Nature Communications (Jul 2024)

Empowering the on-site detection of nucleic acids by integrating CRISPR and digital signal processing

  • Chang Yeol Lee,
  • Hyunho Kim,
  • Ismail Degani,
  • Hanna Lee,
  • Angel Sandoval,
  • Yoonho Nam,
  • Madeleine Pascavis,
  • Hyun Gyu Park,
  • Thomas Randall,
  • Amy Ly,
  • Cesar M. Castro,
  • Hakho Lee

DOI
https://doi.org/10.1038/s41467-024-50588-3
Journal volume & issue
Vol. 15, no. 1
pp. 1 – 12

Abstract

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Abstract Addressing the global disparity in cancer care necessitates the development of rapid and affordable nucleic acid (NA) testing technologies. This need is particularly critical for cervical cancer, where molecular detection of human papillomavirus (HPV) has emerged as an accurate screening method. However, implementing this transition in low- and middle-income countries has been challenging due to the high costs and centralized facilities required for current NA tests. Here, we present CreDiT (CRISPR Enhanced Digital Testing) for on-site NA detection. The CreDiT platform integrates i) a one-pot CRISPR strategy that simultaneously amplifies both target NAs and analytical signals and ii) a robust fluorescent detection based on digital communication (encoding/decoding) technology. These features enable a rapid assay (<35 minutes) in a single streamlined workflow. We demonstrate the sensitive detection of cell-derived HPV DNA targets down to single copies and accurate identification of HPV types in clinical cervical brushing specimens (n = 121).