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Partial Characterization of Glutathione S-Transferase Isozymes Induced by the Herbicide Safener Benoxacor in Maize.

机译:除草剂Safener Benoxacor在玉米中诱导的谷胱甘肽S-转移酶同工酶的部分表征。

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摘要

The effects of the dichloroacetamide safener benoxacor on maize (Zea mays L. var Pioneer 3906) growth and glutathione S-transferase (GST) activity were evaluated, and GST isozymes induced by benoxacor were partially separated, characterized, and identified. Protection from metolachlor injury was closely correlated with GST activity, which was assayed with metolachlor as a substrate, as benoxacor concentration increased from 0.01 to 1 [mu]M. GST activity continued to increase at higher benoxacor concentrations (10 and 100 [mu]M), but no further protection was observed. Total GST activity with metolachlor as a substrate increased 2.6- to 3.8-fold in response to 1 [mu]M benoxacor treatment. Total GST activity from maize treated with or without 1 [mu]M benoxacor was resolved by fast protein liquid chromatography anion-exchange chromatography into four major activities, designated activity peaks A, B, C, and D in their order of elution. These GST activity peaks were enhanced to varying degrees by benoxacor. Activity peak B showed the least induction, whereas activity peak A was absent constitutively and thus highly induced by benoxacor. In contrast to earlier reports, there appear to be not one, but at least two, major constitutive isozymes (activity peaks A and D) having activity with metolachlor as substrate; there were at least three such isozymes in benoxacor-treated maize (activity peaks A, C, and D). The elution volumes of activity peaks A, B, C, and D were compared with those of partially purified maize GST I and GST II; also, the reactivity of polypeptides in these activity peaks with antisera to GST I or GST I/III (mixture) was evaluated. Evidence from these experiments indicated that activity peak B contained GST I, and activity peak C contained GST II and GST III. Activity peaks A and D contained unique GSTs that may play a major role in metolachlor metabolism and in the safening activity of benoxacor in maize. Isozymes present in activity peaks A and D were not detected in earlier reports because of the very low activity with the artificial substrate 1-chloro-2,4-dinitrobenzene. Immunoblotting experiments also indicated the presence of numerous unidentified GST subunits, including multiple subunits in chromatography fractions containing single peaks of GST activity; this is indicative of the likely complexity and diversity of the maize GST enzyme family.
机译:评价了二氯乙酰胺安全性贝诺沙克对玉米(Zea mays L.var Pioneer 3906)生长和谷胱甘肽S-转移酶(GST)活性的影响,并部分分离,表征和鉴定了由贝诺沙克诱导的GST同工酶。甲霜灵的浓度从0.01μM增加到1μM时,保护免受甲草胺的伤害与GST活性密切相关,GST活性以甲草胺为底物进行了分析。在较高的苯甲酸酯浓度(10和100μM)下,GST活性继续增加,但是未观察到进一步的保护作用。响应于1μM的苯甲酸酯处理,以异丙甲草胺为底物的总GST活性增加了2.6-至3.8倍。通过快速蛋白质液相色谱阴离子交换色谱将用或不用1μMbenoxacor处理的玉米的总GST活性分解为四个主要活性,以洗脱顺序命名为活性峰A,B,C和D。苯甲酸酯使这些GST活性峰得到不同程度的增强。活性峰B表现出最少的诱导,而活性峰A组成性地不存在,因此被苯甲酸酯高度诱导。与以前的报道相反,似乎没有一种,但至少有两种主要的组成型同功酶(活性峰A和D)具有以异丙甲草胺为底物的活性。在贝诺沙克处理过的玉米中至少有三种同工酶(活性峰A,C和D)。将活性峰A,B,C和D的洗脱量与部分纯化的玉米GST I和GST II的洗脱量进行比较;还评估了这些活性峰中的多肽对GST I或GST I / III(混合物)的抗血清反应性。这些实验的证据表明,活性峰B包含GST I,而活性峰C包含GST II和GST III。活性峰A和D包含独特的GST,这些GST可能在甲草胺的代谢和苯甲沙星在玉米中的安全活性中起主要作用。早期报道中未检测到活性峰A和D中存在的同功酶,因为人工底物1-氯-2,4-二硝基苯的活性非常低。免疫印迹实验还表明存在大量未鉴定的GST亚基,包括含有GST活性单峰的色谱级分中的多个亚基。这表明玉米GST酶家族可能具有复杂性和多样性。

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