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鉴定控制人类造血干细胞/祖细胞生长和分化的基质微环境的不同成分。

Identification of distinct elements of the stromal microenvironment that control human hematopoietic stem/progenitor cell growth and differentiation.

作者信息

Aiuti A, Friedrich C, Sieff C A, Gutierrez-Ramos J C

机构信息

Center for Blood Research, Inc., Department of Genetics, Harvard Medical School, Boston, Massachusetts, USA.

出版信息

Exp Hematol. 1998 Feb;26(2):143-57.

PMID:9472804
Abstract

Using a novel collection of conditionally immortalized mouse stromal cell clones, we evaluated the role of distinct elements of the hematopoietic microenvironment in supporting and regulating the growth, division, and differentiation of a candidate human stem cell population (CD34+/CD38-). We found functional diversity in the capacity of different stromal cell clones to support the growth of primitive (CD34+/CD38-) and committed (CD34+/CD38+) hematopoietic progenitors and their differentiation into mature hematopoietic cells (CD34-/CD45+). Among the stromal cell clones that supported long-term hematopoiesis, we identified two clones that induced expansion of CD34+ progenitor/stem cells during the first 4 weeks of coculture and that supported the maintenance of this CD34+ population for up to 10 weeks in vitro. However, these two clones appeared to represent two different microenvironments with regard to the signals they provide to the different CD34+ progenitor subpopulations: One stromal clone preserved a pool of undifferentiated, relatively quiescent (CD34+/CD38-) progenitor cells, allowing their differentiation at a low rate into more committed (CD34+/CD38+) progenitors; the other fostered a more extensive and rapid differentiation of all CD34+/CD38- progenitors into CD34+/CD38+ cells, preferentially maintaining this committed population at a higher rate of cell division. These stromal cell clones were also able to support the proliferation and differentiation of CD34+/CD38- cells in conditions in which progenitor-stroma contact was prevented. This collection of stromal cell clones may represent a unique tool for the study of stromal regulators of hematopoiesis as well as for the support of gene transfer into hematopoietic progenitor cells.

摘要

利用一组新的条件永生化小鼠基质细胞克隆,我们评估了造血微环境中不同成分在支持和调节候选人类干细胞群体(CD34+/CD38-)的生长、分裂和分化中的作用。我们发现不同的基质细胞克隆在支持原始(CD34+/CD38-)和定向(CD34+/CD38+)造血祖细胞生长以及它们分化为成熟造血细胞(CD34-/CD45+)的能力上存在功能多样性。在支持长期造血的基质细胞克隆中,我们鉴定出两个克隆,它们在共培养的前4周诱导CD34+祖细胞/干细胞扩增,并在体外支持该CD34+群体维持长达10周。然而,就它们向不同CD34+祖细胞亚群提供的信号而言,这两个克隆似乎代表了两种不同的微环境:一个基质克隆保留了一群未分化、相对静止的(CD34+/CD38-)祖细胞,允许它们以低速率分化为更定向的(CD34+/CD38+)祖细胞;另一个则促进所有CD34+/CD38-祖细胞更广泛、快速地分化为CD34+/CD38+细胞,优先以更高的细胞分裂速率维持这个定向群体。这些基质细胞克隆还能够在阻止祖细胞与基质接触的条件下支持CD34+/CD38-细胞的增殖和分化。这组基质细胞克隆可能是研究造血的基质调节因子以及支持基因导入造血祖细胞的独特工具。

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Identification of distinct elements of the stromal microenvironment that control human hematopoietic stem/progenitor cell growth and differentiation.鉴定控制人类造血干细胞/祖细胞生长和分化的基质微环境的不同成分。
Exp Hematol. 1998 Feb;26(2):143-57.
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