Murakami Mário T, Fernandes-Pedrosa Matheus Freitas, de Andrade Sonia A, Gabdoulkhakov Azat, Betzel Christian, Tambourgi Denise V, Arni Raghuvir K
Department of Physics, IBILCE/UNESP, São José do Rio Preto-SP, Brazil.
Biochem Biophys Res Commun. 2006 Mar 31;342(1):323-9. doi: 10.1016/j.bbrc.2006.01.123. Epub 2006 Feb 3.
Spider venom sphingomyelinases D catalyze the hydrolysis of sphingomyelin via an Mg(2+) ion-dependent acid-base catalytic mechanism which involves two histidines. In the crystal structure of the sulfate free enzyme determined at 1.85A resolution, the metal ion is tetrahedrally coordinated instead of the trigonal-bipyramidal coordination observed in the sulfate bound form. The observed hyperpolarized state of His47 requires a revision of the previously suggested catalytic mechanism. Molecular modeling indicates that the fundamental structural features important for catalysis are fully conserved in both classes of SMases D and that the Class II SMases D contain an additional intra-chain disulphide bridge (Cys53-Cys201). Structural analysis suggests that the highly homologous enzyme from Loxosceles bonetti is unable to hydrolyze sphingomyelin due to the 95Gly-->Asn and 134Pro-->Glu mutations that modify the local charge and hydrophobicity of the interfacial face. Structural and sequence comparisons confirm the evolutionary relationship between sphingomyelinases D and the glicerophosphodiester phosphoesterases which utilize a similar catalytic mechanism.