AI Article Synopsis

  • Array-based comparative genomic hybridization using bacterial artificial chromosomes has been effective in detecting subtle DNA copy-number variations relevant to health and disease.
  • Improvements in technology have led to new microarray platforms with higher resolution and a higher number of oligonucleotide targets.
  • A novel statistical power analysis method revealed that high-density oligonucleotide platforms outperform BAC platforms for detecting copy-number variations under 1 Mb, though all platforms struggle with variations below 100 kb and show different sensitivities to gains and losses.

Article Abstract

Recently, comparative genomic hybridization onto bacterial artificial chromosome (BAC) arrays (array-based comparative genomic hybridization) has proved to be successful for the detection of submicroscopic DNA copy-number variations in health and disease. Technological improvements to achieve a higher resolution have resulted in the generation of additional microarray platforms encompassing larger numbers of shorter DNA targets (oligonucleotides). Here, we present a novel method to estimate the ability of a microarray to detect genomic copy-number variations of different sizes and types (i.e. deletions or duplications). We applied our method, which is based on statistical power analysis, to four widely used high-density genomic microarray platforms. By doing so, we found that the high-density oligonucleotide platforms are superior to the BAC platform for the genome-wide detection of copy-number variations smaller than 1 Mb. The capacity to reliably detect single copy-number variations below 100 kb, however, appeared to be limited for all platforms tested. In addition, our analysis revealed an unexpected platform-dependent difference in sensitivity to detect a single copy-number loss and a single copy-number gain. These analyses provide a first objective insight into the true capacities and limitations of different genomic microarrays to detect and define DNA copy-number variations.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC2779891PMC
http://dx.doi.org/10.1093/dnares/dsm002DOI Listing

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