4.5 Article

Allosteric regulation in CRISPR/Cas1-Cas2 protospacer acquisition mediated by DNA and Cas2

BIOPHYSICAL JOURNAL (2021)

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Journal

BIOPHYSICAL JOURNAL
Volume 120, Issue 15, Pages 3126-3137

Publisher

CELL PRESS
DOI: 10.1016/j.bpj.2021.06.007

Keywords

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Categories

Biophysics

Funding

  1. Special Program for Applied Research on Super Computation of the National Natural Science Foundation of China-Guangdong Joint Fund (the second phase) [U1501501]
  2. Beijing Computational Science Research Center
  3. National Natural Science Foundation of China [12005029, 11775016, 11635002]
  4. Start-up Founding of Chongqing University of Posts and Telecommunications [A2020-029]
  5. Center of Multiscale Cell Fate Research of University of California, Irvine via Natural Science Foundation, Division of Mathematical Sciences [1763272]
  6. Simons Foundation [594598]
  7. start-up funding from University of California, Irvine

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Cas1 and Cas2 are highly conserved proteins that play a significant role in protospacer acquisition. The study shows that PAMc recognition and cleavage at one active site of Cas1-Cas2 may allosterically regulate non-PAMc association or even cleavage at the other site, with potential support from noncatalytic Cas2 and DNA protospacer in mediating the process.
Cas1 and Cas2 are highly conserved proteins across clustered-regularly-interspaced-short-palindromic-repeatCas systems and play a significant role in protospacer acquisition. Based on crystal structure of twofold symmetric Cas1-Cas2 in complex with dual-forked protospacer DNA (psDNA), we conducted all-atom molecular dynamics simulations to study the psDNA binding, recognition, and response to cleavage on the protospacer-adjacent-motif complementary sequence, or PAMc, of Cas1-Cas2. In the simulation, we noticed that two active sites of Cas1 and Cas1' bind asymmetrically to two identical PAMc on the psDNA captured from the crystal structure. For the modified psDNA containing only one PAMc, as that to be recognized by Cas1-Cas2 in general, our simulations show that the non-PAMc association site of Cas1-Cas2 remains destabilized until after the stably bound PAMc being cleaved at the corresponding association site. Thus, long-range correlation appears to exist upon the PAMc cleavage between the two active sites (similar to 10 nm apart) on Cas1-Cas2, which can be allosterically mediated by psDNA and Cas2 and Cas2' in bridging. To substantiate such findings, we conducted repeated runs and further simulated Cas1-Cas2 in complex with synthesized psDNA sequences psL and psH, which have been measured with low and high frequency in acquisition, respectively. Notably, such intersite correlation becomes even more pronounced for the Cas1-Cas2 in complex with psH but remains low for the Cas1-Cas2 in complex with psL. Hence, our studies demonstrate that PAMc recognition and cleavage at one active site of Cas1-Cas2 may allosterically regulate non-PAMc association or even cleavage at the other site, and such regulation can be mediated by noncatalytic Cas2 and DNA protospacer to possibly support the ensued psDNA acquisition.

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