Date published: 2025-9-16

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C6orf162 Activators

Chemical activators of C6orf162 can influence the protein's activity through a variety of cellular mechanisms, predominantly through modulation of intracellular signaling pathways. Forskolin, acting as an adenylate cyclase activator, directly increases the levels of cAMP within the cell. This rise in cAMP facilitates the activation of PKA (protein kinase A), which can then phosphorylate C6orf162, leading to its activation. Similarly, 8-Bromo-cAMP, a cAMP analog, bypasses the need for adenylate cyclase activation and directly activates PKA, which in turn can phosphorylate and activate C6orf162. Ionomycin and A-23187, both acting as calcium ionophores, increase the intracellular calcium concentration. Elevated calcium levels can activate calcium-dependent kinases, which are capable of phosphorylating C6orf162, thereby leading to its activation. PMA, an activator of protein kinase C (PKC), can also phosphorylate serine and threonine residues on proteins, including C6orf162, leading to its functional activation.

Additionally, Spermine NONOate releases nitric oxide, which activates guanylate cyclase, subsequently increasing cGMP levels and activating PKG (protein kinase G). PKG activation can result in the phosphorylation and activation of C6orf162. Zaprinast, by inhibiting phosphodiesterases, increases cGMP levels as well, leading to PKG-mediated activation of C6orf162. Inhibitors of protein phosphatases such as Okadaic Acid and Calyculin A prevent the dephosphorylation of proteins, thus maintaining C6orf162 in a phosphorylated and active state. Anisomycin activates stress-activated protein kinases that may target C6orf162 for phosphorylation and activation. Bisindolylmaleimide I, under specific conditions, can paradoxically activate PKC, which may then phosphorylate and activate C6orf162. Lastly, Thapsigargin, by inhibiting SERCA, disrupts calcium homeostasis, resulting in increased cytosolic calcium levels and activation of kinases capable of phosphorylating and activating C6orf162. Each of these chemicals, through their influence on cellular signaling pathways and kinase activity, can lead to the functional activation of C6orf162.

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