Abstract

When human fibroblasts from different donors are grown in vitro, only a small fraction of the variation in their finite replicative capacity is explained by the chronological age of the donor. Because we had previously shown that telomeres, the terminal guanine-rich sequences of chromosomes, shorten throughout the life-span of cultured cells, we wished to determine whether variation in initial telomere length would account for the unexplained variation in replicative capacity. Analysis of cells from 31 donors (aged 0-93 yr) indicated relatively weak correlations between proliferative ability and donor age (m = -0.2 doubling per yr; r = -0.42; P = 0.02) and between telomeric DNA and donor age (m = -15 base pairs per yr; r = -0.43; P = 0.02). However, there was a striking correlation, valid over the entire age range of the donors, between replicative capacity and initial telomere length (m = 10 doublings per kilobase pair; r = 0.76; P = 0.004), indicating that cell strains with shorter telomeres underwent significantly fewer doublings than those with longer telomeres. These observations suggest that telomere length is a biomarker of somatic cell aging in humans and are consistent with a causal role for telomere loss in this process. We also found that fibroblasts from Hutchinson-Gilford progeria donors had short telomeres, consistent with their reduced division potential in vitro. In contrast, telomeres from sperm DNA did not decrease with age of the donor, suggesting that a mechanism for maintaining telomere length, such as telomerase expression, may be active in germ-line tissue.

Keywords

TelomereTelomeraseBiologySomatic cellProgeriaCell divisionMolecular biologyGeneticsChromosomeDNAAndrologyCellGeneMedicine

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Year
1992
Type
article
Volume
89
Issue
21
Pages
10114-10118
Citations
2205
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Richard Allsopp, Homayoun Vaziri, Cam Patterson et al. (1992). Telomere length predicts replicative capacity of human fibroblasts.. Proceedings of the National Academy of Sciences , 89 (21) , 10114-10118. https://doi.org/10.1073/pnas.89.21.10114

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DOI
10.1073/pnas.89.21.10114