Telomere length set point regulation in human pluripotent stem cells critically depends on the shelterin protein TPP1

Telomere maintenance is essential for the long-term proliferation of human pluripotent stem cells, while their telomere length set point determines the proliferative capacity of their differentiated progeny. The shelterin protein TPP1 is required for telomere stability and elongation, but its role i...

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Veröffentlicht in:Molecular biology of the cell 2020-11, Vol.31 (23), p.2583-2596
Hauptverfasser: Boyle, John M, Hennick, Kelsey M, Regalado, Samuel G, Vogan, Jacob M, Zhang, Xiaozhu, Collins, Kathleen, Hockemeyer, Dirk
Format: Artikel
Sprache:eng
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Zusammenfassung:Telomere maintenance is essential for the long-term proliferation of human pluripotent stem cells, while their telomere length set point determines the proliferative capacity of their differentiated progeny. The shelterin protein TPP1 is required for telomere stability and elongation, but its role in establishing a telomere length set point remains elusive. Here, we characterize the contribution of the shorter isoform of TPP1 (TPP1S) and the amino acid L104 outside the TEL patch, TPP1's telomerase interaction domain, to telomere length control. We demonstrate that cells deficient for TPP1S (TPP1S knockout [KO]), as well as the complete TPP1 KO cell lines, undergo telomere shortening. However, TPP1S KO cells are able to stabilize short telomeres, while TPP1 KO cells die. We compare these phenotypes with those of TPP1 mutant cells, which have short and stable telomeres similar to the TPP1S KO. In contrast to TPP1S KO cells, TPP1 cells respond to increased telomerase levels and maintain protected telomeres. However, TPP1 shows altered sensitivity to expression changes of shelterin proteins suggesting the mutation causes a defect in telomere length feedback regulation. Together this highlights TPP1 as the first shelterin mutant engineered at the endogenous locus of human stem cells with an altered telomere length set point.
ISSN:1059-1524
1939-4586
DOI:10.1091/MBC.E19-08-0447