Bioresource Technology, Vol.102, No.2, 1740-1746, 2011
Enhancement of the thermostability of the maltogenic amylase MAUS149 by Gly312Ala and Lys436Arg substitutions
Based on sequence alignments and homology modeling, Gly 312 and Lys 436 of the maltogenic amylase from Bacillus sp. US149 (MAUS149) were selected as targets for site-directed mutagenesis to improve the thermostability of the enzyme. Variants of MAUS149 with amino acid substitutions G312A, K436R and G312A-K436R had substrate specificities, kinetic parameters and pH optima similar to those of the wild-type enzyme: however, the enzymes with substitutions K436R and G312A-K436R, had an optimal temperature of 45 degrees C instead of the 40 degrees C for the wild-type enzyme. The half-life time at 55 degrees C increased from 15 to 25 min for the double mutant. Molecular modeling suggests that the increase in thermostability was due to new hydrophobic interactions and the formation of a salt bridge and hydrogen bond in the G312A and K436R variants, respectively. The double mutant could be a potential candidate for application in the bread industry. (C) 2010 Elsevier Ltd. All rights reserved.
Keywords:Maltogenic amylase;Site-directed mutagenesis;Thermostability;Salt bridge;Hydrophobic interactions