Cloning and characterization of an intracellular esterase from the wine-associated lactic acid bacterium Oenococcus oeni
Cloning and characterization of an intracellular esterase from the wine-associated lactic acid bacterium Oenococcus oeni
We report the cloning and characterization of EstB28, the first esterase to be so characterized from the wine-associated lactic acid bacterium, Oenococcus oeni. The published sequence for O. oeni strain PSU-1 was used to identify putative esterase genes and design PCR primers in order to amplify the corresponding region from strain Ooeni28, an isolate intended for inoculation of wines. In this way a 912-bp open reading frame (ORF) encoding a putative esterase of 34.5 kDa was obtained. The amino acid sequence indicated that EstB28 is a member of family IV of lipolytic enzymes and contains the GDSAG motif common to other lactic acid bacteria. This ORF was cloned into Escherichia coli using an appropriate expression system, and the recombinant esterase was purified. Characterization of EstB28 revealed that the optimum temperature, pH, and ethanol concentration were 40°C, pH 5.0, and 28% (vol/vol), respectively. EstB28 also retained marked activity under conditions relevant to winemaking (10 to 20°C, pH 3.5, 14% [vol/vol] ethanol). Kinetic constants were determined for EstB28 with p-nitrophenyl (pNP)-linked substrates ranging in chain length from C2 to C18. EstB28 exhibited greatest specificity for C2 to C4 pNP-linked substrates.
6729-6735
Sumby, Krista M.
f54b8f1c-c29e-488b-ab5e-dbb9b2576ba9
Matthews, Angela H.
5aa6e142-a824-4fb1-a994-f741f4288796
Grbin, Paul R.
e1cce428-cbfc-4cd2-aef0-c0e3a076a955
Jiranek, Vladimir
8e5a8dfd-f5b2-43e3-928b-11dff324abc7
November 2009
Sumby, Krista M.
f54b8f1c-c29e-488b-ab5e-dbb9b2576ba9
Matthews, Angela H.
5aa6e142-a824-4fb1-a994-f741f4288796
Grbin, Paul R.
e1cce428-cbfc-4cd2-aef0-c0e3a076a955
Jiranek, Vladimir
8e5a8dfd-f5b2-43e3-928b-11dff324abc7
Sumby, Krista M., Matthews, Angela H., Grbin, Paul R. and Jiranek, Vladimir
(2009)
Cloning and characterization of an intracellular esterase from the wine-associated lactic acid bacterium Oenococcus oeni.
Applied and Environmental Microbiology, 75 (21), .
(doi:10.1128/AEM.01563-09).
Abstract
We report the cloning and characterization of EstB28, the first esterase to be so characterized from the wine-associated lactic acid bacterium, Oenococcus oeni. The published sequence for O. oeni strain PSU-1 was used to identify putative esterase genes and design PCR primers in order to amplify the corresponding region from strain Ooeni28, an isolate intended for inoculation of wines. In this way a 912-bp open reading frame (ORF) encoding a putative esterase of 34.5 kDa was obtained. The amino acid sequence indicated that EstB28 is a member of family IV of lipolytic enzymes and contains the GDSAG motif common to other lactic acid bacteria. This ORF was cloned into Escherichia coli using an appropriate expression system, and the recombinant esterase was purified. Characterization of EstB28 revealed that the optimum temperature, pH, and ethanol concentration were 40°C, pH 5.0, and 28% (vol/vol), respectively. EstB28 also retained marked activity under conditions relevant to winemaking (10 to 20°C, pH 3.5, 14% [vol/vol] ethanol). Kinetic constants were determined for EstB28 with p-nitrophenyl (pNP)-linked substrates ranging in chain length from C2 to C18. EstB28 exhibited greatest specificity for C2 to C4 pNP-linked substrates.
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Published date: November 2009
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Local EPrints ID: 482569
URI: http://eprints.soton.ac.uk/id/eprint/482569
ISSN: 0099-2240
PURE UUID: f70567fe-1232-48f5-844a-a6bcf070285d
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Date deposited: 10 Oct 2023 16:58
Last modified: 18 Mar 2024 04:12
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Author:
Krista M. Sumby
Author:
Angela H. Matthews
Author:
Paul R. Grbin
Author:
Vladimir Jiranek
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