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Mutation Analysis of the Entire PKD1 Gene: Genetic and Diagnostic Implications

包装D1 遗传学 生物 错义突变 无义突变 基因 基因座(遗传学) 突变率 外显子 基因突变 编码区 突变 多囊肾病 分子生物学
作者
Sandro Rossetti,Lana Strmecki,Vicki Gamble,Sarah Burton,Vicky Sneddon,Belén Peral,Sushmita Roy,Ayşı̇n Bakkaloğlu,Radovan Komel,Christopher G. Winearls,Peter C. Harris
出处
期刊:American Journal of Human Genetics [Elsevier BV]
卷期号:68 (1): 46-63 被引量:200
标识
DOI:10.1086/316939
摘要

Mutation screening of the major autosomal dominant polycystic kidney disease (ADPKD) locus, PKD1, has proved difficult because of the large transcript and complex reiterated gene region. We have developed methods, employing long polymerase chain reaction (PCR) and specific reverse transcription-PCR, to amplify all of the PKD1 coding area. The gene was screened for mutations in 131 unrelated patients with ADPKD, using the protein-truncation test and direct sequencing. Mutations were identified in 57 families, and, including 24 previously characterized changes from this cohort, a detection rate of 52.3% was achieved in 155 families. Mutations were found in all areas of the gene, from exons 1 to 46, with no clear hotspot identified. There was no significant difference in mutation frequency between the single-copy and duplicated areas, but mutations were more than twice as frequent in the 3' half of the gene, compared with the 5' half. The majority of changes were predicted to truncate the protein through nonsense mutations (32%), insertions or deletions (29.6%), or splicing changes (6.2%), although the figures were biased by the methods employed, and, in sequenced areas, approximately 50% of all mutations were missense or in-frame. Studies elsewhere have suggested that gene conversion may be a significant cause of mutation at PKD1, but only 3 of 69 different mutations matched PKD1-like HG sequence. A relatively high rate of new PKD1 mutation was calculated, 1.8x10-5 mutations per generation, consistent with the many different mutations identified (69 in 81 pedigrees) and suggesting significant selection against mutant alleles. The mutation detection rate, in this study, of >50% is comparable to that achieved for other large multiexon genes and shows the feasibility of genetic diagnosis in this disorder.
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