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生成无转基因猪中间型诱导多能干细胞。

Generation of transgene-free porcine intermediate type induced pluripotent stem cells.

机构信息

a Department of Veterinary and Animal Sciences, Faculty of Health and Medical Sciences , University of Copenhagen , Frederiksberg C , Denmark.

b Department of Veterinary Clinical Sciences, Faculty of Health and Medical Sciences , University of Copenhagen , Taastrup , Denmark.

出版信息

Cell Cycle. 2018;17(23):2547-2563. doi: 10.1080/15384101.2018.1548790. Epub 2018 Dec 3.

Abstract

Physiologically and anatomically, humans and pigs share many similarities, which make porcine induced pluripotent stem cells (piPSCs) very attractive for modeling human cell therapy as well as for testing safety of iPSC based cell replacement therapies. To date, several integrative and non-integrative strategies have been reported to successfully generate piPSCs, but all resulting piPSCs had integration of transgenes. The use of integrative methods has the disadvantage of potential lack of silencing or inappropriate re-activation of these genes during differentiation, as well as uncertainty regarding disruption of important genomic regions caused by integration. In our study, we performed a non-integrative vector based reprogramming approach using porcine fetal fibroblasts. The resulting four piPSC lines were positive for pluripotency marker and when subjected to in vitro and in vivo differentiation assays, all four lines formed embryoid bodies, capable to differentiate into all three germ layers, and three out of the four cell lines formed teratomas. PCR analysis on genomic and plasmid DNA revealed that the episomal vectors were undetectable in six out of eight subclones derived from one of the piPSC lines (piPSC1) above passage 20. These piPSCs could potentially be ideal cell lines for the generation of porcine in vitro and in vivo models. Furthermore, subsequent analyses of our new transgene independent piPSCs could provide novel insights on the genetic and epigenetic necessities to achieve and maintain piPSCs.

摘要

从生理学和解剖学角度来看,人类和猪有许多相似之处,这使得猪诱导多能干细胞(piPSCs)非常适合用于模拟人类细胞治疗以及测试基于 iPSC 的细胞替代疗法的安全性。迄今为止,已经报道了几种整合和非整合策略来成功生成 piPSCs,但所有生成的 piPSCs 都整合了转基因。整合方法的使用有以下缺点:在分化过程中这些基因可能无法沉默或重新激活不当,以及整合引起重要基因组区域破坏的不确定性。在我们的研究中,我们使用猪胎儿成纤维细胞进行了基于非整合载体的重编程方法。得到的四个 piPSC 系均为多能性标志物阳性,并且当进行体外和体内分化实验时,这四个系均形成了胚状体,能够分化为三个胚层,并且四个系中的三个形成了畸胎瘤。对来自上述 piPSC 系(piPSC1)的八个亚克隆中的六个的基因组和质粒 DNA 的 PCR 分析表明,上述 piPSC 系中的六个亚克隆中均无法检测到附加体载体。这些 piPSCs 可能是生成猪体外和体内模型的理想细胞系。此外,对我们新的非转基因独立 piPSCs 的后续分析可以提供关于实现和维持 piPSCs 的遗传和表观遗传必要性的新见解。

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