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无饲养层和动物来源成分的培养以及重组人 vitronectin 接枝水凝胶上的人胚胎干细胞的分化。

Xeno-free and feeder-free culture and differentiation of human embryonic stem cells on recombinant vitronectin-grafted hydrogels.

机构信息

Department of Chemical and Materials Engineering, National Central University, No. 300, Jhongda RD., Jhongli, Taoyuan, 32001, Taiwan.

出版信息

Biomater Sci. 2019 Sep 24;7(10):4345-4362. doi: 10.1039/c9bm00418a.

Abstract

Recombinant vitronectin-grafted hydrogels were developed by adjusting surface charge of the hydrogels with grafting of poly-l-lysine for optimal culture of human embryonic stem cells (hESCs) under xeno- and feeder-free culture conditions, with elasticity regulated by crosslinking time (10-30 kPa), in contrast to conventional recombinant vitronectin coating dishes, which have a fixed stiff surface (3 GPa). hESCs proliferated on the hydrogels for over 10 passages and differentiated into the cells derived from three germ layers indicating the maintenance of pluripotency. hESCs on the hydrogels differentiated into cardiomyocytes under xeno-free culture conditions with much higher efficiency (80% of cTnT+ cells) than those on conventional recombinant vitronectin or Matrigel-coating dishes just only after 12 days of induction. It is important to have an optimal design of cell culture biomaterials where biological cues (recombinant vitronectin) and physical cues (optimal elasticity) are combined for high differentiation of hESCs into specific cell lineages, such as cardiomyocytes, under xeno-free and feeder-free culture conditions.

摘要

通过调整水凝胶的表面电荷,用聚赖氨酸接枝合成了重组 vitronectin 接枝水凝胶,在无饲养层和异种条件下,为人类胚胎干细胞(hESCs)的最佳培养提供了条件,其弹性可通过交联时间(10-30 kPa)进行调节,与传统的重组 vitronectin 包被培养皿相比,后者具有固定的刚性表面(3 GPa)。hESCs 在水凝胶上增殖超过 10 代,并分化为来自三个胚层的细胞,表明其多能性得以维持。在无饲养层的条件下,hESCs 在水凝胶上分化为心肌细胞的效率比传统的重组 vitronectin 或 Matrigel 包被培养皿高得多(诱导 12 天后 cTnT+细胞的比例为 80%)。在无饲养层和异种条件下,将生物信号(重组 vitronectin)和物理信号(最佳弹性)结合起来,对细胞培养生物材料进行优化设计,对于 hESCs 向特定细胞谱系(如心肌细胞)的高效分化非常重要。

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