CRISPR-driven enhanced hydrocarbon emulsification in an environmental Pseudomonas aeruginosa strain

CRISPR-driven enhanced hydrocarbon emulsification in an environmental Pseudomonas aeruginosa strain

Abstract Background Oil spills are a major concern due to the economic impact and severe effects on the ecosystem. To mitigate oil spills, hydrocarbon dispersion through emulsification is a promising approach, as it makes oil more susceptible to degradation by microorganisms. Environmental strains o...

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Main Authors: Luis M. Salazar-García, Luis C. Damas-Ramos, Luisa M. Trejo-Alarcón, Daniela Rago, Linda Ahonen, Pablo Cruz-Morales, Patricia Ponce-Noyola, Cuauhtémoc Licona-Cassani
Format: Article
Language:English
Published: BMC 2025-07-01
Series:Microbial Cell Factories
Subjects:
Pyocyanin
Rhamnolipids
Pseudomonas aeruginosa
CRISPR/Cas
Environmental strain
Bioremediation
Online Access:https://doi.org/10.1186/s12934-025-02769-y
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Summary:Abstract Background Oil spills are a major concern due to the economic impact and severe effects on the ecosystem. To mitigate oil spills, hydrocarbon dispersion through emulsification is a promising approach, as it makes oil more susceptible to degradation by microorganisms. Environmental strains of Pseudomonas aeruginosa have demonstrated significant potential for producing rhamnolipids (RMLs) and pyocyanin (PYO), secondary metabolites associated to hydrocarbon emulsification. In this study, we isolated and characterized an environmental strain from an oil-contaminated site in the Gulf of Mexico. Upon genome sequencing and taxonomic classification, we developed genetic engineering tools and assessed their capacity to produce PYO and RMLs, molecules relevant for hydrocarbon emulsification. Results Using the CRISPR/Cas9-APOBEC1-UGI system, we generated a targeted cytosine to thymine transition in the rpoS gene to generate a premature STOP codon. The resulting mutant exhibited increased production of PYO and RMLs, along with enhanced gasoline emulsification in cell-free supernatants, demonstrating successful modulation of a key regulatory gene. While the strain IGLPR01 retains certain virulence-associated features, this study contributes to the exploration of environmental isolates as future candidate chassis for biosurfactant production, emphasizing the need for further safety evaluation and rational attenuation strategies. Conclusion This study provides a successful example of implementing CRISPR-based editing in an environmental P. aeruginosa strain. Despite the technical challenges, a genetic editing system was established and validated through a proof of concept to increase production of relevant metabolites. Our work demonstrates the applicability of genetic engineering tools in non-model environmental isolates, facilitating further developments. Importantly, the presence of virulence-associated features highlights the need for in-depth evaluation of pathogenicity and containment strategies before considering any future biotechnological applications.
ISSN:1475-2859

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