AI Article Synopsis

  • The recombinant CpLIP2 lipase/acyltransferase is a promising target for antifungal drug development, particularly for treating candidiasis.
  • The study examined the inhibitory effects of the drug orlistat and flavonols (galangin, kaempferol, quercetin, and myricetin) on CpLIP2, revealing that orlistat and kaempferol were the most effective inhibitors with significant reductions in enzyme activity.
  • The mechanisms behind these inhibitions were explored, showing that orlistat binds at the catalytic site while kaempferol interacts with a specific protein residue, and interactions were largely driven by hydrophobic bonds and electrostatic forces.

Article Abstract

The inhibition of recombinant CpLIP2 lipase/acyltransferase from was considered a key model for novel antifungal drug discovery and a potential therapeutic target for candidiasis. Lipases have identified recently as potent virulence factors in and some other yeasts. The inhibition effects of orlistat and four flavonols (galangin, kaempferol, quercetin and myricetin) characterized by an increasing degree of hydroxylation in B-ring, were investigated using ethyl oleate hydrolysis as the model reaction. Orlistat and kaempferol (14 µM) strongly inhibited CpLIP2 catalytic activity within 1 min of pre-incubation, by 90% and 80%, respectively. The relative potency of flavonols as inhibitors was: kaempferol > quercetin > myricetin > galangin. The results suggested that orlistat bound to the catalytic site while kaempferol interacted with W294 on the protein lid. A static mechanism of interactions between flavonols and CpLIP2 lipase was confirmed by fluorescence quenching analyses, indicating that the interactions were mainly driven by hydrophobic bonds and electrostatic forces. From the Lehrer equation, fractions of tryptophan accessibility to the quencher were evaluated, and a relationship with the calculated number of binding sites was suggested.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC6719172PMC
http://dx.doi.org/10.3390/molecules24162888DOI Listing

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