the tissue from the second cannula, is guided within the lumen of the first cannula to the transplant site. The tissue is then transplanted into the brain by withdrawing the first and second cannulas while the stylet within the second cannula is maintained in a fixed position. The stylet is later removed, leaving only the transplanted tissue in the recipient.
These instruments have in common a number of disadvantages. For example, the diameters of the instruments are relatively large, e.g., 0.9 mm or greater. The use of large diameter transplant instruments to deliver therapeutic agents decreases precision in placement of the injection while increasing trauma and disruption of the graft microenvironment. For example, it has been shown that insertion of a cannula into the brain during standard neural transplant procedures causes localized trauma to the tissue, destruction of neurons, and damage to the blood brain barrier (Perry, V. H. et al. (1993) TINS 16(7): 268-273). This damage in turn results in several undesirable events such as macrophage, T-cell, and blood-derived IgG infiltration to the transplant site. Furthermore, reactive gliosis mounts and production of neurite inhibitory factors (e.g., chondroitin-6-sulfate and cytotactin/tenascin) is upregulated resulting in the formation of a glial scar that hinders neurite outgrowth (McKeon, R. J. et al. (1991) J. Neurosci. 11:3398-3411). These processes, which occur on the cellular and molecular level within the graft's microenvironment, ultimately result in cell death and poor graft integration.
In addition, these instruments do not provide for reliable delivery of very small volumes to a selected site in a subject. Small volumes of fluid injected from these instruments tends to adhere to the relatively large surface area of the cannula and can flow up around the outside wall of the guide cannula. Furthermore, as the large caliber instrument is withdrawn, a greater suction is produced. The suction created by removal of these instruments pulls extruded cell suspension into the tract of the cannula, thereby removing cells from the transplant site and resulting in decreased precision in placement of transplants. Furthermore, when these instruments are used for transplantation, transplants can be placed only along a single tract, each tract requiring removal and repenetration of the instrument into the brain. Therefore, the brain must be entered many times in order to place transplants in a three dimensional configuration. These multiple penetrations or insertions cause further trauma to the brain of the transplant recipient. Thus, the disadvantages inherent in the structure of these instruments contribute to low (5-10% of transplanted cells) and variable graft survival and graft-induced functional recovery of the graft in the recipient. These suboptimal techniques remain the state of the art in neural transplantation.
Thus, there is a need for an instrument which can be used to precisely deliver any volume of a therapeutic agent, e.g., a factor, a compound, a chemical, cells, etc. to a selected site in a subject, e.g., a human, in a manner which incurs an absolute minimum level of tissue damage and which is capable of disseminating numerous grafts in a three dimensional configuration. Such an instrument would improve graft survival and functional integration of the graft in the subject leading to further improvement in the quality of life for the subject.
The invention features systems (hereinafter “delivery systems” “delivery instruments” or “delivery apparatuses or devices”) and methods for delivering a therapeutic agent to a selected site, e.g., a desired location, in a subject. These systems and methods meet the above-cited needs by allowing for precise placement of selected amounts, e.g., very small (e.g., less than about 250, 200, 150, 100, 90, 80, 70, 60, 50, 40, 30, or 20 microliters) or large amounts, of a therapeutic agent to a predetermined site in a subject with minimal trauma to the subject. Use of the systems and methods of the invention to deliver a therapeutic agent to a subject results in a level of tissue damage which is substantially less than that caused by known delivery devices. Moreover, the systems and methods of the invention can be used to disseminate numerous grafts in a three dimensional configuration within a subject with only a minimal number of penetrations into the subject. In addition, if the therapeutic agent to be delivered to the subject includes cells or tissue, the systems and methods of the invention provide for increased survival of the cells or tissue in the subject. The systems and methods of the invention can also be used to remove, with great precision and minimal trauma to a subject, selected substances, cells, and/or tissues from a selected site in the subject.
