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An inducible CRISPR-ON system for controllable gene activation in human pluripotent stem cells

机译:诱导型CRISPR-ON系统,用于人类多能干细胞中可控的基因激活

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摘要

Human pluripotent stem cells (hPSCs) are an important system to study early human development, model human diseases, and develop cell replacement therapies. However, genetic manipulation of hPSCs is challenging and a method to simultaneously activate multiple genomic sites in a controllable manner is sorely needed. Here, we constructed a CRISPR-ON system to efficiently upregulate endogenous genes in hPSCs. A doxycycline (Dox) inducible dCas9-VP64-p65-Rta ( dCas9-VPR ) transcription activator and a reverse Tet transactivator (rtTA) expression cassette were knocked into the two alleles of the AAVS1 locus to generate an iVPR hESC line. We showed that the dCas9-VPR level could be precisely and reversibly controlled by the addition and withdrawal of Dox. Upon transfection of multiplexed gRNA plasmid targeting the NANOG promoter and Dox induction, we were able to control NANOG gene expression from its endogenous locus. Interestingly, an elevated NANOG level promoted na?ve pluripotent gene expression, enhanced cell survival and clonogenicity, and enabled hESCs to integrate with the inner cell mass (ICM) of mouse blastocysts in vitro . Thus, iVPR cells provide a convenient platform for gene function studies as well as high-throughput screens in hPSCs.
机译:人多能干细胞(hPSC)是研究早期人类发育,为人类疾病建模和开发细胞替代疗法的重要系统。然而,hPSC的遗传操作具有挑战性,因此迫切需要一种以可控方式同时激活多个基因组位点的方法。在这里,我们构建了一个CRISPR-ON系统来有效上调hPSC中的内源基因。将强力霉素(Dox)诱导的dCas9-VP64-p65-Rta(dCas9-VPR)转录激活因子和反向Tet反激活因子(rtTA)表达盒敲入AAVS1基因座的两个等位基因,以生成iVPR hESC系。我们表明,通过添加和撤除Dox可以精确且可逆地控制dCas9-VPR水平。转染针对NANOG启动子和Dox诱导的多重gRNA质粒后,我们能够从其内源性基因位点控制NANOG基因的表达。有趣的是,升高的NANOG水平促进了幼稚多能基因表达,增强了细胞存活和克隆形成性,并使hESCs能够在体外与小鼠胚泡的内部细胞团(ICM)整合。因此,iVPR细胞为hPSC中的基因功能研究以及高通量筛选提供了方便的平台。

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