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改良的脾源性鼠纤维细胞无血清培养条件。

Improved serum-free culture conditions for spleen-derived murine fibrocytes.

机构信息

Department of Biochemistry and Cell Biology, Rice University, Houston, Texas 77005-1894, USA.

出版信息

J Immunol Methods. 2010 Dec 15;363(1):9-20. doi: 10.1016/j.jim.2010.09.025. Epub 2010 Oct 1.

Abstract

Both wound repair and fibrosing diseases involve circulating monocytes entering a tissue and differentiating into fibroblast-like cells called fibrocytes. Fibrocyte biology has been extensively studied in both humans and mice. However, current in vitro techniques to culture murine fibrocytes can take up to two weeks and can require multiple mice to obtain enough circulating monocytes for a single experiment. An alternative source of fibrocytes is the splenic reservoir of monocytes, where one can obtain significantly more cells compared to the peripheral blood. We found that in serum-free medium, fibrocytes differentiate from murine spleen cells within 5 days. To maximize fibrocyte yield, we found the optimal purification technique was to digest the spleen with a collagenase/DNase cocktail, pass the cells through a cell strainer, and lyse the red blood cells. We found that IL-13 and M-CSF significantly enhanced fibrocyte differentiation and that the optimal cell density to promote differentiation was 1.75×10⁶ cells/ml. Serum amyloid P (SAP) and cross-linked IgG are two factors known to inhibit the differentiation of human monocytes into fibrocytes. We found that SAP and cross-linked IgG also inhibited the differentiation of murine spleen cells into fibrocytes. These results suggest that culturing murine spleen cells in serum-free medium is a rapid and efficient system to study factors that can affect fibrocyte differentiation.

摘要

伤口修复和纤维化疾病都涉及循环单核细胞进入组织并分化为成纤维细胞样细胞,称为纤维细胞。纤维细胞生物学在人类和小鼠中都得到了广泛的研究。然而,目前用于培养小鼠纤维细胞的体外技术可能需要长达两周的时间,并且可能需要多只小鼠才能获得足够的循环单核细胞进行单次实验。纤维细胞的另一个来源是脾脏中的单核细胞储备,与外周血相比,脾脏中可以获得更多的细胞。我们发现,在无血清培养基中,纤维细胞可以在 5 天内从鼠脾细胞中分化出来。为了最大限度地提高纤维细胞的产量,我们发现最佳的纯化技术是用胶原酶/DNase 鸡尾酒消化脾脏,将细胞通过细胞滤网,并裂解红细胞。我们发现,IL-13 和 M-CSF 显著增强了纤维细胞的分化,促进分化的最佳细胞密度为 1.75×10⁶ 个细胞/ml。血清淀粉样蛋白 P(SAP)和交联 IgG 是两种已知抑制人单核细胞分化为纤维细胞的因子。我们发现 SAP 和交联 IgG 也抑制了鼠脾细胞向纤维细胞的分化。这些结果表明,在无血清培养基中培养鼠脾细胞是研究影响纤维细胞分化的因素的快速有效的系统。

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