Universal DNA array detection of small insertions and deletions in BRCA1 and BRCA2. Academic Article uri icon

Overview

abstract

  • Array-based mutation detection methodology typically relies on direct hybridization of the fluorescently labeled query sequence to surface-bound oligonucleotide probes. These probes contain either small sequence variations or perfect-match sequence. The intensity of fluorescence bound to each oligonucleotide probe is intended to reveal which sequence is perfectly complementary to the query sequence. However, these approaches have not always been successful, especially for detection of small frameshift mutations. Here we describe a multiplex assay to detect small insertions and deletions by using a modified PCR to evenly amplify each amplicon (PCR/PCR), followed by ligase detection reaction (LDR). Mutations were identified by screening reaction products with a universal DNA microarray, which uncouples mutation detection from array hybridization and provides for high sensitivity. Using the three BRCA1 and BRCA2 founder mutations in the Ashkenazi Jewish population (BRCA1 185delAG; BRCA1 5382insC; BRCA2 6174delT) as a model system, the assay readily detected these mutations in multiplexed reactions. Our results demonstrate that universal microarray analysis of PCR/PCR/LDR products permits rapid identification of small insertion and deletion mutations in the context of both clinical diagnosis and population studies.

publication date

  • May 1, 2000

Research

keywords

  • BRCA1 Protein
  • Frameshift Mutation
  • Jews
  • Neoplasm Proteins
  • Oligonucleotide Array Sequence Analysis
  • Transcription Factors

Identity

Scopus Document Identifier

  • 0034121447

Digital Object Identifier (DOI)

  • 10.1038/75452

PubMed ID

  • 10802632

Additional Document Info

volume

  • 18

issue

  • 5