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GENETICS AND MOLECULAR BIOLOGY

Thermoadaptation of α-Galactosidase AgaB1 in Thermus thermophilus

Olafur Fridjonsson, Hildegard Watzlawick, Ralf Mattes
Olafur Fridjonsson
Institut für Industrielle Genetik, Universität Stuttgart, 70569 Stuttgart, Germany
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  • For correspondence: olafur@prokaria.com
Hildegard Watzlawick
Institut für Industrielle Genetik, Universität Stuttgart, 70569 Stuttgart, Germany
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Ralf Mattes
Institut für Industrielle Genetik, Universität Stuttgart, 70569 Stuttgart, Germany
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DOI: 10.1128/JB.184.12.3385-3391.2002
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This article has a correction. Please see:

  • Thermoadaptation of α-Galactosidase AgaB1 in Thermus thermophilus
    - August 01, 2002

ABSTRACT

The evolutionary potential of a thermostable α-galactosidase, with regard to improved catalytic activity at high temperatures, was investigated by employing an in vivo selection system based on thermophilic bacteria. For this purpose, hybrid α-galactosidase genes of agaA and agaB from Bacillus stearothermophilus KVE39, designated agaA1 and agaB1, were cloned into an autonomously replicating Thermus vector and introduced into Thermus thermophilus OF1053GD (ΔagaT) by transformation. This selector strain is unable to metabolize melibiose (α-galactoside) without recombinant α-galactosidases, because the native α-galactosidase gene, agaT, has been deleted. Growth conditions were established under which the strain was able to utilize melibiose as a single carbohydrate source when harboring a plasmid-encoded agaA1 gene but unable when harboring a plasmid-encoded agaB1 gene. With incubation of the agaB1 plasmid-harboring strain under selective pressure at a restrictive temperature (67°C) in a minimal melibiose medium, spontaneous mutants as well as N-methyl-N′-nitro-N-nitrosoguanidine-induced mutants able to grow on the selective medium were isolated. The mutant α-galactosidase genes were amplified by PCR, cloned in Escherichia coli, and sequenced. A single-base substitution that replaces glutamic acid residue 355 with glycine or valine was found in the mutant agaB1 genes. The mutant enzymes displayed the optimum hydrolyzing activity at higher temperatures together with improved catalytic capacity compared to the wild-type enzyme and furthermore showed an enhanced thermal stability. To our knowledge, this is the first report of an in vivo evolution of glycoside-hydrolyzing enzyme and selection within a thermophilic host cell.

  • Copyright © 2002 American Society for Microbiology
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Thermoadaptation of α-Galactosidase AgaB1 in Thermus thermophilus
Olafur Fridjonsson, Hildegard Watzlawick, Ralf Mattes
Journal of Bacteriology Jun 2002, 184 (12) 3385-3391; DOI: 10.1128/JB.184.12.3385-3391.2002

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Thermoadaptation of α-Galactosidase AgaB1 in Thermus thermophilus
Olafur Fridjonsson, Hildegard Watzlawick, Ralf Mattes
Journal of Bacteriology Jun 2002, 184 (12) 3385-3391; DOI: 10.1128/JB.184.12.3385-3391.2002
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KEYWORDS

Adaptation, Physiological
Bacterial Proteins
Directed Molecular Evolution
temperature
Thermus thermophilus
alpha-Galactosidase

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