4.8 Article

Kinetic and structural mechanism for DNA unwinding by a non-hexameric helicase

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NATURE COMMUNICATIONS
卷 12, 期 1, 页码 -

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NATURE PORTFOLIO
DOI: 10.1038/s41467-021-27304-6

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资金

  1. National Institutes of Health [R01 GM120353, R01 GM45948, R35 GM136632]
  2. National Science Foundation Physics Frontiers Center (PFC) program [PHY-1430124]
  3. Blue Waters sustainedpetascale computing project [OCI-0725070, ACI-1238993]
  4. Extreme Science and Engineering Discovery Environment grant [TG-BIO200029]

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The study utilized optical tweezers to directly measure the stepping behavior of UvrD as it processes a DNA hairpin, revealing a variable step size averaging around 3 base pairs. Analysis of ATP hydrolysis kinetics showed that UvrD moves one base pair at a time but non-uniformly releases nascent single strands, suggesting a conserved mechanism among other non-hexameric helicases.
UvrD, a model for non-hexameric Superfamily 1 helicases, utilizes ATP hydrolysis to translocate stepwise along single-stranded DNA and unwind the duplex. Previous estimates of its step size have been indirect, and a consensus on its stepping mechanism is lacking. To dissect the mechanism underlying DNA unwinding, we use optical tweezers to measure directly the stepping behavior of UvrD as it processes a DNA hairpin and show that UvrD exhibits a variable step size averaging similar to 3 base pairs. Analyzing stepping kinetics across ATP reveals the type and number of catalytic events that occur with different step sizes. These single-molecule data reveal a mechanism in which UvrD moves one base pair at a time but sequesters the nascent single strands, releasing them non-uniformly after a variable number of catalytic cycles. Molecular dynamics simulations point to a structural basis for this behavior, identifying the protein-DNA interactions responsible for strand sequestration. Based on structural and sequence alignment data, we propose that this stepping mechanism may be conserved among other non-hexameric helicases.

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