Journal:JBIC:21
From Proteopedia
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Furthermore, Phe197, Met61 and Met184, which are also located at the entrance to the active site, were found to play an important role in Cu uptake. Substitution of a bulky Phe197 to Ala, resulted in higher Cu uptake, while mutations at positions 61 and 184, had an opposite effect. <scene name='55/558329/Cv/18'>The active site of variant F197A</scene> ([[4j6t]]). <span style="color:lime;background-color:black;font-weight:bold;">Six His residues composing the active site are colored in green</span> and are ligating CuA and CuB ions which are shown as spheres. <span style="color:yellow;background-color:black;font-weight:bold;">Alanine residue at position 197 is colored in yellow</span>. In addition, it was found that these residues are also important for enhancing the diphenolase activity of the enzyme. Therefore, we can suggest that a Cu ion entering the active site (CuA) first associates with the methionine residues followed by its transfer to His60 in its flipped out conformation. Following Cu binding, His60 alters its conformation and transfers CuA into the active site in a paddle-like motion. We propose that CuB passes only through Asp205 and Phe197. The proposed pathway clarifies the previously reported observations of TyrBm’s tighter binding of CuA in comparison to CuB. | Furthermore, Phe197, Met61 and Met184, which are also located at the entrance to the active site, were found to play an important role in Cu uptake. Substitution of a bulky Phe197 to Ala, resulted in higher Cu uptake, while mutations at positions 61 and 184, had an opposite effect. <scene name='55/558329/Cv/18'>The active site of variant F197A</scene> ([[4j6t]]). <span style="color:lime;background-color:black;font-weight:bold;">Six His residues composing the active site are colored in green</span> and are ligating CuA and CuB ions which are shown as spheres. <span style="color:yellow;background-color:black;font-weight:bold;">Alanine residue at position 197 is colored in yellow</span>. In addition, it was found that these residues are also important for enhancing the diphenolase activity of the enzyme. Therefore, we can suggest that a Cu ion entering the active site (CuA) first associates with the methionine residues followed by its transfer to His60 in its flipped out conformation. Following Cu binding, His60 alters its conformation and transfers CuA into the active site in a paddle-like motion. We propose that CuB passes only through Asp205 and Phe197. The proposed pathway clarifies the previously reported observations of TyrBm’s tighter binding of CuA in comparison to CuB. | ||
| - | PDB references: Crystal Structure of Tyrosinase from ''Bacillus megaterium'' F197A mutant [[4j6t]]; Crystal Structure of Tyrosinase from ''Bacillus megaterium'' N205A mutant [[4j6u]]; Crystal Structure of Tyrosinase from ''Bacillus megaterium'' N205D mutant [[4j6v]]. | + | '''PDB references:''' Crystal Structure of Tyrosinase from ''Bacillus megaterium'' F197A mutant, [[4j6t]]; Crystal Structure of Tyrosinase from ''Bacillus megaterium'' N205A mutant, [[4j6u]]; Crystal Structure of Tyrosinase from ''Bacillus megaterium'' N205D mutant, [[4j6v]]. |
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<references/> | <references/> | ||
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- ↑ Kanteev M, Goldfeder M, Chojnacki M, Adir N, Fishman A. The mechanism of copper uptake by tyrosinase from Bacillus megaterium. J Biol Inorg Chem. 2013 Dec;18(8):895-903. doi: 10.1007/s00775-013-1034-0. Epub, 2013 Sep 6. PMID:24061559 doi:http://dx.doi.org/10.1007/s00775-013-1034-0
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