Cellular and Structural Basis of Synthesis of the Unique Intermediate Dehydro-F<sub>420</sub>-0 in Mycobacteria

Rhys Grinter; Blair Ney; Rajini Brammananth; Christopher K. Barlow; Paul R. F. Cordero; David L. Gillett; Thierry Izoré; Max J. Cryle; Liam K. Harold; Gregory M. Cook; George Taiaroa; Deborah A. Williamson; Andrew C. Warden; John G. Oakeshott; Matthew C. Taylor; Paul K. Crellin; Colin J. Jackson; Ralf B. Schittenhelm; Ross L. Coppel; Chris Greening

doi:10.1128/mSystems.00389-20

mSystems (Jun 2020)

Cellular and Structural Basis of Synthesis of the Unique Intermediate Dehydro-F<sub>420</sub>-0 in Mycobacteria

Rhys Grinter,
Blair Ney,
Rajini Brammananth,
Christopher K. Barlow,
Paul R. F. Cordero,
David L. Gillett,
Thierry Izoré,
Max J. Cryle,
Liam K. Harold,
Gregory M. Cook,
George Taiaroa,
Deborah A. Williamson,
Andrew C. Warden,
John G. Oakeshott,
Matthew C. Taylor,
Paul K. Crellin,
Colin J. Jackson,
Ralf B. Schittenhelm,
Ross L. Coppel,
Chris Greening

Affiliations

Rhys Grinter: School of Biological Sciences, Monash University, Clayton, VIC, Australia
Blair Ney: School of Biological Sciences, Monash University, Clayton, VIC, Australia
Rajini Brammananth: School of Biological Sciences, Monash University, Clayton, VIC, Australia
Christopher K. Barlow: Department of Biochemistry, Monash Biomedicine Discovery Institute, Monash University, Clayton, VIC, Australia
Paul R. F. Cordero: School of Biological Sciences, Monash University, Clayton, VIC, Australia
David L. Gillett: School of Biological Sciences, Monash University, Clayton, VIC, Australia
Thierry Izoré: Department of Biochemistry, Monash Biomedicine Discovery Institute, Monash University, Clayton, VIC, Australia
Max J. Cryle: Department of Biochemistry, Monash Biomedicine Discovery Institute, Monash University, Clayton, VIC, Australia
Liam K. Harold: Department of Microbiology and Immunology, University of Otago, Dunedin, New Zealand
Gregory M. Cook: Department of Microbiology and Immunology, University of Otago, Dunedin, New Zealand
George Taiaroa: Peter Doherty Institute for Infection and Immunity, University of Melbourne, Melbourne, VIC, Australia
Deborah A. Williamson: Peter Doherty Institute for Infection and Immunity, University of Melbourne, Melbourne, VIC, Australia
Andrew C. Warden: CSIRO Land & Water, Canberra, ACT, Australia
John G. Oakeshott: CSIRO Land & Water, Canberra, ACT, Australia
Matthew C. Taylor: CSIRO Land & Water, Canberra, ACT, Australia
Paul K. Crellin: School of Biological Sciences, Monash University, Clayton, VIC, Australia
Colin J. Jackson: Research School of Chemistry, Australian National University, Canberra, ACT, Australia
Ralf B. Schittenhelm: Department of Biochemistry, Monash Biomedicine Discovery Institute, Monash University, Clayton, VIC, Australia
Ross L. Coppel: Department of Microbiology, Monash Biomedicine Discovery Institute, Monash University, Clayton, VIC, Australia
Chris Greening: School of Biological Sciences, Monash University, Clayton, VIC, Australia

DOI: https://doi.org/10.1128/mSystems.00389-20
Journal volume & issue: Vol. 5, no. 3

Abstract

Read online

ABSTRACT F420 is a low-potential redox cofactor used by diverse bacteria and archaea. In mycobacteria, this cofactor has multiple roles, including adaptation to redox stress, cell wall biosynthesis, and activation of the clinical antitubercular prodrugs pretomanid and delamanid. A recent biochemical study proposed a revised biosynthesis pathway for F420 in mycobacteria; it was suggested that phosphoenolpyruvate served as a metabolic precursor for this pathway, rather than 2-phospholactate as long proposed, but these findings were subsequently challenged. In this work, we combined metabolomic, genetic, and structural analyses to resolve these discrepancies and determine the basis of F420 biosynthesis in mycobacterial cells. We show that, in whole cells of Mycobacterium smegmatis, phosphoenolpyruvate rather than 2-phospholactate stimulates F420 biosynthesis. Analysis of F420 biosynthesis intermediates present in M. smegmatis cells harboring genetic deletions at each step of the biosynthetic pathway confirmed that phosphoenolpyruvate is then used to produce the novel precursor compound dehydro-F420-0. To determine the structural basis of dehydro-F420-0 production, we solved high-resolution crystal structures of the enzyme responsible (FbiA) in apo-, substrate-, and product-bound forms. These data show the essential role of a single divalent cation in coordinating the catalytic precomplex of this enzyme and demonstrate that dehydro-F420-0 synthesis occurs through a direct substrate transfer mechanism. Together, these findings resolve the biosynthetic pathway of F420 in mycobacteria and have significant implications for understanding the emergence of antitubercular prodrug resistance. IMPORTANCE Mycobacteria are major environmental microorganisms and cause many significant diseases, including tuberculosis. Mycobacteria make an unusual vitamin-like compound, F420, and use it to both persist during stress and resist antibiotic treatment. Understanding how mycobacteria make F420 is important, as this process can be targeted to create new drugs to combat infections like tuberculosis. In this study, we show that mycobacteria make F420 in a way that is different from other bacteria. We studied the molecular machinery that mycobacteria use to make F420, determining the chemical mechanism for this process and identifying a novel chemical intermediate. These findings also have clinical relevance, given that two new prodrugs for tuberculosis treatment are activated by F420.

Published in mSystems

ISSN: 2379-5077 (Online)
Publisher: American Society for Microbiology
Country of publisher: United States
LCC subjects: Science: Microbiology
Website: https://journals.asm.org/journal/msystems

About the journal

Abstract

Keywords