Preparation of Enzymes Required for Enzymatic Quantification of 5-Keto-<small>D</small>-gluconate and 2-Keto-<small>D</small>-gluconate

Ittipon SAICHANA; Yoshitaka ANO; Osao ADACHI; Kazunobu MATSUSHITA; Hirohide TOYAMA

doi:10.1271/bbb.70259

This article has now been updated. Please use the final version.

Preparation of Enzymes Required for Enzymatic Quantification of 5-Keto-D-gluconate and 2-Keto-D-gluconate

Ittipon SAICHANA, Yoshitaka ANO, Osao ADACHI, Kazunobu MATSUSHITA, Hirohide TOYAMA

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Keywords: 5-keto D-gluconic acid, 2-keto D-gluconic acid, 5-keto D-gluconate reductase, 2-keto D-gluconate reductase, Gluconobacter

JOURNAL FREE ACCESS Advance online publication

Article ID: 70259

DOI https://doi.org/10.1271/bbb.70259

The final version of this article is now available: Vol. 71 (2007) , No. 10 p.2478

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Abstract

For easy measurement of 5-keto D-gluconate (5KGA) and 2-keto D-gluconate (2KGA), two enzymes, 5KGA reductase (5KGR) and 2KGA reductase (2KGR) are useful. The gene for 5KGR has been reported, and a corresponding gene was found in the genome of Gluconobacter oxydans 621H and was identified as GOX2187. On the other hand, the gene for 2KGR was identified in this study as GOX0417 from the N-terminal amino acid sequence of the partially purified enzyme. Several plasmids were constructed to express GOX2187 and GOX0417, and the final constructed plasmids showed good expression of 5KGR and 2KGR in Escherichia coli. From the two E. coli transformants, large amounts of each enzyme were easily prepared after one column chromatography, and the preparation was ready to use for quantification of 5KGA or 2KGA.

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