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构建具有层粘连蛋白衍生短肽的多功能融合蛋白以促进小鼠诱导多能干细胞的神经分化。

Construction of multifunctional fusion proteins with a laminin-derived short peptide to promote neural differentiation of mouse induced pluripotent stem cells.

机构信息

Department of Life Science and Technology, School of Life Science and Technology, Tokyo Institute of Technology, Yokohama, Japan.

Department of Microbiology, Faculty of Biological Sciences, Jahangirnagar University, Dhaka, Bangladesh.

出版信息

J Biomed Mater Res B Appl Biomater. 2020 Aug;108(6):2691-2698. doi: 10.1002/jbm.b.34600. Epub 2020 Mar 13.

DOI:10.1002/jbm.b.34600
PMID:32167675
Abstract

There is growing interest in the functional roles of the extracellular matrix (ECM) in regulating the fate of pluripotent stem cells (PSCs). An artificially bioengineered ECM provides an excellent model for studying the molecular mechanisms underlying self-renewal and differentiation of PSCs, without multiple unknown and variable factors associated with natural substrates. Here, we have engineered multifunctional fusion proteins that are based on peptides from laminin, including p20, RGD, and elastin-like polypeptide (ELP), where laminin peptides work as cell adhesion molecules (CAMs) and ELP to promote anchorage. The functionality of these chimeric proteins, referred to as ERE-p20 and E-p20, was assessed by determining their ability to immobilize cells on a hydrophobic polystyrene surface, improve mouse induced pluripotent stem cells (miPSCs) attachment, and promote miPSC differentiation to neural progenitors. ERE-p20 and E-p20 proteins showed hydrophobic binding saturation to the polystyrene plates around 500 nM (2.39 μg/cm ) and 750 nM (2.27 μg/cm ) protein concentrations, respectively. The apparent maximum cell binding to ERE-p20 and E-p20 was approximately 81% and 73%, respectively, relative to gelatin. For neural precursors, neurite outgrowth was enhanced by the presence of RGD and p20 peptides. The expression levels of neuronal marker protein MAP2 were upregulated approximately 2.5-fold and threefold by ERE-p20 and E-p20, respectively, relative to laminin. Overall, we have shown that elastin-mimetic fusion proteins consisting of p20 with and without RGD peptides are able to induce neuronal differentiation. In conclusion, our newly designed bioengineered fusion proteins allow preparation of specific bioactive matrices or coating/scaffold for miPSCs differentiation.

摘要

人们对细胞外基质 (ECM) 在调节多能干细胞 (PSCs) 命运方面的功能作用越来越感兴趣。人工生物工程 ECM 为研究 PSCs 自我更新和分化的分子机制提供了一个极好的模型,而不会受到与天然基质相关的多个未知和可变因素的影响。在这里,我们设计了基于层粘连蛋白肽的多功能融合蛋白,包括 p20、RGD 和弹性蛋白样多肽 (ELP),其中层粘连蛋白肽作为细胞黏附分子 (CAM),ELP 促进锚定。通过确定这些嵌合蛋白(称为 ERE-p20 和 E-p20)固定细胞在疏水性聚苯乙烯表面上的能力、提高小鼠诱导多能干细胞 (miPSC) 黏附的能力以及促进 miPSC 分化为神经祖细胞的能力,评估了这些嵌合蛋白的功能。ERE-p20 和 E-p20 蛋白在大约 500 nM(2.39μg/cm )和 750 nM(2.27μg/cm )蛋白浓度时显示出对聚苯乙烯板的疏水性结合饱和,分别为 750 nM(2.27μg/cm )和 750 nM(2.27μg/cm )。相对于明胶,ERE-p20 和 E-p20 对细胞的最大结合率分别约为 81%和 73%。对于神经前体细胞,RGD 和 p20 肽的存在增强了神经突的生长。与层粘连蛋白相比,ERE-p20 和 E-p20 使神经元标志物蛋白 MAP2 的表达水平分别上调约 2.5 倍和 3 倍。总之,我们表明,由 p20 与 RGD 肽组成的弹性蛋白模拟融合蛋白能够诱导神经元分化。总之,我们新设计的生物工程融合蛋白允许制备特定的生物活性基质或涂层/支架用于 miPSC 分化。

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