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以脱落酸 - 蛋白质缀合物作为亲和探针检测拟南芥微粒体蛋白组分中的脱落酸结合蛋白。

Detection of abscisic-acid-binding proteins in the microsomal protein fraction of Arabidopsis thaliana with abscisic-acid-protein conjugates used as affinity probes.

作者信息

Pedron J, Brault M, Nake C, Miginiac E

机构信息

Laboratoire de Physiologie du Développement des Plantes, URA CNRS 2135, Université Pierre et Marie Curie (Paris VI), France.

出版信息

Eur J Biochem. 1998 Mar 15;252(3):385-90. doi: 10.1046/j.1432-1327.1998.2520385.x.

DOI:10.1046/j.1432-1327.1998.2520385.x
PMID:9546653
Abstract

A family of affinity probes has been generated to detect and purify abscisic-acid (ABA)-binding proteins, by coupling ABA onto carrier proteins (ovalbumin or BSA) through the C1 carboxyl group or the C4' carbonyl group of ABA. ELISA detection showed that these ABA-protein conjugates bound efficiently to the solubilized microsomal protein fraction of Arabidopsis thaliana, but not to the soluble protein fraction. Heat or proteolytic treatments inhibited the binding of the conjugates, indicating the protein nature of these binding sites. After membrane purification of the microsomes, the binding sites were found to be preferentially located in the plasma membrane fraction. The binding of the conjugates was independent of the nature of the carrier protein or the ABA-carrier protein linker, but was competitively inhibited with an anti-ABA mAb. Furthermore, the competitive inhibition of the binding of the conjugates with ABA, but not with the inactive ABA methyl ester analog, demonstrated the specificity of the binding and the saturability of the binding sites. The binding of the conjugates was strictly correlated to the ABA/carrier protein molar coupling ratio, confirming that the affinity of the conjugates to the ABA-binding proteins was enhanced by the increase in the probability of binding events. The experimental approach permits a new insight into the nature of membrane-associated ABA-binding proteins.

摘要

通过将脱落酸(ABA)通过其C1羧基或C4'羰基偶联到载体蛋白(卵清蛋白或牛血清白蛋白)上,已生成了一系列亲和探针,用于检测和纯化ABA结合蛋白。酶联免疫吸附测定(ELISA)检测表明,这些ABA-蛋白偶联物能有效地结合拟南芥可溶性微粒体蛋白组分,但不能结合可溶性蛋白组分。加热或蛋白酶处理会抑制偶联物的结合,这表明这些结合位点具有蛋白质性质。对微粒体进行膜纯化后,发现结合位点优先位于质膜组分中。偶联物的结合与载体蛋白的性质或ABA-载体蛋白连接子无关,但会被抗ABA单克隆抗体竞争性抑制。此外,偶联物与ABA而非无活性的ABA甲酯类似物的结合竞争抑制,证明了结合的特异性和结合位点的可饱和性。偶联物的结合与ABA/载体蛋白的摩尔偶联比严格相关,证实了偶联物与ABA结合蛋白的亲和力因结合事件概率的增加而增强。该实验方法为膜相关ABA结合蛋白的性质提供了新的见解。

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