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Cooperative actions of Tra2 alpha with 9G8 and SRp30c in the RNA splicing of the gonadotropin-releasing hormone gene transcript

Authors
Park, EHan, JSon, GHLee, MSChung, SPark, SHPark, KLee, KHChoi, SSeong, JYKim, K
Issue Date
6-1월-2006
Publisher
AMER SOC BIOCHEMISTRY MOLECULAR BIOLOGY INC
Citation
JOURNAL OF BIOLOGICAL CHEMISTRY, v.281, no.1, pp.401 - 409
Indexed
SCIE
SCOPUS
Journal Title
JOURNAL OF BIOLOGICAL CHEMISTRY
Volume
281
Number
1
Start Page
401
End Page
409
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/123170
DOI
10.1074/jbc.M505814200
ISSN
0021-9258
Abstract
In earlier studies, we demonstrated that excision of the first intron ( intron A) from the gonadotropin-releasing hormone ( GnRH) transcript is highly cell type- and developmental stage-specific. The removal of GnRH intron A requires exonic splicing enhancers on exons 3 and 4 (ESE3 and ESE4, respectively). Tra2 alpha, a serine/arginine- rich (SR)- like protein, specifically binds to ESE4, although it requires additional nuclear co-factors for efficient removal of this intron. In the present study, we demonstrate the cooperative action of multiple SR proteins in the regulation of GnRH pre-mRNA splicing. SRp30c specifically binds to both ESE3 and ESE4, whereas 9G8 binds to an element in exon 3 and strongly enhances the excision of GnRH intron A in the presence of minimal amount of other nuclear components. Interestingly, Tra2 alpha can interact with either 9G8 or SRp30c, whereas no interaction between 9G8 and SRp30c is observed. Tra2 alpha has an additive effect on the RNA binding of these proteins. Overexpression or knock-down of these three proteins in cultured cells further suggests their essential role in intron A excision activities, and their presence in GnRH neurons of the mouse preoptic area further strengthens this possibility. Together, these results indicate that interaction of Tra2 alpha with 9G8 and SRp30c appears to be crucial for ESE-dependent GnRH pre-mRNA splicing, allowing efficient generation of mature mRNA in GnRH- producing cells.
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