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在炭疽菌与菜豆相互作用中形成的生物营养界面特异性真菌富含脯氨酸糖蛋白的表达克隆。

Expression cloning of a fungal proline-rich glycoprotein specific to the biotrophic interface formed in the Colletotrichum-bean interaction.

作者信息

Perfect S E, O'Connell R J, Green E F, Doering-Saad C, Green J R

机构信息

School of Biological Sciences, University of Birmingham, UK.

出版信息

Plant J. 1998 Jul;15(2):273-9. doi: 10.1046/j.1365-313x.1998.00196.x.

DOI:10.1046/j.1365-313x.1998.00196.x
PMID:9721685
Abstract

The monoclonal antibody, UB25, recognises a glycoprotein specifically located at the biotrophic interface formed in the Colletotrichum lindemuthianum-bean interaction. The antibody labels the walls of intracellular hyphae and the interfacial matrix which separates them from the invaginated host plasma membrane. In Western blots, UB25 recognises a ladder of bands which are multiples of M(r) 40.5 kDa. A full length cDNA encoding the glycoprotein recognised by UB25 has been isolated by expression cloning and designated CIH1 (Colletotrichum Intracellular Hypha 1). In vitro transcription/translation of CIH1, and transfection of mammalian COS cells, showed that UB25 recognized the expressed product in both procedures confirming that the clones isolated were true positives. Southern analysis of bean and C. lindemuthianum genomic DNA indicated that the CIH1 glycoprotein is fungally encoded and Northern analysis showed that it is only expressed in planta. Analysis of the deduced amino acid sequence of CIH1 indicates the presence of an N-terminal signal sequence and two possible sites for N-glycosylation. The N-terminal domain of the mature protein is rich in proline and contains several short repetitive motifs. CIH1 is thus a fungal proline-rich glycoprotein which appears to form a cross-linked structure in planta and, as such, resembles plant cell wall proline- and hydroxyproline-rich proteins. Possible functions for the CIH1 protein in the establishment and maintenance of biotrophy are discussed.

摘要

单克隆抗体UB25识别一种糖蛋白,该糖蛋白特异性位于炭疽菌与菜豆相互作用形成的活体营养界面处。该抗体标记细胞内菌丝的细胞壁以及将它们与内陷的宿主质膜分隔开的界面基质。在蛋白质免疫印迹中,UB25识别一系列条带,其分子量为40.5 kDa的倍数。通过表达克隆分离出编码UB25识别的糖蛋白的全长cDNA,并将其命名为CIH1(炭疽菌细胞内菌丝1)。CIH1的体外转录/翻译以及哺乳动物COS细胞的转染表明,在这两种操作中UB25都能识别表达产物,证实分离得到的克隆是真正的阳性克隆。对菜豆和炭疽菌基因组DNA的Southern分析表明,CIH1糖蛋白是由真菌编码的,Northern分析表明它仅在植物中表达。对CIH1推导的氨基酸序列的分析表明存在一个N端信号序列和两个可能的N糖基化位点。成熟蛋白的N端结构域富含脯氨酸,并包含几个短的重复基序。因此,CIH1是一种真菌富含脯氨酸的糖蛋白,它似乎在植物中形成交联结构,因此类似于植物细胞壁富含脯氨酸和羟脯氨酸的蛋白。文中讨论了CIH1蛋白在活体营养建立和维持中的可能功能。

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