TWI566774B - 治療關節疾病的組成物及其方法 - Google Patents
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- TWI566774B TWI566774B TW103134710A TW103134710A TWI566774B TW I566774 B TWI566774 B TW I566774B TW 103134710 A TW103134710 A TW 103134710A TW 103134710 A TW103134710 A TW 103134710A TW I566774 B TWI566774 B TW I566774B
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Description
本發明係關於一種醫藥組成物,尤其是關於一種包含間質幹細胞、透明質酸及醫藥學上可接受之載劑的組成物。
骨關節炎(osteoarthritis,簡稱OA)於老年人口中係為一世界性的健康問題,其影響55至70歲間的超過70%美國人,肇因於慢性外傷或疾病所引起的漸進性軟骨損傷,由於關節軟骨不具有血管且其細胞有絲分裂活性較低,故其修復具有容量限制。
多種病理機制參與骨關節炎的形成,包括細胞外基質(extracellular matrix,以下稱為ECM)的酵素性降解、缺乏新基質形成、細胞死亡、以及軟骨細胞的異常活化及肥大分化(hypertrophic differentiation)。目前業已發展許多治療方法以減輕骨關節炎所引起之疼痛且改善受影響的功能,然而,目前的治療策略,例如:全關節置換術(total joint arthroplasty)仍無法恢復軟骨的天然結構,甚至可能進一步增加關節受損的風險。
目前已開發由骨髓間質幹細胞(bone marrow mesenchymal stem cells,以下稱為BMSC)所製備成的骨和軟骨用於骨關節炎的治療,雖然此種技術是有吸引力的,但骨髓的收穫是痛苦的,特別是在老年人中,產生有限數量的幹細胞。因此,需要延伸擴大培養幹細胞。脂肪衍生的間質幹細胞(adipose-derived mesenchymal stem cells,以下稱為ASC)是目前最好的選擇,由於可大量獲得ASC且其發病率較小,並且可容易在體外擴大培養。除了再生(regeneration)活性外,ASC亦具有免疫抑制特性。近期,已於髕骨下脂肪墊(infra-patellar fat pad,以下稱為IFP)發現具有幹細胞特性的細胞。
ECM提供細胞微環境以維持動態平衡(homeostasis)且分化為特定組織。在ECM中,透明質酸(hyaluronan,簡稱HA)是軟骨間質的糖胺聚多醣(glycosaminoglycan),在軟骨組織中係天然的。其作為關節軟骨基質的主要生理成分,HA在滑液(synovial fluid)中尤其豐富,此聚合物在軟骨之動態平衡中發揮作用,且參與細胞過程,例如:細胞的形態形成(morphogenesis)、增殖和傷口修復。其亦被廣泛用於關節內的關節炎治療。然而,少有報導HA微環境於間質幹細胞(Mesenchymal stem cells,以下稱為MSC)分化上的影響。
本發明提供一種醫藥組成物,其包含間質幹細胞、透明質酸及醫藥上可接受之載劑。
於本發明之一具體實施例中,該組成物係用於治療關節疾病,其中,該關節疾病為關節軟骨缺陷、慢性關節風濕症、變形性關節炎或肩關節周炎者。
於本發明之一具體實施例中,該間質幹細胞係培養至第3至第6繼代。又於一具體實施例中,係包含1.6×107至1×109個間質幹細胞,而該間質幹細胞係選自髕骨下脂肪墊基質細胞、骨髓間質幹細胞、華頓氏膠幹細胞及脂肪衍生幹細胞所組成群組之至少一者。較佳者,該間質幹細胞係為髕骨下脂肪墊基質細胞。
於本發明之一具體實施例中,該間質幹細胞係被誘導產生糖胺聚多糖。
