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Simple and efficient method for generation of induced pluripotent stem cells using piggyBac transposition of doxycycline-inducible factors and an EOS reporter system.

机译:使用强力霉素诱导因子的piggyBac换位和EOS报告系统,简单有效地生成诱导多能干细胞的方法。

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摘要

PiggyBac (PB) transposition of reprogramming factors (Oct3/4 (O), Sox2 (S), Klf4 (K) and c-Myc) is a safe, nonviral method for generating induced pluripotent stem cells (iPSCs). However, compared with retroviral methods, the reprogramming efficiency of the PB-mediated methods is relatively low. In this study, we describe a simple and efficient system for generating high-quality iPSCs by a single transfection of multiple plasmids that does not require the use of a virus, special instruments or skilled techniques. To improve reprogramming efficiency, we modified the components of the polycistronic 2A vectors used in this study and also investigated the combination of another reprogramming-related factor (L-Myc). By simultaneous transposition of multiple PB vectors containing an EOS (early transposon promoter and Oct3/4 and Sox2 enhancers) reporter and modified polycistronic doxycycline (Dox)-inducible factors, we reprogrammed mouse somatic cells with an efficiency higher than is usually obtained with retroviral methods and we established some iPSC lines that contributed highly to chimeras. By using the Dox-inducible system, we also showed that the appropriate elimination of exogenous-factor expression at appropriate time accelerated the induction of Oct3/4 when a combination of OKS and c-Myc vectors were used.
机译:重编程因子(Oct3 / 4(O),Sox2(S),Klf4(K)和c-Myc)的PiggyBac(PB)转座是一种安全,非病毒的方法,用于产生诱导性多能干细胞(iPSC)。但是,与逆转录病毒方法相比,PB介导的方法的重编程效率相对较低。在这项研究中,我们描述了一种简单高效的系统,可通过一次转染多个质粒来生成高质量的iPSC,而无需使用病毒,专用仪器或熟练技术。为了提高重编程效率,我们修改了本研究中使用的多顺反子2A载体的成分,并研究了另一个与重编程相关的因子(L-Myc)的组合。通过同时转置包含EOS(早期转座子启动子和Oct3 / 4和Sox2增强子)报道基因和修饰的多顺反子多西环素(Dox)诱导因子的多个PB载体,我们以比通常使用逆转录病毒方法更高的效率对小鼠体细胞进行了重新编程我们建立了一些iPSC产品线,这些产品对嵌合体起到了很大的作用。通过使用Dox诱导系统,我们还显示,当使用OKS和c-Myc载体结合使用时,在适当的时间适当消除外源因子表达可加速Oct3 / 4的诱导。

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