Germline Sequencing of DNA Damage Repair Genes in Two Hereditary Prostate Cancer Cohorts Reveals New Disease Risk-Associated Gene Variants

被引:1
作者
Foley, Georgea R. [1 ]
Marthick, James R. [1 ]
Lucas, Sionne E. [1 ]
Raspin, Kelsie [1 ]
Banks, Annette [1 ]
Stanford, Janet L. [2 ]
Ostrander, Elaine A. [3 ]
Fitzgerald, Liesel M. [1 ]
Dickinson, Joanne L. [1 ]
机构
[1] Univ Tasmania, Menzies Inst Med Res, Hobart, Tas 7000, Australia
[2] Fred Hutchinson Canc Ctr, 1100 Fairview Ave N,M4-B874, Seattle, WA 98109 USA
[3] NIH, Natl Human Genome Res Inst, Canc Genet & Comparat Genom Branch, Bethesda, MD 20892 USA
基金
美国国家卫生研究院; 澳大利亚研究理事会;
关键词
rare high-risk genes; prostate cancer; DNA repair; genetic susceptibility; germline variants; MUTATIONS; EXPRESSION; FAMILIES;
D O I
10.3390/cancers16132482
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
Simple Summary An urgent demand exists to identify inherited genetic risk variants for prostate cancer (PrCa), particularly in DNA damage repair genes targetable with precision medicine-based strategies. Though the most heritable common cancer, discovery of rare germline PrCa risk variants is hampered by their low frequency, even in sizeable population datasets. Through utilising two large, independent, familial PrCa resources and their likely enrichment of rare causative variants, we provide robust evidence for several novel risk variants in DNA damage repair genes.Abstract Rare, inherited variants in DNA damage repair (DDR) genes have a recognised role in prostate cancer (PrCa) susceptibility. In addition, these genes are therapeutically targetable. While rare variants are informing clinical management in other common cancers, defining the rare disease-associated variants in PrCa has been challenging. Here, whole-genome and -exome sequencing data from two independent, high-risk Australian and North American familial PrCa datasets were interrogated for novel DDR risk variants. Rare DDR gene variants (predicted to be damaging and present in two or more family members) were identified and subsequently genotyped in 1963 individuals (700 familial and 459 sporadic PrCa cases, 482 unaffected relatives, and 322 screened controls), and association analyses accounting for relatedness (MQLS) undertaken. In the combined datasets, rare ERCC3 (rs145201970, p = 2.57 x 10-4) and BRIP1 (rs4988345, p = 0.025) variants were significantly associated with PrCa risk. A PARP2 (rs200603922, p = 0.028) variant in the Australian dataset and a MUTYH (rs36053993, p = 0.031) variant in the North American dataset were also associated with risk. Evaluation of clinicopathological characteristics provided no evidence for a younger age or higher-grade disease at diagnosis in variant carriers, which should be taken into consideration when determining genetic screening eligibility criteria for targeted, gene-based treatments in the future. This study adds valuable knowledge to our understanding of PrCa-associated DDR genes, which will underpin effective clinical screening and treatment strategies.
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