於本發明之一具體實施例中,該透明質酸濃度範圍為25%(v/v)至75%(v/v)。較佳者,該透明質酸濃度範圍為25%(v/v)至50%(v/v)。最佳者,該透明質酸濃度係為25%(v/v)。
本發明進一步提供一種治療關節疾病的方法,其包含以有效量之包含間質幹細胞、透明質酸及醫藥上可接受之載劑之組成物投予至個體之受損關節組織中。
於本發明之一具體實施例中,係以注射方式將本發明之醫藥組成物投予至個體之受損關節組織中。其中,該關節疾病為關節軟骨缺陷、慢性關節風濕症、變形性關節炎或肩關節周炎者。
於本發明之一具體實施例中,該間質幹細胞係培養至第3至第6繼代,而該間質幹細胞之數量係包含1.6×107至1×109個細胞。
於本發明之一具體實施例中,該間質幹細胞係選自髕骨下脂肪墊基質細胞、骨髓間質幹細胞、華頓氏膠幹細胞及脂肪衍生幹細胞所組成群組之至少一者。較佳者,該間質幹細胞係為髕骨下脂肪墊基質細胞。
第1圖係顯示髕骨下脂肪墊基質細胞(IFPSC)之細胞表面標誌;(A)髕骨下脂肪墊基質細胞(IFPSC);(B)骨髓間質幹細胞(BMSC);(C)華頓氏膠幹細胞(WJSC)以及(D)脂肪衍生幹細胞(ASC);第2圖係顯示髕骨下脂肪墊基質細胞(IFPSC)、骨髓間質幹細胞(BMSC)、華頓氏膠幹細胞(WJSC)和自腹部皮下脂肪之脂肪衍生幹細胞(ASC)的生長動力學;第3圖係顯示不同來源之間質幹細胞趨化成為軟骨細胞之條件培養基(conditioned medium,簡稱CM);第4圖係顯示髕骨下脂肪墊基質細胞(IFPSC)之多效分化能力;(A)油紅染色之脂質形成;(B)茜紅素染色之成骨形成;(C)及(D)阿爾辛藍染色之軟骨形成,在(A)及(B)中之比例尺為100μm,在(C)及(D)中之比例尺為1000μm;第5圖係顯示髕骨下脂肪墊基質細胞(IFPSC)較其他幹細胞更具軟骨性;(A)各種間質幹細胞於第14天及第21天之阿爾辛藍染色;(B)在OD595下測量阿爾辛藍染色量;藉由qRT-PCR量測不同誘導天數之(C)SOX9及(D)COL2A1基因之表現量,*P<0.05;第6圖係顯示25%(v/v)透明質酸(HA)增強人類髕骨下
脂肪墊基質細胞(IFPSCs)之脂肪形成、骨形成以及軟骨生成,該IFPSC在不同濃度之HA下分別藉由茜紅素、油紅及阿爾辛藍染色所顯示之脂肪形成、骨形成以及軟骨生成之(A)圖片(B)含量,*P<0.05、**P<0.01及***P<0.001;第7圖係顯示透明質酸(HA)在髕骨下脂肪墊基質細胞(IFPSC)的增殖上無影響,以25%(v/v)、50%(v/v)、75%(v/v)及100%(v/v)之HA培養5天後之IFPSC的(A)圖片(B)不同濃度之HA不影響IFPSC之增殖,比例尺為1000μm。
以下係藉由特定的具體實施例說明本發明之實施方式,熟習此專業之人士可由本說明書所揭示之內容輕易地瞭解本發明之優點及功效。本發明亦可藉由其它不同之實施方式加以施行或應用,本說明書中的各項細節亦可基於不同觀點與應用,在不悖離本發明所揭示之精神下賦予不同之修飾與變更。
除非文中另有說明,否則說明書及所附申請專利範圍中所使用之單數形式「一」及「該」包括複數個體。
除非文中另有說明,否則說明書及所附申請專利範圍中所使用之術語「或」包括「及/或」之含義。
本發明提供一種醫藥組成物,其包含間質幹細胞、透明質酸及醫藥上可接受之載劑。根據本發明之一具體實施例,該組成物係用於治療關節疾病,其中,該關節疾病為關節軟骨缺陷、慢性關節風濕症、變形性關節炎或肩關節周炎者。本發明提出用於治療關節疾病,特定言之用於修
復關節軟骨並促進多種軟骨修復。
