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国家自然科学基金(81125003)

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用KOSR优化山羊克隆胚的培养体系
2012年
体细胞核移植重构胚的体外培养一直是影响山羊克隆效率的一个重要因素,为了排除成分复杂的胎牛血清(fetal bovine serum,FBS)对克隆重构胚发育的潜在抑制作用,本研究采用成分明确的血清替代品(knockout serum replacement,KOSR)进行山羊体细胞克隆重构胚胎的体外培养,并比较KOSR与FBS对重构胚的发育效率的影响。结果显示,KOSR组山羊重构胚培养体系的分裂率明显高于FBS组(80.67±0.63%.vs 49.02±4.85%,P<0.01),2组在重构胚重编程过程中的8细胞率具有显著差异(48.89±1.92%vs.28.59±3.13%,P<0.05);2组不同培养体系的受孕率也有明显不同(33.3%vs.10%,P<0.05)。研究结果表明,KOSR培养体系能有效提高山羊重构胚的发育效率,特别是有利于重构胚的早期重编程,为获得健康的转基因克隆山羊奠定了良好的基础。
陈威胡伟曹辉李凯王清泉蔡勤蔡琳琳刘宇习书斌李华陈美珏黄英黄淑帧曾凡一
关键词:重构胚重编程发育
Integration-free Methods for Generating Induced Pluripotent Stem Cells被引量:3
2013年
Induced pluripotent stem (iPS) cells by exogenous expression of four factors, Oct4, can be generated from mouse or human fibroblasts Sox2, Klf4 and c-Myc, and hold great potential for transplantation therapies and regenerative medicine. However, use of retroviral vectors during iPS cell generation has limited the techniques clinical application due to the potential risks resulting from genome integration of transgenes, including insertional mutations and altered differentiation potentials of the target cells, which may lead to pathologies such as tumorigenesis. Here we review recent progress in generating safer transgene-free or integration-free iPS cells, including the use of non-integrating vectors, excision of vectors after integration, DNA-free delivery of factors and chemical induction of pluripotency.
Yi-ye ZhouFanyi Zeng
关键词:VECTOR
Shared Gene Regulation during Human Somatic Cell Reprogramming被引量:2
2012年
Human induced pluripotent stem (iPS) cells have the ability to differentiate into all somatic cells and to maintain unlimited self- renewal. Therefore, they have great potential in both basic research and clinical therapy for many diseases. To identify potentially universal mechanisms of human somatic cell reprogramming, we studied gene expression changes in three types of cells undergoing reprogramming. The set of 570 genes commonly regulated during induction of iPS cells includes known embryonic stem (ES) cell markers and pluripotency related genes. We also identified novel genes and biological categories which may be related to somatic cell reprogramming. For example, some of the down-regulated genes are predicted targets of the pluripotency microRNA cluster miR302/367, and the proteins from these putative target genes interact with the stem cell pluripotency factor POU5F1 according to our network analysis. Our results identified candidate gene sets to guide research on the mechanisms operating during somatic cell reprogramming.
Xiang WangXuesong ChenHuijun ZhangWenyi QinYan XueFanyi Zeng
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