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以过酸形成作为用卤过氧化物酶转化的植物抗感染基础的评估。

Evaluation of peracid formation as the basis for resistance to infection in plants transformed with haloperoxidase.

作者信息

Jacks T J, Rajasekaran K, Stromberg K D, De Lucca A J, van Pée K-H

机构信息

Southern Regional Research Center, Agricultural Research Service, U.S. Department of Agriculture, 1100 Robert E. Lee Boulevard, New Orleans, Louisiana 70124, USA.

出版信息

J Agric Food Chem. 2002 Feb 13;50(4):706-9. doi: 10.1021/jf011006q.

Abstract

Nonheme haloperoxidase (HPO-P) isolated from Pseudomonas pyrrocinia catalyzed the peroxidation of alkyl acids to peracids. Among acids tested as substrates, acetic acid was most readily peroxidized. The reaction product peracetate possessed potent antifungal activity: 50% death (LD(50)) of Aspergillus flavus occurred at 25 microM peracetate. Viability of A. flavus was inhibited by up to 80% by leaf extracts of tobacco plants transformed with the HPO-P gene from P. pyrrocinia compared to viability of fungi exposed to extracts from controls. To elucidate if peracid formation by HPO-P was the basis for antifungal activity in transgenic leaf tissues, lethalities of hydrogen peroxide-acetate-HPO-P combinations against A. flavus were examined in vitro. LD(50) of A. flavus exposed to the combinations occurred at 30 mM acetate when concentrations of hydrogen peroxide and HPO-P were held constant. This value was identical to the LD(50) produced by 30 mM acetate in the absence of hydrogen peroxide-HPO-P and therefore did not account for enhanced antifungal activity in transgenic plants. For clarification, kinetics of the enzymic reaction were examined. According to the concentration of acetate needed for enzyme saturation (K(m) = 250 mM), acetate was lethal prior to its oxidation to peracetate. Results indicate that peracid generation by HPO-P was not the basis for enhanced antifungal activity in transgenic plants expressing the HPO-P gene.

摘要

从吡咯假单胞菌中分离出的非血红素卤过氧化物酶(HPO-P)催化脂肪酸过氧化生成过酸。在所测试的作为底物的酸中,乙酸最容易被过氧化。反应产物过乙酸具有强大的抗真菌活性:黄曲霉50%死亡(半数致死剂量,LD(50))发生在25微摩尔的过乙酸浓度下。与接触对照提取物的真菌活力相比,用来自吡咯假单胞菌的HPO-P基因转化的烟草植株叶片提取物可将黄曲霉的活力抑制高达80%。为了阐明HPO-P形成过酸是否是转基因叶片组织中抗真菌活性的基础,在体外检测了过氧化氢-乙酸-HPO-P组合对黄曲霉的致死率。当过氧化氢和HPO-P的浓度保持恒定时,接触该组合的黄曲霉的LD(50)出现在30毫摩尔乙酸浓度下。该值与在无过氧化氢-HPO-P情况下30毫摩尔乙酸产生的LD(50)相同,因此不能解释转基因植物中增强的抗真菌活性。为了弄清楚,研究了酶促反应的动力学。根据酶饱和所需的乙酸浓度(米氏常数K(m)=250毫摩尔),乙酸在氧化成过乙酸之前就具有致死性。结果表明,HPO-P产生过酸不是表达HPO-P基因的转基因植物中增强抗真菌活性的基础。

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