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A new function of glucocorticoid receptor: regulation of mRNA stability

Authors
Park, Ok HyunDo, EunjinKim, Yoon Ki
Issue Date
31-Jul-2015
Publisher
KOREAN SOCIETY BIOCHEMISTRY & MOLECULAR BIOLOGY
Keywords
Glucocorticoid receptor; mRNA decay; PNRC2; UPF1; Chemotaxis
Citation
BMB REPORTS, v.48, no.7, pp.367 - 368
Indexed
SCIE
SCOPUS
KCI
Journal Title
BMB REPORTS
Volume
48
Number
7
Start Page
367
End Page
368
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/92973
DOI
10.5483/BMBRep.2015.48.7.131
ISSN
1976-6696
Abstract
It has long been thought that glucocorticoid receptor (GR) functions as a DNA-binding transcription factor in response to its ligand (a glucocorticoid) and thus regulates various cellular and physiological processes. It is also known that GR can bind not only to DNA but also to mRNA; this observation points to the possible role of GR in mRNA metabolism. Recent data revealed a molecular mechanism by which binding of GR to target mRNA elicits rapid mRNA degradation. GR binds to specific RNA sequences regardless of the presence of a ligand. In the presence of a ligand, however, the mRNA-associated GR can recruit PNRC2 and UPF1, both of which are specific factors involved in nonsense-mediated mRNA decay (NMD). PNRC2 then recruits the decapping complex, consequently promoting mRNA degradation. This mode of mRNA decay is termed "GR-mediated mRNA decay" (GMD). Further research demonstrated that GMD plays a critical role in chemotaxis of immune cells by targeting CCL2 mRNA. All these observations provide molecular insights into a previously unappreciated function of GR in posttranscriptional regulation of gene expression.
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