Journal of Ginseng Research
- Volume 9 Issue 2
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- Pages.154-162
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- 1985
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- 1226-8453(pISSN)
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- 2093-4947(eISSN)
A New Method on the Measurement of Catalase Activity of Panax ginseng C.A. Meyer Tissues
인삼조직에서 Catalase Activity측정에 관한 새로운 Method
- Yang, Deok-Cho (Department of Biology, Chungbuk National University) ;
- Chae, Quae (Department of Chemistry, Chungbuk National University) ;
- Yoon, Jae-Jun (Department of Biology, Chungbuk National University) ;
- Lee, Sung-Jong (Department of Biology, Chungbuk National University) ;
- Lee, Ae-Ra (Department of Biology, Chungbuk National University)
- 양덕조 (충북대학교 자연대 생물학과) ;
- 채쾌 (충북대학교 자연대 화학과) ;
- 윤재준 (충북대학교 자연대 생물학과) ;
- 이성종 (충북대학교 자연대 생물학과) ;
- 이애라 (충북대학교 자연대 생물학과)
- Published : 1985.12.01
Abstract
We report a newassay method on the measurement of the catalase activity, whose utilzation value is considered to be remarkable in the field of plant biochemistry. We named this method as a De-Coupling method. The essence of de-coupling method is the separation between the enzyme reaction and the indicator reaction. The optimum condition of the enzyme reaction was found to be following: on addition of 1 ml of substrate (H2O2: 20mM) to the fixture of the crude extract of enzyme (volume: 0.2 ml) and the ammonium phosphate buffer (volume: 1.8 ml; 0.93 M phosphate, 1.6M NHB, 2.5 M methanol, pH 7.0). After 30, 60 and 90 seconds of the enzyme reactions are proceeded, the reactions are terminated by 25% of tai-chloro-acetate (final concentration of 5%), respectively. The precipitated materials by tai-chloro-acetate was removed by the centrifugation (2000g, 10minutes). Formaldehyde produced in the enzymatic reaction was reacted with 2ml of acetylacetone (60mM). The indicator reaction -(HANTSCH REAKT10N)- in which lutidine is formed, was proceeded for 60 minutes at
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