首页> 外文OA文献 >Hubungan Aktivitas Enzim Dan Konsentrasi Substrat Pada Pola Deteksi Secara Hplc Hasil Transglikosilasi Naringenin Oleh Enzim Selulase Penicillium SP. Lbkurcc27
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Hubungan Aktivitas Enzim Dan Konsentrasi Substrat Pada Pola Deteksi Secara Hplc Hasil Transglikosilasi Naringenin Oleh Enzim Selulase Penicillium SP. Lbkurcc27

机译:青霉纤维素酶SP对柚皮素转糖基化结果的Hplc检测模式中酶活性和底物浓度的关系。 Lbkurcc27

摘要

Transglycosylation of naringenin was carried out by concentrated cellulase enzyme of Penicillium sp. LBKURCC27. Enzymatic transglycosylation of naringenin was successfully carried out by cellulase from Penicillium sp. LBKURCC27, however the reproducibility of the reaction is low, making detection by reverse phase HPLC (High Performance Liquid Chromatography) difficult when the enzyme activity decreases. It is believe that the flavonoid concentration used in the transglycosylation naringenin by cellulase Penicillium sp. LBKURCC27 influences the detection pattern of transglycosylation product of HPLC. The reaction was carried out for 30 hours at 40°C with acetate buffer 0.05 M pH 5.5 and 170 rpm shaking. Carboxymethyl Cellulose (CMC) was used as glycosyl donor. Results of HPLC analysis showed that cellulase Penicillium sp. LBKURCC27 with an activity of (0.670±0.023 U/mL) were not able to convert naringenin to a detectable glycosylated product when the initial substrate concentration was 6 mg/mL. In the 0.6 mg/mL of naringenin concentration, the glycosylation product was formed with 100% of percent convertion.
机译:柚皮素的转糖基化是通过青霉菌的浓缩纤维素酶进行的。 LBKURCC27。柚皮素的纤维素酶成功地实现了柚皮素的酶促糖基化。 LBKURCC27,但是反应的重现性低,当酶活性降低时,很难通过反相HPLC(高效液相色谱)进行检测。相信纤维素酶青霉属(Penicillium sp。)在转糖基柚皮素中使用的类黄酮浓度。 LBKURCC27影响HPLC转糖基化产物的检测模式。反应在40℃下用0.05M pH 5.5的乙酸盐缓冲液和170rpm摇动进行30小时。羧甲基纤维素(CMC)用作糖基供体。 HPLC分析结果表明纤维素酶青霉属。当初始底物浓度为6 mg / mL时,活性为(0.670±0.023 U / mL)的LBKURCC27无法将柚皮苷转化为可检测的糖基化产物。在浓度为0.6 mg / mL的柚皮素中,糖基化产物的转化率为100%。

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