Date published: 2025-10-11

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CAMSAP1L1 Inhibitors

CAMSAP1L1 inhibitors constitute a diverse array of chemical compounds that diminish the activity of CAMSAP1L1. For instance, microtubule-destabilizing agents such as Nocodazole and Vinblastine reduce the density and stability of microtubules, respectively, thereby attenuating CAMSAP1L1's intrinsic ability to bind and stabilize microtubule minus-ends. Conversely, microtubule-stabilizing drugs like Taxol and MCC950 sodium salt could interfere with CAMSAP1L1's function by hyper-stabilizing microtubules, which may reduce the protein's binding affinity and localization to microtubules. These inhibitors do not simply prevent the assembly or disassembly of microtubules but rather alter the dynamic equilibrium required for CAMSAP1L1 to function effectively. Chemicals like Colchicine and Podophyllotoxin further contribute to this effect by binding to tubulin, the building block of microtubules, thus preventing the formation of the microtubule structures essential for CAMSAP1L1's role in cellular architecture. Moreover, the impact of kinase inhibitors like Staurosporine on CAMSAP1L1 activity is mediated through the inhibition of phosphorylation events that are critical for the protein's stability and interaction with the cytoskeleton. Sspecific compounds like S-Trityl-L-cysteine and the kinesin Eg5 inhibitor Monastrol disrupt microtubule polymerization and spindle fiber formation, respectively, which indirectly limits CAMSAP1L1's stabilizing actions. Additionally, the IGF-1R signaling inhibitor BMS-754807 exemplifies a compound that can alter intracellular signaling pathways, resulting in downstream effects that may compromise microtubule dynamics and, consequently, CAMSAP1L1's role in microtubule stabilization. Collectively, these inhibitors work in concert through various mechanisms to impair the functional ability of CAMSAP1L1, effectively diminishing its activity without directly altering its expression or employing general cellular pathways.

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