Identification of Microdeletions in Candidate Genes for Cleft Lip and/or Palate

被引:48
|
作者
Shi, Min [2 ]
Mostowska, Adrianna [1 ,3 ]
Jugessur, Astanand [4 ]
Johnson, Marla K. [1 ]
Mansilla, Maria Adela [1 ]
Christensen, Kaare [5 ]
Lie, Rolv T. [6 ]
Wiicox, Allen J. [7 ]
Murray, Jeffrey C. [1 ]
机构
[1] Univ Iowa, Dept Pediat, Carver Coll Med, Iowa City, IA 52242 USA
[2] Natl Inst Environm Hlth Sci, Biostat Branch, NIH, Res Triangle Pk, NC USA
[3] Univ Med Sci, Dept Biochem & Mol Biol, PL-60781 Poznan, Poland
[4] Royal Childrens Hosp, Murdoch Childrens Res Inst, Melbourne, Vic, Australia
[5] Univ So Denmark, Inst Publ Hlth, DK-5000 Odense C, Denmark
[6] Univ Bergen, Dept Publ Hlth & Primary Hlth Care, Sect Epidemiol & Med Stat, Bergen, Norway
[7] Natl Inst Environm Hlth Sci, Epidemiol Branch, Res Triangle Pk, NC USA
关键词
cleft lip; cleft palate; microdeletion; SNP; CNV; candidate genes; MATERNAL SMOKING; HUMAN GENOME; ORAL CLEFTS; REGION;
D O I
10.1002/bdra.20571
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
BACKGROUND: Genome-wide association studies are now used routinely to identify genes implicated in complex traits. The panels used for such analyses can detect single nucleotide polymorphisms and copy number variants, both of which may help to identify small deleted regions of the genome that may contribute to a particular disease. METHODS: We performed a candidate gene analysis involving 1,221 SNPs in 333 candidate genes for orofacial clefting, using 2,823 samples from 725 two- and three-generation families with a proband having cleft lip with or without cleft palate. We used SNP genotyping, DNA sequencing, high-resolution DNA microarray analysis, and long-range PCR to confirm and characterize the deletion events. RESULTS: This dataset, had a high duplicate reproducibility rate (99.98%), high Mendelian consistency rate (99.93%), and low missing data rate (0.55%), which provided a powerful opportunity for deletion detection. Apparent Mendelian inconsistencies between parents and children suggested deletion events in 15 individuals in 11 genomic regions. We confirmed deletions involving CYP1B1, FGF10, SP8, SUMO1, TBX1, TFAP2A, and UGT7A1, including both de novo and familial cases. Deletions of SUMO1, TBX1, and TFAP2A are likely to be etiologic. CONCLUSIONS: These deletions suggest the potential roles of genes or regulatory elements contained within deleted regions in the etiology of clefting. Our analysis took advantage of genotypes from a candidate-gene-based SNP survey and proved to be an efficient analytical approach to interrogate genes potentially involved in clefting. This can serve as a model to find genes playing a role in complex traits in general. Birth Defects Research (Part A) 85:42-51, 2009. (C) 2009 Wiley-Liss, Inc.
引用
收藏
页码:42 / 51
页数:10
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