Detection of BRCA1/2 large genomic rearrangement including BRCA1 promoter-region deletions using next-generation sequencing
- Author(s)
- Eunhee Han; Jaeeun Yoo; Hyojin Chae; Seungok Lee; Do-Hoon Kim; Kwang Joong Kim; Yonggoo Kim; Myungshin Kim
- Keimyung Author(s)
- Kim, Do Hoon
- Department
- Dept. of Laboratory Medicine (진단검사의학)
- Journal Title
- Clinica chimica acta; international journal of clinical chemistry
- Issued Date
- 2020
- Volume
- 505
- Keyword
- BRCA1; BRCA2; Next-generation sequencing; Single-nucleotide variations; Large genomic rearrangements; Copy-number variations
- Abstract
- Background:
Germline mutations in BRCA1 and BRCA2 (BRCA1/2) have been conventionally analyzed by Sanger sequencing and multiplex ligation-dependent probe amplification (MLPA). Nowadays, next-generation sequencing (NGS) is increasingly being used in clinical genetics. The aim of this study was to evaluate the performance of NGS BRCA1/2 assays by comparing them with the conventional method.
Materials and methods:
We did BRCA1/2 NGS assays of 108 breast and/or ovarian cancer patients whose BRCA1/2 mutation had been previously analyzed by Sanger sequencing and MLPA using TruSeq Custom Amplicon Design AFP2. Single-nucleotide variations (SNVs) and small insertions or deletions (InDels) were evaluated. In addition, we analyzed large genomic rearrangements (LGRs) using a coverage-based algorithm as well as a revised BRCA1/2 NGS assay (BRCAaccuTest PLUS), which additionally covered a BRCA1 promoter region.
Results:
The NGS BRCA1/2 assay detected all 20 SNVs and 21 small InDels in 56 patients. Among seven LGRs detected by MLPA, six exonic LGRs were well identified by both NGS BRCA1/2 assays. One pathogenic LGR, located on a BRCA1 promoter region, was successfully identified using revised BRCAaccuTestPLUS.
Conclusions:
These results indicated that an NGS BRCA1/2 assay could detect most LGRs including BRCA1 promoter-region deletion as well as SNVs and small InDels. Therefore, it was applicable to clinical BRCA1/2 mutation tests.
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