Date published: 2025-9-18

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GM2-AP Inhibitors

Chemical inhibitors of GM2-AP can exert their inhibitory effects through various mechanisms affecting the protein's lipid environment and cellular trafficking. Methyl-β-cyclodextrin affects GM2-AP functionality by extracting cholesterol from cellular membranes, thereby disrupting lipid rafts where GM2-AP is active. Similarly, Filipin binds to cholesterol, perturbing the lipid rafts and consequently inhibiting the raft-associated activities of GM2-AP. U18666A disrupts intracellular cholesterol trafficking, leading to its accumulation and potential disturbance of the cholesterol-rich microenvironments crucial for GM2-AP activity. Genistein inhibits tyrosine kinases that may be involved in GM2-AP's localization and function, suggesting an indirect means of inhibition through interference with protein trafficking and cellular signaling pathways. Progesterone modulates sphingolipid metabolism, which can affect GM2-AP by altering the lipid composition of the membranes where GM2-AP functions.

Chlorpromazine and Imipramine both act as inhibitors of acid sphingomyelinase, which in turn can lead to changes in lipid composition, affecting GM2-AP indirectly by disrupting its lipid-dependent processes. GW4869 similarly inhibits acid sphingomyelinase, influencing the lipid composition and potentially the lipid raft domains essential for GM2-AP's activity. NB-DNJ and D-PDMP are inhibitors of glucosylceramide synthase, which can impact GM2-AP by reducing the synthesis of glycosphingolipids, thus affecting the pool of lipid substrates required for GM2-AP's function. Thapsigargin disrupts calcium homeostasis by inhibiting the sarco/endoplasmic reticulum Ca2+ ATPase, which can affect GM2-AP by modifying its conformation or trafficking, processes that rely on calcium. Lastly, Bafilomycin A1 inhibits the vacuolar type H+-ATPase, which can increase lysosomal pH, negatively impacting the acidic environment GM2-AP needs for optimal functioning.

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