JPS6163613A - Sustained release preparation - Google Patents
Sustained release preparationInfo
- Publication number
- JPS6163613A JPS6163613A JP18367184A JP18367184A JPS6163613A JP S6163613 A JPS6163613 A JP S6163613A JP 18367184 A JP18367184 A JP 18367184A JP 18367184 A JP18367184 A JP 18367184A JP S6163613 A JPS6163613 A JP S6163613A
- Authority
- JP
- Japan
- Prior art keywords
- drug
- polylactic acid
- sustained release
- organisms
- additional matter
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Pending
Links
Abstract
Description
【発明の詳細な説明】
(産業上の利用分野)
本発明は生体内(二おける生理活性物質の放出速度が制
御された顆粒状に調製された徐放性製剤に関する。DETAILED DESCRIPTION OF THE INVENTION (Field of Industrial Application) The present invention relates to a sustained release preparation prepared in the form of granules in which the release rate of a physiologically active substance in the body is controlled.
(従来の技術)
最近の制ガン療法では制ガン薬をガン患部周辺のみに分
布させ、正常細胞個所への副作用を防止し、同時に樹脂
などの高分子賦形剤を用いて薬効の持続を考慮した投与
方法や剤形の研究が盛んにおこなわれている。(Conventional technology) In recent anticancer therapy, anticancer drugs are distributed only around the cancerous area to prevent side effects on normal cells, and at the same time, polymeric excipients such as resins are used to maintain drug efficacy. Research on the administration methods and dosage forms is being actively conducted.
患部周辺のみに長時間にわたって継続的に有効濃度の薬
物を供給する、いわゆる徐放性局部投与方法として、例
えば制ガン薬をカプセル中に入れたり、または錠剤ない
しペレット状に成形した製剤を、ガン患部の局部周辺に
埋め込む方法や、制ガン薬なコアセルベイジョンにより
重合物波膜でマイクロカプセル化、または重合物?1容
媒に溶解し、これに薬な溶解または懸濁させた後マイク
ロスフイアに調製したものを、局部周辺の筋肉内ないし
は血管内に注入し、局部周辺の血管の、マイクロカプセ
ルまたはマイクロスフイアで塞栓して閉枠された局部血
管のみに薬剤が浸出するのを利用する方法などが挙げら
れる。As a so-called sustained-release local administration method that continuously supplies an effective concentration of a drug only to the affected area over a long period of time, for example, an anticancer drug is placed in a capsule, or a preparation formed into a tablet or pellet is used to treat cancer. A method of implanting it around the affected area, micro-encapsulation with a polymeric wave membrane through coacervasion, which is an anticancer drug, or a polymeric material? After dissolving or suspending the medicinal substance in 1 volume, it is prepared into microspheres and injected into the muscles or blood vessels around the local area to form microcapsules or microspheres in the blood vessels around the local area. Examples include a method that utilizes the fact that the drug seeps only into the local blood vessels that are closed off by embolization.
従来、重合物の被膜やマトリックスを用いて微小球に賦
形したものには、エチルセルローズやワックスを用いて
製剤したもの(特開昭54−163808)や、無毒の
生体内分解性高分子材料であるポリ乳酸などを用いてマ
イクロカプセルまたはマイクロスフイアに調製したもの
(特開昭54−55717 。Conventionally, microspheres formed using polymer coatings or matrices include those formulated using ethyl cellulose or wax (Japanese Patent Application Laid-Open No. 163808/1982), and non-toxic biodegradable polymer materials. prepared into microcapsules or microspheres using polylactic acid, etc. (Japanese Patent Laid-Open No. 54-55717).
特開昭59−33214 )などが知られている。しが
しながらポリ乳酸はガラス転移温度が低く、溶融粘度が
高いなどの物性上の制約があり、この生体内分解性高分
子材料では均一なマイクロカプセル化された微小球は得
られがたいとされている。特に薬物粒子の形状が不均一
の場合は完全にカプセル化されていない粒子もあり、従
ってポリ乳酸によりマイクロカプセル化された製剤を患
部に投与した場合、投与初期の薬物放出速度が非常に速
くて長時間に亘っての徐放性が得られず、常に一定濃度
で薬物が供給される徐放効果は得られ難い。JP-A-59-33214) is known. However, polylactic acid has physical property limitations such as a low glass transition temperature and high melt viscosity, and it is difficult to obtain uniform microencapsulated microspheres with this biodegradable polymer material. has been done. Particularly when the shape of the drug particles is non-uniform, some particles may not be completely encapsulated. Therefore, when a preparation microencapsulated with polylactic acid is administered to the affected area, the drug release rate at the initial stage of administration is very fast. Sustained release over a long period of time cannot be obtained, and it is difficult to obtain a sustained release effect in which the drug is always supplied at a constant concentration.
