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正常人骨髓细胞的体外扩增能力取决于实验条件:细胞浓度、血清及CD34+细胞选择在无基质培养中的作用。

The ex vivo expansion capacity of normal human bone marrow cells is dependent on experimental conditions: role of the cell concentration, serum and CD34+ cell selection in stroma-free cultures.

作者信息

Poloni A, Giarratana M C, Firat H, Kobari L, Gorin N C, Douay L

机构信息

Centre Claude Bernard, CHU Saint-Antoine, Paris, France.

出版信息

Hematol Cell Ther. 1997 Apr;39(2):49-58. doi: 10.1007/s00282-997-0049-9.

Abstract

The present study was conducted to establish defined culture conditions for ex vivo expansion of normal human bone marrow cells. We investigated the role of three experimental expansion parameters: the cell concentration in the initial culture medium, the role of animal serum, human plasma and serum-free substitute, and the expansion potential of mononucleated cells (MNC) versus CD34+ cells. Cells were cultured in suspension with stem cell factor (SCF), IL3, IL6 and Erythropoietin (Epo) for 10 days. 1) Reducing the cell concentration from 3 x 10(4) to 1.5 x 10(3)/ml increased total cell expansion almost 20 fold, progenitor expansion more than 3 fold, and the maintenance of long term culture-initiating cells (LTC-IC). 2) In medium containing a serum-free substitute, total and CD34+ cell expansion was 3 times greater than in medium containing 1-10% human AB plasma or 25% animal serum. 3) The expansion potential of selected CD34+ cells was significantly greater than that of the total MNC population. However, taking into account the cell loss due to CD34+ selection, the overall results for quantitative expansion in relation to the initial number of MNCS favor the use of non-selected MNCS. 4) SCF + IL3 + IL6 was clearly the best combination of early cytokines for LTC-IC maintenance, with or without lineage-restricted cytokines, whereas the presence of IL1 beta in any combination augmented the decrease in LTC-IC. Addition of G-CSF to the medium resulted in 1 log increase in total cell expansion and a 2-fold increase in CFU-GM expansion. Addition of Epo always induced a dramatic proliferation of erythroid cells (up to 2000 fold) as well as of CFU-GM (up to 4 fold), without exhausting the LTC-IC pool. We concluded that the expansion of hemopoietic cells for clinical purposes needs establishment of controlled, reproducible and reliable culture conditions.

摘要

本研究旨在建立正常人骨髓细胞体外扩增的特定培养条件。我们研究了三个实验性扩增参数的作用:初始培养基中的细胞浓度、动物血清、人血浆和无血清替代品的作用,以及单核细胞(MNC)与CD34+细胞的扩增潜力。细胞在含有干细胞因子(SCF)、白细胞介素3(IL3)、白细胞介素6(IL6)和促红细胞生成素(Epo)的悬浮液中培养10天。1)将细胞浓度从3×10⁴/ml降至1.5×10³/ml,总细胞扩增几乎增加了20倍,祖细胞扩增超过3倍,并维持了长期培养起始细胞(LTC-IC)。2)在含有无血清替代品的培养基中,总细胞和CD34+细胞的扩增比含有1-10%人AB血浆或25%动物血清的培养基大3倍。3)所选CD34+细胞的扩增潜力明显大于总MNC群体。然而,考虑到由于CD34+选择导致的细胞损失,与初始MNC数量相关的定量扩增总体结果有利于使用未选择的MNC。4)SCF + IL3 + IL6显然是维持LTC-IC的早期细胞因子的最佳组合,无论是否存在谱系限制性细胞因子,而任何组合中IL1β的存在都会加剧LTC-IC的减少。向培养基中添加粒细胞集落刺激因子(G-CSF)导致总细胞扩增增加1个对数,集落形成单位-粒细胞-巨噬细胞(CFU-GM)扩增增加2倍。添加Epo总是会诱导红系细胞显著增殖(高达2000倍)以及CFU-GM增殖(高达4倍),而不会耗尽LTC-IC池。我们得出结论,用于临床目的的造血细胞扩增需要建立可控、可重复和可靠的培养条件。

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