Accordingly, the invention features a system for delivering a therapeutic agent to a selected site in a subject which includes a guide cannula for penetrating a selected site in a subject to a predetermined depth and a delivery cannula for delivering the therapeutic agent to the subject. The guide cannula has an axial bore extending therethrough which has an open proximal end and an opening at a distal portion thereof. The delivery cannula has an axial bore extending therethrough, a flexible distal end portion, and an outer diameter which is less than the inner diameter of the guide cannula. The shape of the delivery cannula enables the delivery cannula to be inserted within the bore of the guide cannula and also allows for movement of the delivery cannula along the bore of the guide cannula. The delivery cannula can be manufactured of an inert, e.g., nontoxic and nonreactive with host tissue and components thereof, material which can be formed into various shapes and sizes with selected specifications and which is flexible. As used herein, the term “flexible” refers to at least a portion, e.g., a distal portion, of the delivery cannula of the invention which is capable of being deformed or bent without breaking. The flexible portion of the delivery cannula is capable of returning to its original position or form upon removal of a force which causes it to deform or bend. Typically, at least a portion of the delivery cannula can be deflected at an angle from the guide cannula to deliver the therapeutic agent to a selected site in a subject. The flexibility of the delivery cannula allows for placement of a therapeutic agent in a three dimensional array in a subject with minimal trauma to the subject. Preferably, the material from which the delivery cannula is produced is flexible or pliable when formed into cannulas having very small diameters at their distal ends, e.g., from about 1 to about 200 micrometers, preferably from about 10 to about 190 micrometers, more preferably from about 20 to about 180 micrometers, yet more preferably from about 30 to about 170 micrometers, still more preferably from about 40 to about 160 micrometers, and most preferably from about 50 to about 100 to about 150 micrometers. The material can be manufactured from a variety of materials such as glass, polymeric materials e.g., polycarbonate, polypropylene, or other polymeric material described herein, and metals, e.g., stainless steel. In an embodiment, the delivery cannula is manufactured of a glass e.g., borosilicate, soda-lime glass. In another embodiment, the delivery cannula is manufactured of silicon dioxide either in the form of fused quartz or fused silica. In an alternative embodiment, the delivery cannula can be manufactured from more than one, e.g., a combination of the materials described herein. For example, the delivery cannula can be composed at its distal portion of the flexible material described herein and at its proximal portion of a more rigid material such as a metal, e.g., stainless steel.
In one embodiment, the luminal walls of the delivery cannula are coated or covered with an anti-adhesive compound. Anti-adhesive compounds include compounds which inhibit or prevent adhesion of agents described herein, e.g., therapeutic agents or agents which excite or inhibit neurons, or components thereof, to the luminal wall of the delivery cannula. In one embodiment, an anti-adhesive compound is a silicon (e.g., silane, e.g., silane the substituent groups of which can be any combination of nonreactive, inorganically reactive, and organically reactive groups). In one embodiment, the anti-adhesive compound is a polymer (e.g., polyethylene glycol), peptide, protein (e.g., albumin, e.g., bovine serum albumin, gelatin), glycoprotein (e.g., anti-sticking factor-I (ASF-I, Roy and Majumder (1989) Biochimica et Biophysica Acta 991(1):114-122; anti-sticking factor II (ASF-II, Roy and Majumder (19 Feb. 2004) Journal of Cellular Biochemistry 44(4):265-274), polysaccharide, or lipid or a solution of any of the foregoing (.e.g, serum, bovine serum, milk).
