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Different quaternary structures of human RECQ1 are associated with its dual enzymatic activity
Authors:Muzzolini Laura  Beuron Fabienne  Patwardhan Ardan  Popuri Venkateswarlu  Cui Sheng  Niccolini Benedetta  Rappas Mathieu  Freemont Paul S  Vindigni Alessandro
Institution:1, International Centre for Genetic Engineering and Biotechnology, Trieste, Italy;2, Division of Molecular Biosciences, Faculty of Natural Sciences, Imperial College London, London, United Kingdom;National Cancer Institute–National Institutes of Health, United States of America
Abstract:RecQ helicases are essential for the maintenance of chromosome stability. In addition to DNA unwinding, some RecQ enzymes have an intrinsic DNA strand annealing activity. The function of this dual enzymatic activity and the mechanism that regulates it is, however, unknown. Here, we describe two quaternary forms of the human RECQ1 helicase, higher-order oligomers consistent with pentamers or hexamers, and smaller oligomers consistent with monomers or dimers. Size exclusion chromatography and transmission electron microscopy show that the equilibrium between the two assembly states is affected by single-stranded DNA (ssDNA) and ATP binding, where ATP or ATPγS favors the smaller oligomeric form. Our three-dimensional electron microscopy reconstructions of human RECQ1 reveal a complex cage-like structure of approximately 120 Å × 130 Å with a central pore. This oligomeric structure is stabilized under conditions in which RECQ1 is proficient in strand annealing. In contrast, competition experiments with the ATPase-deficient K119R and E220Q mutants indicate that RECQ1 monomers, or tight binding dimers, are required for DNA unwinding. Collectively, our findings suggest that higher-order oligomers are associated with DNA strand annealing, and lower-order oligomers with DNA unwinding.
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