Chemical inhibitors of C1orf156 can exert their inhibitory action through multiple mechanisms, primarily by targeting the methyltransferase activity that is central to the function of C1orf156. Sinefungin, a known methyltransferase inhibitor, can directly inhibit the methylation function of C1orf156 by competing with the S-adenosylmethionine (SAM) binding site, a critical methyl donor for these enzymes. Similarly, adenosine dialdehyde acts by inhibiting S-adenosylhomocysteine hydrolase, leading to the accumulation of S-adenosylhomocysteine, a potent inhibitor of methylation processes, thereby impeding the enzymatic activity of C1orf156. Compounds like BIX-01294 and chaetocin, although initially characterized for their inhibitory effects on other specific histone methyltransferases, can also inhibit C1orf156 due to the similarities in the catalytic sites and mechanisms of these enzyme families.
Further, methylthioadenosine, a byproduct of polyamine synthesis, can inhibit C1orf156 by mimicking the structure of the enzyme's native substrates, thus blocking its active site. RG108, while a direct inhibitor of DNA methyltransferases, could also extend its inhibitory action to proteins like C1orf156 due to the overlap in the biochemical pathways involving methylation. Decitabine and azacitidine, both nucleoside analogs of cytidine, inhibit DNA methyltransferases and thus could indirectly inhibit C1orf156 by a general reduction in methylation activity within the cell. Disulfiram, with its metal-binding properties, can inhibit C1orf156 by disrupting the metal-dependent catalytic activity that is often a feature of methyltransferase enzymes. Anacardic acid, a known inhibitor of histone acetyltransferases, can also inhibit methyltransferases like C1orf156 by binding to the active site or altering the conformation of the enzyme. Quercetin and epigallocatechin gallate, known for their broad-spectrum kinase inhibition, can inhibit C1orf156 due to the conserved nature of binding sites across these protein families, thus preventing the proper enzymatic activity of C1orf156.
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