Examples of polymers that can be used as anti-adhesive compounds or as components of the delivery or guide cannulas described herein include acrylates including methyl acrylate, ethyl acrylate, propyl acrylate, n-butyl acrylate (BA), isobutyl acrylate, 2-ethyl acrylate, and t-butyl acrylate; methacrylates including ethyl methacrylate, n-butyl methacrylate, and isobutyl methacrylate; acrylonitriles; methacrylonitrile; vinyls including vinyl acetate, vinylversatate, vinylpropionate, vinylformamide, vinylacetamide, vinylpyridines, and vinylimidazole; aminoalkyls including amino alkylacrylates, aminoalkylmethacrylates, and aminoalkyl(meth)acrylamides; styrenes; cellulose acetate phthalate; cellulose acetate succinate; hydroxypropylmethylcellulose phthalate; poly(D,L-lactide); poly(D,L-lactide-co-glycolide); poly(glycolide); poly(hydroxybutyrate); poly(alkylcarbonate); poly(orthoesters); polyesters; poly(hydroxyvaleric acid); polydioxanone; poly(ethylene terephthalate); poly(malic acid); poly(tartronic acid); polyanhydrides; polyphosphazenes; poly(amino acids) and their copolymers (see generally, Svenson, S (ed.)., Polymeric Drug Delivery: Volume I: Particulate Drug Carriers. 2006; ACS Symposium Series; Amiji, M. M (ed.)., Nanotechnology for Cancer Therapy. 2007; Taylor & Francis Group, LLP; Nair et al. Prog. Polym. Sci. (2007) 32: 762-798); hydrophobic peptide-based polymers and copolymers based on poly(L-amino acids) (Lavasanifar, A., et al., Advanced Drug Delivery Reviews (2002) 54:169-190); poly(ethylene-vinyl acetate) (“EVA”) copolymers; silicone rubber; polyethylene; polypropylene; polydienes (polybutadiene, polyisoprene and hydrogenated forms of these polymers); maleic anhydride copolymers of vinyl methylether and other vinyl ethers; polyamides (nylon 6,6); polyurethane; poly(ester urethanes); poly(ether urethanes); and poly(ester-urea).
The guide cannula is typically produced from an inert material which provides sufficient rigidity to stabilize the delivery cannula in the subject, e.g., which is stiff or rigid to such a degree as to be able to penetrate the subject such that at least its distal portion is adjacent to or in proximity to a selected site in the subject. In one embodiment, the guide cannula includes or comprises a metal, e.g., stainless steel, gold, and gold alloy, a glass, e.g., borosilicate, soda-lime glass, silicon dioxide either in the form of fused quartz or fused silica or other material that transmits light, or a plastic, e.g., a plastic comprising a polymer or other non-plastic polymeric material. In one embodiment, the delivery cannula includes or comprises a plastic, e.g., a polymer having a molecular weight of from about 10,000 to about 6,000,000 daltons, e.g., from about 10,000 to about 3,000,000 daltons, e.g., from about 10,000 to about 1,00,000 daltons, e.g., from about 10,000 to about 500,000 daltons. Examples of polymers that can be used in the guide cannula include synthetic rubber, bakelite, neoprene, nylon, polyvinyl chloride, polystyrene, polyethylene, polypropylene, polyacrylonitrile, polyvinyl butyral, silicone, and other polymers described herein.
In addition, the guide cannula can be manufactured from a combination of such materials.
In a preferred embodiment, the distal end of the guide cannula is a blunt end which minimizes damage to the tissue of the subject upon insertion of the guide cannula into the subject. The distal opening of the guide cannula can be disposed at the distal end of the guide cannula, coaxial with the lumen thereof, or it can be a side wall mounted opening disposed in a side wall of the guide cannula. If the opening at the distal portion of the guide cannula is a side wall mounted opening disposed in a side wall, the side wall of the guide cannula opposite the side wall mounted opening increases in thickness distally to converge with a distal aspect of the side wall mounted opening.
