Abstract

The aim of this work was to transform ginsenoside extract into the pharmacologically active minor ginsenoside 20(S)-Rg3 by three thermostable glycosidases. The GH1 thermostable beta-glucosidase Tpebgl1 from Thermotoga petrophlia was found to have the ability to convert ginsenosides Rb1 and Rb2. Its properties concerning ginsenoside conversion were systematically investigated. It had high specific activity on pNPG (162·20Umg-1 ) and pNPArp (22·14Umg-1 ). The Km and Vmax of Tpebgl1 for pNPG were 0·28mmoll-1 and 470·2Umg-1 and for pNPArp were 17·30mmoll-1 and 74·28Umg-1 . Therefore, it could successfully convert ginsenosides Rb1 and Rb2 into ginsenoside Rd, which has been proven byexperiments in this paperthen. Tpebgl1 also had good tolerance to glucose and some organic solvents. These made Tpebgl1 a good catalyst candidate for industrial application. Finally, it was applied to convert ginsenoside extract into the pharmacologically active minor ginsenoside 20(S)-Rg3, combined with thermostable ginsenoside Rc converting α-1,6-l-arabinofranosidase Tt-Afs and ginsenoside Rd converting β-glucosidase Tpebgl3. A quantity of 10gl-1 of ginsenoside extract was transformed into 3·93gl-1 of Rg3 at 90°C, pH 5·0 for 3h, with a corresponding molar conversion of 98·19%. The thermostable enzyme Tpebgl1 was found to be a ginsenoside-converting enzyme and successfully applied in the preparation ofginsenoside 20(S)-Rg3 from ginsenoside extract. The three-stepcooperate transformation system of ginsenoside extract was established by using Tpebgl1,Tt-Afs (athermostable ginsenoside Rc converting α-1,6-l-arabinofranosidase) and Tpebgl3 (athermostableginsenoside Rb1 converting β-glucosidase). Converting all the major ginsenosides into protopanaxadiol-type ginsenoside extract would greatly reduce the cost of ginsenoside Rg3 preparation. Enzymes from thermophilic bacteria can meet the requirement of higher reaction temperatures in industrial reactions for substrate solubility promotion and bacterial contamination prevention.

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