TY - JOUR
T1 - Polyvalent guide RNAs for CRISPR antivirals
AU - Bagchi, Rammyani
AU - Tinker-Kulberg, Rachel
AU - Salehin, Mohammad
AU - Supakar, Tinku
AU - Chamberlain, Sydney
AU - Ligaba-Osena, Ayalew
AU - Josephs, Eric A.
PY - 2022/11/18
Y1 - 2022/11/18
N2 - CRISPR effector Cas13 recognizes and degrades RNA molecules that are complementary to its guide RNA (gRNA) and possesses potential as an antiviral biotechnology because it can degrade viral mRNA and RNA genomes. Because multiplexed targeting is a critical strategy to improve viral suppression, we developed a strategy to design of gRNAs where individual gRNAs have maximized activity at multiple viral targets, simultaneously, by exploiting the molecular biophysics of promiscuous target recognition by Cas13. These “polyvalent” gRNA sequences (“pgRNAs”) provide superior antiviral elimination across tissue/organ scales in a higher organism (Nicotiana benthamiana) compared to conventionally-designed gRNAs—reducing detectable viral RNA by >30-fold, despite lacking perfect complementarity with either of their targets and, when multiplexed, reducing viral RNA by >99.5%. Pairs of pgRNA-targetable sequences are abundant in the genomes of RNA viruses, and this work highlights the need for specific approaches to the challenges of targeting viruses in eukaryotes using CRISPR.
AB - CRISPR effector Cas13 recognizes and degrades RNA molecules that are complementary to its guide RNA (gRNA) and possesses potential as an antiviral biotechnology because it can degrade viral mRNA and RNA genomes. Because multiplexed targeting is a critical strategy to improve viral suppression, we developed a strategy to design of gRNAs where individual gRNAs have maximized activity at multiple viral targets, simultaneously, by exploiting the molecular biophysics of promiscuous target recognition by Cas13. These “polyvalent” gRNA sequences (“pgRNAs”) provide superior antiviral elimination across tissue/organ scales in a higher organism (Nicotiana benthamiana) compared to conventionally-designed gRNAs—reducing detectable viral RNA by >30-fold, despite lacking perfect complementarity with either of their targets and, when multiplexed, reducing viral RNA by >99.5%. Pairs of pgRNA-targetable sequences are abundant in the genomes of RNA viruses, and this work highlights the need for specific approaches to the challenges of targeting viruses in eukaryotes using CRISPR.
KW - Biocomputational method
KW - Biological sciences tools
KW - Computational bioinformatics
UR - https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=85140413634&origin=inward
UR - https://www.scopus.com/inward/citedby.uri?partnerID=HzOxMe3b&scp=85140413634&origin=inward
U2 - 10.1016/j.isci.2022.105333
DO - 10.1016/j.isci.2022.105333
M3 - Article
SN - 2589-0042
VL - 25
JO - iScience
JF - iScience
IS - 11
M1 - 105333
ER -