In one embodiment, the delivery cannula tapers from a point or location, e.g., a proximal portion, which is a selected distance from the distal end to form a tube having a diameter at its distal end which is smaller than the diameter at its proximal end. Preferably, the delivery cannula tapers such that the distal end of the delivery cannula is at least about ten fold, preferably at least about 20 fold, more preferably at least about 50 fold, and most preferably at least about 100 fold or more smaller than the diameter of the proximal end of the delivery cannula. In one embodiment, the guide cannula has a diameter of about 0.5 millimeters to about 3 millimeters and the delivery cannula tapers from a point or location which is a selected distance from the distal end to a distal end to form a tube having a diameter at its distal end of about 1 micrometer to about 200 micrometers. In one embodiment, the delivery cannula includes or comprises a hinge mechanism which allows a first portion of the delivery cannula to move relative to a second portion of the delivery cannula such that the delivery cannula exits the guide cannula at a selected angle relative to the guide cannula, e.g., at a selected angle relative to the guide cannula, e.g., at an angle greater than 30 degrees relative to the guide cannula, e.g., greater than 35, 40, 45, 50, 55, 60, 65, 70, 75, 80, 85, or 90 degrees relative to the guide cannula. For example, the hinge mechanism can be placed at any portion (e.g., a distal portion which is located about 3, 2.5, 2, 1.5, 1, or 0.5 centimeter(s) from the distal opening of the delivery cannula) of the delivery cannula such that the second portion is able to move as it exits the guide relative to the guide cannula as described herein. In one embodiment, the delivery cannula includes or comprises a distal opening which can be at the distal end of the delivery cannula, coaxial with the lumen thereof, or in a side wall, e.g., a side wall opening.
The systems of the invention can further include or comprise means for moving the delivery cannula relative to the guide cannula, means for moving the guide cannula relative to the selected site in the subject (e.g., a motorized drive), means for aspirating and expelling the contents of the delivery cannula, means for supplementing the contents, e.g., therapeutic agent, of the delivery cannula while it remains in the subject, e.g., in the tissue of the subject, during a surgical procedure, means for recording electrophyisological events at the selected site in the subject (e.g., by using devices such as the Guideline 4000 LP+™ from FHC, Bowdoin, Me., and compatible software), means for detecting an obstruction in the delivery cannula, e.g, means for measuring pressure at the site in the subject, e.g., including use of pressure transducers such as strain gages, variable capacitor, and piezoelectric sensors, and/or means for transmitting selected wavelengths of light to the distal portion of the delivery cannula. In one embodiment, components of a stereotaxic apparatus provide the means for moving the delivery cannula relative to the guide cannula, the means for moving the guide cannula relative to the selected site in the subject, and the means for aspirating and expelling the contents of the delivery cannula. In one embodiment, the systems of the invention include means for locking or securing the delivery cannula in a selected position, e.g., a stationary position, such that the delivery cannula does not move, e.g., does not move in any axis (e.g., it is secured or locked such that it cannot be withdrawn, advanced, or rotated), during delivery of the agents described herein.
In one embodiment, the delivery cannula or the guide cannula is manufactured such that it includes a selected configuration of a material which has free electrons or charge carriers (“luminal material”), e.g., a metal (e.g., copper, silver, gold, palladium, platinum, iron, and ruthenium) along a side of a lumen, e.g., a strip of metal which can extend for a selected length of the delivery or guide cannula and which can have length, width, and thickness dimensions of from about 5 nanometers to 300 microns, e.g., from about 1 micron to about 300 microns, e.g., from about 5 microns to about 250 microns. In one embodiment, the luminal material strip, e.g., metal strip, in the delivery cannula or the guide cannula can extend the length of the cannula and have a width of about 10 microns and a thickness of about 2 microns. This luminal material coating, e.g., metal coating in the lumen of the guide or delivery cannula, allows for recording electrophysiological events at the selected site in the subject. In addition, such coatings allow for sensing of other conditions, e.g., impedance, temperature, at the selected site. In one embodiment, the delivery cannula or guide cannula is manufactured such that it includes a compound (e.g., thermosetting polymer, e.g., UV-curable epoxies, and solvent based polymers, e.g., polyurethane, polyimide, a ceramic) which provides structural support to the cannula. Methods for manufacturing the delivery cannula or the guide cannula such that it includes a selected configuration of metal are know in the art, e.g., see manufacturing information from Optomec, St. Paul, Minn. and Albuquerque, N. Mex.
