Intronic alterations in BRCA1 and BRCA2: effect on mRNA splicing fidelity and expression

Germline mutations in the human breast cancer susceptibility genes BRCA1 and BRCA2 account for the majority of hereditary breast and ovarian cancer. In spite of the large number of sequence variants identified in BRCA1 and BRCA2 mutation analyses, many of these genetic alterations are still classifi...

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Bibliographic Details
Published in:Human mutation 2006-05, Vol.27 (5), p.427-435
Main Authors: Chen, Xiaowei, Truong, Tuyet-Trinh N., Weaver, JoEllen, Bove, Betsy A., Cattie, Kimberly, Armstrong, Brock A., Daly, Mary B., Godwin, Andrew K.
Format: Article
Language:English
Subjects:
Antimetabolites, Antineoplastic - pharmacology
Base Sequence
BRCA1
BRCA1 Protein - chemistry
BRCA1 Protein - genetics
BRCA2
BRCA2 Protein - chemistry
BRCA2 Protein - genetics
breast cancer
Cell Line
DNA Mutational Analysis
Female
Humans
Introns
Molecular Sequence Data
Mutation
NMD
nonsense-mediated mRNA decay
ovarian cancer
Polymorphism, Genetic
Puromycin - pharmacology
RNA Splice Sites
RNA Splicing
RNA, Messenger - metabolism
Sequence Analysis, Protein
splicing
variants of unknown significance
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Summary:Germline mutations in the human breast cancer susceptibility genes BRCA1 and BRCA2 account for the majority of hereditary breast and ovarian cancer. In spite of the large number of sequence variants identified in BRCA1 and BRCA2 mutation analyses, many of these genetic alterations are still classified as variants of unknown significance (VUS). In this study, we evaluated 12 BRCA1/2 intronic variants in order to differentiate their pathogenic or polymorphic effects on the mRNA splicing process. We detected the existence of aberrant splicing in three BRCA1 variants (c.301‐2delA/IVS6‐2delA, c.441+1G>A/IVS7+1G>A, and c.4986+6T>G/IVS16+6T>G) and two BRCA2 variants (c.8487+1G>A/IVS19+1G>A and c.8632‐2A>G/IVS20‐2A>G). All but one of the aberrant transcripts arise from mutations affecting the conserved splice acceptor or donor sequences and all would be predicted to result in expression of truncated BRCA1 or BRCA2 proteins. However, we demonstrated that four of these splice‐site mutations (i.e., c.301‐2delA, c.441+1G>A, c.4986+6T>G, and c.8632‐2A>G) with premature termination codons were highly unstable and were unlikely to encode for abundant expression of a mutant protein. Three variants of BRCA1 (c.212+3A>G/IVS5+3A>G, c.593+8A>G/IVS9+8A>G, and c.4986‐20A>G/IVS16‐20A>G) and four variants of BRCA2 (c.516‐19C>T/IVS6‐19C>T, c.7976‐4_7976_3delTT/IVS17‐4delTT, c.8487+19A>G/IVS19+19A>G, and c.9256‐ 18C>A/IVS24‐ 18C>A) in our studies show no effects on the normal splicing process, and they are considered to be benign polymorphic alterations. Our studies help to clarify the aberrant splicing in BRCA1 and BRCA2 as well as provide information that can be used clinically to help counsel breast/ovarian cancer prone families. Hum Mutat 27(5), 427–435, 2006. Published 2006 Wiley‐Liss, Inc.
ISSN:1059-7794
1098-1004
DOI:10.1002/humu.20319