Study on the germline mutation of MSH6 gene in Chinese hereditary nonpolyposis colorectal cancer pedigrees using PCR based sequencing.

Shi-yan Yan; Xiao-yan Zhou; San-jun Cai; Bao-hua YU; Tai-ming Zhang; Xiao-mei LI; Yong-ming LU; Heng-hua Zhou; Shan-jing MO; Xiang DU; Da-ren Shi

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Study on the germline mutation of MSH6 gene in Chinese hereditary nonpolyposis colorectal cancer pedigrees using PCR based sequencing.

Author: Shi-yan YAN ¹ ; Xiao-yan ZHOU ; San-jun CAI ; Bao-hua YU ; Tai-ming ZHANG ; Xiao-mei LI ; Yong-ming LU ; Heng-hua ZHOU ; Shan-jing MO ; Xiang DU ; Da-ren SHI
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1. Department of Pathology, Cancer Hospital, Fudan University, Shanghai, 200032 PR China.
Publication Type:Journal Article
MeSH: Adult; Asian Continental Ancestry Group; genetics; Base Pair Mismatch; genetics; Colorectal Neoplasms, Hereditary Nonpolyposis; genetics; pathology; DNA Mutational Analysis; DNA Repair Enzymes; genetics; Female; Germ-Line Mutation; genetics; Humans; Male; Middle Aged; MutS DNA Mismatch-Binding Protein; genetics; MutS Homolog 2 Protein; genetics; Pedigree; Polymerase Chain Reaction
From: Chinese Journal of Medical Genetics 2007;24(6):640-645
CountryChina
Language:Chinese
Abstract:
OBJECTIVETo detect the germline mutation of mismatch repair gene (MSH6) in hereditary nonpolyposis colorectal cancer (HNPCC) kindreds fulfilling different clinical criteria.
METHODSThe germline mutations of MSH6 gene were detected by PCR based DNA sequencing in 39 unrelated HNPCC probands fulfilling different clinical criteria in which MSH2 and MLH1 mutations were excluded. The exons with missense mutations were analyzed using PCR sequencing in the germline genomic DNA of 137 healthy persons. The expression of MSH6 protein was detected by Envision immunohistochemistry staining in the tumor tissues of the mutational probands.
RESULTSSix germline mutations of MSH6 gene were detected in 39 probands of Chinese HNPCC kindreds, and the mutations distributed in the exon 4, 6, 9 and 10. Four out of six mutations were missense mutation, one was nonsense mutation and the remaining one was insertion mutation in splice site. The results of sequecing for the exons with above four missense mutations in 137 healthy persons' genomic DNA showed that 5 of 137 persons had the missense mutation of c.3488 A to T at codon 1163 of the 6th exon. The mutational rate was approximately 3.65% (5/137), so the mutation could be a single nucleotide polymorphism (SNP). The remaining missense mutations were not found in any germline genomic DNA of 137 healthy persons. Positive expression of MSH6 protein had been identified in the tumor of the SNP proband while the tumors had negative MSH6 protein expression in the rest probands of germline mutation MSH6 gene. The types of mutations and their potential significance were determined by comparing the following databases: http://www.ncbi.nlm.nih.gov/, http://www.ensembl.org/homo-sapies, and http://www.insight-group.org. Five out of the six mutations had not been reported previously and they were new pathological mutations, the rest one was a new SNP.
CONCLUSIONGermline mutations of MSH6 gene may play an important role in Chinese HNPCC kindreds fulfilling different clinical criteria. It is necessary to analyze the germline mutations of MSH6 gene using sequencing to identify HNPCC families in the probands in which MSH2 and MLH1 mutation were excluded.