Date published: 2025-9-15

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Cyp2c29 Inhibitors

Chemical inhibitors of Cyp2c29 act through various mechanisms to impede the protein's function. Sulfaphenazole is a selective inhibitor that targets the Cyp2c29 enzyme directly by binding to its active site. This binding precludes endogenous substrates from interacting with the enzyme, effectively halting its metabolic activity. Similarly, quercetin serves as a competitive inhibitor to Cyp2c29, occupying the active site of the enzyme and thereby preventing the catalysis of its natural substrates. Montelukast, while primarily known for another pharmacological action, also demonstrates inhibitory effects on Cyp2c29 by attaching to its active site, negating the enzyme's typical catalytic processes.

Nifedipine, a calcium channel blocker, extends its influence to Cyp2c29 by non-selectively binding to the protein's active site, diminishing the enzyme's capacity to metabolize substrates. Trimethoprim exhibits its inhibitory effect on Cyp2c29 by occupying the active site, directly obstructing the enzyme's function in metabolizing its substrates. Fluconazole, another inhibitor, interacts with the heme group within the Cyp2c29 active site, which is essential for the enzyme's activity, thereby inhibiting its function. The metabolites of Clopidogrel can form an irreversible bond with the active site of Cyp2c29, leading to sustained inhibition. Proadifen, or SKF-525A, acts as a non-selective inhibitor, binding to the active site of Cyp2c29 and impeding the enzyme's ability to process its substrates. Ketoconazole targets the heme group of Cyp2c29 as well, blocking the electron transfer which is vital for the enzyme's activity. Methimazole serves as a mechanism-based inhibitor, covalently attaching to the enzyme post-activation by Cyp2c29 itself, culminating in irreversible inhibition. α-Naphthoflavone competes for the Cyp2c29 active site, hindering substrate metabolism. Finally, Phenylbutazone binds to the active site of the enzyme, interfering with the normal catalytic function of Cyp2c29 and thereby inhibiting substrate metabolism. Each chemical presents a unique mode of interaction with Cyp2c29, but all culminate in the functional inhibition of this metabolic protein.

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