Peptidoglycan Remodeling in Mycobacterium Tuberculosis: Comparison of Structures and Catalytic Activities of RipA and RipB

Overview

Journal J Mol Biol

Publisher Elsevier

Specialties Microbiology
Molecular Biology

Date 2011 Aug 26

PMID 21864539

Citations 35

Authors

Dominic Both

Gunter Schneider

Robert Schnell

Affiliations

Soon will be listed here.

Abstract

The success of Mycobacterium tuberculosis in sustaining long-term survival within the host macrophages partly relies on its unique cell envelop that also confers low susceptibility to several antibiotics. Remodeling of the septal peptidoglycan (PG) has been linked to the putative PG hydrolases RipA and RipB. The crystal structures of RipB (Rv1478) and the homologous module of RipA (Rv1477) were determined to 1.60 Å and 1.38 Å resolution, respectively. Both proteins contain a C-terminal core domain resembling the NlpC-type PG hydrolases. However, the structure of RipB exhibits striking differences to the structures of this domain in RipA reported here and previously by others. Major structural differences were found in the N-terminal segments of 70 amino acids and in an adjacent loop, which form part of the substrate binding groove. Both RipA and RipB are able to bind PG. RipA, its C-terminal module and RipB cleave defined PG fragments between d-glutamate and meso-diaminopimelate with pH optima of 5 and 6, respectively. The peptidase module of RipA is also able to degrade Bacillus subtilis PG, which displays peptide stems and cross-links identical with those found in mycobacterial murein. RipB did not show comparable hydrolase activity with this substrate. Removal of the N-terminal segments previously suggested to have a role in auto-inhibition did not change the activity of either RipA or RipB. A comparison of the putative active-site clefts in the two enzymes provides structural insights into the basis of the differences in their substrate specificity.

Citing Articles

Elucidating the molecular properties and anti-mycobacterial activity of cysteine peptidase domain of D29 mycobacteriophage endolysin.

Gangakhedkar R, Jain V J Virol. 2024; 98(10):e0132824.

PMID: 39287392 PMC: 11494882. DOI: 10.1128/jvi.01328-24.

Functional Analysis of Genes in Action Against Autophagosome-Lysosome Fusion.

Sundaram K, Vajravelu L Indian J Microbiol. 2024; 64(2):367-375.

PMID: 39011011 PMC: 11246336. DOI: 10.1007/s12088-024-01227-4.

Comparison of the transcriptome, lipidome, and c-di-GMP production between BCGΔBCG1419c and BCG, with Mincle- and Myd88-dependent induction of proinflammatory cytokines in murine macrophages.

Flores-Valdez M, Peterson E, Aceves-Sanchez M, Baliga N, Morita Y, Sparks I Sci Rep. 2024; 14(1):11898.

PMID: 38789479 PMC: 11126594. DOI: 10.1038/s41598-024-61815-8.

MtrA modulates Mycobacterium tuberculosis cell division in host microenvironments to mediate intrinsic resistance and drug tolerance.

Peterson E, Brooks A, Reiss D, Kaur A, Do J, Pan M Cell Rep. 2023; 42(8):112875.

PMID: 37542718 PMC: 10480492. DOI: 10.1016/j.celrep.2023.112875.

Identification and classification of papain-like cysteine proteinases.

Ozhelvaci F, Steczkiewicz K J Biol Chem. 2023; 299(6):104801.

PMID: 37164157 PMC: 10318531. DOI: 10.1016/j.jbc.2023.104801.