Functional characterization of the endolysins derived from mycobacteriophage PDRPxv

Kandasamy Eniyan; Avni Sinha; Shazeb Ahmad; Urmi Bajpai

doi:10.1007/s11274-020-02858-7

Functional characterization of the endolysins derived from mycobacteriophage PDRPxv

World J Microbiol Biotechnol. 2020 May 28;36(6):83. doi: 10.1007/s11274-020-02858-7.

Authors

Kandasamy Eniyan¹, Avni Sinha¹, Shazeb Ahmad¹, Urmi Bajpai²

Affiliations

¹ Department of Biomedical Science, Acharya Narendra Dev College (University of Delhi), Govindpuri, New Delhi, 110019, India.
² Department of Biomedical Science, Acharya Narendra Dev College (University of Delhi), Govindpuri, New Delhi, 110019, India. urmibajpai@andc.du.ac.in.

PMID: 32468233
DOI: 10.1007/s11274-020-02858-7

Abstract

Bacteriophage-derived endolysin enzymes play a critical role in disintegration of the host bacterial cell wall and hence have gained considerable attention as possible therapeutics for the treatment of drug-resistant infections. Endolysins can target both dividing and non-dividing cells and given the vital role peptidoglycan plays in bacterial survival, bacteria are less likely to modify it even if continuously exposed to lysins. Hence, probability of bacteria developing resistance to lysins appear bleak. Endolysins from mycobacteriophages offer great potential as alternative therapeutics for the drug-resistant TB. However, considering that a large number of mycobacteriophages have been discovered so far, the information on endolysins come from only a few mycobacteriophages. In this study, we report the structural and functional characterization of endolysins (LysinA and LysinB) encoded by mycobacteriophage PDRPxv which belongs to B1 sub cluster. On in silico analysis, we found LysinA to be a modular protein having peptidase domain at the N-terminal (104 aa), a central amidase domain (174 aa) and the peptidoglycan binding domain (62 aa) at the C-terminal. Additionally, 'H-X-H', which is a conserved motif and characteristic of peptidase domains, and the conserved residues His-His-Asp, which are characteristic of amidase domain were also observed. In LysinB enzyme, a single α/β hydrolase domain having a catalytic triad (Ser-Asp-His) and G-X-S-X-G motif, which are characteristic of the serine esterase enzymes were predicted to be present. Both the enzymes were purified as recombinant proteins and their antimycobacterial activity against M. smegmatis was demonstrated through turbidimetric experiments and biochemical assay. Interesting observation in this study is the secretory nature of LysinA evident by its periplasmic expression in E.coli, which might explain the ability of PDRPxv to lyse the bacterial host in the absence of transmembrane Holin protein.

Keywords: Endolysins; Esterase; Mycobacteriophage PDRPxv; Periplasmic expression.

MeSH terms

Anti-Bacterial Agents / biosynthesis
Computer Simulation
Endopeptidases* / biosynthesis
Endopeptidases* / chemistry
Endopeptidases* / isolation & purification
Endopeptidases* / pharmacology
Escherichia coli / metabolism
Mycobacteriophages / enzymology*
Mycobacterium smegmatis / drug effects
Recombinant Proteins / biosynthesis
Recombinant Proteins / chemistry
Recombinant Proteins / isolation & purification
Viral Proteins / biosynthesis
Viral Proteins / chemistry
Viral Proteins / isolation & purification
Viral Proteins / pharmacology

Substances

Anti-Bacterial Agents
Recombinant Proteins
Viral Proteins
Endopeptidases
endolysin

Grants and funding

2014-2015/Innovation and entrepreneurship development center (IEDC) cell at ANDC funded by the National Science & Technology Entrepreneurship Development Board (NSTEDB), Department of Science and Technology (DST), India.