根據本發明之一具體實施例,關節軟骨中包含細胞密度範圍從6800到24000細胞/立方毫米(cells/mm3)的軟骨細胞,因此,針對此細胞密度的軟骨再生,估計可能需要1.6×107個細胞以用於修復600mm3區域的軟骨。因此,根據本發明之一具體實施例,製備針對修復軟骨組織的IFPSC時間包括個體髕骨下脂肪墊的切除以及人工處理及分離IFPSC大約需一小時。隨後將該IFPSC培養4至5天以增長至亞匯合(sub-confluence)程度,再經過10天(第3繼代(passage))的培養以擴大至1.6×107個細胞,估計該製劑可在兩週內完成。根據本發明之一具體實施例,較佳者,該間質幹細胞培養至第3至第6繼代時,該間質幹細胞之範圍係介於1.6×107至1×109個細胞之間。最佳者,該間質幹細胞培養至第5繼代時,該間質幹細胞具有1×108個細胞。
根據本發明之一具體實施例,該間質幹細胞係選自髕骨下脂肪墊基質細胞(infra-patellar fat pad stromal cell,以下簡稱IFPSC)、骨髓間質幹細胞(bone marrow stem cell,以下簡稱BMSC)、華頓氏膠幹細胞(Wharton’s jelly stem cell,以下簡稱WJSC)及脂肪衍生幹細胞(adipose derived stem cell,以下簡稱ASC)所組成群組之至少一者。較佳者,該間質幹細胞係為髕骨下脂肪墊基質細胞。
根據本發明之一具體實施例,本發明顯示該IFPSC細胞表面標誌物輪廓(profile)與生長動力學(growth kinetics)是與腹部皮下脂肪之脂肪衍生幹細胞(adipose derived stem
cells,以下簡稱ASC)一致的。CD34和CD45的含量在該IFPSC(9.0%和11.0%)中較高,相較於骨髓幹細胞(bone marrow stem cells,以下簡稱BMSC)分別為0.3%和0.5%。雖然該IFPSC具有大部分ASC的表面標誌物,但在該IFPSC中CD45含量較高(0.4%)。
根據本發明之一具體實施例,在軟骨培養基的存在下,間質幹細胞(包括IFPSC、ASC、BMSC和WJSC)被誘導而產生糖胺聚多糖,該糖胺聚多糖係軟骨組織之細胞外基質的主要成分,並且可以藉由阿爾辛藍染色。相較於其他間質幹細胞(包括ASC、BMSC和WJSC),該IFPSC顯示在軟骨誘導上更顯著的阿爾辛藍染色,且其軟骨細胞基因(例如:SOX9和COL2A1)的表現量較高。
根據本發明之一具體實施例,本發明亦顯示間質幹細胞具有朝向軟骨細胞的趨化活性,指出該間質幹細胞朝向受傷軟骨的潛在導向,由於非關節來源之間質細胞亦表現優良,因此表示此種趨化作用似乎沒有組織特異性。
根據本發明之一具體實施例,捐贈者的年齡不影響間質幹細胞之增殖率、倍增時間(doubling time)、端粒的長度(telomere length)、或成骨及軟骨分化能力。幹細胞在培養至第3至6繼代時具有穩定及可與前驅細胞(progenitor cells)比較之細胞特性,在複製至第10繼代時常會發生細胞衰老。
根據本發明之一具體實施例,不同濃度的透明質酸(hyaluronan,以下稱為HA)對間質幹細胞的增殖無促進作
用。但HA可能對間質幹細胞的軟骨形成具有促進作用。由於HA可作為軟骨組織之天然成分,HA係用於關節中自其前驅細胞的軟骨細胞誘導,且HA對於細胞聚集之細胞-細胞橋接間是必須的。此外,HA亦為圍繞IFP之滑液主成分,因此,滑液中HA可創造微環境,其係在受傷組織修復期間可誘導該間質幹細胞的軟骨分化。於本發明中,HA的濃度係以體積百分比濃度表示之,用於本發明之HA濃度範圍係介於0%(v/v)至100%(v/v),較佳係介於25%(v/v)至75%(v/v),而濃度為25%(v/v)之HA對於軟骨分化具有最佳效果,此表示HA可提供軟骨生長之適宜微環境,且亦增強間質幹細胞之軟骨分化作用。
根據本發明之一具體實施例,本發明將間質幹細胞(包括IFPSC、ASC、BMSC及WJSC)與HA聯合注射於受損之關節組織中顯示具有較佳之軟骨形成效果。
根據本發明之一具體實施例,含有間質幹細胞、透明質酸及醫藥學上可接受之載劑的組成物中,舉例而言,用於固體形式之組成物時,醫藥學上可接受之載劑可包括黏結劑、潤滑劑、崩散劑、賦形劑、增溶劑、分散劑、安定劑、懸浮劑、著色劑及香料;用於液體形式之組成物時,醫藥學上可接受之載劑可包括緩衝劑、保藏劑、止痛劑、增溶劑、等張劑及安定劑。
