AI Article Synopsis

  • * Researchers created a method using biotinylated DNA probes to capture viral genetic fragments, significantly improving the detection sensitivity of viral sequences compared to traditional approaches.
  • * This new method is cost-effective and versatile, enabling the study of proviruses’ transcriptional and epigenetic regulation, which has been difficult to investigate until now.

Article Abstract

The recent development and advancement of next-generation sequencing (NGS) technologies have enabled the characterization of the human genome at extremely high resolution. In the retrovirology field, NGS technologies have been applied to integration-site analysis and deep sequencing of viral genomes in combination with PCR amplification using virus-specific primers. However, virus-specific primers are not available for some epigenetic analyses, like chromatin immunoprecipitation sequencing (ChIP-seq) assays. Viral sequences are poorly detected without specific PCR amplification because proviral DNA is very scarce compared to human genomic DNA. Here, we have developed and evaluated the use of biotinylated DNA probes for the capture of viral genetic fragments from a library prepared for NGS. Our results demonstrated that viral sequence detection was hundreds or thousands of times more sensitive after enrichment, enabling us to reduce the economic burden that arises when attempting to analyze the epigenetic landscape of proviruses by NGS. In addition, the method is versatile enough to analyze proviruses that have mismatches compared to the DNA probes. Taken together, we propose that this approach is a powerful tool to clarify the mechanisms of transcriptional and epigenetic regulation of retroviral proviruses that have, until now, remained elusive.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4913254PMC
http://dx.doi.org/10.1038/srep28324DOI Listing

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