一方、たとえば前記特開昭59−33214号公報に記
載されているような方法で得られたポリ乳酸をマトリッ
クスに用いたマイクロスフイア製剤を投与した場合、長
時間に亘っての徐放効果は得られるものの、薬物含有率
や用いるポリ乳酸の分子量には殆んど無関係に、投与後
24時間以降の放出速度が非常に低くなることがわかっ
た。On the other hand, when a microsphere preparation using polylactic acid as a matrix obtained by the method described in JP-A-59-33214 is administered, the sustained release effect over a long period of time is However, it was found that the release rate after 24 hours after administration became extremely low, almost regardless of the drug content and the molecular weight of the polylactic acid used.
一般に薬物の生理活性における薬理作用として、薬物に
よっては一定期間中は患部に一定濃度以上に存在してい
なければ薬理効果が得られない場合もあり、それに必要
な一定期間内は放出速度の増大をはかる必要もある。In general, depending on the pharmacological action of the physiological activity of a drug, some drugs may not have a pharmacological effect unless they are present at a certain concentration in the affected area for a certain period of time, and the release rate must be increased within the necessary certain period of time. There is also a need to measure it.
(発明が解決しようとする問題点)
前記のように、ポリ乳酸を用いた従来技術の徐放性製剤
では放出持続性がないか、または極端に放出時間が長す
ぎるため活性濃度が希薄で薬理効果の乏いか、のいずれ
かであった。(Problems to be Solved by the Invention) As mentioned above, conventional sustained-release preparations using polylactic acid do not have sustained release or have an extremely long release time, resulting in dilute active concentrations and poor pharmacology. They were either ineffective or not.
本発明者らは、これらの問題を解決するため鋭意検討の
結果本発明を完成するに至ったものであり、従って本発
明の目的は、薬物活性が必要な期間中は常に必要な活性
濃度を維持可能な、放出速度を制御出来る徐放性製剤な
提供することである。The present inventors have completed the present invention as a result of intensive studies to solve these problems. Therefore, the purpose of the present invention is to maintain the necessary active concentration at all times during the period when drug activity is required. The purpose of the present invention is to provide a sustained release formulation that can be maintained and whose release rate can be controlled.
(問題を解決するための手段)
本発明は、生体内分解性高分子であるポリ乳酸を用いた
注射用または埋込(−用いるマイクロスフイア構造の徐
放性製剤を提供するものであり、該徐放性製剤の製造に
際して、生体内で消化されうる脂溶性添加物を薬物の放
出速度制御のために添加して、これをポリ乳酸類と均一
に固化析出せしめ、かつ顆粒状に調製した徐放性製剤で
ある。従って本発明の顆粒状に調製された徐放性製剤と
は、ポリ乳酸またはその共重合体に少量添加された脂溶
性添加物がマ)リツクスとなり、徐放される薬物と均質
に分散した粒径10乃至500μを有するマイクロスフ
イア構造の製剤であり、これにより、従来のポリ乳酸の
みを用いたマイクロスフイア構造の徐放性製剤の欠点で
あった、投与後の一定時間経過後の活性成分の放出速度
の低下が防止できる。(Means for Solving the Problems) The present invention provides a microsphere-structure sustained release preparation for injection or implantation using polylactic acid, which is a biodegradable polymer, During the production of the sustained-release preparation, a fat-soluble additive that can be digested in vivo was added to control the release rate of the drug, and this was uniformly solidified and precipitated with polylactic acids, and was prepared into granules. It is a sustained-release preparation. Therefore, the sustained-release preparation prepared in the form of granules of the present invention is a matrix in which a small amount of a fat-soluble additive is added to polylactic acid or its copolymer, and the drug is released in a sustained manner. It is a microsphere-structured preparation with a particle size of 10 to 500μ that is homogeneously dispersed with the drug, and this makes it possible to eliminate the shortcomings of conventional microsphere-structured sustained-release preparations using only polylactic acid after administration. It is possible to prevent a decrease in the release rate of the active ingredient after a certain period of time has elapsed.
