AI Article Synopsis

  • The study reveals that the human CRH receptor type 2 (CRHR2) gene is regulated by multiple promoters and alternate splicing, affecting its overall expression.
  • Promoter activity is driven by specific flanking regions near the gene's first exons, and conserved promoter elements across species may influence how this gene functions in different tissues.
  • Novel transcripts from alternate splicing of the CRHR2beta indicate a complex regulatory mechanism, which has important implications for distinguishing between different CRHR2 variants and their functional roles.

Article Abstract

We demonstrate that multiple promoters and alternate splicing regulate expression of the human CRH receptor type 2 (CRHR2) gene. We show that flanking regions to the first exons drive promoter activity in both endogenously and nonendogenously expressing cell lines. Putative promoter elements have been identified that are conserved between species, including the comparison of CRHR2gamma in nonhuman primates that was previously known only in humans, which may be responsible for subtype tissue specific regulation. We have identified novel transcripts produced by alternate splicing of the first exon of CRHR2beta (beta1a) with various combinations of the 5' exons including a novel exon (beta1c) spliced to the common exons. The 5' structure of the gene permits many other combinations of alternate splicing that may arise as part of a regulatory mechanism controlling functional receptor expression. The 5'-untranslated region of the first exons has been extended; and 3' acceptor sites identified within the 5' untranslated region of CRHR2gamma and CRHR2alpha are used during alternate splicing of CRHR2beta upstream exons. This has important implications because various reports on the expression of CRHR2gamma and CRHR2alpha have been unable to discriminate between the functional receptor and CRHR2beta alternate splice variants. Only the described sequences upstream of the 3' splice site are unique to CRHR2gamma and CRHR2alpha.

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Source
http://dx.doi.org/10.1210/me.2002-0302DOI Listing

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