Abstract
Pluripotent stem cells (PSCs), including embryonic and induced pluripotent stem cells (iPSCs), show atypical cell cycle regulation characterized by a high proliferation rate and a shorter G1 phase compared with somatic cells. The mechanisms by which somatic cells remodel their cell cycle to achieve the high proliferation rate of PSCs during reprogramming are unclear. Here we identify that the Ink4 protein p18, which is expressed at high levels in somatic cells but at low levels in PSCs, is a roadblock to successful reprogramming. Mild inhibition of p18 expression enhances reprogramming efficiency, while ectopic expression of p18 completely blocks reprogramming. Mechanistic studies show that expression of wild-type p18, but not a p18D68N mutant which cannot inhibit Cdk4/6, down-regulates expression of Cdk4/6 target genes involved in DNA synthesis (TK, TS, DHFR, PCNA) and cell cycle regulation (CDK1 and CCNA2) and thus inhibits reprogramming. These results indicate that p18 blocks reprogramming by targeting Cdk4/6-mediated cell cycle regulation. Taken together, our results define a novel pathway that inhibits somatic cell reprogramming, and provide a new target to enhance reprogramming efficiency.
Highlights
Pluripotent stem cells (PSCs), including embryonic and induced pluripotent stem cells, show atypical cell cycle regulation characterized by a high proliferation rate and a shorter G1 phase compared with somatic cells
To screen for crucial cell cycle regulators that restrict reprogramming, mRNA expression data of different embryonic stem cells (ESCs) lines, induced pluripotent stem cells (iPSCs) lines and fibroblast lines were downloaded from the NCBI website (Supplementary Table 2)
We showed that p18 restricts somatic cell reprogramming by targeting the cyclin-dependent kinase (Cdk)[4] and Cdk[6] pathways
Summary
Pluripotent stem cells (PSCs), including embryonic and induced pluripotent stem cells (iPSCs), show atypical cell cycle regulation characterized by a high proliferation rate and a shorter G1 phase compared with somatic cells. Mechanistic studies show that expression of wild-type p18, but not a p18D68N mutant which cannot inhibit Cdk4/6, down-regulates expression of Cdk4/6 target genes involved in DNA synthesis (TK, TS, DHFR, PCNA) and cell cycle regulation (CDK1 and CCNA2) and inhibits reprogramming. These results indicate that p18 blocks reprogramming by targeting Cdk4/6-mediated cell cycle regulation. Ectopic expression of p18 leads to decreased expression of Cdk4/6 target genes involved in DNA synthesis and cell cycle regulation, and blocks reprogramming
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