島根大学農学部
ISSN:0370-940X
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島根大学農学部研究報告 20
1986-12-20 発行
キノチアミンおよびL-システインエチルエステルを基質とする新チアミナーゼ活性測定法
A New Method for the Determination of Thiaminase Activity by the Use of Quinothiamine and L-Cysteine Ethylester as Substrates
持田 和男
尾添 嘉久
中村 利家
長尾 敏夫
鈴木 喜六
ファイル
内容記述(抄録等)
A new method for the determination of transferase activity of thiaminase I and II was proposed. Thiaminase II which has been classified into a hydrolase showed transferase activity by the use of quinothiamine (Pm-quinoline) and L-cysteine ethylester as substrates.
Transferase activity of thiaminase I or II at 37℃ was able to be evaluated from the time course of absorbance (315 nm) for the reaction solution prepared by mixing 0.3 ml of 2 mM Pm-quinoline, 0.3 ml of 500 mM L-cysteine ethylester, 2.0 ml of 0.1 M Tris-HCl buffer (pH 8.8), and 0.4 ml of the enzyme solution. The Km values for Pm-quinoline and L-cysteine ethylester were determined to be 0.025 and 7.1 mM, respectively, in the case of thiaminase I and 0.094 and 0.9 mM, respectively, in the case of thiaminase II.
Transferase activity of thiaminase I or II at 37℃ was able to be evaluated from the time course of absorbance (315 nm) for the reaction solution prepared by mixing 0.3 ml of 2 mM Pm-quinoline, 0.3 ml of 500 mM L-cysteine ethylester, 2.0 ml of 0.1 M Tris-HCl buffer (pH 8.8), and 0.4 ml of the enzyme solution. The Km values for Pm-quinoline and L-cysteine ethylester were determined to be 0.025 and 7.1 mM, respectively, in the case of thiaminase I and 0.094 and 0.9 mM, respectively, in the case of thiaminase II.
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AN00108015
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PP. 191 - 195