AI Article Synopsis

  • The study focuses on the characterization of two endolysins, Skl and Pal, with Pal being particularly significant for its effectiveness against severe diseases.
  • Both endolysins are identified as cysteine-amidases and have a structural similarity to the enzyme papain, with unique active sites for breaking down bacterial components.
  • Skl is highlighted as a potent anti-pneumococcal agent, effective against resistant strains, but its initial lysis efficiency is limited, which suggests a complex interaction with bacterial targets.

Article Abstract

We have structurally and functionally characterized Skl and Pal endolysins, the latter being the first endolysin shown to kill effectively , a leading cause of deathly diseases. We have proved that Skl and Pal are cysteine-amidases whose catalytic domains, from CHAP and Amidase_5 families, respectively, share an αβ-fold with papain-like topology. Catalytic triads are identified (for the first time in Amidase_5 family), and residues relevant for substrate binding and catalysis inferred from models, including a calcium-binding site accounting for Skl dependence on this cation for activity. Both endolysins contain a choline-binding domain (CBD) with a β-solenoid fold (homology modeled) and six conserved choline-binding loci whose saturation induced dimerization. Remarkably, Pal and Skl dimers display a common overall architecture, preserved in choline-bound dimers of pneumococcal lysins with other catalytic domains and bond specificities, as disclosed using small angle X-ray scattering (SAXS). Additionally, Skl is proved to be an efficient anti-pneumococcal agent that kills multi-resistant strains and clinical emergent-serotype isolates. Interestingly, Skl and Pal time-courses of pneumococcal lysis were sigmoidal, which might denote a limited access of both endolysins to target bonds at first stages of lysis. Furthermore, their DTT-mediated activation, of relevance for other cysteine-peptidases, cannot be solely ascribed to reversal of catalytic-cysteine oxidation.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC8586454PMC
http://dx.doi.org/10.3389/fmicb.2021.740914DOI Listing

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