Inhibition of the SARS-CoV-2 helicase at single-nucleotide resolution

Author:

Marx Sinduja K.ORCID,Mickolajczyk Keith J.ORCID,Craig Jonathan M.ORCID,Thomas Christopher A.ORCID,Pfeffer Akira M.,Abell Sarah J.,Carrasco Jessica D.,Franzi Michaela C.,Huang Jesse R.,Kim Hwanhee C.,Brinkerhoff Henry D.ORCID,Kapoor Tarun M.ORCID,Gundlach Jens H.,Laszlo Andrew H.ORCID

Abstract

AbstractThe genome of SARS-CoV-2 encodes for a helicase called nsp13 that is essential for viral replication and highly conserved across related viruses, making it an attractive antiviral target. Here we use nanopore tweezers, a high-resolution single-molecule technique, to gain detailed insight into how nsp13 turns ATP-hydrolysis into directed motion along nucleic acid strands. We measured nsp13 both as it translocates along single-stranded DNA or unwinds short DNA duplexes. Our data confirm that nsp13 uses the inchworm mechanism to move along the DNA in single-nucleotide steps, translocating at ~1000 nt/s or unwinding at ~100 bp/s. Nanopore tweezers’ high spatio-temporal resolution enables observation of the fundamental physical steps taken by nsp13 even as it translocates at speeds in excess of 1000 nucleotides per second enabling detailed kinetic analysis of nsp13 motion. As a proof-of-principle for inhibition studies, we observed nsp13’s motion in the presence of the ATPase inhibitor ATPγS. Our data reveals that ATPγS interferes with nsp13’s action by affecting several different kinetic processes. The dominant mechanism of inhibition differs depending on the application of assisting force. These advances demonstrate that nanopore tweezers are a powerful method for studying viral helicase mechanism and inhibition.

Publisher

Cold Spring Harbor Laboratory

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