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通过拟胚体诱导人类诱导多能干细胞分化:一种实用且稳定的方法。

Inducing human induced pluripotent stem cell differentiation through embryoid bodies: A practical and stable approach.

作者信息

Guo Ning-Ning, Liu Li-Ping, Zheng Yun-Wen, Li Yu-Mei

机构信息

Institute of Regenerative Medicine, Affiliated Hospital of Jiangsu University, Jiangsu University, Zhenjiang 212001, Jiangsu Province, China.

出版信息

World J Stem Cells. 2020 Jan 26;12(1):25-34. doi: 10.4252/wjsc.v12.i1.25.

DOI:10.4252/wjsc.v12.i1.25
PMID:32110273
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7031760/
Abstract

Human induced pluripotent stem cells (hiPSCs) are invaluable resources for producing high-quality differentiated cells in unlimited quantities for both basic research and clinical use. They are particularly useful for studying human disease mechanisms by making it possible to circumvent the ethical issues of human embryonic stem cell research. However, significant limitations exist when using conventional flat culturing methods especially concerning cell expansion, differentiation efficiency, stability maintenance and multicellular 3D structure establishment, differentiation prediction. Embryoid bodies (EBs), the multicellular aggregates spontaneously generated from iPSCs in the suspension system, might help to address these issues. Due to the unique microenvironment and cell communication in EB structure that a 2D culture system cannot achieve, EBs have been widely applied in hiPSC-derived differentiation and show significant advantages especially in scaling up culturing, differentiation efficiency enhancement, simulation, and organoid establishment. EBs can potentially also be used in early prediction of iPSC differentiation capability. To improve the stability and feasibility of EB-mediated differentiation and generate high quality EBs, critical factors including iPSC pluripotency maintenance, generation of uniform morphology using micro-pattern 3D culture systems, proper cellular density inoculation, and EB size control are discussed on the basis of both published data and our own laboratory experiences. Collectively, the production of a large quantity of homogeneous EBs with high quality is important for the stability and feasibility of many PSCs related studies.

摘要

人诱导多能干细胞(hiPSC)是用于基础研究和临床应用的无限量生产高质量分化细胞的宝贵资源。它们对于研究人类疾病机制特别有用,因为可以规避人类胚胎干细胞研究中的伦理问题。然而,使用传统的平面培养方法存在重大局限性,特别是在细胞扩增、分化效率、稳定性维持、多细胞三维结构建立以及分化预测方面。胚状体(EB)是在悬浮系统中由iPSC自发形成的多细胞聚集体,可能有助于解决这些问题。由于EB结构中存在二维培养系统无法实现的独特微环境和细胞通讯,EB已广泛应用于hiPSC衍生的分化,并显示出显著优势,特别是在扩大培养规模、提高分化效率、模拟和类器官建立方面。EB还可能用于iPSC分化能力的早期预测。为了提高EB介导的分化的稳定性和可行性并生成高质量的EB,基于已发表的数据和我们自己的实验室经验,讨论了包括iPSC多能性维持、使用微图案三维培养系统生成均匀形态、适当的细胞密度接种和EB大小控制等关键因素。总体而言,大量生产高质量的均匀EB对于许多PSC相关研究的稳定性和可行性很重要。

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