MARCH2 Activators are a collection of chemical entities that indirectly enhance the ubiquitin ligase function of MARCH2 through a variety of intracellular signaling modifications. Forskolin and IBMX elevate cAMP levels, indirectly promoting the activation of protein kinase A (PKA), which can lead to phosphorylation events enhancing MARCH2 activity. PMA activates protein kinase C (PKC), which may affect MARCH2 through phosphorylation of proteins that interact with it. Similarly, calcium ionophores like Ionomycin and A23187 increase intracellular calcium, which can activate calcium-dependent signaling pathways that might interface with MARCH2's ubiquitination processes. The inhibition of PI3K by LY294002 and mTOR by Rapamycin shifts cellular signaling in ways that could enhance MARCH2's function in autophagy and ubiquitination, respectively.
In parallel, proteostatic stressors such as MG-132, Brefeldin A, Chloroquine, and Tunicamycin modify the cellular environment to potentially increase the utilization of MARCH2's E3 ligase activity. MG-132 prevents proteasomal degradation of ubiquitinated proteins, possibly increasing the functional demand for MARCH2. Brefeldin A disrupts Golgi apparatus functions, which could enhance the role of MARCH2 in the degradation of membrane proteins. Chloroquine's inhibition ofautophagosome-lysosome fusion may lead to a compensatory increase in MARCH2's activity to manage autophagic processes. Lastly, Tunicamycin-induced ER stress and Thapsigargin's elevation of cytosolic calcium levels can trigger cellular pathways where MARCH2's ubiquitin ligase activity is essential for the degradation of misfolded proteins and regulation of calcium signaling proteins. Through these diverse mechanisms, each activator indirectly facilitates the enhancement of MARCH2's role in cellular ubiquitination processes without directly modifying its expression levels or requiring direct activation of the protein itself.
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