中华实验眼科杂志
中華實驗眼科雜誌
중화실험안과잡지
CHINESE JOURNAL OF EXPERIMENTAL OPHTHALMOLOGY
2014年
7期
583-587
,共5页
孟倩丽%杨培增%郭海科%崔颖
孟倩麗%楊培增%郭海科%崔穎
맹천려%양배증%곽해과%최영
树突状细胞%巨噬细胞%抗原递呈%表型特征%葡萄膜%组织分布%荧光抗体技术%激光扫描共焦显微镜
樹突狀細胞%巨噬細胞%抗原遞呈%錶型特徵%葡萄膜%組織分佈%熒光抗體技術%激光掃描共焦顯微鏡
수돌상세포%거서세포%항원체정%표형특정%포도막%조직분포%형광항체기술%격광소묘공초현미경
Dendritic cell%Macrophage%Antigen presentation%Phenotype character%Uvea%Tissue distribution%Fluorescent antibody technique%Laser confocal microscope
背景 以往对组织中抗原递呈细胞(APCs)的研究多采用体外免疫组织化学的方法,其结果易受到多种因素的影响,曾有研究者采用前房注射荧光素标记抗体的方法对眼前节组织中的APCs进行研究,但易损伤角膜等组织.采用活体标记的方法探讨虹膜和睫状体中APCs的表型特征,对进一步阐明APCs在维持眼部免疫平衡状态中的作用及机制具有重要意义. 目的 探讨正常小鼠虹膜中APCs的表型特征、分布和形态学特点.方法 6~8周龄的SPF级雌性BALB/c小鼠51只按照随机数字表法分为17个组,在生物解剖显微镜下用玻璃微量注射针于角巩膜缘后0.5 mm处刺入玻璃体腔内注射2.0 μl AlexaFluor594或Alexa Fluor 488标记的卵清蛋白(OVA)、抗CD11c、主要组织相容性复合体分子Ⅱ(MHC-Ⅱ)、F4/80、B7-1和B7-2单克隆抗体或其两两抗体的混合液,注射24 h后取小鼠虹膜组织,结合平片技术和激光扫描共焦显微镜观察虹膜中APCs的表型特征、分布及形态学特点,并用体外染色实验验证体内染色结果. 结果 正常小鼠虹膜中存在大量呈规则网络状分布的OVA+、F4/80+、CD11c+、MHC-Ⅱ+、B7-1+和B7-2+细胞,Alexa Fluor 594标记的阳性细胞呈红色荧光,Alexa Fluor 488标记的阳性细胞呈绿色荧光.双重染色实验结果可见,虹膜中约有90%的F4/80+细胞为OVA+,约有60%的F4/80+细胞和CD11c+细胞表达MHC-Ⅱ,约有35%的F4/80+细胞和CD11c+细胞同时表达B7-1和B7-2,70%以上的OVA+细胞为MHC-Ⅱ+.根据标记细胞的形态不同可分为树突状细胞(DC)和多形性细胞两大类.结论 活体玻璃体腔内注射荧光素标记抗体的方法可以准确观察正常小鼠虹膜中的APCs.虹膜中APCs的表型特征、分布和形态学特点与眼免疫偏离和炎症密切相关.
揹景 以往對組織中抗原遞呈細胞(APCs)的研究多採用體外免疫組織化學的方法,其結果易受到多種因素的影響,曾有研究者採用前房註射熒光素標記抗體的方法對眼前節組織中的APCs進行研究,但易損傷角膜等組織.採用活體標記的方法探討虹膜和睫狀體中APCs的錶型特徵,對進一步闡明APCs在維持眼部免疫平衡狀態中的作用及機製具有重要意義. 目的 探討正常小鼠虹膜中APCs的錶型特徵、分佈和形態學特點.方法 6~8週齡的SPF級雌性BALB/c小鼠51隻按照隨機數字錶法分為17箇組,在生物解剖顯微鏡下用玻璃微量註射針于角鞏膜緣後0.5 mm處刺入玻璃體腔內註射2.0 μl AlexaFluor594或Alexa Fluor 488標記的卵清蛋白(OVA)、抗CD11c、主要組織相容性複閤體分子Ⅱ(MHC-Ⅱ)、F4/80、B7-1和B7-2單剋隆抗體或其兩兩抗體的混閤液,註射24 h後取小鼠虹膜組織,結閤平片技術和激光掃描共焦顯微鏡觀察虹膜中APCs的錶型特徵、分佈及形態學特點,併用體外染色實驗驗證體內染色結果. 結果 正常小鼠虹膜中存在大量呈規則網絡狀分佈的OVA+、F4/80+、CD11c+、MHC-Ⅱ+、B7-1+和B7-2+細胞,Alexa Fluor 594標記的暘性細胞呈紅色熒光,Alexa Fluor 488標記的暘性細胞呈綠色熒光.雙重染色實驗結果可見,虹膜中約有90%的F4/80+細胞為OVA+,約有60%的F4/80+細胞和CD11c+細胞錶達MHC-Ⅱ,約有35%的F4/80+細胞和CD11c+細胞同時錶達B7-1和B7-2,70%以上的OVA+細胞為MHC-Ⅱ+.根據標記細胞的形態不同可分為樹突狀細胞(DC)和多形性細胞兩大類.結論 活體玻璃體腔內註射熒光素標記抗體的方法可以準確觀察正常小鼠虹膜中的APCs.虹膜中APCs的錶型特徵、分佈和形態學特點與眼免疫偏離和炎癥密切相關.
