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慢速旋转侧向血管生物反应器可改善小鼠胚胎干细胞的胚状体形成和心脏发生分化。

Slow turning lateral vessel bioreactor improves embryoid body formation and cardiogenic differentiation of mouse embryonic stem cells.

作者信息

Rungarunlert Sasitorn, Klincumhom Nuttha, Tharasanit Theerawat, Techakumphu Mongkol, Pirity Melinda K, Dinnyes Andras

机构信息

1 BioTalentum Ltd ., Gödöllö, H-2100, Hungary .

出版信息

Cell Reprogram. 2013 Oct;15(5):443-58. doi: 10.1089/cell.2012.0082. Epub 2013 Sep 10.

DOI:10.1089/cell.2012.0082
PMID:24020697
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3787388/
Abstract

Embryonic stem cells (ESCs) have the ability to form aggregates, which are called embryoid bodies (EBs). EBs mimic early embryonic development and are commonly produced for cardiomyogenesis. Here, we describe a method of EB formation in hydrodynamic conditions using a slow-turning lateral vessel (STLV) bioreactor and the subsequent differentiation of EBs into cardiomyocytes. EBs formed in the STLV were compared with conventional techniques, such as hanging drop (HD) or static suspension cell culture (SSC), for homogeneity of EB size, shape, proliferation, apoptosis, and in vitro cardiac differentiation. After 3 days of culture, a four-fold improvement in the yield of EB formation/mL, a six-fold enhancement in total yield of EB/mL, and a nearly 10-fold reduction of cells that failed to incorporate into EBs were achieved in STLV versus SSC. During cardiac differentiation, a 1.5- to 4.2-fold increase in the area of cardiac troponin T (cTnT) per single EB in STLV versus SSC and HD was achieved. These results demonstrate that the STLV method improves the quality and quantity of ES cells to form EBs and enhances the efficiency of cardiac differentiation. We have demonstrated that the mechanical method of cell differentiation creates different microenvironments for the cells and thus influences their lineage commitments, even when genetic origin and the culture medium are the same. Ascorbic acid (ASC) improved further cardiac commitment in differentiation assays. Hence, this culture system is suitable for the production of large numbers of cells for clinical cell replacement therapies and industrial drug testing applications.

摘要

胚胎干细胞(ESC)具有形成聚集体的能力,这些聚集体被称为胚状体(EB)。EB模拟早期胚胎发育,常用于心肌生成研究。在此,我们描述了一种在流体动力学条件下使用慢速旋转侧管(STLV)生物反应器形成EB的方法,以及随后将EB分化为心肌细胞的过程。将在STLV中形成的EB与传统技术(如悬滴法(HD)或静态悬浮细胞培养(SSC))在EB大小、形状、增殖、凋亡以及体外心脏分化的同质性方面进行比较。培养3天后,与SSC相比,STLV在每毫升EB形成产量上提高了四倍,每毫升EB总产量提高了六倍,未整合到EB中的细胞数量减少了近10倍。在心脏分化过程中,与SSC和HD相比,STLV中单个EB中心肌肌钙蛋白T(cTnT)的面积增加了1.5至4.2倍。这些结果表明,STLV方法提高了ES细胞形成EB的质量和数量,并提高了心脏分化效率。我们已经证明,即使遗传来源和培养基相同,细胞分化的机械方法也会为细胞创造不同的微环境,从而影响它们的谱系定向。在分化试验中,抗坏血酸(ASC)进一步促进了心脏定向分化。因此,这种培养系统适用于为临床细胞替代疗法和工业药物测试应用生产大量细胞。

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本文引用的文献

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Biol Pharm Bull. 2012;35(3):308-16. doi: 10.1248/bpb.35.308.
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