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引发过敏反应的烟草基因的克隆

Cloning of tobacco genes that elicit the hypersensitive response.

作者信息

Karrer E E, Beachy R N, Holt C A

机构信息

Scripps Research Institute, Division of Plant Biology BCC 206, La Jolla, CA 90237, USA.

出版信息

Plant Mol Biol. 1998 Mar;36(5):681-90. doi: 10.1023/a:1005949304445.

DOI:10.1023/a:1005949304445
PMID:9526500
Abstract

We used a functional screening method to isolate genes whose products elicit the hypersensitive response (HR) pathway of defense against plant pathogens. A cDNA library derived from tobacco leaves undergoing the HR was cloned into a tobacco mosaic virus (TMV)-based expression vector. Infectious transcripts were generated and used to inoculate tobacco plants lacking the N resistance gene (genotype Xanthi nn). Approximately 1/1000 of the infectious transcripts produced local lesions, and may thus elicit the HR. The cDNA inserts from 50 lesion-forming clones were recovered by RT-PCR, and 12 unique clones were sequenced. Comparisons with protein databases revealed homologies to (a) ubiquitin, (b) tobacco tumor-related protein, similar to Kunitz-type trypsin inhibitors and (c) ribosomal protein S14. The remaining nine clones revealed no homology to known proteins and are thus considered novel. Five clones were able to induce the expression of PR2, a gene which is specifically activated in the tobacco HR. Northern and western blot analyses of leaves infected by the clone encoding ubiquitin strongly suggest that the infection produced a co-suppression response; the endogenous level of ubiquitin mRNA and protein in infected leaves are ca. 50% less than those found in healthy leaves. This observation supports a previous report on the involvement of the ubiquitin system in the tobacco HR [2], and validates and utility of the functional cloning method.

摘要

我们采用一种功能筛选方法来分离其产物引发植物病原体防御过敏反应(HR)途径的基因。将来自经历HR的烟草叶片的cDNA文库克隆到基于烟草花叶病毒(TMV)的表达载体中。产生感染性转录本并用于接种缺乏N抗性基因的烟草植株(基因型Xanthi nn)。大约1/1000的感染性转录本产生局部病斑,因此可能引发HR。通过RT-PCR回收来自50个形成病斑克隆的cDNA插入片段,并对12个独特克隆进行测序。与蛋白质数据库的比较揭示了与(a)泛素、(b)烟草肿瘤相关蛋白(类似于Kunitz型胰蛋白酶抑制剂)和(c)核糖体蛋白S14的同源性。其余9个克隆与已知蛋白无同源性,因此被认为是新的。5个克隆能够诱导PR2的表达,PR2是在烟草HR中特异性激活的基因。对受编码泛素的克隆感染的叶片进行Northern和Western印迹分析强烈表明,感染产生了共抑制反应;感染叶片中泛素mRNA和蛋白的内源水平比健康叶片中低约50%。这一观察结果支持了先前关于泛素系统参与烟草HR的报道[2],并验证了功能克隆方法的有效性和实用性。

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