p53 isoforms regulate aging- and tumor-associated replicative senescence in T lymphocytes
Abdul M. Mondal, … , David P. Lane, Curtis C. Harris
Abdul M. Mondal, … , David P. Lane, Curtis C. Harris
Published November 15, 2013
Citation Information: J Clin Invest. 2013;123(12):5247-5257. https://doi.org/10.1172/JCI70355.
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Research Article Aging

p53 isoforms regulate aging- and tumor-associated replicative senescence in T lymphocytes

Abstract

Cellular senescence contributes to aging and decline in tissue function. p53 isoform switching regulates replicative senescence in cultured fibroblasts and is associated with tumor progression. Here, we found that the endogenous p53 isoforms Δ133p53 and p53β are physiological regulators of proliferation and senescence in human T lymphocytes in vivo. Peripheral blood CD8+ T lymphocytes collected from healthy donors displayed an age-dependent accumulation of senescent cells (CD28CD57+) with decreased Δ133p53 and increased p53β expression. Human lung tumor-associated CD8+ T lymphocytes also harbored senescent cells. Cultured CD8+ blood T lymphocytes underwent replicative senescence that was associated with loss of CD28 and Δ133p53 protein. In poorly proliferative, Δ133p53-low CD8+CD28 cells, reconstituted expression of either Δ133p53 or CD28 upregulated endogenous expression of each other, which restored cell proliferation, extended replicative lifespan and rescued senescence phenotypes. Conversely, Δ133p53 knockdown or p53β overexpression in CD8+CD28+ cells inhibited cell proliferation and induced senescence. This study establishes a role for Δ133p53 and p53β in regulation of cellular proliferation and senescence in vivo. Furthermore, Δ133p53-induced restoration of cellular replicative potential may lead to a new therapeutic paradigm for treating immunosenescence disorders, including those associated with aging, cancer, autoimmune diseases, and HIV infection.

Authors

Abdul M. Mondal, Izumi Horikawa, Sharon R. Pine, Kaori Fujita, Katherine M. Morgan, Elsa Vera, Sharlyn J. Mazur, Ettore Appella, Borivoj Vojtesek, Maria A. Blasco, David P. Lane, Curtis C. Harris

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Figure 1

Senescent phenotypes in CD28CD57+ subsets of CD8+ T lymphocytes in vivo.

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Senescent phenotypes in CD28–CD57+ subsets of CD8+ T lymphocytes in vivo...
(A) CD28+CD57 subsets decreased and CD28CD57+ subsets increased with donor age. (B) High-throughput quantitative FISH revealed shortened telomeres in CD28CD57+ subsets. n represents total number of telomere spots analyzed per subset. (C) Summary of SA-β-gal activity (donors 4, 6, and 7). (D) Representative images for HP1-γ foci by immunofluorescence staining (donor 4). (E) Quantitative analysis of HP1-γ foci per cell (donors 4, 6, and 7). (F) Representative images for γ-H2AX foci (donor 26). Irradiated (2 Gy) CD28+CD57 cells were used as a positive control. IR, irradiation. (G) Summary of γ-H2AX foci per cell (donors 26–28). (H) Quantitative RT-PCR analysis for SASP factors (donors 1–6). B2M was used for normalization. Data are mean ± SEM (B) or mean ± SD (C, E, G, and H). Scale bars: 5 μm (D and F). *P < 0.05; **P < 0.01; ***P < 0.001.