Alternative splicing of GTBP in normal human tissues

Hiromi O. Shiwaku; Shigeru Wakatsuki; Yuriko Mori; Shinichi Fukushige; Akira Horii

doi:10.1093/dnares/4.5.359

Alternative splicing of GTBP in normal human tissues

Hiromi O. Shiwaku, Shigeru Wakatsuki, Yuriko Mori, Shinichi Fukushige, Akira Horii

School of Medicine

Research output: Contribution to journal › Article › peer-review

1 Scopus citations

Abstract

GTBP is one of the functional homologues of the bacterial mismatch repair gene mutS, whose product forms a heterodimer with hMSH2 to bind to the mismatched region of double-stranded DNA. We determined the expression of the GTBP gene and found that two forms of the transcripts were ubiquitously expressed in normal human tissues. These transcripts, termed GTBP-N and GTBP-ALT, were generated by the alternative splicing machinery. These two transcripts share 3172 bp from the translation initiation codon that codes for 1057 amino acids. GTBP-ALT lacked a region that codes for a highly conserved region between GTBP-N, hMSH2, and hMSH3 in their C-termini.

Original language	English (US)
Pages (from-to)	359-362
Number of pages	4
Journal	DNA Research
Volume	4
Issue number	5
DOIs	https://doi.org/10.1093/dnares/4.5.359
State	Published - 1997

Keywords

Alternative splicing
DNA mismatch repair
GTBP

ASJC Scopus subject areas

Molecular Biology
Genetics

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10.1093/dnares/4.5.359

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title = "Alternative splicing of GTBP in normal human tissues",

abstract = "GTBP is one of the functional homologues of the bacterial mismatch repair gene mutS, whose product forms a heterodimer with hMSH2 to bind to the mismatched region of double-stranded DNA. We determined the expression of the GTBP gene and found that two forms of the transcripts were ubiquitously expressed in normal human tissues. These transcripts, termed GTBP-N and GTBP-ALT, were generated by the alternative splicing machinery. These two transcripts share 3172 bp from the translation initiation codon that codes for 1057 amino acids. GTBP-ALT lacked a region that codes for a highly conserved region between GTBP-N, hMSH2, and hMSH3 in their C-termini.",

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T1 - Alternative splicing of GTBP in normal human tissues

AU - Shiwaku, Hiromi O.

AU - Wakatsuki, Shigeru

AU - Mori, Yuriko

AU - Fukushige, Shinichi

AU - Horii, Akira

PY - 1997

Y1 - 1997

N2 - GTBP is one of the functional homologues of the bacterial mismatch repair gene mutS, whose product forms a heterodimer with hMSH2 to bind to the mismatched region of double-stranded DNA. We determined the expression of the GTBP gene and found that two forms of the transcripts were ubiquitously expressed in normal human tissues. These transcripts, termed GTBP-N and GTBP-ALT, were generated by the alternative splicing machinery. These two transcripts share 3172 bp from the translation initiation codon that codes for 1057 amino acids. GTBP-ALT lacked a region that codes for a highly conserved region between GTBP-N, hMSH2, and hMSH3 in their C-termini.

AB - GTBP is one of the functional homologues of the bacterial mismatch repair gene mutS, whose product forms a heterodimer with hMSH2 to bind to the mismatched region of double-stranded DNA. We determined the expression of the GTBP gene and found that two forms of the transcripts were ubiquitously expressed in normal human tissues. These transcripts, termed GTBP-N and GTBP-ALT, were generated by the alternative splicing machinery. These two transcripts share 3172 bp from the translation initiation codon that codes for 1057 amino acids. GTBP-ALT lacked a region that codes for a highly conserved region between GTBP-N, hMSH2, and hMSH3 in their C-termini.

KW - Alternative splicing

KW - DNA mismatch repair

KW - GTBP

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Alternative splicing of GTBP in normal human tissues

Abstract

Keywords

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