Date published: 2025-9-11

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Apobec-1 Inhibitors

Chemical inhibitors of Apobec-1 include a variety of compounds that can inhibit its function through different mechanisms. Bisphenol A can disrupt the mRNA editing process that is a key function of Apobec-1, rendering the protein unable to perform its role in RNA editing. Similarly, Resveratrol can interfere with the RNA-binding ability of Apobec-1, which is essential for its editing function. This interference halts the ability of Apobec-1 to bind to and edit RNA molecules as it normally would. S-Adenosylmethionine serves as a competitive inhibitor for Apobec-1, binding to its active site and preventing the interaction with its natural substrates, which inhibits the RNA editing activity of Apobec-1. Chloroquine inhibits Apobec-1 activity by altering the endosomal/lysosomal pH, a condition necessary for the optimal activity of Apobec-1, leading to a reduction in its functional capacity.

Curcumin binds to Apobec-1 and inhibits its RNA editing activity through steric hindrance, which physically obstructs the protein from interacting with its RNA substrate. Epigallocatechin gallate can also bind to Apobec-1 and inhibit its function by blocking the catalytic domain, which is crucial for its RNA editing activity. Quercetin's inhibition of Apobec-1 is achieved by competing with RNA substrates, thereby reducing the protein's ability to edit RNA. Oleuropein inhibits the activity of Apobec-1 by binding to its active site, which prevents the protein from accessing its RNA substrates. Ly294002, PD98059, SB203580, and SP600125 inhibit Apobec-1 indirectly through the inhibition of various signaling pathways such as PI3K/Akt, MEK/ERK, p38 MAPK, and JNK, respectively, which are all involved in the regulation of Apobec-1. Inhibition of these pathways leads to a decrease in the regulatory mechanisms that control the activity and function of Apobec-1, therefore inhibiting the protein's overall function in the cell.

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