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构建胚状体微环境以引导胚胎干细胞分化。

Engineering the embryoid body microenvironment to direct embryonic stem cell differentiation.

作者信息

Bratt-Leal Andrés M, Carpenedo Richard L, McDevitt Todd C

机构信息

The Wallace H. Coulter Dept. of Biomedical Engineering, Georgia Institute of Technology/Emory University, Atlanta, GA, USA.

出版信息

Biotechnol Prog. 2009 Jan-Feb;25(1):43-51. doi: 10.1002/btpr.139.

Abstract

Embryonic stem cells (ESCs) are pluripotent cells capable of differentiating into all somatic and germ cell types. The intrinsic ability of pluripotent cells to generate a vast array of different cells makes ESCs a robust resource for a variety of cell transplantation and tissue engineering applications, however, efficient and controlled means of directing ESC differentiation is essential for the development of regenerative therapies. ESCs are commonly differentiated in vitro by spontaneously self-assembling in suspension culture into 3D cell aggregates called embryoid bodies (EBs), which mimic many of the hallmarks of early embryonic development, yet the 3D organization and structure of EBs also presents unique challenges to effectively direct the differentiation of the cells. ESC differentiation is strongly influenced by physical and chemical signals comprising the local extracellular microenvironment, thus current methods to engineer EB differentiation have focused primarily on spatially controlling EB size, adding soluble factors to the media, or culturing EBs on or within natural or synthetic extracellular matrices. Although most such strategies aim to influence differentiation from the exterior of EBs, engineering the microenvironment directly within EBs enables new opportunities to efficiently direct the fate of the cells by locally controlling the presentation of morphogenic cues.

摘要

胚胎干细胞(ESCs)是能够分化为所有体细胞和生殖细胞类型的多能细胞。多能细胞产生大量不同细胞的内在能力使胚胎干细胞成为各种细胞移植和组织工程应用的强大资源,然而,有效且可控地引导胚胎干细胞分化的方法对于再生疗法的发展至关重要。胚胎干细胞通常在体外通过在悬浮培养中自发自组装成称为胚状体(EBs)的三维细胞聚集体进行分化,这些胚状体模拟了早期胚胎发育的许多特征,然而,胚状体的三维组织和结构也给有效引导细胞分化带来了独特的挑战。胚胎干细胞的分化受到构成局部细胞外微环境的物理和化学信号的强烈影响,因此目前设计胚状体分化的方法主要集中在空间控制胚状体大小、向培养基中添加可溶性因子,或将胚状体培养在天然或合成细胞外基质上或内部。尽管大多数此类策略旨在从胚状体外部影响分化,但直接在胚状体内构建微环境能够通过局部控制形态发生线索的呈现为有效引导细胞命运带来新的机会。

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