Database of articles cited by EMDB/PDB/SASBDB data

Keywords
Structure methods	All X-ray diffraction NMR electron microscopy small angle scattering neutron diffraction fiber diffraction powder diffraction infrared spectroscopy EPR fluorescence transfer theoretical model Hybrid
Author
Journal
IF	>30 >20 >10 >5 all

Title	Heterogeneity in E. coli RecBCD Helicase-DNA Binding and Base Pair Melting.
Journal, issue, pages	J Mol Biol, Vol. 433, Issue 18, Page 167147, Year 2021
Publish date	Sep 3, 2021
Authors	Linxuan Hao / Rui Zhang / Timothy M Lohman /
PubMed Abstract	E. coli RecBCD, a helicase/nuclease involved in double stranded (ds) DNA break repair, binds to a dsDNA end and melts out several DNA base pairs (bp) using only its binding free energy. We examined ...E. coli RecBCD, a helicase/nuclease involved in double stranded (ds) DNA break repair, binds to a dsDNA end and melts out several DNA base pairs (bp) using only its binding free energy. We examined RecBCD-DNA initiation complexes using thermodynamic and structural approaches. Measurements of enthalpy changes for RecBCD binding to DNA ends possessing pre-melted ssDNA tails of increasing length suggest that RecBCD interacts with ssDNA as long as 17-18 nucleotides and can melt at least 10-11 bp upon binding a blunt DNA end. Cryo-EM structures of RecBCD alone and in complex with a blunt-ended dsDNA show significant conformational heterogeneities associated with the RecB nuclease domain (RecB) and the RecD subunit. In the absence of DNA, 56% of RecBCD molecules show no density for the RecB nuclease domain, RecB, and all RecBCD molecules show only partial density for RecD. DNA binding reduces these conformational heterogeneities, with 63% of the molecules showing density for both RecD and RecB. This suggests that the RecB domain is dynamic and influenced by DNA binding. The major RecBCD-DNA structural class in which RecB is docked onto RecC shows melting of at least 11 bp from a blunt DNA end, much larger than previously observed. A second structural class in which RecB is not docked shows only four bp melted suggesting that RecBCD complexes transition between states with different extents of DNA melting and that the extent of melting regulates initiation of helicase activity.
External links	J Mol Biol / PubMed:34246654 / PubMed Central
Methods	EM (single particle)
Resolution	3.6 - 4.5 Å
Structure data	23952 7mr0 EMDB-23952, PDB-7mr0: Cryo-EM structure of RecBCD with docked RecBNuc and flexible RecD Method: EM (single particle) / Resolution: 3.7 Å 23953 7mr1 EMDB-23953, PDB-7mr1: Cryo-EM structure of RecBCD with undocked RecBNuc and flexible RecD C-terminus Method: EM (single particle) / Resolution: 4.2 Å 23954 7mr2 EMDB-23954, PDB-7mr2: Cryo-EM structure of RecBCD with undocked RecBNuc and flexible RecD Method: EM (single particle) / Resolution: 4.3 Å 23955 7mr3 EMDB-23955, PDB-7mr3: Cryo-EM structure of RecBCD-DNA complex with docked RecBNuc and stabilized RecD Method: EM (single particle) / Resolution: 3.6 Å 23956 7mr4 EMDB-23956, PDB-7mr4: Cryo-EM structure of RecBCD-DNA complex with undocked RecBNuc and flexible RecD Method: EM (single particle) / Resolution: 4.5 Å
Source	escherichia coli k12 (bacteria) escherichia coli (strain k12) (bacteria) synthetic construct (others)
Keywords	HYDROLASE / SF1 helicase / complex / DNA repair / motor protein / HYDROLASE/DNA / HYDROLASE-DNA complex