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Structure basis for RNA-guided DNA degradation by Cascade and Cas3.

Yibei XiaoMin LuoAdam E DolanMaofu LiaoAilong Ke
Published in: Science (New York, N.Y.) (2018)
Type I CRISPR-Cas system features a sequential target-searching and degradation process on double-stranded DNA by the RNA-guided Cascade (CRISPR associated complex for antiviral defense) complex and the nuclease-helicase fusion enzyme Cas3, respectively. Here, we present a 3.7-angstrom-resolution cryo-electron microscopy (cryo-EM) structure of the Type I-E Cascade/R-loop/Cas3 complex, poised to initiate DNA degradation. Cas3 distinguishes Cascade conformations and only captures the R-loop-forming Cascade, to avoid cleaving partially complementary targets. Its nuclease domain recruits the nontarget strand (NTS) DNA at a bulged region for the nicking of single-stranded DNA. An additional 4.7-angstrom-resolution cryo-EM structure captures the postnicking state, in which the severed NTS retracts to the helicase entrance, to be threaded for adenosine 5'-triphosphate-dependent processive degradation. These snapshots form the basis for understanding RNA-guided DNA degradation in Type I-E CRISPR-Cas systems.
Keyphrases
  • crispr cas
  • genome editing
  • circulating tumor
  • single molecule
  • nucleic acid
  • cell free
  • transcription factor
  • genome wide
  • gene expression
  • mass spectrometry
  • protein kinase