Therapeutic agents which can be delivered to a subject using the systems and the methods of the invention include agents which have a therapeutic effect, e.g., reduce or eliminate deleterious symptoms or undesirable effects caused by, for example, disease or injury, and/or which preserve health, in a subject. The therapeutic agents can be delivered alone or in combination with a pharmaceutically acceptable carrier or diluent through the diameter of the delivery cannula to the selected site in the subject. Pharmaceutically acceptable carriers or diluents are art recognized formulations and include saline, aqueous buffer solutions, solvents and/or dispersion media. The use of such carriers and diluents is well known in the art. These carriers or diluents are preferably sterile and fluid to the extent that easy syringability exists. Preferably, the solution is stable under the conditions of manufacture and storage and preserved against the contaminating action of microorganisms. Such therapeutic agents include small molecules, toxins, lysed cell products, cells, e.g., neural cells, e.g., such as mesencephalic cells and striatal cells, glial cells, stem cells, e.g., stem cells which are precursors to neural or glial cells, and tissues, peptides or proteins (e.g., a microbial opsin, an antibody, a growth factor, e.g., a neurotrophic factor, e.g., a ciliary neurotrophic factor for treatment of amyotrophic lateral sclerosis, brain-derived neurotrophic factor for treatment of Parkinson's disease, glial growth factors for treatment of multiple sclerosis and Parkinson's disease, and a nerve growth factor for treatment of Alzheimer's disease), lipids, and viruses. These growth factors can be delivered to a subject together with cells or tissues using the delivery systems of the invention. The cells delivered to the subject using the delivery systems of the invention can be obtained from any source, e.g., mammals such as pigs, rodents, and primates e.g., humans and monkeys.
Other examples of therapeutic agents include chemotherapeutic agents, e.g., small molecule or protein chemotherapeutic agents, which cross the blood brain barrier such as carmustine and chemotherapeutic agents, e.g., small molecule or protein chemotherapeutic agents, which do not cross the blood brain barrier such as cisplatin, photodynamic drugs or agents such as porphyrin analogues or derivatives, and antimicrobial agents such as antibiotics. In one embodiment, the chemotherapeutic agent is an anti-angiogenic agent. In one embodiment, the delivery systems of the invention can be used to deliver concentrated doses of chemotherapeutic agents directly to brain tumors, e.g., brain carcinomas, thereby bypassing systemic administration and its accompanying undesirable side effects. Similarly, the delivery systems of the invention can be used to deliver antibiotics to focal infectious processes in the brain of a subject, e.g., brain abscesses. Selected concentrations of these antibiotics can be locally administered using these systems without the limitation of the antibiotic's ability to cross the blood brain barrier. Photodynamic drugs or agents can be locally administered using the delivery systems of the invention, allowed to accumulate in precancerous or cancerous cells, and subsequently illuminated by light transmitted through the delivery cannula. Illumination of the cells containing the photodynamic drugs activates the drug which in turn results in destruction of the precancerous or cancerous cells.
Other therapeutic agents which are used to treat acute events such as trauma and cerebral ischemia, or agents which can be used to treat chronic pathological processes can also be delivered by employing the delivery systems of the invention. Examples of these agents include nitric oxide synthase inhibitors and superoxide dismutase to inhibit oxidative stress caused by trauma, ischemia, and neurodegenerative disease, thrombolytics, e.g., streptokinase, urokinase, for direct dissolution of intracerebral thrombosis, and angiogenic factors to help reestablish circulation to traumatized or infarcted areas.
Still other examples of therapeutic agents which can be delivered to a subject using the delivery systems of the invention include nucleic acids, e.g., nucleic acids alone, e.g., naked DNA, RNA (e.g., regulatory RNA, e.g., RNAi (e.g., siRNA, microRNA, antisense RNA) and nucleic acids, e.g., DNA or RNA in delivery vehicles such as plasmids, lipid (e.g., lipidoids) or lipoprotein delivery vehicles and viruses or particles, e.g., microparticles, e.g., nanoparticles (e.g., particles having a size in their greatest dimension of between about 10 nm to about 1000 nm). For example, nucleic acids which can be delivered to a subject using the systems of the invention can encode foreign tissue antigens that cause tumors, e.g., brain carcinomas, to be attacked by the immune system. In addition, further examples of nucleic acids which can be delivered to a subject using the systems of the invention include nucleic acids which encode immunostimulators (e.g., cytokines, IL-2, IL-12, γ-interferon) to boost the immune system, nucleic acids which encode antigens which render tumor cells more vulnerable or more susceptible to chemotherapy, e.g., Allovectin-7, and nucleic acids which encode apoptotic proteins which cause the tumor cells to self-destruct. Alternatively, nucleic acids encoding neurotrophic factors, deficient proteins, specialized receptors, et cetera can also be delivered to a subject using the delivery systems of the invention. Regulatory RNAs which can be delivered to a subject using the systems of the invention can target genes associated with neurodegenerative diseases, e.g., the huntingtin gene.
