Differential Selectivity of the Escherichia coli Cell Membrane Shifts the Equilibrium for the Enzyme-Catalyzed Isomerization of Galactose to Tagatose

An Escherichia coli galactose kinase gene knockout (ΔgalK) strain, which contains the L-arabinose isomerase gene (araA) to isomerize D-galactose to D-tagatose, showed a high conversion yield of tagatose compared with the original galK strain because galactose was not metabolized by endogenous galact...

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Veröffentlicht in:Applied and Environmental Microbiology 2008-04, Vol.74 (8), p.2307-2313
Hauptverfasser: Kim, Jin-Ha, Lim, Byung-Chul, Yeom, Soo-Jin, Kim, Yeong-Su, Kim, Hye-Jung, Lee, Jung-Kul, Lee, Sook-Hee, Kim, Seon-Won, Oh, Deok-Kun
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Sprache:eng
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Zusammenfassung:An Escherichia coli galactose kinase gene knockout (ΔgalK) strain, which contains the L-arabinose isomerase gene (araA) to isomerize D-galactose to D-tagatose, showed a high conversion yield of tagatose compared with the original galK strain because galactose was not metabolized by endogenous galactose kinase. In whole cells of the ΔgalK strain, the isomerase-catalyzed reaction exhibited an equilibrium shift toward tagatose, producing a tagatose fraction of 68% at 37°C, whereas the purified L-arabinose isomerase gave a tagatose equilibrium fraction of 36%. These equilibrium fractions are close to those predicted from the measured equilibrium constants of the isomerization reaction catalyzed in whole cells and by the purified enzyme. The equilibrium shift in these cells resulted from the higher uptake and lower release rates for galactose, which is a common sugar substrate, than for tagatose, which is a rare sugar product. A ΔmglB mutant had decreased uptake rates for galactose and tagatose, indicating that a methylgalactoside transport system, MglABC, is the primary contributing transporter for the sugars. In the present study, whole-cell conversion using differential selectivity of the cell membrane was proposed as a method for shifting the equilibrium in sugar isomerization reactions.
ISSN:0099-2240
1098-5336
1098-6596
DOI:10.1128/AEM.02691-07