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体外混合集落形成过程中造血干细胞的自我更新

Self-renewal of hemopoietic stem cells during mixed colony formation in vitro.

作者信息

Humphries R K, Eaves A C, Eaves C J

出版信息

Proc Natl Acad Sci U S A. 1981 Jun;78(6):3629-33. doi: 10.1073/pnas.78.6.3629.

Abstract

Replating experiments have shown that the self-renewal of pluripotent hemopoietic stem cells can be studied in vitro by clonal analysis techniques. The number of daughter stem cells detectable in individual primary clones produced in vitro varies markedly from one clone to another. These findings are consistent with a general model of stem cell differentiation in which the choice to self-replicate or not is ultimately determined at the single-cell level by a mechanism involving a random-event component that is intrinsic to the stem cell itself. Hemopoietic stem cells were identified by their ability to generate macroscopic-sized colonies having a visible erythroid component (i.e., gross red color) in standard methylcellulose assays containing medium conditioned by pokeweed mitogen-treated spleen cells and erythropoietin. In assays of replated primary or secondary colonies, inclusion of irradiated marrow-cell feeders was found to be an additional requirement. The mixed erythroid-megakaryocyte-granulocyte nature of colonies identified simply as macroscopic and erythroid was confirmed by cytochemical stains for lineage-specific markers. Marked variation in self-renewal was a feature of marrow stem cells both before and after maintenance in flask culture, although the overall self-renewal capacity exhibited by flask-cultured cells was approximately 5-fold higher. Variation in self-renewal was not correlated with primary colony size, which also varied over a wide range (0.2-9 X 10(5) nucleated cells per colony). Variation in stem cell self-renewal has been previously associated with hemopoietic stem cell proliferation in vivo. Its persistence in vitro in assays of dilute single-cell suspensions casts doubt on the significance of microenvironmental influences in directing stem cell differentiation.

摘要

再接种实验表明,多能造血干细胞的自我更新可以通过克隆分析技术在体外进行研究。在体外产生的单个初级克隆中可检测到的子代干细胞数量在不同克隆之间存在显著差异。这些发现与干细胞分化的一般模型一致,即在该模型中,自我复制与否的选择最终在单细胞水平上由一种涉及干细胞自身内在随机事件成分的机制决定。造血干细胞通过在含有经商陆有丝分裂原处理的脾细胞和促红细胞生成素条件培养基的标准甲基纤维素测定中产生具有可见红系成分(即明显红色)的宏观大小集落的能力来鉴定。在对再接种的初级或次级集落的测定中,发现加入经辐照的骨髓细胞饲养层是一项额外要求。通过针对谱系特异性标志物的细胞化学染色,证实了简单鉴定为宏观且红系的集落在红系、巨核细胞系和粒细胞系方面的混合性质。自我更新的显著差异是骨髓干细胞在烧瓶培养前后的一个特征,尽管烧瓶培养细胞表现出的总体自我更新能力大约高5倍。自我更新能力差异与初级集落大小无关,初级集落大小也在很宽范围内变化(每个集落0.2 - 9×10⁵个有核细胞)。干细胞自我更新的差异先前已与体内造血干细胞增殖相关联。其在体外稀释单细胞悬液测定中的持续存在使人对微环境影响在指导干细胞分化中的重要性产生怀疑。

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