4.6 Review

Cancer Biomarkers Discovery of Methylation Modification With Direct High-Throughput Nanopore Sequencing

Journal

FRONTIERS IN GENETICS
Volume 12, Issue -, Pages -

Publisher

FRONTIERS MEDIA SA
DOI: 10.3389/fgene.2021.672804

Keywords

nanopore sequencing; cancer biomarker; Cas9 enrichment; DNA methylation; RNA methylation

Funding

  1. National Natural Science Foundation of China [82060524]
  2. Science and Technology Innovation Outstanding Young Talents Training Program of Jiangxi Province [20192BCBL23017]
  3. Youth Jinggang Scholars Program in Jiangxi Province

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Nanopore sequencing technology allows for direct detection of base modifications in DNA and RNA, compared to bisulfite sequencing. The CRISPR/Cas9-targeted enrichment nanopore sequencing techniques are simple and cost-effective, particularly when targeting specific genomic regions.
Cancer is a complex disease, driven by a combination of genetic and epigenetic alterations. DNA and RNA methylation modifications are the most common epigenetic events that play critical roles in cancer development and progression. Bisulfite converted sequencing is a widely used technique to detect base modifications in DNA methylation, but its main drawbacks lie in DNA degradation, lack of specificity, or short reads with low sequence diversity. The nanopore sequencing technology can directly detect base modifications in native DNA as well as RNA without harsh chemical treatment, compared to bisulfite sequencing. Furthermore, CRISPR/Cas9-targeted enrichment nanopore sequencing techniques are straightforward and cost-effective when targeting genomic regions are of interest. In this review, we mainly focus on DNA and RNA methylation modification detection in cancer with the current nanopore sequencing approaches. We also present the respective strengths, weaknesses of nanopore sequencing techniques, and their future translational applications in identification of epigenetic biomarkers for cancer detection and prognosis.

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