Development and Evaluation of Bacteriophage Cocktail to Eradicate Biofilms Formed by an Extensively Drug-Resistant (XDR) Pseudomonas aeruginosa

Author:

Vashisth Medhavi12ORCID,Jaglan Anu Bala13,Yashveer Shikha2,Sharma Priya1,Bardajatya Priyanka1,Virmani Nitin1,Bera Bidhan Chand1,Vaid Rajesh Kumar1ORCID,Anand Taruna1

Affiliation:

1. ICAR-National Research Centre on Equines, Hisar 125001, India

2. Department of Molecular Biology and Biotechnology, College of Biotechnology, Chaudhary Charan Singh Haryana Agricultural University, Hisar 125004, India

3. Department of Zoology and Aquaculture, College of Basic Sciences and Humanities, Chaudhary Charan Singh Haryana Agricultural University, Hisar 125004, India

Abstract

Extensive and multiple drug resistance in P. aeruginosa combined with the formation of biofilms is responsible for its high persistence in nosocomial infections. A sequential method to devise a suitable phage cocktail with a broad host range and high lytic efficiency against a biofilm forming XDR P. aeruginosa strain is presented here. Out of a total thirteen phages isolated against P. aeruginosa, five were selected on the basis of their high lytic spectra assessed using spot assay and productivity by efficiency of plating assay. Phages, after selection, were tested individually and in combinations of two-, three-, four-, and five-phage cocktails using liquid infection model. Out of total 22 combinations tested, the cocktail comprising four phages viz. φPA170, φPA172, φPA177, and φPA180 significantly inhibited the bacterial growth in liquid infection model (p < 0.0001). The minimal inhibitory dose of each phage in a cocktail was effectively reduced to >10 times than the individual dose in the inhibition of XDR P. aeruginosa host. Field emission-scanning electron microscopy was used to visualize phage cocktail mediated eradication of 4-day-old multi-layers of XDR P. aeruginosa biofilms from urinary catheters and glass cover slips, and was confirmed by absence of any viable cells. Differential bacterial inhibition was observed with different phage combinations where multiple phages were found to enhance the cocktail’s lytic range, but the addition of too many phages reduced the overall inhibition. This study elaborates an effective and sequential method for the preparation of a phage cocktail and evaluates its antimicrobial potential against biofilm forming XDR strains of P. aeruginosa.

Funder

ICAR-National Fellow project

National Agricultural Science Fund

Publisher

MDPI AG

Subject

Virology,Infectious Diseases

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