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人骨髓间充质基质细胞表达 CD14 交叉反应性表位。

Human mesenchymal stromal cells express CD14 cross-reactive epitopes.

机构信息

Center for Regenerative Medicine (ZRM), UKT, Eberhard-Karls University, Tübingen, Germany.

出版信息

Cytometry A. 2011 Aug;79(8):635-45. doi: 10.1002/cyto.a.21073. Epub 2011 Jul 6.

DOI:10.1002/cyto.a.21073
PMID:21735544
Abstract

Mesenchymal stromal cells (MSCs) do not express a unique definite epitope or marker gene. As such, minimal criteria were recently established for defining multipotent MSC. These criteria include expression of CD73, CD90, CD105, and a lack of hematopoietic marker expression. However, we detected binding of a CD14 antibody on bone marrow- and placenta-derived MSC and investigated the staining of CD14 antibodies on these MSC in more detail. The MSC were isolated from human bone marrow and placenta tissue, expanded, characterized by quantitative RT-PCR, flow cytometry, and immunocytochemistry and differentiated to generate osteoblasts, chondrocytes, and adipocytes. The CD14-cross-reactive MSCs were enriched by cell sorting. Human peripheral blood mononuclear cells, fibroblasts, and hematopoietic cell lines served as controls. Utilizing four different clones of CD14 monoclonal antibodies, we found that three CD14 reagents stained the MSC. Two CD14 antibodies (HCD14 and M5E2) clearly marked the CD90(+) MSC population with distinct intensities, clone 134 620 generated a shift in flow cytometry histograms, but clone MΦP9 did not stain MSC. Transcripts encoding CD14 or the CD14 protein were not detected in MSC. We confirm that bone marrow- and placenta-derived MSC do not express CD14 and that the CD14 antibody MΦP9 discriminates between monocytes and MSC more efficiently than the other antibodies employed here. This investigation does not contradict previous work but provides a more accurate characterization of MSC.

摘要

间充质基质细胞(MSCs)不表达独特的明确表位或标记基因。因此,最近为定义多能 MSC 确立了最小标准。这些标准包括 CD73、CD90、CD105 的表达和缺乏造血标记物的表达。然而,我们在骨髓和胎盘来源的 MSC 上检测到 CD14 抗体的结合,并更详细地研究了这些 MSC 上 CD14 抗体的染色情况。MSC 从人骨髓和胎盘组织中分离出来,进行扩增,通过定量 RT-PCR、流式细胞术和免疫细胞化学进行特征鉴定,并分化为成骨细胞、软骨细胞和脂肪细胞。通过细胞分选富集 CD14 交叉反应性 MSC。人外周血单核细胞、成纤维细胞和造血细胞系用作对照。利用四种不同的 CD14 单克隆抗体克隆,我们发现三种 CD14 试剂染色 MSC。两种 CD14 抗体(HCD14 和 M5E2)清楚地标记 CD90(+) MSC 群体,具有明显的强度,克隆 134 620 在流式细胞术直方图中产生偏移,但克隆 MΦP9 不染色 MSC。在 MSC 中未检测到编码 CD14 或 CD14 蛋白的转录本。我们证实骨髓和胎盘来源的 MSC 不表达 CD14,并且 CD14 抗体 MΦP9 比这里使用的其他抗体更有效地区分单核细胞和 MSC。这项研究并没有与以前的工作相矛盾,但提供了对 MSC 更准确的描述。

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