Genome Biology (Jun 2020)

Direct-seq: programmed gRNA scaffold for streamlined scRNA-seq in CRISPR screen

  • Qingkai Song,
  • Ke Ni,
  • Min Liu,
  • Yini Li,
  • Lixia Wang,
  • Yingying Wang,
  • Yingzheng Liu,
  • Zhenxing Yu,
  • Yinyao Qi,
  • Zhike Lu,
  • Lijia Ma

DOI
https://doi.org/10.1186/s13059-020-02044-w
Journal volume & issue
Vol. 21, no. 1
pp. 1 – 15

Abstract

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Abstract CRISPR-based genome perturbation provides a new avenue to conveniently change DNA sequences, transcription, and epigenetic modifications in genetic screens. However, it remains challenging to assay the complex molecular readouts after perturbation at high resolution and at scale. By introducing an A/G mixed capture sequence into the gRNA scaffold, we demonstrate that gRNA transcripts could be directly reverse transcribed by poly (dT) primer together with the endogenous mRNA, followed by high-content molecular phenotyping in scRNA-seq (Direct-seq). With this method, the CRISPR perturbation and its transcriptional readouts can be profiled together in a streamlined workflow.