在本發明之一具體實施例中,HA亦增強ASC之軟骨分化作用,在濃度為25%(v/v)之HA中,IFPSC之軟骨形成效果係大於ASC。
髕骨下脂肪墊(以下稱為IFP)和關節軟骨組織的取得
自成年男性進行關節鏡以單離出初代人類關節軟骨片段,獲得佛教慈濟綜合醫院的研究倫理委員會批准,並從參與者獲得知情同意後,於全膝關節置換手術獲得IFPs,且同時獲得其他來源幹細胞(BMSC、ASC和WJSC)。IFPs的體積大約是2×2×2立方厘米(cm3)。患者(n=2,皆女性)年齡皆大於60歲(分別為65歲和68歲)。
本文中之結果以平均值±標準差表示。學生t-檢驗(Student’s t-test)係用於評估控制組和實驗組間的平均差異。P<0.05的數值被認為是統計學上顯著的。藉由使用多重比較的曼-惠特尼U檢驗(Mann-Whitney U test)比較IFPSC與其他三種不同來源幹細胞的增殖率。
該所得的IFPs進行了一系列以磷酸鹽緩衝鹽食鹽水洗滌(PBS,Biowest,Nuaille,法國),並在37℃下以0.1毫克/毫升(mg/ml)膠原酶Ia分解60分鐘(Sigma公司,聖路易斯,密蘇里州,美國)。酵素消化後,收集所得細胞並培養於含有5%胎牛血清(以下稱為FBS)(Biological Industry,Kibbutz,Israel)、N-乙醯半胱氨酸(NAC)及L-抗壞血酸2-磷酸酯(Sigma-Aldrich公司,聖路易斯,密蘇里州,美國)之角質形成細胞的無血清培養基(KSFM,Gibco公司,Grand island,NY,USA)。於培養的第二天移除培
養皿中的上清液及碎片,將所得IFPSC培養物標記為第0代。為了防止自發性的分化,將該培養物維持在亞匯合(sub-confluent)的程度(小於80%的匯合)。使用2.5%胰蛋白酶/0.23毫摩耳(mM)EDTA(Gibco,Grand island,NY,USA)進行繼代培養。在96孔培養皿中,以細胞密度大約2000cell/cm2於第0、3及7天進行XTT細胞增殖測定(Roche,Mannheim,Germany)。
由佛教慈濟綜合醫院之骨髓庫提供BMSC(N=1),以補充有10% FBS(Biological Industry,Kibbutz,Israel)之α-MEM培養基(Gibco,Grand Island,NY,USA)培養BMSC。
ASC係衍生自接受婦科手術患者(N=1,女性,60歲)的皮下組織,將人體脂肪組織切成小塊(1至2立方毫米(mm3)),以0.1毫克(mg)膠原酶Ia(Sigma,St.Louis,MO,USA)分解,且於37℃下培養60分鐘,收集所得細胞並培養於含有5% FBS、NAC及L-抗壞血酸2-磷酸酯之KSFM培養基中(添加表皮生長因子和牛垂體萃取物,Gibco,17005-042,Grand island,NY,USA)。於培養第2天,自培養皿移除上清液和碎片。為了防止自發性的分化,將培養物維持在亞匯合的程度(小於80%匯合)。
將所收集的人類臍帶組織(n=1)藉由剪刀在中線方向進行機械切割,該臍動脈、靜脈及概述膜(outlining membranes)的血管分離自華頓氏膠,然後將該膠體切割成
小於0.5cm3的片段,以膠原酶第1型(Sigma,St.Louis,MO,USA)處理,且於95%空氣/5% CO2的潮濕環境中,37℃下培養14至18小時。然後,於95%空氣/5% CO2的潮濕環境中,在37℃下,將該外植體(explants)培養於含有10% FBS和抗生素的DMEM培養基中(Gibco,Grand Island,NY,USA),隨後,將該外植體靜置5至7天,該WJSC自外植體遷移出。
