The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植病原原核生究得最清楚是胡萝卜软腐菌果胶酸内裂解酶。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

与果胶酸裂解酶底同。胡萝卜软腐欧氏菌多个亚种产生此酶，但菊欧氏菌不产生。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件细胞异柠檬酸裂解酶活性和异柠檬酸脱氢酶活性分别是对照1.48倍和75%。

The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植物病原原核生物中研究得最清楚是胡萝卜软腐菌果胶酸内裂解。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

与果胶酸裂解底物同。胡萝卜软腐欧氏菌多个亚种产生此，但菊欧氏菌不产生。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件下细胞异柠檬酸裂解活性和异柠檬酸活性分别是对照1.48倍和75%。

The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植物病原原核生物中研究得最清楚的是胡萝卜软腐菌的果胶内裂解酶。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

与果胶裂解酶的底物同。胡萝卜软腐欧氏菌的多个亚种产生此酶，但菊欧氏菌不产生。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件下的细胞异裂解酶活性和异脱氢酶活性分别是对照的1.48倍和75%。

The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植物病原原核生物中研究得最清楚是胡萝卜软腐胶酸内裂解。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

胶酸裂解底物同。胡萝卜软腐欧氏个亚种产生此，但菊欧氏不产生。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件下细胞异柠檬酸裂解活性和异柠檬酸脱氢活性分别是对照1.48倍和75%。

The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植物病原原核生物中研究得最清楚是胡萝卜软腐菌果胶内裂解酶。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

与果胶裂解酶底物同。胡萝卜软腐欧氏菌多个亚种产生此酶，但菊欧氏菌不产生。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件下细胞异柠裂解酶活性和异柠氢酶活性分别是对照1.48倍和75%。

The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植物病原原核生物中研究得最清楚的是胡萝软菌的果胶酸内。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

与果胶酸的底物同。胡萝软欧氏菌的多个亚种产生此，但菊欧氏菌不产生。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件下的细胞异柠檬酸活性和异柠檬酸脱氢活性分别是对照的1.48倍和75%。

The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植物病原原核生物中研究得最清楚的是胡萝卜软腐菌的果胶酸酶。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

与果胶酸酶的底物同。胡萝卜软腐欧氏菌的多产生此酶，但菊欧氏菌不产生。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件下的细胞异柠檬酸酶活性和异柠檬酸脱氢酶活性分别是对照的1.48倍和75%。

The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植物病原原核生物中研究得最清楚是胡萝卜软腐菌果胶酸内裂解。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

与果胶酸裂解底物同。胡萝卜软腐欧氏菌多个亚种产生此，但菊欧氏菌不产生。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件下细胞异柠檬酸裂解活性和异柠檬酸活性分别是对照1.48倍和75%。

The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植物病物中研究得最清楚的是胡萝卜软腐菌的果胶酸内裂解酶。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

与果胶酸裂解酶的底物同。胡萝卜软腐欧氏菌的多个亚种产此酶，但菊欧氏菌不产。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件下的柠檬酸裂解酶活性和柠檬酸脱氢酶活性分别是对照的1.48倍和75%。

The best studied inducible and repressible enzyme in phytopathogenic prokaryotes is endo-pectate lyase in E. carotovora.

植物病原原核生物中研究得最清楚的是胡萝卜软腐菌的果胶酸酶。

Polygalacturonase has the same substrate specificity as pectate lyase. This enzyme is produced by Erwinia carotovora subspp. but not by Erwinia chyrsanthemi.

与果胶酸酶的底物同。胡萝卜软腐欧氏菌的多产生此酶，但菊欧氏菌不产生。

Moreover, the activities of isocitrate lyase and isocitrate dehydrogenase in the 0 P-treated cells were 1.48 and 0.75 times higher than in the control at day 8 of the treatment.

在第8 d，缺磷条件下的细胞异柠檬酸酶活性和异柠檬酸脱氢酶活性分别是对照的1.48倍和75%。