The therapeutic agents can be chronically infused into a subject using the delivery systems of the invention. Chronic infusion can be accomplished by advancing the delivery cannula to the target site, e.g., target brain site, securing it to the surrounding bone structures, e.g., skull, with, for example, acrylic, and attaching a constant infusion device, such as a mini-osmotic pump loaded with the therapeutic agent to be infused or delivered.
In one embodiment, the delivery systems of the invention can be used to deliver neural cells to a selected site, e.g., putamen, caudate, substantia nigra, nucleus accumbens, or hippocampus, in the central nervous system. For example, when neural cells, e.g., mesencephalic cells, are transplanted into subjects having Parkinson's disease, the cells are typically delivered to the putamen and caudate nucleus. In addition, neural cells, e.g., GABAergic neurons, can be delivered using the delivery systems of the invention to epileptic foci in the brain of a subject. Furthermore, the delivery systems of the invention can be used to deliver cortical neurons, e.g., hNT neurons, to repopulate areas of neurodegeneration caused by stroke or trauma.
The invention also features methods for delivering a therapeutic agent to a selected site in a subject. Subjects who can be treated using this method include mammals, e.g., primates such as humans and monkeys, pigs, and rodents. Selected sites in a subject include locations to which it is desirable to deliver a therapeutic agent. Examples of such locations include areas of neurodegeneration in the central nervous system of a subject. These methods include the steps of inserting a guide cannula having the features described herein such that its distal portion is proximal to a selected site in the subject and inserting a delivery cannula, which releasably holds a therapeutic agent, into the guide cannula. The delivery cannula is inserted into the guide cannula a predetermined distance such that the distal end of the delivery cannula is proximal to an opening at the distal portion of the guide cannula. The methods then include the steps of extending the delivery cannula through the opening at the distal portion of the guide cannula along a first extension path to the selected site in the subject, and releasing the therapeutic agent from the delivery cannula into the selected site in the subject to form an injection site. In an alternative embodiment, the delivery cannula is inserted into the guide cannula prior to insertion of the guide cannula into the subject. In yet another alternative embodiment, the delivery cannula is loaded with the therapeutic agent to be delivered to the subject after it is inserted into the guide cannula. The delivery cannula can taper from a point or location at a selected distance from a distal end to the distal end to form a tube having a diameter at its distal end which is smaller than the diameter at its proximal end.
In another embodiment, the method further includes or comprises, after the step of releasing the therapeutic agent to the selected site, the steps of retracting the delivery cannula a predetermined distance from the first injection site, and releasing, e.g., by injection, the therapeutic agent from the delivery cannula into a second selected site in the subject to form a second injection site. These additional steps can be repeated as desired, e.g., at least twice.
In yet another embodiment, the invention further includes or comprises, after the step of releasing the therapeutic agent to the selected site or a series of sites along one path, the steps of retracting the delivery cannula such that the distal end of the delivery cannula does not extend beyond the opening at the distal portion of the guide cannula, rotating the guide cannula a predetermined angle from the first extension path of the delivery cannula, extending the delivery cannula through the opening at the distal portion of the guide cannula along a second extension path to a second selected site or series of sites in the subject, and releasing the therapeutic agent from the delivery cannula into the second selected site in the subject to form a second injection site or sites. These additional steps can also be repeated as desired, e.g., at least twice. This method results in placement of transplants in a three dimensional configuration in the subject with minimal trauma to the tissues of the subject.