藉由流式細胞儀定性第三或第四繼代培養之IFPSC和BMSC的表面分子。以含有2mM EDTA之PBS分離細胞、以含有2%牛血清白蛋白和0.1%疊氮化鈉(Sigma,St.Louis,MO,USA)的PBS洗滌,並分別與異硫氰酸熒光素(fluorescein isothiocyanate)或藻紅素(phycoerythrin)共軛之抗體,包括CD29、CD34、CD44、CD45、CD73、CD90、HLA-ABC和HLA-DR(BD,PharMingen)培養。此後,使用Becton Dickinson公司之流式細胞儀(Becton Dickinson,San Jose,CA,USA)分析該細胞。
實施例1至3之結果顯示該IFPSC具有類似脂肪衍生幹細胞表現型。如第1圖所示,在培養至繼代第3代,該衍生IFPSC具有高度同質化的類纖維細胞外觀,且容易在培養14天中達到匯合,類似MSCs,該IFPSC表現CD29、CD44、CD73、CD90和HLA-ABC的表面標誌物。然而,如第1圖所示,與BMSC不同,該IFPSC表現較高含量之CD34及CD45。如第1圖及表1所示,相較於BMSC、WJSC及
ASC,該IFPSC具有類似於ASC且不同於BMSC之細胞表面標誌物。如第2圖所示,將於第0天、第3天及第7天觀察IFPSC、BMSC、WJSC及ASC之細胞數,於培養至第7天,該IFPSC之生長動力學明顯優於ASC、BMSC及WJSC(P<0.05)。
將軟骨碎片切碎成1mm3,並以第2型膠原酶(0.1%,Worthington,Lakewood,NJ,USA)溶液於37℃水解過夜,然後將所水解的內容物通過100μm(微米)的過濾器過濾且以PBS洗滌,然後將該分離的軟骨細胞以每5000cells/cm2接
種,並生長在含有2mM L-麩醯胺酸、10% FBS(Gibco)、1×青黴素/鏈黴素、50μg/mL的去抗壞血酸及0.1M非必須胺基酸(Gibco,Invitrogen,Grand Island,NY,USA)的DMEM/F12(Gibco)中生長至匯合。藉由進一步培養在補充10% FBS及1%青黴素/鏈黴素之高葡萄糖DMEM(Gibco)培養軟骨細胞來收集軟骨細胞條件培養基(chondrocyte-conditioned medium)48小時。
將該IFPSC、BMSC、ASC、及WJSC接種於24孔通透Boyden腔室之上層孔中(8μm孔徑;Costar,Corning Inc.,Corning,NY,USA),且使其轉移至置於底層孔之衍生自軟骨細胞的無細胞培養基中,測試遷移48小時後,將該遷移之細胞以結晶紫染色(Sigma-Aldrich,St Louis,MO,USA),使用亮視野顯微鏡(bright field microscopy)計數。
實施例4結果顯示該IFPSC趨化成為軟骨細胞。如第3圖所示,在控制組培養基中,該IFPSC的基本遷移活性是類似於ASC和WJSC但小於BMSC。包括IFPSC的所有細胞皆是高度趨向軟骨細胞的條件培養基。儘管如此,該IFPSC具有高於控制組培養基2.95倍之遷移率。
以密度為每孔5×104細胞,將該IFPSC接種於12孔盤之脂質培養基(補充有10% FBS、1μmol/L的地塞米松(dexamethasone)(Sigma-Aldrich,St.Louis,MO,USA)、5μg/mL的胰島素(Sigma-Aldrich,St.Louis,MO,USA)、0.5
mmol/L的異丁基甲基黃嘌呤(Sigma-Aldrich,St.Louis,MO,USA)以及60μmol/L的吲哚美辛(indomethacin)(Sigma-Aldrich,St.Louis,MO,USA)之DMEM)。然後,使該等IFPSC生長7天,每3天更換培養基,然後以油紅(oil red)(Sigma-Aldrich,St.Louis,MO,USA)染色,以PBS洗滌兩次後,以1ml 100%異丙醇(Sigma-Aldrich,St.Louis,MO,USA)萃取樣品中脂質,並輕輕搖動5分鐘。根據在510nm處吸光度測量脂質濃度,各樣品中的脂質含量以三重複測量。
