首页> 美国卫生研究院文献>The Journal of Experimental Medicine >Preferential Proliferation of Murine Colony-forming Units in Culture in a Chemically Defined Condition with a Macrophage Colony-stimulating Factor–negative Stromal Cell Clone
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Preferential Proliferation of Murine Colony-forming Units in Culture in a Chemically Defined Condition with a Macrophage Colony-stimulating Factor–negative Stromal Cell Clone

机译:在化学定义的条件下具有巨噬细胞集落刺激因子阴性基质细胞克隆的化学条件下培养的小鼠集落形成单位的优先增殖。

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摘要

The establishment of culture conditions that selectively support hematopoietic stem cells is an important goal of hematology. In this study, we investigated the possibility of using for this purpose a defined medium, mSFO2, which was developed for stromal cell–dependent bone marrow cultures. We found that a combination of epidermal growth factor (EGF), the OP9 stromal cell line, which lacks macrophage colony-stimulating factor, recombinant stem cell factor, and the chemically defined medium mSFO2 provides a microenvironment where c-Kit+ Thy-1+/lo Mac-1+/lo B220 TER119 commonβ+ IL-2Rγ + gp130+ cells are selectively propagated from normal, unfractionated bone marrow cells. This cell population produced an in vitro colony at a very high efficiency (50%), whereas it has only limited proliferative ability in the irradiated recipient. Thus, the cells selected in this culture condition might represent colony-forming units in culture (CFU-c) with short-term reconstituting ability. Transferring this cell population into medium containing differentiation signals resulted in the rapid production of mature myelomonocytic and B cell lineages in vitro and in vivo. The fact that a similar culture condition was created by erb-B2–transduced OP9 in the absence of EGF indicated that EGF exerts its effect by acting on OP9 rather than directly on CFU-c. These results suggested that the balance between self-renewal and differentiation of CFU-c can be regulated by extracellular signals.
机译:建立选择性支持造血干细胞的培养条件是血液学的重要目标。在这项研究中,我们调查了为此目的使用定义的培养基mSFO2的可能性,该培养基专为基质细胞依赖性骨髓培养而开发。我们发现表皮生长因子(EGF),OP9基质细胞系(缺乏巨噬细胞集落刺激因子,重组干细胞因子)和化学成分确定的培养基mSFO2的组合提供了微环境,其中c-Kit + < / sup> Thy-1 + / lo Mac-1 + / lo B220 - TER119 -常见β + IL-2Rγ + gp130 + 细胞从正常的普通骨髓细胞中选择性繁殖。该细胞群以非常高的效率(50%)产生了体外菌落,而在受辐照的受体中其增殖能力有限。因此,在这种培养条件下选择的细胞可能代表具有短期重构能力的培养菌落形成单位(CFU-c)。将该细胞群转移到含有分化信号的培养基中,导致在体外和体内快速产生成熟的单核细胞和B细胞谱系。在没有EGF的情况下erb-B2转导的OP9产生了类似的培养条件,这一事实表明EGF通过作用于OP9而不是直接作用于CFU-c发挥了作用。这些结果表明,CFU-c的自我更新与分化之间的平衡可以通过细胞外信号来调节。

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