배경 이왕대조직중항원체정세포(APCs)적연구다채용체외면역조직화학적방법,기결과역수도다충인소적영향,증유연구자채용전방주사형광소표기항체적방법대안전절조직중적APCs진행연구,단역손상각막등조직.채용활체표기적방법탐토홍막화첩상체중APCs적표형특정,대진일보천명APCs재유지안부면역평형상태중적작용급궤제구유중요의의. 목적 탐토정상소서홍막중APCs적표형특정、분포화형태학특점.방법 6~8주령적SPF급자성BALB/c소서51지안조수궤수자표법분위17개조,재생물해부현미경하용파리미량주사침우각공막연후0.5 mm처자입파리체강내주사2.0 μl AlexaFluor594혹Alexa Fluor 488표기적란청단백(OVA)、항CD11c、주요조직상용성복합체분자Ⅱ(MHC-Ⅱ)、F4/80、B7-1화B7-2단극륭항체혹기량량항체적혼합액,주사24 h후취소서홍막조직,결합평편기술화격광소묘공초현미경관찰홍막중APCs적표형특정、분포급형태학특점,병용체외염색실험험증체내염색결과. 결과 정상소서홍막중존재대량정규칙망락상분포적OVA+、F4/80+、CD11c+、MHC-Ⅱ+、B7-1+화B7-2+세포,Alexa Fluor 594표기적양성세포정홍색형광,Alexa Fluor 488표기적양성세포정록색형광.쌍중염색실험결과가견,홍막중약유90%적F4/80+세포위OVA+,약유60%적F4/80+세포화CD11c+세포표체MHC-Ⅱ,약유35%적F4/80+세포화CD11c+세포동시표체B7-1화B7-2,70%이상적OVA+세포위MHC-Ⅱ+.근거표기세포적형태불동가분위수돌상세포(DC)화다형성세포량대류.결론 활체파리체강내주사형광소표기항체적방법가이준학관찰정상소서홍막중적APCs.홍막중APCs적표형특정、분포화형태학특점여안면역편리화염증밀절상관.
Background The conventional study of antigen-presenting cells(APCs)in eye relies on in vitro histoimmunochemistry,but its outcome is influenced by many factors.The anterior chamber injection of fluoresceinmarked antibody was used as a new approach before,however,it is liable to lead to injury of cornea.The intravitreal injection of fluorescein-labeled antibody may be important for the in vivo study of the phenotype features of APCs in iris,which is significant for evaluating the function of APCs in immune homeostasis.Objective This study was to investigate the phenotype characters,distribution and morphology of different types of APCs in the normal murine iris.Methods Fifty-one SPF female BALB/c mice(from 6-to 8-week old)were randomized into 17 groups according to the injection of different antibodies.Alexa Fluor 594 or Alexa Fluor 488-tagged ovalbumin (OVA),CD11 c,major histocompatibility complex Ⅱ (MHC-Ⅱ),F4/80,B7-1 and B7-2 monoclonal antibodies or mixtures of two antibodies (2.0 μl)were intravitreally injected at 0.5 mm far from corneal limbus with microneedle under the biomicroscope.The iris tissues were isolated 24 hours after injection.The phenotype characters,precise distribution and morphology of different types of APCs were identified by epifluorescence microscope and laser confocal microscope.In vitro staining was also performed to validate the in vivo staining results.Results After in vivo staining via intravitreal injection,the cell positive for OVA as well as MHC-Ⅱ,F4/80,CD11 c,B7-1 and B7-2 were exhibited with the regular networkline appearance throughout the normal murine iris.Positive cells tagged with Alexa Fluor 594 or Alexa Fluor 488 presented the red or green fluorescence.Double-fluorescein staining showed that about 90% of F4/80+ cells were OVA+,and MHC-Ⅱ was expressed in about 60% of F4/80+ cells and CD11c+cells,and about 35% of F4/80+ cells and CD1 1 c+ cells expressed B7-1 and B7-2 simultaneously,and over 70% of OVA+ cells were positive to MHC-Ⅱ.These labeled cells were identified as two populations based on their shape.One type was dendritiform cell (DC) with a small cell body and many long dendrites,including OVA+,CD1 1 c+,F4/80+ cells and MHC-Ⅱ + cells ; and the other types were polymorphic population being round,pleomorphic or irregular shape with a large cell body and a few short dendrities,including B7-1 + and B7-2+ cells.Conclusions In vivo intravitreal injection of labeled antibodies can be adapted to visualize the labeled cells in the murine iris.APCs with distinct morphologies,phenotypes and distribution may contribute to the immunologically privileged feature and inflammation of the eye.
