Docking Simulation and Competitive Experiments Validate the Interaction Between the 2,5-Xylidine Inhibitor and Rigidoporus lignosus Laccase

被引:53
作者
Cambria, Maria Teresa [3 ]
Di Marino, Daniele [1 ,2 ]
Falconi, Mattia [1 ,2 ]
Garavaglia, Silvia [4 ]
Cambria, Antonio [5 ]
机构
[1] Univ Roma Tor Vergata, Dipartimento Biol, I-00133 Rome, Italy
[2] Ctr Interdipartimentale Biostat & Bioinformat, CIBB, I-00133 Rome, Italy
[3] Univ Catania, Dipartimento Sci Chim, I-95125 Catania, Italy
[4] Univ Piemonte Orientale, DISCAFF INFM, I-28100 Novara, Italy
[5] Consorzio Interuniv, Ist Nazl Biostrutture & Biosistemi, I-00136 Rome, Italy
关键词
CRYSTAL-STRUCTURE; TRAMETES-VERSICOLOR; FUNGAL LACCASES; FULL COMPLEMENT; SUBSTRATE; PROTEINS; NETWORK;
D O I
10.1080/07391102.2010.10507334
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Laccases are polyphenol oxidases which oxidize a broad range of reducing Substrates, preferably phenolic compounds. and their use in biotechnological applications is increasing. Recently. the first X-ray structure of active laccase from white rot fungus Rigidoporus lignosus has been reported containing a full complement of copper ions. Comparison among selected fungal laccases of known 3D structure has shown that the Rigidoporus lignosus laccase has a very high similarity with the Trametes versicolor laccase that, being co-crystallized with 2.5-xylidine, shows a well defined binding pocket for the substrate. Global sequence alignment between Rigidoporus lignosus and Trametes versicolor laccases shows 73% of identity but, surprisingly, there is no identity and neither conservative substitutions between the residues composing the loops directly contacting the 2.5-xylidine. Moreover the structural alignment of these two enzymes identifies in these loops a striking structural similarity proposing the question if 2.5-xylidine may bind in same enzyme pocket. Here we report the protein-ligand docking simulation of 3D structure of Rigidoporus lignosus laccase and 2,5-xylidine. Docking simulation analyses show that spatial conformation of the two 2,5-xylidine binding pockets, despite differences in the residues directly contacting the ligand, may arrange a similar pocket that allows a comparable accommodation of the inhibitor. To validate these results the binding of 2,5-xylidine in the substrate cavity has been confirmed by kinetic competitive experiments.
引用
收藏
页码:501 / 509
页数:9
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