本発明に用いられる放出速度制御用添加物は、有機溶剤
を用いたポリ乳酸溶液から得られる公知のマイクロスフ
イアの製造時に添加されるものであり、従って添加物は
、該有機溶剤に溶けしかも生体内で消化される脂溶性の
ものでなければならない。これら添加物としては、植物
油、カカオ脂、中鎖(CS乃至C22)脂肪酸トリグリ
セリド、低級(C6以下)脂肪酸トリグリセリド、プロ
ピレングリコールのジ脂肪酸エステル、中鎖または高級
(C8以上)脂肪酸アルキルエステル、乳酸アルキルエ
ステル、などのほかに芳香族モノまたはジカルボン酸ア
ルキルエステルなども使用できるが、特に脂肪酸エステ
ル類は好ましい添加物である。The release rate controlling additive used in the present invention is added during the production of known microspheres obtained from a polylactic acid solution using an organic solvent, and therefore, the additive may be dissolved in the organic solvent. It must be fat-soluble and digested within the body. These additives include vegetable oil, cocoa butter, medium chain (CS to C22) fatty acid triglycerides, lower (C6 or lower) fatty acid triglycerides, difatty acid esters of propylene glycol, medium chain or higher (C8 or higher) fatty acid alkyl esters, and alkyl lactates. In addition to esters, aromatic mono- or dicarboxylic acid alkyl esters can also be used, but fatty acid esters are particularly preferred additives.
添加物の使用量はその種類及び薬物の種類、投与形態に
もとづく放出速度量により適宜法められるが、通常ポリ
乳酸類100重駄部に対して5〜100屯量部の範囲内
で使用される。The amount of additive used is determined as appropriate depending on the type of additive, the type of drug, and the release rate based on the dosage form, but it is usually used within the range of 5 to 100 parts by weight per 100 parts by weight of polylactic acid. Ru.
本発明の徐放性製剤の調製は、常法に従い、例えば以下
のようにして得られる。すなわちポリ乳酸類及び添加物
を塩化メチレンなどの有機溶剤(=完全に溶解してこれ
に薬物を溶解または懸濁し、これをゼラチンなどの保護
コロイドの存在する水性媒体中に攪拌下に滴下懸濁させ
、次いで溶剤を蒸発除去して得られる顆粒状のマイクロ
スフイアを水性媒体からr過分能すればよい。The sustained release preparation of the present invention can be prepared according to a conventional method, for example, as follows. In other words, polylactic acids and additives are completely dissolved in an organic solvent such as methylene chloride, and the drug is dissolved or suspended in this, and this is dropped and suspended in an aqueous medium containing a protective colloid such as gelatin while stirring. The granular microspheres obtained by evaporating and removing the solvent may be superfractionated from an aqueous medium.
本発明(=用いられる薬物は、従来より徐放i生が望ま
れる薬物として知られている薬物なら全てに適用+41
′能であるが、特にその作用の時間依存性の大きな制ガ
ン薬などに適用すれば効果が大きく、そのほか、インシ
ュリン、プロスタグランジン類、局所麻酔薬、などにも
使用できる。The present invention (=applicable to all drugs that are conventionally known as drugs for which sustained release is desired)
However, it is especially effective when applied to anticancer drugs whose action is highly time-dependent, and can also be used for insulin, prostaglandins, local anesthetics, etc.
本発明に用いるポリ乳酸類、すなわちポリ乳酸を主材料
とした生体内分解性重合物とは、ポリ−4−乳酸、ポリ
ーd、l−乳酸、または乳酸−グリコール酸の共重合物
であり、ポリ−1−乳酸の場合は、l一体の分子量10
,000〜200.000のものが適しており、またd
、l一体の場合は固有粘度0.6〜1.2(クロロホル
ム中、25℃で測定)程度のものが適している。The polylactic acids used in the present invention, that is, the biodegradable polymers mainly made of polylactic acid, are poly-4-lactic acid, poly-d, l-lactic acid, or a copolymer of lactic acid-glycolic acid, In the case of poly-1-lactic acid, the molecular weight of 1 is 10
,000 to 200,000 is suitable, and d
, l is suitable for use with an intrinsic viscosity of about 0.6 to 1.2 (measured in chloroform at 25°C).
