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人脂肪来源干细胞向搏动性心肌细胞的分化。

Differentiation of human adipose-derived stem cells into beating cardiomyocytes.

机构信息

O'Brien Institute, Melbourne, Australia.

出版信息

J Cell Mol Med. 2010 Apr;14(4):878-89. doi: 10.1111/j.1582-4934.2010.01009.x. Epub 2010 Jan 11.

Abstract

Human adipose-derived stem cells (ASCs) may differentiate into cardiomyocytes and this provides a source of donor cells for tissue engineering. In this study, we evaluated cardiomyogenic differentiation protocols using a DNA demethylating agent 5-azacytidine (5-aza), a modified cardiomyogenic medium (MCM), a histone deacetylase inhibitor trichostatin A (TSA) and co-culture with neonatal rat cardiomyocytes. 5-aza treatment reduced both cardiac actin and TropT mRNA expression. Incubation in MCM only slightly increased gene expression (1.5- to 1.9-fold) and the number of cells co-expressing nkx2.5/sarcomeric alpha-actin (27.2% versus 0.2% in control). TSA treatment increased cardiac actin mRNA expression 11-fold after 1 week, which could be sustained for 2 weeks by culturing cells in cardiomyocyte culture medium. TSA-treated cells also stained positively for cardiac myosin heavy chain, alpha-actin, TropI and connexin43; however, none of these treatments produced beating cells. ASCs in non-contact co-culture showed no cardiac differentiation; however, ASCs co-cultured in direct contact co-culture exhibited a time-dependent increase in cardiac actin mRNA expression (up to 33-fold) between days 3 and 14. Immunocytochemistry revealed co-expression of GATA4 and Nkx2.5, alpha-actin, TropI and cardiac myosin heavy chain in CM-DiI labelled ASCs. Most importantly, many of these cells showed spontaneous contractions accompanied by calcium transients in culture. Human ASC (hASC) showed synchronous Ca(2+) transient and contraction synchronous with surrounding rat cardiomyocytes (106 beats/min.). Gap junctions also formed between them as observed by dye transfer. In conclusion, cell-to-cell interaction was identified as a key inducer for cardiomyogenic differentiation of hASCs. This method was optimized by co-culture with contracting cardiomyocytes and provides a potential cardiac differentiation system to progress applications for cardiac cell therapy or tissue engineering.

摘要

人脂肪来源的干细胞(ASCs)可分化为心肌细胞,这为组织工程提供了供体细胞来源。在这项研究中,我们使用 DNA 去甲基化剂 5-氮杂胞苷(5-aza)、改良的心肌生成培养基(MCM)、组蛋白去乙酰化酶抑制剂曲古抑菌素 A(TSA)以及与新生大鼠心肌细胞共培养来评估心肌生成分化方案。5-aza 处理降低了心脏肌动蛋白和 TropT mRNA 的表达。仅在 MCM 中孵育略微增加了基因表达(1.5-1.9 倍),并且共表达 nk2.5/肌节 alpha-actin 的细胞数量(对照为 0.2%,而对照为 0.2%)。TSA 处理在 1 周后使心脏肌动蛋白 mRNA 表达增加 11 倍,通过在心肌细胞培养基中培养细胞可维持 2 周。用 TSA 处理的细胞也对心肌肌球蛋白重链、alpha-actin、TropI 和连接蛋白 43 染色呈阳性;然而,这些处理均未产生搏动细胞。非接触共培养中的 ASC 没有表现出心脏分化;然而,在直接接触共培养中,ASC 的心脏肌动蛋白 mRNA 表达随时间呈依赖性增加(在第 3 天至第 14 天之间增加了 33 倍)。免疫细胞化学显示在 CM-DiI 标记的 ASC 中共同表达 GATA4 和 Nkx2.5、alpha-actin、TropI 和心肌肌球蛋白重链。最重要的是,许多这些细胞在培养中显示出自发性收缩并伴有钙瞬变。人 ASC(hASC)显示与周围大鼠心肌细胞(106 次/分钟)同步的 Ca(2+)瞬变和收缩。通过染料转移观察到它们之间也形成了缝隙连接。总之,细胞间相互作用被确定为 hASC 心肌生成分化的关键诱导剂。通过与收缩的心肌细胞共培养优化了该方法,并提供了一种潜在的心脏分化系统,以推进心脏细胞治疗或组织工程的应用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0b85/3823119/ca5d9d0f098d/jcmm0014-0878-f1.jpg

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