| Literature DB >> 33749238 |
Vijay Kumar1, Snigdha A Mathure1, Mijoon Lee2, Jacob Boorman1, Ximin Zeng3, Jun Lin3, Dusan Hesek2, Elena Lastochkin2, Shahriar Mobashery2, Focco van den Akker1.
Abstract
The soluble lytic transglycosylase Cj0843c from Campylobacter jejuni breaks down cell-wall peptidoglycan (PG). Its nonhydrolytic activity sustains cell-wall remodeling and repair. We report herein our structure-function studies probing the substrate preferences and recognition by this enzyme. Our studies show that Cj0843c exhibits both exolytic and endolytic activities and forms the N-acetyl-1,6-anhydromuramyl (anhMurNAc) peptidoglycan termini, the typical transformation catalyzed by lytic transglycosylase. Cj0843c shows a trend toward a preference for substrates with anhMurNAc ends and those with peptide stems. Mutagenesis revealed that the catalytic E390 is critical for activity. In addition, mutagenesis showed that R388 and K505, located in the positively charged pocket near E390, also serve important roles. Mutation of R326, on the opposite side of this positively charged pocket, enhanced activity. Our data point to different roles for positively charged residues in this pocket for productive binding of the predominantly negatively charged PG. We also show by X-ray crystallography and by molecular dynamics simulations that the active site of Cj0843c is still capable of binding GlcNAc containing di- and trisaccharides without MurNAc moieties, without peptide stems, and without the anhMurNAc ends.Entities:
Mesh:
Substances:
Year: 2021 PMID: 33749238 PMCID: PMC9067259 DOI: 10.1021/acs.biochem.1c00027
Source DB: PubMed Journal: Biochemistry ISSN: 0006-2960 Impact factor: 3.321