ポリ乳酸類の使用量は、得られるマイクロスフイア10
0重量部に対し、ポリ乳酸類を30〜90重量部、好ま
しくは50〜80重量部用いる。とくに30重計部未満
では所望の強度および均一なマイクロスフイアは得(二
くい。また、添加物の使用量は前述したよう(二、ポリ
乳酸類100重量部(二対し5〜100重量部であり、
また薬物は、通常、マイクロスフイア100重量部中に
は、10〜50重量部含有されているが、薬物使用量が
多ければ添加物の使用は少なくてよい。The amount of polylactic acids used is 10
0 parts by weight, polylactic acids are used in an amount of 30 to 90 parts by weight, preferably 50 to 80 parts by weight. In particular, if the amount is less than 30 parts by weight, the desired strength and uniform microspheres cannot be obtained (2. and
Further, the drug is usually contained in 10 to 50 parts by weight in 100 parts by weight of microspheres, but if the amount of drug used is large, the amount of additives may be small.
(作用、及び発明の効果)
ポリ乳酸類、添加物、及び薬物よりなる本発明の徐放性
製剤は、注射用または埋込み用として使用できるマイク
ロスフイア構造の徐放性製剤であり、添加物の種類とそ
の使用割合を適宜選択することにより、薬物の放出速度
が制御でき、した゛がってその一定の濃度を維持できる
。また生体内の酵素によってポリ乳酸、添加物ともに加
水分解されて無害物質となるため、体外に取り出す必要
もなく、体内に残留もしない。(Actions and Effects of the Invention) The sustained-release preparation of the present invention comprising polylactic acids, additives, and drugs is a sustained-release preparation with a microsphere structure that can be used for injection or implantation. By appropriately selecting the type of drug and the ratio of its use, the release rate of the drug can be controlled and its concentration can therefore be maintained at a constant level. Furthermore, since both polylactic acid and additives are hydrolyzed by enzymes in the body and become harmless substances, there is no need to take them out of the body and they do not remain in the body.
実施例−1
固有粘度値(yJ ) = 1.32を有するボ9−1
−乳酸(クロロホルム中25℃で測定、分子量43,0
00)1.81を塩化メチレン40.9に攪拌しながら
溶解した後、イソプロピルミリステー)(IPM)0.
4gを溶かし、さらにブレオマイシン帆6gを加えて、
その懸濁液を得た。Example-1 Bo 9-1 having intrinsic viscosity value (yJ) = 1.32
-Lactic acid (measured in chloroform at 25°C, molecular weight 43.0
00) 1.81 in methylene chloride 40.9 with stirring, isopropyl myrite) (IPM) 0.
Dissolve 4g, add 6g of bleomycin,
A suspension was obtained.
別に、アルカリ処理のゼラチン〔宮城化学■製、ゼリー
強度250プルーム〕2gを、198gの水に加え50
℃で加温溶解して1%水溶液を作成し、室温迄冷却した
。Separately, add 2 g of alkali-treated gelatin [manufactured by Miyagi Chemical, jelly strength 250 Plume] to 198 g of water, and add 50 g of gelatin to 198 g of water.
A 1% aqueous solution was prepared by heating and dissolving at °C, and the mixture was cooled to room temperature.
500コピーカー中に該ゼラチン水溶液を移しこれに該
塩化メチレン溶液を加え5(mの櫂型攪拌羽根を用いて
500 rpmで攪拌、乳化したのち、減圧上塩化メチ
レンを蒸発させ、塩化メチレン臭が完全に消失したこと
を確認してマイクロスフイア化を終えた。上層の若干の
凝集物を除去したのち濾過し、蒸留水で水洗したのち室
温で減圧乾燥して粒子径180〜200μの白色球状の
マイクロスフイア2.Ogを得た。The aqueous gelatin solution was transferred to a 500-meter copy car, and the methylene chloride solution was added thereto, stirred at 500 rpm using a 5-meter paddle-type stirring blade, and emulsified. After confirming that it had completely disappeared, microsphere formation was completed. After removing some aggregates in the upper layer, it was filtered, washed with distilled water, and dried under reduced pressure at room temperature to form white spherical particles with a particle size of 180 to 200μ. Microspheres of 2.0 g were obtained.
得られたマイクロスフイアは、溶剤抽出を行ってプレオ
マイシンを完全に単離し、290 nmにおける吸光度
測定による定量分析の結果、マイクロスフイア中のプレ
オマイシンの含有率は15.1%であった。The obtained microspheres were subjected to solvent extraction to completely isolate pleomycin, and as a result of quantitative analysis by absorbance measurement at 290 nm, the content of pleomycin in the microspheres was 15.1%. .
