AI Article Synopsis

  • Bacterial phospholipase A1 (PLA1) is valuable in industries for processing phospholipids and refining plant oils, but it can be toxic to bacterial cells when produced internally.
  • This study successfully addressed the toxicity issue by utilizing a secretion-based production method, which involves the ABC transporter complex from SIK-W1 to release the PLA1 protein outside the bacterial cell.
  • A new bacterial strain, ZYAI, was engineered to control PLA1 expression, allowing for high yields of a functional protein that is effective in the oil degumming process, highlighting its industrial application potential.

Article Abstract

Bacterial phospholipase A1 (PLA1) is used in various industrial fields because it can catalyze the hydrolysis, esterification, and transesterification of phospholipids to their functional derivatives. It also has a role in the degumming process of crude plant oils. However, bacterial expression of the foreign PLA1-encoding gene was generally hampered because intracellularly expressed PLA1 is inherently toxic and damages the phospholipid membrane. In this study, we report that secretion-based production of recombinant PlaA, a bacterial PLA1 gene, or co-expression of PlaS, an accessory gene, minimizes this harmful effect. We were able to achieve high-level PlaA production via secretion-based protein production. Here, TliD/TliE/TliF, an ABC transporter complex of SIK-W1, was used to secrete recombinant proteins to the extracellular medium. In order to control the protein expression with induction, a new strain of , which had the operon repressor gene , was constructed and named ZYAI strain. The bacteriotoxic PlaA protein was successfully produced in a bacterial host, with help from ABC transporter-mediated secretion, induction-controlled protein expression, and fermentation. The final protein product is capable of degumming oil efficiently, signifying its application potential.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7074900PMC
http://dx.doi.org/10.3390/microorganisms8020239DOI Listing

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