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Biochemical and Structural Properties of Fungal Holliday Junction-Resolving Enzymes

Author(s)
Liu, YijinFreeman, AlasdairDeclais, Anne-CecileGartner, AntonLilley, David M. J.
Issued Date
2018
DOI
10.1016/bs.mie.2017.11.021
URI
https://scholarworks.unist.ac.kr/handle/201301/27476
Fulltext
https://www.sciencedirect.com/science/article/pii/S0076687917303592?via%3Dihub
Citation
MECHANISMS OF DNA RECOMBINATION AND GENOME REARRANGEMENTS: METHODS TO STUDY HOMOLOGOUS RECOMBINATION, v.600, pp.543 - 568
Abstract
Four-way Holliday junctions in DNA are the central intermediates of genetic recombination and must be processed into regular duplex species. One mechanism for achieving this is called resolution, brought about by structure-selective nucleases. GEN1 is an important junction-resolving enzyme in eukaryotic cells, a member of the FEN1/EXO1 superfamily of nucleases. While human GEN1 is difficult to work with because of aggregation, orthologs from thermophilic fungi have been identified using bioinformatics and have proved to have excellent properties. Here, the expression and purification of this enzyme from Chaetomium thermophilum is described, together with the means of investigating its biochemical properties. The enzyme is quite similar to junction-resolving enzymes from lower organisms, binding to junctions in dimeric form, introducing symmetrical bilateral cleavages, the second of which is accelerated to promote productive resolution. Crystallization of C. thermophilum GEN1 is described, and the structure of a DNA-product complex. Juxtaposition of complexes in the crystal lattice suggests how the structure of a dimeric enzyme with an intact junction is organized.
Publisher
ELSEVIER ACADEMIC PRESS INC
ISSN
0076-6879
Keyword
4-WAY DNA JUNCTIONCRUCIFORM FORMATIONSUPERCOILED DNAINVERTED REPEATHUMAN GEN1ENDONUCLEASERESOLUTIONMECHANISMFLUORESCENCECCE1

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