試験例−1
実施例−1で得られたプレオマインン15.1%含有の
マイクロスフイア100m9を5Qmlの生理食塩水に
入れ、各測定時に直接1〜3 mlサンプリングして2
90 nmにおける吸光度を測定した。同時に実施例−
1と全く同じ条件下で、添加剤IPMを全く加えない場
合得られたマイクロスフイアの生理食塩水中の290
nmにおける吸光度も比較試験として測定した。Test Example-1 100 m9 of microspheres containing 15.1% pleomine obtained in Example-1 were placed in 5 Q ml of physiological saline, and 1 to 3 ml was directly sampled at each measurement time.
Absorbance was measured at 90 nm. Example at the same time
290 in saline of microspheres obtained under exactly the same conditions as in 1 without adding any additive IPM.
The absorbance at nm was also measured as a comparative test.
これらの吸光度より計算して第1図のような経過時間と
放出率との関係を得た。By calculating from these absorbances, the relationship between elapsed time and release rate as shown in FIG. 1 was obtained.
実施例−2、及び試験例−2
固有粘度0.88を有するポリ−d 、 l−乳酸を用
いた以外は、実施例−1と全く同じ方法でプレオマイシ
ン含有のマイクロスフイアを得た。マイクロスフイア中
のプレオマイシン含有量は16.0%であった。Example 2 and Test Example 2 Pleomycin-containing microspheres were obtained in exactly the same manner as in Example 1, except that poly-d,l-lactic acid having an intrinsic viscosity of 0.88 was used. Pleomycin content in the microspheres was 16.0%.
得られたマイクロスフイア製剤を試験例−1と同様な方
法でin vitro放出試験を行い、第2図のような
結果を得た。The obtained microsphere preparation was subjected to an in vitro release test in the same manner as in Test Example 1, and the results shown in FIG. 2 were obtained.
第1および2図は、本発明の実施例の製剤の1nvi
tro放出試験における経過時間と薬物放出率との関係
を、IPMを含まない製剤の場合と比較したちのである
。
△:実施例の製剤の場合
○:IPMを含まない製剤の場合
特許出願人 三井東圧化学株式会社
第1図
時開(!our)Figures 1 and 2 show 1nvi of formulations of examples of the invention.
The relationship between elapsed time and drug release rate in the tro release test was compared with that of a formulation without IPM. △: In the case of the formulation of the example ○: In the case of the formulation that does not contain IPM Patent applicant Mitsui Toatsu Chemical Co., Ltd. Figure 1 Jikai (!our)
Claims (3)
ポリ乳酸を溶解する有機溶媒に溶け、しかも生体内で消
化されうる脂溶性の添加物、及び薬物よりなる顆粒状に
調製された徐放性製剤。(1) A biodegradable polymer mainly made of polylactic acid,
A sustained release preparation prepared in the form of granules, comprising a drug and a fat-soluble additive that is soluble in an organic solvent that dissolves polylactic acid and can be digested in vivo.
の範囲第1項記載の製剤。(2) The preparation according to claim 1, wherein the fat-soluble additive is a fatty acid ester.
の製剤。(3) The preparation according to claim 1, wherein the drug is an anticancer drug.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP18367184A JPS6163613A (en) | 1984-09-04 | 1984-09-04 | Sustained release preparation |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP18367184A JPS6163613A (en) | 1984-09-04 | 1984-09-04 | Sustained release preparation |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| JPS6163613A true JPS6163613A (en) | 1986-04-01 |
Family
ID=16139887
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| JP18367184A Pending JPS6163613A (en) | 1984-09-04 | 1984-09-04 | Sustained release preparation |
Country Status (1)
| Country | Link |
|---|---|
| JP (1) | JPS6163613A (en) |
Cited By (12)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US4853226A (en) * | 1986-10-07 | 1989-08-01 | Chugai Seiyaku Kabushiki Kaisha | Sustained-release particulate preparation and process for preparing the same |
| WO1991009612A1 (en) * | 1989-12-25 | 1991-07-11 | Koken Co., Ltd. | Tumor cell growth inhibitor |
| JPH0474117A (en) * | 1990-07-16 | 1992-03-09 | Kokuritsu Eisei Shikenjo | New microsphere |
| WO1998024427A3 (en) * | 1996-12-02 | 1998-10-01 | Angiotech Pharm Inc | Compositions and methods for treating or preventing inflammatory diseases |
