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生长素受体的特性描述。

Characterisation of auxin receptors.

作者信息

Venis M A, Napier R M

机构信息

AFRC Institute of Horticultural Research, Kent, UK.

出版信息

Symp Soc Exp Biol. 1990;44:55-65.

PMID:1966638
Abstract

Many auxin-binding systems, both membrane-bound and soluble, have been studied, but most lack credibility as receptors. The exception and best candidate as a valid auxin receptor is the auxin-binding protein of maize coleoptile membranes. This protein can be readily solubilised from the membranes and has been purified to homogeneity. It is a glycosylated homodimer of 22 kDa subunits. Preparations of minimum 50% purity were used to immunise rats and five monoclonal antibodies have been derived. Two of these can be mapped to epitopes within a C-terminal 1 kDa region, while the epitope of a third is within 7 kDa of the N-terminus. Immunotitration of receptor abundance in different tissues of maize seedlings shows that roots contain 40-fold less receptor protein per gram of fresh weight than coleoptiles. Pure receptor was produced by native PAGE and used to generate a high titer polyclonal antiserum in rabbits, capable of detecting receptor protein from as little as 1 mg of coleoptile tissue. The polyclonal specifically precipitates the 22 kDa polypeptide from maize membrane extracts, concomitant with removal of auxinbinding activity. The antiserum also detects homologous polypeptides in maize supernatant and in several other species, both monocots and dicots. In some cases, differences in chromatographic behaviour or size have been found. An auxin-induced conformational change in the receptor has been detected with a sandwich ELISA. The receptor gene has been cloned in four laboratories and the sequence data with knowledge of antibody epitopes can be used to identify parts of the protein involved in conformational changes (and perhaps auxin action). We are currently raising antibodies to a polypeptide thought to be part of the auxin binding site. Most of the auxin-binding protein is found in the endoplasmic reticulum but electrophysiological evidence, using polyclonal antiserum and impermeant auxin conjugates on protoplasts, suggests that a small population of functional receptor is accessible at the exterior face of the plasma membrane. Evidence bearing on the localisation and structure of the receptors is discussed.

摘要

人们已经对许多生长素结合系统进行了研究,包括膜结合型和可溶型,但大多数作为受体缺乏可信度。作为有效的生长素受体的例外且最佳候选者是玉米胚芽鞘膜的生长素结合蛋白。这种蛋白质可以很容易地从膜中溶解出来,并已纯化至同质。它是由22 kDa亚基组成的糖基化同型二聚体。使用纯度至少为50%的制剂免疫大鼠,已获得五种单克隆抗体。其中两种可以定位到C末端1 kDa区域内的表位,而第三种的表位在N末端的7 kDa范围内。对玉米幼苗不同组织中受体丰度的免疫滴定表明,根中每克鲜重所含的受体蛋白比胚芽鞘少40倍。通过天然聚丙烯酰胺凝胶电泳制备了纯受体,并用于在兔中产生高滴度的多克隆抗血清,该抗血清能够从低至1 mg的胚芽鞘组织中检测到受体蛋白。多克隆抗体能从玉米膜提取物中特异性沉淀出22 kDa的多肽,同时去除生长素结合活性。该抗血清还能检测玉米上清液以及其他几个物种(单子叶植物和双子叶植物)中的同源多肽。在某些情况下,已发现色谱行为或大小存在差异。用夹心酶联免疫吸附测定法检测到受体中生长素诱导的构象变化。该受体基因已在四个实验室中克隆,结合抗体表位的序列数据可用于识别蛋白质中参与构象变化(可能还有生长素作用)的部分。我们目前正在制备针对一种被认为是生长素结合位点一部分的多肽的抗体。大多数生长素结合蛋白存在于内质网中,但使用多克隆抗血清和原生质体上的非渗透性生长素缀合物的电生理证据表明,一小部分功能性受体可在质膜外表面被检测到。文中讨论了有关受体定位和结构的证据。

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