2019
DOI: 10.1093/nar/gkz004
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Determining the effects of DNA sequence on Hel308 helicase translocation along single-stranded DNA using nanopore tweezers

Abstract: Motor enzymes that process nucleic-acid substrates play vital roles in all aspects of genome replication, expression, and repair. The DNA and RNA nucleobases are known to affect the kinetics of these systems in biologically meaningful ways. Recently, it was shown that DNA bases control the translocation speed of helicases on single-stranded DNA, however the cause of these effects remains unclear. We use single-molecule picometer-resolution nanopore tweezers (SPRNT) to measure the kinetics of translocation alon… Show more

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Cited by 38 publications
(42 citation statements)
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“…The complementary strand has a poly-T 20 tail with a 3’ cholesterol, which associates with the bilayer and increases the concentration of analyte near the pore, improving the event rate( 7, 24, 25 ). For sequencing, we used the mutant nanopore M2 MspA( 26 ) with a cup-like shape( 27 ) that separates the anchoring enzyme by ~10 nm from the constriction of the pore where the blockage of ion current occurs ( 28 ). For the DNA-translocating motor enzyme, we used Hel308 DNA helicase because its observable half-nucleotide ~0.33 nm steps, when pulling ssDNA through MspA( 23 ), are approximately the same as single-amino acid steps.…”
Section: Figurementioning
confidence: 99%
“…The complementary strand has a poly-T 20 tail with a 3’ cholesterol, which associates with the bilayer and increases the concentration of analyte near the pore, improving the event rate( 7, 24, 25 ). For sequencing, we used the mutant nanopore M2 MspA( 26 ) with a cup-like shape( 27 ) that separates the anchoring enzyme by ~10 nm from the constriction of the pore where the blockage of ion current occurs ( 28 ). For the DNA-translocating motor enzyme, we used Hel308 DNA helicase because its observable half-nucleotide ~0.33 nm steps, when pulling ssDNA through MspA( 23 ), are approximately the same as single-amino acid steps.…”
Section: Figurementioning
confidence: 99%
“…The induced and natural competency of many archaeal species permit genetic manipulations, most dependent on HR-directed gene conversion and integrations of new DNA. The archaeal Hel308 enzyme, believed to be responsible for strand displacement during SDSA, has been extensively studied for use in nanopore sequencing [67]. DSB repair is also an essential process for CRISPR viral defense systems found in~85% of Archaea, in which Cas enzymes generate guided double-strand breaks which are subsequently repaired by non-HR DSB repair pathways, NHEJ, and MMEJ [26].…”
Section: New Resources Emerging From Dsb Repair Pathwaysmentioning
confidence: 99%
“…For example, Roche has been quietly developing a protein nanopore-based technology acquired from startup Genia as a potential tool for clinical diagnostics, and Ontera is working on a handheld device that uses solid-state nanopores that can potentially identify nucleic acids, proteins, and even pathogens present in a given sample. And at the University of Washington, Jens Gundlach's team has been using nanopore proteins derived from the microbe Mycobacterium smegmatis to study the dynamic interplay between nucleic acids and various 'motor proteins' , such as the helicase enzymes that unwind DNA 15 .…”
Section: Opening the Floodgatesmentioning
confidence: 99%