| US6287587B2 (en) | 1997-07-15 | 2001-09-11 | Takeda Chemical Industries, Ltd. | Process for producing sustained-release preparation by in-water drying |
| WO2001080835A1 (en) * | 2000-04-24 | 2001-11-01 | Tanabe Seiyaku Co., Ltd. | Process for producing microsphere |
| US6495579B1 (en) | 1996-12-02 | 2002-12-17 | Angiotech Pharmaceuticals, Inc. | Method for treating multiple sclerosis |
| US7527809B2 (en) | 2003-05-02 | 2009-05-05 | Canon Kabushiki Kaisha | Polyhydroxyalkanoate-containing magnetic structure, and manufacturing method and use thereof |
| US7615233B2 (en) | 2001-07-10 | 2009-11-10 | Canon Kabushiki Kaisha | Particulate construct comprising polyhydroxyalkanoate and method for producing it |
| US8795726B2 (en) | 2010-01-19 | 2014-08-05 | Polypid Ltd. | Sustained-release nucleic acid matrix compositions |
| US8877242B2 (en) | 2008-07-14 | 2014-11-04 | Polypid Ltd. | Sustained-release drug carrier composition |
| US8992979B2 (en) | 2009-07-14 | 2015-03-31 | Polypid Ltd. | Sustained-release drug carrier composition |
-
1984
- 1984-09-04 JP JP18367184A patent/JPS6163613A/en active Pending
Cited By (19)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US4853226A (en) * | 1986-10-07 | 1989-08-01 | Chugai Seiyaku Kabushiki Kaisha | Sustained-release particulate preparation and process for preparing the same |
| WO1991009612A1 (en) * | 1989-12-25 | 1991-07-11 | Koken Co., Ltd. | Tumor cell growth inhibitor |
| JPH0474117A (en) * | 1990-07-16 | 1992-03-09 | Kokuritsu Eisei Shikenjo | New microsphere |
| US6689803B2 (en) | 1996-12-02 | 2004-02-10 | Angiotech Pharmaceuticals, Inc. | Compositions and methods for treating surgical adhesions |
| WO1998024427A3 (en) * | 1996-12-02 | 1998-10-01 | Angiotech Pharm Inc | Compositions and methods for treating or preventing inflammatory diseases |
| EP1090637A3 (en) * | 1996-12-02 | 2001-09-12 | Angiotech Pharmaceuticals, Inc. | Compositions and methods for treating or preventing inflammatory diseases |
| EP1092433A3 (en) * | 1996-12-02 | 2001-09-12 | Angiotech Pharmaceuticals, Inc. | Compositions and methods for treating or preventing inflammatory diseases |
| EP1070502A3 (en) * | 1996-12-02 | 2001-10-17 | Angiotech Pharmaceuticals, Inc. | Compositions and methods for treating or preventing inflammatory diseases |
| US6495579B1 (en) | 1996-12-02 | 2002-12-17 | Angiotech Pharmaceuticals, Inc. | Method for treating multiple sclerosis |
| US6515016B2 (en) | 1996-12-02 | 2003-02-04 | Angiotech Pharmaceuticals, Inc. | Composition and methods of paclitaxel for treating psoriasis |
| US6287587B2 (en) | 1997-07-15 | 2001-09-11 | Takeda Chemical Industries, Ltd. | Process for producing sustained-release preparation by in-water drying |
| WO2001080835A1 (en) * | 2000-04-24 | 2001-11-01 | Tanabe Seiyaku Co., Ltd. | Process for producing microsphere |
| US7615233B2 (en) | 2001-07-10 | 2009-11-10 | Canon Kabushiki Kaisha | Particulate construct comprising polyhydroxyalkanoate and method for producing it |
| US7527809B2 (en) | 2003-05-02 | 2009-05-05 | Canon Kabushiki Kaisha | Polyhydroxyalkanoate-containing magnetic structure, and manufacturing method and use thereof |
| US8877242B2 (en) | 2008-07-14 | 2014-11-04 | Polypid Ltd. | Sustained-release drug carrier composition |
| US10682412B2 (en) | 2008-07-14 | 2020-06-16 | Polypid Ltd. | Sustained-release drug carrier composition |
| US8992979B2 (en) | 2009-07-14 | 2015-03-31 | Polypid Ltd. | Sustained-release drug carrier composition |
| US8795726B2 (en) | 2010-01-19 | 2014-08-05 | Polypid Ltd. | Sustained-release nucleic acid matrix compositions |
| US9616032B2 (en) | 2010-01-19 | 2017-04-11 | Polypid Ltd. | Sustained-release nucleic acid matrix compositions |
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