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悬浮状态下的滤泡树突状细胞:鉴定、富集及初步表征,显示其具有免疫复合物捕获能力且缺乏黏附及吞噬活性

Follicular dendritic cells in suspension: identification, enrichment, and initial characterization indicating immune complex trapping and lack of adherence and phagocytic activity.

作者信息

Schnizlein C T, Kosco M H, Szakal A K, Tew J G

出版信息

J Immunol. 1985 Mar;134(3):1360-8.

PMID:3968423
Abstract

Antigen-retaining follicular dendritic cells (FDC) have been identified and studied in sections of lymph nodes and spleen, but studies of these cells in culture have been extremely limited. The purpose of this study was to establish techniques to release these fragile cells from mouse lymph nodes in a viable state and to identify these cells routinely in lymph node cell suspensions. FDC were obtained from passively or actively immunized popliteal lymph nodes of mice injected in the footpads with 125I-labeled human serum albumin (HSA) or horseradish peroxidase (HRP). Lymph nodes were removed 1 hr after the footpads had been injected with collagenase. After another hour of incubation in vitro with collagenase, protease, and deoxyribonuclease, FDC were released by gentle teasing and enriched by centrifugation on a low density bovine serum albumin (BSA) or Percoll gradient. Most FDC with the associated radiolabel floated at densities greater than 1.06 g/ml on BSA or Percoll gradients. Slides of the FDC-enriched fraction were prepared, using a cytobucket which allowed the cells to be affixed to glass slides by centrifugation in a less disruptive manner than by cytocentrifugation. FDC that were air-dried and fixed with 3% glutaraldehyde had a characteristic pink acidophilic cytoplasm after Wright's staining, and had a faintly basophilic euchromatic nucleus frequently with peripherally-clumped chromatin. In addition, these cells were large and irregularly shaped (up to 60 micron long). Fixation of FDC with 0.6% paraformaldehyde/ 0.9% glutaraldehyde on poly-L-lysine-coated slides resulted in a preservation of FDC which made possible visualization of long dendritic processes by Nomarski optics. Antigen presence on the cell surface was confirmed by autoradiography and, in the case of HRP, was also visualized enzymatically using diaminobenzidine. In contrast to resident peritoneal macrophages or some contaminating lymph node macrophages present on the same slides, FDC did not phagocytize opsonized sheep red blood cells (SRBC) or adhere to plastic surfaces although they did form rosettes with opsonized SRBC. Cell marker studies indicated FDC have a distinctive phenotype. They were positive for Ia, Fc receptor, and leukocyte common antigen, but negative for Thy-1, Ly-1, Ly-2, endogenous Ig, Mac-1, Mac-2, Mac-3, and F4/80, and negative to weakly positive for nonspecific esterase. Cultured FDC remained viable and retained radiolabeled antigen-antibody complexes on their surfaces and were significantly enriched for FDC.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

抗原保留滤泡树突状细胞(FDC)已在淋巴结和脾脏切片中得到鉴定和研究,但对这些细胞进行培养的研究极为有限。本研究的目的是建立从小鼠淋巴结中以活态释放这些脆弱细胞的技术,并在淋巴结细胞悬液中常规鉴定这些细胞。FDC取自经足垫注射125I标记的人血清白蛋白(HSA)或辣根过氧化物酶(HRP)的被动或主动免疫的小鼠腘窝淋巴结。在足垫注射胶原酶1小时后取出淋巴结。在体外与胶原酶、蛋白酶和脱氧核糖核酸酶再孵育1小时后,通过轻柔拨弄释放FDC,并通过在低密度牛血清白蛋白(BSA)或Percoll梯度上离心进行富集。大多数带有相关放射性标记的FDC在BSA或Percoll梯度上漂浮在密度大于1.06 g/ml处。制备富含FDC部分的玻片,使用细胞桶,通过离心使细胞以比细胞离心更不易破坏的方式附着在玻片上。经空气干燥并用3%戊二醛固定的FDC在瑞氏染色后具有特征性的粉红色嗜酸性细胞质,并且具有通常带有周边聚集染色质的淡嗜碱性常染色质核。此外,这些细胞大且形状不规则(长达60微米)。在聚-L-赖氨酸包被的玻片上用0.6%多聚甲醛/0.9%戊二醛固定FDC可使FDC得以保存,从而通过相差显微镜观察到长的树突状突起。通过放射自显影证实细胞表面存在抗原,对于HRP,还使用二氨基联苯胺进行酶促显色。与同一玻片上存在的驻留腹膜巨噬细胞或一些污染的淋巴结巨噬细胞不同,FDC不吞噬调理过的绵羊红细胞(SRBC),也不粘附于塑料表面,尽管它们确实与调理过的SRBC形成玫瑰花结。细胞标志物研究表明FDC具有独特的表型。它们对Ia、Fc受体和白细胞共同抗原呈阳性,但对Thy-1、Ly-1、Ly-2、内源性Ig、Mac-1、Mac-2、Mac-3和F4/80呈阴性,对非特异性酯酶呈阴性至弱阳性。培养的FDC保持存活并在其表面保留放射性标记的抗原 - 抗体复合物,并且FDC显著富集。(摘要截短于400字)

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