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The next generation of CRISPR-Cas technologies and applications

Journal

NATURE REVIEWS MOLECULAR CELL BIOLOGY
Volume 20, Issue 8, Pages 490-507

Publisher

NATURE PORTFOLIO
DOI: 10.1038/s41580-019-0131-5

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Funding

  1. Allen Distinguished Investigator Award from the Paul G. Allen Frontiers Group
  2. US National Institutes of Health [R01DA036865, R01AR069085, R21NS103007, R33DA041878, P30AR066527, R41GM119914, R41AI136755, U01HG007900, UM1HG009428, UG3TR002142]
  3. National Science Foundation [EFRI-1830957, DMR-1709527]
  4. Pfizer-NCBiotech Distinguished Postdoctoral Fellowship
  5. Open Philanthropy

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The prokaryote-derived CRISPR-Cas genome editing systems have transformed our ability to manipulate, detect, image and annotate specific DNA and RNA sequences in living cells of diverse species. The ease of use and robustness of this technology have revolutionized genome editing for research ranging from fundamental science to translational medicine. Initial successes have inspired efforts to discover new systems for targeting and manipulating nucleic acids, including those from Cas9, Cas12, Cascade and Cas13 orthologues. Genome editing by CRISPR-Cas can utilize non-homologous end joining and homology-directed repair for DNA repair, as well as single-base editing enzymes. In addition to targeting DNA, CRISPR-Cas-based RNA-targeting tools are being developed for research, medicine and diagnostics. Nuclease-inactive and RNA-targeting Cas proteins have been fused to a plethora of effector proteins to regulate gene expression, epigenetic modifications and chromatin interactions. Collectively, the new advances are considerably improving our understanding of biological processes and are propelling CRISPR-Cas-based tools towards clinical use in gene and cell therapies.

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