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造血细胞去分化诱导因子的鉴定

Identification of a Hematopoietic Cell Dedifferentiation-Inducing Factor.

作者信息

Li Yunyuan, Adomat Hans, Guns Emma Tomlinson, Hojabrpour Payman, Duronio Vincent, Curran Terry-Ann, Jalili Reza Baradar, Jia William, Delwar Zahid, Zhang Yun, Elizei Sanam Salimi, Ghahary Aziz

机构信息

Department of Surgery, University of British Columbia, Vancouver, British Columbia, Canada.

Vancouver Prostate Centre, Vancouver, British Columbia, Canada.

出版信息

J Cell Physiol. 2016 Jun;231(6):1350-63. doi: 10.1002/jcp.25239. Epub 2016 Feb 8.

DOI:10.1002/jcp.25239
PMID:26529564
Abstract

It has long been realized that hematopoietic cells may have the capacity to trans-differentiate into non-lymphohematopoietic cells under specific conditions. However, the mechanisms and the factors for hematopoietic cell trans-differentiation remain unknown. In an in vitro culture system, we found that using a conditioned medium from proliferating fibroblasts can induce a subset of hematopoietic cells to become adherent fibroblast-like cells (FLCs). FLCs are not fibroblasts nor other mesenchymal stromal cells, based on their expression of type-1 collagen, and other stromal cell marker genes. To identify the active factors in the conditioned medium, we cultured fibroblasts in a serum-free medium and collected it for further purification. Using the fractions from filter devices of different molecular weight cut-offs, and ammonium sulfate precipitation collected from the medium, we found the active fraction is a protein. We then purified this fraction by using fast protein liquid chromatography (FPLC) and identified it by mass spectrometer as macrophage colony-stimulating factor (M-CSF). The mechanisms of M-CSF-inducing trans-differentiation of hematopoietic cells seem to involve a tyrosine kinase signalling pathway and its known receptor. The FLCs express a number of stem cell markers including SSEA-1 and -3, OCT3/4, NANOG, and SOX2. Spontaneous and induced differentiation experiments confirmed that FLCs can be further differentiated into cell types of three germ layers. These data indicate that hematopoietic cells can be induced by M-CSF to dedifferentiate to multipotent stem cells. This study also provides a simple method to generate multipotent stem cells for clinical applications.

摘要

长期以来人们已经认识到,造血细胞在特定条件下可能具有转分化为非淋巴造血细胞的能力。然而,造血细胞转分化的机制和因素仍然未知。在体外培养系统中,我们发现使用增殖成纤维细胞的条件培养基可以诱导一部分造血细胞成为贴壁的成纤维细胞样细胞(FLCs)。基于其I型胶原蛋白及其他基质细胞标记基因的表达,FLCs不是成纤维细胞,也不是其他间充质基质细胞。为了鉴定条件培养基中的活性因子,我们在无血清培养基中培养成纤维细胞并收集用于进一步纯化。使用来自不同分子量截留的过滤装置的组分以及从培养基中收集的硫酸铵沉淀,我们发现活性组分是一种蛋白质。然后我们通过快速蛋白质液相色谱(FPLC)纯化该组分,并通过质谱仪鉴定为巨噬细胞集落刺激因子(M-CSF)。M-CSF诱导造血细胞转分化的机制似乎涉及酪氨酸激酶信号通路及其已知受体。FLCs表达多种干细胞标记物,包括SSEA-1和-3、OCT3/4、NANOG和SOX2。自发和诱导分化实验证实,FLCs可以进一步分化为三个胚层的细胞类型。这些数据表明,造血细胞可以被M-CSF诱导去分化为多能干细胞。本研究还提供了一种简单的方法来生成用于临床应用的多能干细胞。

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