The present invention relates to a drug delivery system to posterior segments such as a retina, a choroid and an optic nerve.
Diseases of posterior segments such as a retina, a choroid and an optic nerve are often intractable, and a development of an effective treatment method is eagerly desired. Though ophthalmopathy is most generally treated by instillation of drugs, the drugs are hardly delivered to the posterior segments such as a retina, choroid and an optic nerve. Even if the drugs are delivered to the posterior segments, it is very difficult to sustain a drug concentration in those tissues.
In view of this, an intravenous injection, oral administration and a vitreous injection are attempted to administer the drugs for the diseases of the posterior segments. However, the intravenous injection and the oral administration can deliver only a very minute amount of drugs to the posterior segments which are target sites, and sometimes causes unexpected strong systemic actions (side effects) of the drugs.
In the case of the vitreous injection, since the drug is directly injected into eyes, the amount of the drug to be delivered to the posterior segments is larger than those of the intravenous injection and the oral administration. The delivery to the posterior segments by the vitreous injection is summarized in Journal of ocular pharmacology and therapeutics, (2001) 17/4, 393-401 as a review. However, the vitreous injection is a method of administration which requires skilled procedure and is accompanied by a considerable pain. Accordingly, burdens on patients are heavy, and it is very difficult to administer the drug plural times.
Unlike these methods of administration, a periocular injection, of which procedure is relatively easy, hardly causes disorders of ophthalmic tissues and burdens on patients are light, compared with the vitreous injection. A delivery of a drug to the posterior segments after the periocular injection was reported (Invest. Ophthalmol. Visual Sci. 18 (3) 250-255, 1979), but its half-life was remarkably short, and it was difficult to sustain a drug concentration in the posterior segment tissues for a long period. Accordingly, frequent administration is required in order to sustain the drug concentration in the tissues, but the frequent administration increases the burdens on patients.
Known methods of sustaining the drug concentration in eyes without doing the frequent administration are exemplified by a method of administrating a conjugate of a drug with a polymer intravenously (Invest. Ophthalmol. Visual Sci. 40 (1), 2690-2696, 1999), a method of injecting a microsphere containing a drug into a vitreous body (Japanese Laid-open Patent Publication No. 247871/2000).
Since it was difficult to sustain the concentration of the drug injected periocularlly into the tissues by the conventional techniques as mentioned above, it was desired to develop a sustained drug delivery system to the posterior segments by the periocular injection.
Studying precisely, the present inventors found that periocular administration of sustained release fine particles containing a drug is very useful as a sustaining drug delivery system to posterior segments.
The present invention relates to the drug delivery system to the posterior segments to be used in order to administer the fine particles containing the drug periocularlly. The present invention also relates to a periocular injection which comprises the fine particles containing the drug and enables the drug to deliver to the posterior segments. The delivery of drug to the posterior is excellent and systemic side effects are hardly caused by administering the fine particles containing the drug compared with an intravenous injection and oral administration. Procedure is easy and burdens on patients are light compared with a vitreous injection. Further, a drug concentration in the target tissue can be sustained for a long period by using the fine particles containing the drug.
Preferred materials which are used to form the fine particles in the present invention are biodegradable or biosoluble polymers, and specific examples thereof are biodegradable polymers such as poly(lactic acid), lactic acid-glycolic acid copolymers, lactic acid-caprolactone copolymers, polyanhydrides, poly (ortho ester), poly-ε-caprolactone, polyacrylcyanoacrylates, polyhydroxyalkanoates, polyphosphoesters, polyamino acids and poly α-hydroxyacids; natural polymers such as gelatin, collagen, hyaluronic acid, dextran, starch, sodium alginate, agar, pullulan, albumin, carageenan, pectin, xanthan gum, gellan gum, casein, chitosan and fibrinogen; and synthetic polymers such as methacrylic acid copolymers, polyvinyl alcohol, hydroxypropylmethylcellulose, hydroxypropylmethylcellulose acetate, hydroxyethyl cellulose, carboxymethylcellulose, methyl cellulose, polyvinyl pyrrolidone, polyethylene glycol and poly N-alkylacrylamide.
Molecular weight of these polymeric substances is not particularly limited and can be appropriately selected depending on the kind of drug contained in the fine particles, an effective drug concentration for treatment, a release period of the drug or the like.
A particle diameter of the fine particles in the present invention is preferably 50 nm to 150 μm. It is difficult to produce fine particles having a particle diameter of 50 nm or less. The particle diameter of 150 μm or more is too large to use the fine particles in the form of injections. A more preferred particle diameter is 200 nm to 75 μm.
