Functional interactions between gyrase subunits are optimized in a species-specific manner

Daniela Weidlich; Dagmar Klostermeier

doi:10.1074/jbc.RA119.010245

Functional interactions between gyrase subunits are optimized in a species-specific manner

J Biol Chem. 2020 Feb 21;295(8):2299-2312. doi: 10.1074/jbc.RA119.010245. Epub 2020 Jan 17.

Authors

Daniela Weidlich¹, Dagmar Klostermeier²

Affiliations

¹ Institute for Physical Chemistry, University of Muenster, Corrensstrasse 30, D-48149 Muenster, Germany.
² Institute for Physical Chemistry, University of Muenster, Corrensstrasse 30, D-48149 Muenster, Germany. Electronic address: dagmar.klostermeier@uni-muenster.de.

Abstract

DNA gyrase is a bacterial DNA topoisomerase that catalyzes ATP-dependent negative DNA supercoiling and DNA decatenation. The enzyme is a heterotetramer comprising two GyrA and two GyrB subunits. Its overall architecture is conserved, but species-specific elements in the two subunits are thought to optimize subunit interaction and enzyme function. Toward understanding the roles of these different elements, we compared the activities of Bacillus subtilis, Escherichia coli, and Mycobacterium tuberculosis gyrases and of heterologous enzymes reconstituted from subunits of two different species. We show that B. subtilis and E. coli gyrases are proficient DNA-stimulated ATPases and efficiently supercoil and decatenate DNA. In contrast, M. tuberculosis gyrase hydrolyzes ATP only slowly and is a poor supercoiling enzyme and decatenase. The heterologous enzymes are generally less active than their homologous counterparts. The only exception is a gyrase reconstituted from mycobacterial GyrA and B. subtilis GyrB, which exceeds the activity of M. tuberculosis gyrase and reaches the activity of the B. subtilis gyrase, indicating that the activities of enzymes containing mycobacterial GyrB are limited by ATP hydrolysis. The activity pattern of heterologous gyrases is in agreement with structural features present: B. subtilis gyrase is a minimal enzyme, and its subunits can functionally interact with subunits from other bacteria. In contrast, the specific insertions in E. coli and mycobacterial gyrase subunits appear to prevent efficient functional interactions with heterologous subunits. Understanding the molecular details of gyrase adaptations to the specific physiological requirements of the respective organism might aid in the development of species-specific gyrase inhibitors.

Keywords: ATPase; DNA binding protein; DNA gyrase; DNA topoisomerase; DNA-protein interaction; GyrA; GyrB; decatenation; genome integrity; heterologous protein-protein interaction; species specificity; subunit interaction; supercoiling mechanism.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Adenosine Triphosphatases / metabolism
Bacteria / enzymology*
DNA Gyrase / metabolism*
DNA, Bacterial
DNA, Superhelical
Kinetics
Models, Molecular
Protein Binding
Protein Multimerization
Protein Subunits / metabolism*
Species Specificity
Structural Homology, Protein

Substances

DNA, Bacterial
DNA, Superhelical
Protein Subunits
Adenosine Triphosphatases
DNA Gyrase

Associated data

PDB/4DDQ
PDB/3NUH
PDB/6GAV
PDB/1ZI0
PDB/3UC1
PDB/4XTJ