Mechanistic characterization of the DEAD-box RNA helicase Ded1 from yeast as revealed by a novel technique using single-molecule magnetic tweezers.

Nucleic Acids Res

Laboratoire de Physique de l'Ecole normale supérieure, ENS, Université PSL, CNRS, Sorbonne Université, Université Paris-Diderot, Sorbonne Paris Cité, Paris, France.

Published: April 2019

AI Article Synopsis

  • DEAD-box helicases are crucial for RNA metabolism and work as ATP-dependent proteins that can displace RNA duplexes but lack processivity, making their exact functioning unclear.
  • A new single-molecule assay using magnetic tweezers allows for sensitive measurement of RNA displacement times to better understand helicase activity, with the ability to analyze multiple molecules simultaneously.
  • Research on the yeast helicase Ded1 demonstrates that it requires RNA substrates and ATP hydrolysis for unwinding activity, suggesting that ATP-bound Ded1 stabilizes partially unwound RNA duplexes and may need multiple binding events for effective displacement.

Article Abstract

DEAD-box helicases are involved in all steps of RNA metabolism. They are ATP-dependent RNA binding proteins and RNA-dependent ATPases. They can displace short duplexes, but they lack processivity. Their mechanism and functioning are not clearly understood; classical or bulk biochemical assays are not sufficient to answer these questions. Single-molecule techniques provide useful tools, but they are limited in cases where the proteins are nonprocessive and give weak signals. We present here a new, magnetic-tweezers-based, single-molecule assay that is simple and that can sensitively measure the displacement time of a small, hybridized, RNA oligonucleotide. Tens of molecules can be analyzed at the same time. Comparing the displacement times with and without a helicase gives insights into the enzymatic activity of the protein. We used this assay to study yeast Ded1, which is orthologous to human DDX3. Although Ded1 acts on a variety of substrates, we find that Ded1 requires an RNA substrate for its ATP-dependent unwinding activity and that ATP hydrolysis is needed to see this activity. Further, we find that only intramolecular single-stranded RNA extensions enhance this activity. We propose a model where ATP-bound Ded1 stabilizes partially unwound duplexes and where multiple binding events may be needed to see displacement.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC6468243PMC
http://dx.doi.org/10.1093/nar/gkz057DOI Listing

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