以密度為每孔1×104細胞,將該IFPSC接種於12孔盤中,且以成骨培養基培養(補充有10% FBS之DMEM、0.1μmol/L的地塞米松、10mmol/L β-甘油磷酸鹽(Sigma-Aldrich,St.Louis,MO,USA)及50μmol/L的抗壞血酸(Sigma-Aldrich,St.Louis,MO,USA)),且每三天更換一次。使細胞生長21天,然後以茜素紅(Alizarin Red)(Sigma-Aldrich,St.Louis,MO,USA)染色。對於染色的定量,將800μL 10%(V/V)之醋酸(Baker,Phillipsburg,NJ,USA)加入至各孔中,並將該盤於室溫下震盪培養30分鐘。然後以細胞刮刀(Corning Inc.,Corning,NY,USA)自該盤刮取單層細胞(係鬆散地附著在該盤上),並以10%(V/V)醋酸轉移至1.5mL具有寬口吸管之微離心管。
於渦動(vortex)30秒後,將漿液以500μL礦物油(Sigma-Aldrich,St.Louis,MO,USA)覆蓋,加熱至恰好85℃保持10分鐘,並轉移至冰上5分鐘。然後將漿液於
20,000g離心15分鐘,將500μL的上清液轉移到新的1.5mL微量離心管(Scientific Specialties Inc.,Lodi,CA,USA)。然後,將200μL之10%(V/V)氫氧化銨(Baker,Phillipsburg,NJ,USA)加入以中和酸。將等分試樣的上清液(150μL)於使用不透明壁、透明底盤之96孔型式(Costar,Corning Inc.,Corning,NY,USA)中,於405nm下以三重複讀取。
以密度為每孔1×105cells/cm2,將該IFPSC、ASC、BMSC及WJSC接種於12孔盤中,且以成骨培養基培養,該成骨培養基包含DMEM、10% FBS、10ng/mL TGF-β1(Pepro Tech Inc.,Rocky Hill,NJ,USA)、50μg/mL的抗壞血酸-2-磷酸鹽(Sigma-Aldrich,St.Louis,MO,USA)以及6.25μg/mL的胰島素(Sigma-Aldrich,St.Louis,MO,USA),每三天更換一次培養基。將該細胞以軟骨細胞培養基在37℃、5% CO2培養三星期。於固定在多聚甲醛(para-formaldehyde)後(Bionovas,Toronto,Canada),將細胞固定在載玻片上,並使用標準的阿爾辛藍(Alcian Blue)(Fluka,Sigma-Aldrich Chemie GmbH,Buchs,Switzerland)方案染色。對於阿爾辛藍摻入豐富蛋白多醣的細胞外基質的定量分析,將培養物以6M胍鹽酸鹽(Sigma-Aldrich,St.Louis,MO,USA)培養過夜,並在595nm的光密度下進行光度測量。
實施例5結果顯示該IFPSC可分化成脂肪、骨和軟骨細胞。在培養基中之分化誘導上,該IFPSC容易地分化為脂肪、骨、軟骨譜系。如第4圖A及4圖B所示,藉由在形成脂肪及形成骨條件培養基中14天後誘導,該經分離之
IFPSC顯示在細胞質中具有大、油紅呈陽性之脂質液滴,且以茜素紅染色後呈現細胞形態為長方體形狀的變化。如第4圖C及4圖D所示,藉由21天之軟骨形成誘導,該IFPSC顯示以阿爾辛藍染色後的細胞聚集現象。
依據製造商的說明,使用RNeasy ®(Qiagen)萃取總RNA。進行SOX9和COL2A1基因(引子及降溫溫度列於表2)的即時PCR分析。使用SuperScript III One-Step RT-PCR套組(Invitrogen,Grand Island,NY,USA)合成互補DNA,且以AmpliTaq黃金套組(Applied Biosystems,Foster City,CA,USA)擴增,使用FastStart universal SYBR green master(ROX,Roche,Indianapolis,IN,USA)及定量即時PCR檢測系統(ABI Step One Plus system,Applied Biosystems,Foster City,CA,USA)進行及監測即時PCR,以GAPDH基因作為參考基因分析該基因產物,然後以2△△Ct計算各目標基因的表現量,針對各目標基因進行各實驗樣品的四個讀數,且該實驗重複至少三次。