The invention also features methods for testing or monitoring selected neuronal circuitry in a subject, e.g., a mammal, e.g., a primate such as a human, monkey, pig, or rodent. These methods include the steps of inserting a guide cannula having the features described herein such that its distal portion is proximal to a selected site in the subject and inserting a delivery cannula, which releasably holds an agent that can excite or inhibit a neuron when exposed to light, e.g., a microbial opsin, (e.g., channelrhodopsins ChR2 and VChR1 to excite neurons, and halorhodopsin (NpHR), archaerhodopsin (Arch), and fungal opsins such as leptosphaeria maculansopsin (Mac) to inhibit neurons) into the guide cannula. The delivery cannula is inserted into the guide cannula a predetermined distance such that the distal end of the delivery cannula is proximal to an opening at the distal portion of the guide cannula. The methods then include the steps of extending the delivery cannula through the opening at the distal portion of the guide cannula along a first extension path to the selected site in the subject, releasing the agent that can excite or inhibit a neuron from the delivery cannula into the selected site in the subject to form an injection site, delivering light to excite or inhibit the neurons, and then recording the activity, e.g., electrical activity, of the neurons. In one embodiment, the light is transmitted through either of the delivery cannula or the guide cannula. In one embodiment, the activity, e.g., electrical activity, of the neurons is measured using a means for electrophysiological recording. In one embodiment, the method further includes the step of administering a therapeutic agent at the site of neuronal activity, or a site in promimity thereto, e.g., within a centimeter of the site of neuronal activity, in order to assess its affect on the neuronal activity. In these methods, one or more delivery cannulas can be used to deliver the agent that can excite or inhibit a neuron when exposed to light and the therapeutic agent. In these methods, the system can include various additional means for accomplishing each step in the methods, e.g., the system can include means for moving the delivery cannula relative to the guide cannula, means for moving the guide cannula relative to the selected site in the subject (e.g., a motorized drive), means for aspirating and expelling the contents of the delivery cannula, means for supplementing the contents, e.g., therapeutic agent, of the delivery cannula while it remains in the subject, e.g., in the tissue of the subject, during a surgical procedure, means for recording electrophyisological events at the selected site in the subject (e.g., by using devices such as the Guideline 4000 LP+™ from FHC, Bowdoin, Me., and compatible software), means for detecting an obstruction in the delivery cannula, e.g, means for measuring pressure at the site in the subject, e.g., including use of pressure transducers such as strain gages, variable capacitor, and piezoelectric sensors, means for transmitting selected wavelengths of light to the distal portion of the delivery cannula, means for measuring the distance of extension of the delivery cannula from an opening, e.g., a side wall opening, in the guide cannula; and/or means for uncoupling the delivery cannula from the guide cannula, e.g., in order to remove the delivery cannula from the guide cannula.
In an alternative embodiment, the delivery cannula is inserted into the guide cannula prior to insertion of the guide cannula into the subject. In yet another alternative embodiment, the delivery cannula is loaded with the agent that can excite or inhibit a neuron when exposed to light to be delivered to the subject after it is inserted into the guide cannula. The delivery cannula can taper from a point or location at a selected distance from a distal end to the distal end to form a tube having a diameter at its distal end which is smaller than the diameter at its proximal end.
This invention is further illustrated by the following figures which in no way should be construed as being further limiting. The contents of all cited references (including literature references, issued patents, published patent applications, and co-pending patent applications) cited throughout this application are hereby expressly incorporated by reference.
