Date published: 2025-9-23

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Klk26 Inhibitors

Chemical inhibitors of Klk26 can act on the protein through various mechanisms to impede its enzymatic function. Aprotinin forms a tight stoichiometric complex with Klk26, effectively hindering its ability to cleave peptide substrates. Benzamidine competes with natural substrates for the active site of Klk26, thereby obstructing its proteolytic activity. AEBSF covalently modifies the serine residue within the catalytic triad of Klk26, leading to irreversible inhibition of its enzymatic activity. Similarly, leupeptin interacts with serine proteases, including Klk26, by reversibly binding to the enzyme and inhibiting proteolysis. Gabexate mimics the transition state of peptide bond hydrolysis, which allows it to bind to the active site of Klk26 and prevent substrate cleavage.

Camostat and nafamostat share a mode of action where they inhibit Klk26's proteolytic function by occupying the active site, which precludes substrate interaction and subsequent peptide bond cleavage. Chymostatin also inhibits Klk26 by active site binding, thus preventing substrate hydrolysis. SBTI, or Soybean trypsin inhibitor, targets Klk26 and blocks substrate access by binding to its active site. E-64, although typically a cysteine protease inhibitor, can inhibit Klk26 through interaction with its active site, demonstrating cross-class inhibition. Pepstatin A, known for aspartic protease inhibition, can interact with Klk26's active site due to similarities in substrate specificity, leading to inhibition. Lastly, phosphoramidon, primarily a metalloprotease inhibitor, can interact with Klk26 by binding to metal ions that may play a role in the structural conformation or substrate binding of Klk26, resulting in inhibition of the protein's function. Each chemical utilizes a distinct approach to disrupt the catalytic proficiency of Klk26, ensuring the protein's enzymatic activity is effectively suppressed.

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