實施例6結果顯示該IFPSC較衍生自其他位置之間質幹細胞(例如:BMSC、ASC及WJSC)更具軟骨性。如第5圖A至第5圖B所示,在軟骨分化的誘導上,在第21天,相較於經誘導之BMSC、ASC及WJSC,該經誘導之IFPSC表現較大量之糖胺聚多醣。如第5圖C至第5圖D所示,該IFPSC逐步表現軟骨性基因,例如:SOX9和COL2A1,反之,此兩基因在ASC及WJSC上表現較少,或在BMSC的不同誘導期間具有不一致的表現。
將不同含量透明質酸溶解於培養基後所製備之透明質酸溶液(分子量5000至10000kDa,20mg/2mL,Suplasyn,BIONICHE,Galway,愛爾蘭)加入至12孔盤中,最終濃度(V/V)為25%、50%、75%和100%,並使其在室內空氣中固化。將該IFPSC以5000個細胞的密度接種於含有5% FBS、NAC及L-抗壞血酸-2-磷酸鹽之100μL KSFM中,每2天更換培養基維持14天,收集該細胞以用於在不同時間點進一步的分化和增殖分析。
實施例7結果顯示HA之微環境增強IFPSC的分化但對其生長呈中性。在不同濃度下,將HA塗佈在培養盤中,
並測試HA對IFPSC的分化和生長的影響。除了75%(v/v)之HA塗佈的培養之外,此顯示較差的分化能力,無論是培養在25%(v/v)或50%(v/v)HA之IFPSC具有增強之成骨、成脂和軟骨分化。如第6圖A及B所示,針對軟骨形成,相較於無HA的培養上,培養在25%(v/v)HA之IFPSC顯示具有2至3倍增加的分化能力。再者,如第7圖A及B所示,以濃度範圍為25%(v/v)至75%(v/v)之HA塗佈培養不影響IFPSC的增殖。
Claims (11)
- 一種醫藥組成物,其包含間質幹細胞、透明質酸及醫藥上可接受之載劑,其中,係包含1.6×107至1×109個該間質幹細胞,該透明質酸濃度範圍為25%(v/v)至75%(v/v),該間質幹細胞係髕骨下脂肪墊基質細胞。
- 如申請專利範圍第1項所述之組成物,其係用於治療關節疾病。
- 如申請專利範圍第2項所述之組成物,其中,該關節疾病為關節軟骨缺陷、慢性關節風濕症、變形性關節炎或肩關節周炎者。
- 如申請專利範圍第1項所述之組成物,其中,該間質幹細胞係培養至第3至第6繼代。
- 如申請專利範圍第1項所述之組成物,其中,該間質幹細胞係被誘導產生糖胺聚多糖。
- 如申請專利範圍第1項所述之組成物,其中,該透明質酸濃度範圍為25%(v/v)至50%(v/v)。
- 如申請專利範圍第6項所述之組成物,其中,該透明質酸濃度係為25%(v/v)。
- 一種申請專利範圍第1至7項任一項所述之組成物之用途,係用於製備治療關節疾病的藥物。
- 如申請專利範圍第8項所述之用途,其中,該投予方式係為注射。
- 如申請專利範圍第8項所述之用途,其中,該關節疾病為關節軟骨缺陷、慢性關節風濕症、變形性關節炎 或肩關節周炎者。
- 如申請專利範圍第8項所述之用途,其中,該間質幹細胞係培養至第3至第6繼代。
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US20200261508A1 (en) | 2020-08-20 |
JP2016074648A (ja) | 2016-05-12 |
JP5960777B2 (ja) | 2016-08-02 |
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