Date published: 2025-9-13

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ADAM39 Activators

Chemical activators of a disintegrin and metallopeptidase domain 39 (ADAM39) include a variety of metal ions that serve as essential cofactors for its activity. Zinc acetate provides zinc ions that bind to the metalloprotease domain, which is a crucial component of the protein's proteolytic function. This binding is essential for the catalytic activity of ADAM39 as it facilitates the correct orientation of water molecules for hydrolysis of peptide bonds in substrates. Similarly, manganese from Manganese(II) sulfate enhances ADAM39's enzymatic activity by serving as a cofactor. The manganese ions may assist in the electron transfer processes necessary for the proteolysis carried out by ADAM39. Copper from Copper(II) sulfate also interacts with the metalloprotease domain of ADAM39, which can lead to an increase in its functional activity. This interaction is vital for the protein's structural conformation that enables substrate cleavage.

Furthermore, ions such as magnesium from Magnesium chloride and calcium from Calcium chloride contribute to the structural integrity of ADAM39, ensuring its active conformation and stability, which are prerequisites for substrate interaction and protease activation. Other chemicals like Sodium orthovanadate can enhance the phosphorylation state of ADAM39 by inhibiting tyrosine phosphatases, which increases the protein's activity. Phorbol 12-myristate 13-acetate (PMA) activates protein kinase C, which can subsequently phosphorylate and activate ADAM39. Forskolin, by raising cAMP levels, indirectly activates protein kinase A which may phosphorylate ADAM39, enhancing its enzymatic function. Additionally, oxidative modifications induced by Hydrogen peroxide can augment the proteolytic action of ADAM39. Sodium nitroprusside releases nitric oxide, which can lead to S-nitrosylation of ADAM39, another modification that can increase its activity. Finally, the presence of cobalt from Cobalt(II) chloride and nickel from Nickel(II) sulfate can serve as alternative cofactors, which may also enhance the proteolytic efficiency of ADAM39, demonstrating the diverse chemical milieu that can regulate the activity of this metalloproteinase.

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