4.8 Article

Reduced nuclear export of HuR mRNA by HuR is linked to the loss of HuR in replicative senescence

Journal

NUCLEIC ACIDS RESEARCH
Volume 38, Issue 5, Pages 1547-1558

Publisher

OXFORD UNIV PRESS
DOI: 10.1093/nar/gkp1114

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Funding

  1. Major State Basic Research Development Program of China [2007CB507400]
  2. National Science Foundation of China [30672202, 30621002]
  3. Ministry of Education of People's Republic of China [B07001]
  4. National Institute on Aging-IRP, National Institutes of Health

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The RNA-binding protein, HuR, associates with the HuR mRNA, but the consequences of this interaction are unknown. Here, we use human diploid fibroblasts (HDFs) and cervical carcinoma cells to study this regulatory paradigm. Ectopic overexpression of HuR potently enhanced the translation and cytoplasmic levels of endogenous HuR, but did not affect HuR mRNA levels. Inhibition of CRM1 function by Lemptomycin B or by knockdown of CRM1 greatly diminished the cytoplasmic levels of endogenous HuR mRNA and hence blocked the induction of endogenous HuR by exogenous HuR. Further studies showed that HuR interacted with the 3'-untranslated region (UTR) of HuR and that overexpression of HuR increased the cytoplasmic levels of a chimeric luciferase-HuR 3'-UTR reporter transcript, as well as luciferase activity; conversely, HuR knockdown reduced both parameters. Moreover, the loss of HuR in senescent, late-passage HDFs was accompanied by a reduced cytoplasmic presence of endogenous HuR mRNA, ectopic Luc-HuR-3'UTR reporter transcript, and luciferase activity relative to what was observed in young, early-passage cells. Our results reveal a positive feedback mechanism for the regulation of HuR, which may play an important role in the regulation of HuR during replicative senescence.

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