4.8 Article

CRISPR-mediated live imaging of genome editing and transcription

Journal

SCIENCE
Volume 365, Issue 6459, Pages 1301-+

Publisher

AMER ASSOC ADVANCEMENT SCIENCE
DOI: 10.1126/science.aax7852

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Funding

  1. NSF GRFP
  2. Li Ka Shing Foundation
  3. National Institutes of Health Common Fund 4D Nucleome Program [U01 EB021240]
  4. Pew Scholar Foundation
  5. Alfred P. Sloan Foundation

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We report a robust, versatile approach called CRISPR live-cell fluorescent in situ hybridization (LiveFISH) using fluorescent oligonucleotides for genome tracking in a broad range of cell types, including primary cells. An intrinsic stability switch of CRISPR guide RNAs enables LiveFISH to accurately detect chromosomal disorders such as Patau syndrome in prenatal amniotic fluid cells and track multiple loci in human T lymphocytes. In addition, LiveFISH tracks the real-time movement of DNA double-strand breaks induced by CRISPR-Cas9-mediated editing and consequent chromosome translocations. Finally, by combining Cas9 and Cas13 systems, LiveFISH allows for simultaneous visualization of genomic DNA and RNA transcripts in living cells. The LiveFISH approach enables real-time live imaging of DNA and RNA during genome editing, transcription, and rearrangements in single cells.

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