Structure-function relationships underlying the dual N-acetylmuramic and N-acetylglucosamine specificities of the bacterial peptidoglycan deacetylase PdaC

Laia Grifoll-Romero; María Angela Sainz-Polo; David Albesa-Jové; Marcelo E Guerin; Xevi Biarnés; Antoni Planas

doi:10.1074/jbc.RA119.009510

Structure-function relationships underlying the dual N-acetylmuramic and N-acetylglucosamine specificities of the bacterial peptidoglycan deacetylase PdaC

J Biol Chem. 2019 Dec 13;294(50):19066-19080. doi: 10.1074/jbc.RA119.009510. Epub 2019 Nov 5.

Authors

Laia Grifoll-Romero¹, María Angela Sainz-Polo², David Albesa-Jové^{2

3}, Marcelo E Guerin^{2

3}, Xevi Biarnés¹, Antoni Planas⁴

Affiliations

¹ Laboratory of Biochemistry, Institut Químic de Sarrià, University Ramon Llull, 08017 Barcelona, Spain.
² Structural Biology Unit, Center for Cooperative Research in Biosciences (CIC bioGUNE), Bizkaia Technology Park, Ed. 801A, 48160 Derio, Spain.
³ Basque Foundation for Science (IKERBASQUE), 48011 Bilbao, Spain.
⁴ Laboratory of Biochemistry, Institut Químic de Sarrià, University Ramon Llull, 08017 Barcelona, Spain antoni.planas@iqs.edu.

Abstract

Bacillus subtilis PdaC (BsPdaC) is a membrane-bound, multidomain peptidoglycan N-deacetylase acting on N-acetylmuramic acid (MurNAc) residues and conferring lysozyme resistance to modified cell wall peptidoglycans. BsPdaC contains a C-terminal family 4 carbohydrate esterase (CE4) catalytic domain, but unlike other MurNAc deacetylases, BsPdaC also has GlcNAc deacetylase activity on chitooligosaccharides (COSs), characteristic of chitin deacetylases. To uncover the molecular basis of this dual activity, here we determined the X-ray structure of the BsPdaC CE4 domain at 1.54 Å resolution and analyzed its mode of action on COS substrates. We found that the minimal substrate is GlcNAc₃ and that activity increases with the degree of glycan polymerization. COS deacetylation kinetics revealed that BsPdaC operates by a multiple-chain mechanism starting at the internal GlcNAc units and leading to deacetylation of all but the reducing-end GlcNAc residues. Interestingly, BsPdaC shares higher sequence similarity with the peptidoglycan GlcNAc deacetylase SpPgdaA than with other MurNAc deacetylases. Therefore, we used ligand-docking simulations to analyze the dual GlcNAc- and MurNAc-binding specificities of BsPdaC and compared them with those of SpPgdA and BsPdaA, representing peptidoglycan deacetylases highly specific for GlcNAc or MurNAc residues, respectively. BsPdaC retains the conserved Asp-His-His metal-binding triad characteristic of CE4 enzymes acting on GlcNAc residues, differing from MurNAc deacetylases that lack the metal-coordinating Asp residue. BsPdaC contains short loops similar to those in SpPgdA, resulting in an open binding cleft that can accommodate polymeric substrates. We propose that PdaC is the first member of a new subclass of peptidoglycan MurNAc deacetylases.

Keywords: N-acetylglucosamine; N-acetylmuramic; N-acetylmuramic acid; bacterial pathogenesis; cell wall; chitooligosaccharides; crystal structure; deacetylase; ligand-docking simulations; molecular docking; peptidoglycan; specificity.

Publication types

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

MeSH terms

Acetylglucosamine / chemistry
Acetylglucosamine / metabolism*
Amidohydrolases / chemistry
Amidohydrolases / metabolism*
Bacillus subtilis / enzymology*
Chitin / analogs & derivatives
Chitin / chemistry
Chitin / metabolism*
Crystallography, X-Ray
Models, Molecular
Muramic Acids / chemistry
Muramic Acids / metabolism*
Phylogeny
Structure-Activity Relationship
Substrate Specificity

Substances

Muramic Acids
Chitin
N-acetylmuramic acid
Amidohydrolases
polysaccharide deacetylase
Acetylglucosamine

Associated data

PDB/2C1G
PDB/6H8L
PDB/6H8N
PDB/1W1B
PDB/6AVE
PDB/1TWQ
PDB/9LYZ
PDB/1LZC