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在猪成纤维细胞向诱导多能干细胞的标准重编程过程中诱导滋养层细胞集落的生成。

Generation of colonies of induced trophoblast cells during standard reprogramming of porcine fibroblasts to induced pluripotent stem cells.

机构信息

Bond Life Sciences Center and Division of Animal Sciences, University of Missouri, Columbia, Missouri, USA.

出版信息

Biol Reprod. 2011 Oct;85(4):779-87. doi: 10.1095/biolreprod.111.092809. Epub 2011 Jul 6.

Abstract

During reprogramming of porcine mesenchymal cells with a four-factor (POU5F1/SOX2/KLF4/MYC) mixture of vectors, a fraction of the colonies had an atypical phenotype and arose earlier than the recognizable porcine induced pluripotent stem (iPS) cell colonies. Within days after each passage, patches of cells with an epithelial phenotype formed raised domes, particularly under 20% O(2) conditions. Relative to gene expression of the iPS cells, there was up-regulation of genes for transcription factors associated with trophoblast (TR) lineage emergence, e.g., GATA2, PPARG, MSX2, DLX3, HAND1, GCM1, CDX2, ID2, ELF5, TCFAP2C, and TEAD4 and for genes required for synthesis of products more typical of differentiated TR, such as steroids (HSD17B1, CYP11A1, and STAR), pregnancy-associated glycoproteins (PAG6), and select cytokines (IFND, IFNG, and IL1B). Although POU5F1 was down-regulated relative to that in iPS cells, it was not silenced in the induced TR (iTR) cells over continued passage. Like iPS cells, iTR cells did not senesce on extended passage and displayed high telomerase activity. Upon xenografting into immunodeficient mice, iTR cells formed nonhemorrhagic teratomas composed largely of layers of epithelium expressing TR markers. When cultured under conditions that promoted embryoid body formation, iTR cells formed floating spheres consisting of a single epithelial sheet whose cells were tethered laterally by desmosome-like structures. In conclusion, reprogramming of porcine fibroblasts to iPS cells generates, as a by-product, colonies composed of self-renewing populations of TR cells, possibly containing TR stem cells.

摘要

在使用包含四个因子(POU5F1/SOX2/KLF4/MYC)的载体混合物对猪间充质细胞进行重编程的过程中,一部分集落表现出非典型表型,且比可识别的猪诱导多能干细胞(iPS)集落更早出现。在每次传代后的几天内,具有上皮表型的细胞斑块形成凸起的穹顶,特别是在 20%O2 条件下。与 iPS 细胞的基因表达相比,与滋养层(TR)谱系出现相关的转录因子的基因上调,例如 GATA2、PPARG、MSX2、DLX3、HAND1、GCM1、CDX2、ID2、ELF5、TCFAP2C 和 TEAD4,以及合成更分化的 TR 产物所需的基因,例如类固醇(HSD17B1、CYP11A1 和 STAR)、妊娠相关糖蛋白(PAG6)和选择细胞因子(IFND、IFNG 和 IL1B)。虽然 POU5F1 的表达相对于 iPS 细胞下调,但在持续传代的诱导 TR(iTR)细胞中并未沉默。与 iPS 细胞一样,iTR 细胞在延长传代过程中不会衰老,并且具有高端粒酶活性。在异种移植到免疫缺陷小鼠中时,iTR 细胞形成了主要由表达 TR 标志物的上皮层组成的非出血性畸胎瘤。当在促进类胚体形成的条件下培养时,iTR 细胞形成了由单层上皮组成的悬浮球体,其细胞通过桥粒样结构侧向连接。总之,将猪成纤维细胞重编程为 iPS 细胞会产生自我更新的 TR 细胞群体组成的集落,可能包含 TR 干细胞。

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