The drug delivery system of the present invention is used for treatment or prevention of diseases of a retina, a choroid membrane and an optic nerve. Specific examples of diseases are inflammation due to various causes, viral or bacterial infections, diseases due to angiogenesis of a retina-choroid, diseases due to ischemia of a retina and optic nerve disorders due to glaucoma. Further specific examples of diseases are uveitis, cytomegalovirus retinitis, age-related macular degeneration, diabetic retinopathy, proliferative vitreoretinopathy, retinal detachment, pigmentary retinal degeneration, central retinal vein occlusion and central retinal artery occlusion.
The drugs contained in the fine particles are not particularly limited, and drugs suited for object diseases can be selected. Specific examples of drugs are steroids or derivatives thereof such as betamethasone, dexamethasone, triamcinolone, prednisolone, fluorometholone, hydrocortisone and progesterone; anti-inflammatories such as bromofenac and diclofenac; cytokine inhibitors such as TNF-α inhibitors, PDE-IV inhibitors and ICE inhibitors; immunosuppressors such as ciclosporin and tacrolimus; antivirals such as ganciclovir, aciclovir and interferon-β; antimicrovials such as ofloxacin, clarithromycin and erythromycin; carcinostatic agents such as fluorouracil, methotrexate and MMP inhibitors; angiogenesis inhibitors such as endostatin, VEGF inhibitors, antisense oligonucleotide, PKC inhibitors, adhesion factor inhibitors and vascular resting steroid; neural protectants-neural nutrition factors such as MK-801, timolol, creatine, taurine and BDNF; carbonate dehydratase inhibitors such as acetazolamide; and thrombolytic drugs such as urokinase. Preferred forms of the fine particles containing the drug are a matrix-type wherein the drug is dispersed uniformly in the fine particles and a capsule-type wherein the drug as a core is encapsulated with the fine particles.
An amount of the drug contained in the fine particles can be appropriately increased or reduced depending on the kind of drug, the effective drug concentration for treatment, the release period of the drug, symptoms of diseases or the like. A drug content is 0.01 to 95% by weight, preferably 0.1 to 20% by weight in the fine particles.
The fine particles can be produced by a grinding method using a mill, a phase separation method (a coacervation method), a spray drying method, a supercritical fluid method, an interfacial deposition method or an interfacial reaction method, which is known, and the method is not limited to them. More specific examples of methods are a submerged drying method, which is the interfacial deposition method (J. Control. Release, 2, 343-352, (1985)), an interfacial polymerization method, which is an interfacial reaction method (Int. J. Pharm., 28, 125-132 (1986)) and a self-emulsification solvent diffusion method (J. Control. Release, 25, 89-98 (1993)). An appropriate process for production can be selected among these processes for production considering the particle diameter of the fine particles, the kind, properties or a content of the contained drug or the like.
A practical production example of drug-containing fine particles will be illustrated later in which fine particles contain betamethasone, an anti-inflammatory, and the material of the fine particles is polylactic acid.
Effects of the present invention will be described later in detail in a section of “drug concentration in retina-choroid measurement tests”. Administering the fine particles containing betamethasone periocularlly and measuring a drug concentration in a retina-choroid, it was found that the drug concentration in the retina-choroid is sustained.
The fine particles in the drug delivery system of the present invention are administered periocularly. The periocular administration can be carried out using an ordinary periocular injection. The procedure of the periocular injection is relatively easy, and the burdens on patients are light as described in the section of “Background Art”.
Further, since the drug can be efficiently delivered to the posterior segments such as a retina, a choroid and an optic nerve by using the system of the present invention, a dosage of the drug can be reduced, and consequently side effects can also be reduced.
To administer periocularlly the fine particles to be used for the drug delivery system of the present invention, preferred dosage forms are injections. The injections can be prepared by widely-used formulation techniques of injections. For example, the preparations can be prepared by adding an additive to be usually used such as an osmotic pressure adjustor such as sodium chloride, a buffer such as sodium phosphate, a surfactant such as polysorbate 80 or a thickener such as methyl cellulose and the fine particles to distilled water for injections. When a high pressure syringe having no needle is used, the fine particles can be administered as they are without rendering them the injection.
A production example of the fine particles, an example of the preparation and results of drug concentration measurement tests and choroidal neovascularization inhibition tests are illustrated below.
1. Process for Producing Drug-Containing Fine Particles
A production example of fine particles which can be used for a drug delivery system of the present invention is illustrated below.