One embodiment of the delivery cannula of the invention is illustrated in
A preferred embodiment of the guide cannula is illustrated in
In addition, the delivery cannula of the delivery systems of the invention can be guided through the guide cannula such that it bends and exits through an opening at the distal portion of the guide cannula at an angle to allow for approach of a selected target site while avoiding or bypassing important anatomical structures adjacent to and/or surrounding the site. Using the delivery systems of the invention, neural cells can be delivered to remote or high risk targets such as the substantia nigra with minimal inflammation and edema and with minimal risk of damaging important anatomical structures, e.g., the brain stem. Thus, the delivery systems or delivery apparatuses of the invention can be used to discretely and consistently place small volumes of a therapeutic agent at selected anatomical site(s) while preserving local cytoarchitecture. If cells are delivered using the delivery systems of the invention, cell survival in the subject can be increased two fold or more over that seen with the techniques presently used for human neural transplantation. In situations where it is desirable to use fetuses from humans or other mammals as a source of cells or tissue to be transplanted, this increase in cell survival using the delivery systems of the invention decreases the number of fetuses required to provide the same level of clinical improvement in the recipient subject. For example, if 10 fetuses from which cells are harvested for transplantation are normally required using the delivery devices in the art to produce a desired level of clinical improvement in a human, only 5 fetuses would be required using the delivery system of the invention to produce the same level of clinical improvement in a subject. The delivery systems or delivery apparatuses of the invention can also be used to deliver therapeutic agents, with minimal disruption, to spinal cord locations, peripheral nervous system locations and locations in and around, e.g., eye chambers, the eye, et cetera.
Additional applications of the delivery systems of the invention are diverse and include use in microbiopsy, electrophysiological recording, and photodynamic therapy. Just as tissue can be discretely placed in a selected site in a subject in one, two or three dimensional arrays, tissue can be removed from discrete, selected sites in a subject using the delivery systems of the invention in a one, two or three dimensional array. This is achieved by aspirating cells into the tip of the delivery cannula, or by first injecting a small volume of enzyme, such as trypsin, allowing a short incubation, and then aspirating the dissociated cells into the tip of the delivery cannula. In this embodiment, the delivery cannula becomes a removal cannula. Microbiopsies of aberrant cells, e.g., cancerous cells, using the systems of the invention can be performed with minimal trauma to the subject while reducing the risk of seeding, e.g., leaving a path of aberrant cells, normal tissue with aberrant cells. In addition, aberrant cells, e.g., cancer cells, can be removed using the systems of the invention, genetically manipulated in culture, and delivered to the subject as a vaccine with extremely high tumor specificity.
The delivery systems of the invention can also be used to record electrical, e.g., neural, activity, in a subject. For example, areas of abnormal electrical activity, e.g., epileptic foci, can be located using the systems of the invention. In this embodiment, the carrier of the therapeutic agent can include an electrolytic solution and the delivery cannula can serve as an electrode. Once the site of abnormal electrical activity is located, the therapeutic agent, can be delivered to the site also using the systems of the invention and characterized using standard electroencephalography. Moreover, because the therapeutic agent to be delivered can be in an electrolytic solution, recording and then delivery or injection can be achieved in one step.
An additional application for the delivery systems of the invention is in the field of photodynamic therapy for the destruction of cancer cells within precise foci. Photodynamic therapy is performed by injecting a photoreactive agent into a tumor site which preferentially accumulates within the tumor cells. With the delivery cannula still in position after delivery of the photoreactive agent, light is transmitted to the tip (distal portion) of the cannula (which can be designed to emit light) to thereby activate the photoreactive agent and destroy the tumor cells. Further description of methods of performing photodynamic therapy can be found in Fisher, A. M. et al. (1995) Lasers Surg. Med. 17(1):2-31 and Stables, G. I. et al. (1995) Cancer Treat. Rev. 21(4):311-323.
Those skilled in the art will recognize, or be able to ascertain using no more than routine experimentation, many equivalents of the specific embodiments of the invention described herein. Such equivalents are intended to be encompassed by the following claims.
This application claims priority to U.S. Ser. No. 61/348,064, filed May 25, 2010, the contents of which are considered part of and are incorporated by reference in the disclosure of the present application.
Filing Document | Filing Date | Country | Kind | 371c Date |
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PCT/US11/37867 | 5/25/2011 | WO | 00 | 11/21/2012 |
Number | Date | Country | |
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61348064 | May 2010 | US |