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成年鼠骨髓造血干细胞中醛脱氢酶活性的不同水平与植入和细胞周期状态有关。

Varying levels of aldehyde dehydrogenase activity in adult murine marrow hematopoietic stem cells are associated with engraftment and cell cycle status.

机构信息

British Columbia Cancer Agency/Terry Fox Laboratory, Vancouver, British Columbia, Canada.

出版信息

Exp Hematol. 2012 Oct;40(10):857-66.e5. doi: 10.1016/j.exphem.2012.05.014. Epub 2012 Jun 6.

Abstract

Aldehyde dehydrogenase (ALDH) activity is a widely used marker for human hematopoietic stem cells (HSCs), yet its relevance and role in murine HSCs remain unclear. We found that murine marrow cells with a high level of ALDH activity as measured by Aldefluor staining (ALDH(br) cells) do not contain known HSCs or progenitors. In contrast, highly enriched murine HSCs defined by the CD48(-)EPCR(+) and other phenotypes contain two subpopulations, one that stains dimly with Aldefluor (ALDH(dim)) and one that stains at intermediate levels (ALDH(int)). The CD48(-)EPCR(+)ALDH(dim) cells are virtually all in G(0) and yield high levels of engraftment via both intravenous and intrabone routes. In contrast the CD48(-)EPCR(+)ALDH(int) cells are virtually all in G(1), have little intravenous engraftment potential, and yet can engraft long-term after intrabone transplantation. These data demonstrate that Aldefluor staining of unfractionated murine marrow does not identify known HSCs or progenitors. However, varying levels of Aldefluor staining when combined with CD48 and EPCR detection can identify novel populations in murine marrow including a highly enriched population of resting HSCs and a previously unknown HSC population in G(1) with an intravenous engraftment defect.

摘要

醛脱氢酶(ALDH)活性是人类造血干细胞(HSCs)的广泛应用标志物,但在小鼠 HSCs 中的相关性和作用尚不清楚。我们发现,用 Aldefluor 染色(ALDH(br)细胞)测量的高水平 ALDH 活性的鼠骨髓细胞不含有已知的 HSCs 或祖细胞。相比之下,通过 CD48(-)EPCR(+)和其他表型高度富集的小鼠 HSCs 包含两个亚群,一个用 Aldefluor 染色呈弱荧光(ALDH(dim)),另一个染色呈中等水平(ALDH(int))。CD48(-)EPCR(+)ALDH(dim)细胞几乎全部处于 G(0)期,通过静脉内和骨髓内途径均能产生高水平的植入。相比之下,CD48(-)EPCR(+)ALDH(int)细胞几乎全部处于 G(1)期,静脉内植入潜力很小,但在骨髓内移植后仍能长期植入。这些数据表明,未分馏的鼠骨髓的 Aldefluor 染色不能识别已知的 HSCs 或祖细胞。然而,当与 CD48 和 EPCR 检测结合使用时,不同水平的 Aldefluor 染色可以识别鼠骨髓中的新型群体,包括高度富集的静止 HSCs 群体和以前未知的处于 G(1)期的具有静脉内植入缺陷的 HSC 群体。

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