Betamethasone (0.025 g) and polylactic acid (0.25 g) having weight-average molecular weight of 20,000 were dissolved in benzyl alcohol (1.5 ml). The obtained solution was referred to as a drug/polymer solution. A 2.0% (w/v) aqueous polyvinyl alcohol solution (30 ml) was homogenized with a homogenizer (5,000 rpm), and the drug/polymer solution was added dropwise to the homogenized solution. The mixture was homogenized for five minutes after finishing dropping to prepare an O/W emulsion. Ultrapure water (300 ml) was stirred (300 rpm) with a stirrer, thereto the prepared O/W emulsion was added dropwise followed by stirring for one hour after finishing dropping. After stirring, the obtained suspension was centrifuged, and the resulting supernatant was removed. In order to wash the resulting precipitate, ultrapure water (30 ml) was added to the precipitate to disperse it, the dispersion was centrifuged again, and the resulting supernatant was removed. This operation was repeated one more time. The washed precipitate was sieved to give particles having particle diameters of 50 nm to 75 μm. The obtained particles were lyophilized to give betamethasone-containing microsphere.
2. Process for Preparing Preparation
Betamethasone-containing microsphere powder (442 mg) was dispersed in a solvent (4 ml of an aqueous solution containing 0.4% (w/v) of polysorbate 80 and 2.6% (w/v) of glycerin). The obtained dispersion was referred to as a betamethasone-containing microsphere injection.
3. Measurement of Drug Concentration in Retina-Choroid
Using the betamethasone-containing microsphere injection, a beta met has one concentration in a retina-choroid was measured according to the method below. As a control, using a betamethasone suspension, a concentration was measured in the same manner. A betamethasone concentration in the retina-choroid of a microsphere administration group was compared with that of a suspension administration group. The betamethasone suspension was prepared by suspending betamethasone in a solvent (an aqueous solution containing 0.4% (w/v) of polysorbate 80 and 2.6% (w/v) of glycerin).
Results of changes in drug concentration with time are shown in Table 1. As apparent from Table 1, in the case of the betamethasone suspension, the betamethasone concentration in the retina-choroid was about 0.96 μg/g tissue after seven days, but it was a detection limit or lower after 14 days. To the contrary, in the case of the betamethasone-containing microsphere, the betamethasone concentration in the retina-choroid was about 0.09 μg/g tissue even after 28 days, and the drug concentration in the retina-choroid was sustained.
(In Table 1, the betamethasone concentrations in the retina-choroids represent the average of three or four eyes±standard error. The value after seven days of the microsphere injection represents the average of two eyes since the concentrations were the detection limit or lower in two eyes of four eyes.)
4. Choroidal Neovascularization Inhibition Tests
Inhibitory effects of the betamethasone-containing microsphere injection on choroidal neovascularization were studied by the method below using laser-induced rat choroidal neovascularization models. As a control, using a microsphere injection containing only the solvent (an aqueous solution containing 0.4% (w/v) of polysorbate 80 and 2.6% (w/v) of glycerin), operation was carried out in the same manner.
Neovascularization exhibition rate (%)=(fluorescence di ape des is spot number/laser irradiation spot number)×100.
The obtained results are expressed in the average±standard error. A Student's t test was used for statistical analysis. Each level of significance was taken as 5% on both sides.
Inhibitory effects of the betamethasone-containing microsphere on the choroidal neovascularization are shown in Table 2. While a neovascularization exhibition rate of the control group 14 days after the photocoagulation was 60.9±4.4%, a neovascularization exhibition rate of a betamethasone-containing microsphere group was 12.5±2.4%, and the betamethasone-containing microsphere exhibited a statistically significant inhibitory action on the choroidal neovascularization. Even 28 days after the photocoagulation, while a neovascularization exhibition rate of the control group was 73.4±6.0%, a neovascularization exhibition rate of the betamethasone-containing microsphere group was 12.5±2.4%, and the betamethasone-containing microsphere exhibited the statistically significant inhibitory action on the choroidal neovascularization. The above-mentioned results mean that the periocularlly-administered betamethasone-containing microsphere exhibits the inhibitory action on the choroidal neovascularization even 14 and 28 days after the administration.
(In Table 2, the neovascularization exhibition rates of the respective groups represent the average of eight eyes±standard error.)
The present invention can provide an excellent drug delivery system to posterior segments by periocular administration.
Number | Date | Country | Kind |
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2002-46355 | Feb 2002 | JP | national |
Filing Document | Filing Date | Country | Kind |
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PCT/JP03/01897 | 2/21/2003 | WO |