人脐带血造血祖细胞:与成人骨髓细胞相同吗?

Blood cells Pub Date : 1994-01-01
C M Traycoff, M R Abboud, J Laver, D W Clapp, R Hoffman, P Law, E F Srour
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引用次数: 0

摘要

为了扩大单个脐带血(CB)的造血祖细胞(HPC)含量,我们研究了CB CD34+细胞的体外增殖潜力以及这些细胞在不同细胞因子组合下从细胞周期G0/G1期退出的速率。在最初的实验中,对CB和成人骨髓(BM) CD34+细胞的表型定义群体进行了HPC含量检测,结果显示,与BM相反,CB CD34+人白细胞A (HLA)-DR+细胞似乎含有大部分原始HPC。在干细胞因子(SCF)+白细胞介素-3 (IL-3)培养的BM CD34+ HLA-DR+细胞中,CD34+细胞在5天内增加了5倍,而CB CD34+ HLA-DR+培养的CD34+细胞在相同条件下增加了11倍,说明CB CD34+ HLA-DR+细胞的增殖潜力比成人BM的类似细胞增强。此外,在补充SCF和IL-3的培养中,在第5天观察到仍然存在于G0/G1中的CB CD34+数量增加了6.2倍,这表明体外产生了大量原始HPC。然后检测SCF对G0/G1的CB和BM CD34+ HLA-DR+细胞退出的影响。暴露于SCF 36至48小时后,45%的静止CB细胞进入G0/G1,而静止BM细胞仅为13%。在仅添加SCF或IL-3的无血清培养基中,除非同时添加SCF和IL-3,否则CB CD34+ HLA-DR+细胞不会像存在CB血浆时那样迅速退出细胞周期的G0/G1期。总的来说,这些结果表明,CB CD34+细胞对细胞因子刺激,特别是SCF更敏感,可能比BM细胞更适合体外扩增HPC。此外,这些数据说明了BM细胞亚群和CB细胞亚群中HPC含量的潜在重要生物学差异,以及这些亚群对细胞因子刺激的反应。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Human umbilical cord blood hematopoietic progenitor cells: are they the same as their adult bone marrow counterparts?

In an attempt to expand the hematopoietic progenitor cell (HPC) content of a single collection of umbilical cord blood (CB), we investigated the ex vivo proliferative potential of CB CD34+ cells and the rate of exit of these cells from G0/G1 phases of cell cycle in response to different cytokine combinations. Initial experiments in which phenotypically defined populations of CB and adult bone marrow (BM) CD34+ cells were examined for their HPC content revealed that, contrary to BM, CB CD34+ human leukocyte A (HLA)-DR+ cells appeared to contain the majority of primitive HPC. In cultures of BM CD34+ HLA-DR+ cells incubated with stem cell factor (SCF)+interleukin-3 (IL-3), CD34+ cells increased five-fold over 5 days, while CD34+ cells from CB CD34+ HLA-DR+ cultures increased 11-fold under these same conditions, illustrating an enhanced proliferative potential of CB CD34+ HLA-DR+ cells vs. similar cells from adult BM. Furthermore, a 6.2-fold increase in the number of CB CD34+ still residing in G0/G1 was observed on day 5 in cultures supplemented with SCF and IL-3, suggesting the generation of large numbers of primitive HPC in vitro. The effect of SCF on the exit of CB and BM CD34+ HLA-DR+ cells from G0/G1 was then examined. Following 36- to 48-hour exposure to SCF, 45% of quiescent CB cells exited G0/G1 in contrast to only 13% of quiescent BM cells. In serum-free media supplemented with either SCF or IL-3 alone, CB CD34+ HLA-DR+ cells did not exit G0/G1 phases of cell cycle as rapidly as when CB plasma was present, unless SCF and IL-3 were added simultaneously. Collectively, these results suggest that CB CD34+ cells are more responsive to cytokine stimulation, especially SCF, and may represent more suitable candidates for ex vivo expansion of HPC than BM cells. Furthermore, these data illustrate potentially important biologic differences between the HPC content of subpopulations of BM and CB cells, and the response of these subpopulations to cytokine stimulation.

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