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人原始造血祖细胞在体外的长期生成与扩增

Long-term generation and expansion of human primitive hematopoietic progenitor cells in vitro.

作者信息

Srour E F, Brandt J E, Briddell R A, Grigsby S, Leemhuis T, Hoffman R

机构信息

Department of Medicine, Hematology/Oncology, Indiana University School of Medicine, Indianapolis 46202-5121.

出版信息

Blood. 1993 Feb 1;81(3):661-9.

PMID:7678996
Abstract

Although sustained production of committed human hematopoietic progenitor cells in long-term bone marrow cultures (LTBMC) is well documented, evidence for the generation and expansion of human primitive hematopoietic progenitor cells (PHPC) in such cultures is lacking. For that purpose, we attempted to determine if the human high proliferative potential colony-forming cell (HPP-CFC), a primitive hematopoietic marrow progenitor cell, is capable of generation and expansion in vitro. To that effect, stromal cell-free LTBMC were initiated with CD34+ HLA-DR-CD15- rhodamine 123dull bone marrow cells and were maintained with repeated addition of c-kit ligand and a synthetic interleukin-3/granulocyte-macrophage colony-stimulating factor fusion protein. By day 21 of LTBMC, a greater than twofold increase in the number of assayable HPP-CFC was detected. Furthermore, the production of HPP-CFC in LTBMC continued for up to 4 weeks, resulting in a 5.5-fold increase in HPP-CFC numbers. Weekly phenotypic analyses of cells harvested from LTBMC showed that the number of CD34+ HLA-DR- cells increased from 10(4) on day 0 to 56 CD34+ HLA-DR- cells increased from 10(4) on day 0 to 56 x 10(4) by day 21. To examine further the nature of the in vitro HPP-CFC expansion, individual HPP-CFC colonies were serially cloned. Secondary cloning of individual, day 28 primary HPP-CFC indicated that 46% of these colonies formed an average of nine secondary colony-forming unit--granulocyte-macrophage (CFU-GM)--derived colonies, whereas 43% of primary HPP-CFC gave rise to between one and six secondary HPP-CFC colonies and 6 to 26 CFU-GM. These data show that CD34+ HLA-DR- CD15- rhodamine 123dull cells represent a fraction of human bone marrow highly enriched for HPP-CFC and that based on their regeneration and proliferative capacities, a hierarchy of HPP-CFC exists. Furthermore, these studies indicate that in the presence of appropriate cytokine stimulation, it is possible to expand the number of PHPC in vitro.

摘要

尽管长期骨髓培养(LTBMC)中定向人类造血祖细胞的持续产生已有充分记录,但在此类培养中人类原始造血祖细胞(PHPC)的生成和扩增证据仍很缺乏。为此,我们试图确定人类高增殖潜能集落形成细胞(HPP-CFC),一种原始造血骨髓祖细胞,是否能够在体外生成和扩增。为此,用CD34+HLA-DR-CD15-罗丹明123暗淡的骨髓细胞启动无基质LTBMC,并通过反复添加c-kit配体和一种合成的白细胞介素-3/粒细胞-巨噬细胞集落刺激因子融合蛋白来维持培养。到LTBMC培养的第21天,可检测到的HPP-CFC数量增加了两倍多。此外,LTBMC中HPP-CFC的产生持续了长达4周,导致HPP-CFC数量增加了5.5倍。对从LTBMC收获的细胞进行的每周表型分析表明,CD34+HLA-DR-细胞的数量从第0天的10⁴增加到第21天的56×10⁴。为了进一步研究体外HPP-CFC扩增的性质,对单个HPP-CFC集落进行了连续克隆。对第28天的单个初级HPP-CFC进行二次克隆表明,这些集落中有46%平均形成了9个源自二级集落形成单位-粒细胞-巨噬细胞(CFU-GM)的集落,而43%的初级HPP-CFC产生了1至6个二级HPP-CFC集落以及6至26个CFU-GM。这些数据表明,CD34+HLA-DR-CD15-罗丹明123暗淡细胞代表了人类骨髓中高度富集HPP-CFC的一部分,并且基于它们的再生和增殖能力,存在一个HPP-CFC等级体系。此外,这些研究表明,在适当的细胞因子刺激下,有可能在体外扩增PHPC的数量。

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