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从人脐带血来源的内皮祖细胞分化而来的内皮细胞培养物的免疫学和超微结构特征

Immunological and ultrastructural characterization of endothelial cell cultures differentiated from human cord blood derived endothelial progenitor cells.

作者信息

Neumüller Josef, Neumüller-Guber Sylvia-Emanuela, Lipovac Markus, Mosgoeller Wilhelm, Vetterlein Monika, Pavelka Margit, Huber Johannes

机构信息

Center for Anatomy and Cell Biology, Department of Cell Biology and Ultrastructure Research, Medical University of Vienna, Schwarzspanierstrasse 17, 1090 Vienna, Austria.

出版信息

Histochem Cell Biol. 2006 Dec;126(6):649-64. doi: 10.1007/s00418-006-0201-6. Epub 2006 Jun 10.

DOI:10.1007/s00418-006-0201-6
PMID:16767408
Abstract

The replacement of endothelium by endothelial progenitor cells (EPCs) for therapeutic use in order to ameliorate the vascular status of ischemic organs is now in the focus of vascular research. The aim of our studies was to investigate whether EPCs derived from peripheral blood mononuclear cells (PBMNCs-derived EPCs) or EPCs propagated from CD34(+) hematopoietic stem cells (HSCs-derived EPCs), both isolated from human cord blood, are able to differentiate into early mature endothelial cells (ECs) under certain in vitro conditions. We characterized both cell populations by flow cytometry, phase contrast microscopy, fluorescence microscopy and confocal laser scanning microscopy as well as ultrastructurally using transmission and scanning electron microscopy. While PBMNCs gave rise to clusters of spindle-like EPCs after few days but did not further mature under in vitro conditions, mature ECs could only be successfully propagated from a starting population of isolated HSCs. Both, PBMNCs- and HSCs-derived EPCs, took up Dil-labeled acetylated low density lipoprotein (Dil-Ac-LDL) and could be positively stained for CD31, CD105, the vascular endothelial growth factor receptor 2 (VEGFR-2, KDR) and ulex europaeus agglutinin 1 (UEA-1) at the cell surface. EPC showed surface expression of CD54 and CD106. However, only a small portion of HSCs-derived EPCs was positive for CD54 but negative for CD106. Intracellular staining for von Willebrand factor (vWF) provided a homogenous stain in PBMNC-derived EPCs while in HSCs-derived EPCs, during cultivation for 2-3 weeks, more and more a typical punctuated staining pattern related to Weibel-Palade bodies (WPBs) was visible. By phase contrast and scanning electron microscopy, an arrangement of PBMNCs-derived EPCs in cord-like structures could be demonstrated. In these formations, cells showed parallel alignment but exhibited only few cell contacts. Well-developed WPBs could never be found in PBMNCs-derived EPCs. In contrast, differentiating HSCs-derived EPCs developed adherence junctions, interdigitating junctions as well as syndesmos. During maturation, spindle-like cell types appeared with abundant WPBs as well as cobblestone-like cell types with a fewer content of these organelles. WPBs, in the spindle-like cell types displayed conspicuous shapes and were concentrated in close proximity to mitochondria-rich areas. HSCs-derived EPCs exhibited signs of high synthetic activity such as a well-developed rough endoplasmic reticulum (RER) and multiple Golgi complexes. In the trans-Golgi network (TGN), close to the Golgi complex, a new formation of WPBs could be observed. These morphological features correlated well with a high growing capacity. Although it was not possible to demonstrate the complete differentiation line from HSCs to early matured ECs by immunologic markers because of the limited number of cells available for such investigations, distinct morphologic maturation stages could be shown at light and electron microscopical levels. In conclusion, the study presented here characterizes not only the different cell populations involved in the differentiation of early EPCs into mature ECs but also the transition stage where the maturation step takes place by demonstration of the new formation of WPBs. In this respect, these investigations provide new insights into the in vitro differentiation which could have some in vivo correlation.

摘要

为改善缺血器官的血管状态,采用内皮祖细胞(EPCs)替代内皮进行治疗性应用,现已成为血管研究的焦点。我们研究的目的是调查从人脐带血中分离的外周血单个核细胞来源的EPCs(PBMNCs - 来源的EPCs)或从CD34(+)造血干细胞增殖而来的EPCs(HSCs - 来源的EPCs)在特定体外条件下是否能够分化为早期成熟的内皮细胞(ECs)。我们通过流式细胞术、相差显微镜、荧光显微镜和共聚焦激光扫描显微镜以及使用透射和扫描电子显微镜进行超微结构分析,对这两种细胞群体进行了表征。虽然PBMNCs在几天后产生了纺锤样EPCs簇,但在体外条件下并未进一步成熟,而成熟的ECs只能从分离的HSCs起始群体中成功增殖。PBMNCs - 来源的EPCs和HSCs - 来源的EPCs都摄取了Dil标记的乙酰化低密度脂蛋白(Dil - Ac - LDL),并且在细胞表面CD31、CD105、血管内皮生长因子受体2(VEGFR - 2,KDR)和荆豆凝集素1(UEA - 1)可呈阳性染色。EPC显示CD54和CD106的表面表达。然而,只有一小部分HSCs - 来源的EPCs对CD54呈阳性而对CD106呈阴性。对血管性血友病因子(vWF)的细胞内染色在PBMNCs - 来源的EPCs中呈现均匀染色,而在HSCs - 来源的EPCs中,在培养2 - 3周期间,越来越多地可见与魏尔-帕拉德小体(WPBs)相关的典型点状染色模式。通过相差显微镜和扫描电子显微镜,可以证明PBMNCs - 来源的EPCs排列成索状结构。在这些结构中,细胞显示平行排列,但细胞间接触很少。在PBMNCs - 来源的EPCs中从未发现发育良好的WPBs。相反,正在分化的HSCs - 来源的EPCs形成了黏附连接、交错连接以及桥粒。在成熟过程中,出现了具有丰富WPBs的纺锤样细胞类型以及这些细胞器含量较少的鹅卵石样细胞类型。在纺锤样细胞类型中,WPBs呈现明显的形状,并集中在富含线粒体的区域附近。HSCs - 来源的EPCs表现出高合成活性的迹象,如发达的粗面内质网(RER)和多个高尔基体复合体。在高尔基体复合体附近的反式高尔基体网络(TGN)中,可以观察到WPBs的新形成。这些形态学特征与高生长能力密切相关。尽管由于可用于此类研究的细胞数量有限,无法通过免疫标记证明从HSCs到早期成熟ECs的完整分化谱系,但在光学和电子显微镜水平上可以显示出不同的形态成熟阶段。总之,本文的研究不仅表征了参与早期EPCs分化为成熟ECs的不同细胞群体,还通过证明WPBs的新形成表征了成熟步骤发生的过渡阶段。在这方面,这些研究为体外分化提供了新的见解,这可能与体内情况存在一定关联。

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