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转化植物合成农杆碱所需的一个T-DNA基因,在功能和进化上与根癌土壤杆菌菌株分解农杆碱所需的一个Ti质粒基因相关。

A T-DNA gene required for agropine biosynthesis by transformed plants is functionally and evolutionarily related to a Ti plasmid gene required for catabolism of agropine by Agrobacterium strains.

作者信息

Hong S B, Hwang I, Dessaux Y, Guyon P, Kim K S, Farrand S K

机构信息

Department of Crop Sciences, University of Illinois at Urbana-Champaign, Urbana 61801, USA.

出版信息

J Bacteriol. 1997 Aug;179(15):4831-40. doi: 10.1128/jb.179.15.4831-4840.1997.

Abstract

The mechanisms that ensure that Ti plasmid T-DNA genes encoding proteins involved in the biosynthesis of opines in crown gall tumors are always matched by Ti plasmid genes conferring the ability to catabolize that set of opines on the inducing Agrobacterium strains are unknown. The pathway for the biosynthesis of the opine agropine is thought to require an enzyme, mannopine cyclase, coded for by the ags gene located in the T(R) region of octopine-type Ti plasmids. Extracts prepared from agropine-type tumors contained an activity that cyclized mannopine to agropine. Tumor cells containing a T region in which ags was mutated lacked this activity and did not contain agropine. Expression of ags from the lac promoter conferred mannopine-lactonizing activity on Escherichia coli. Agrobacterium tumefaciens strains harboring an octopine-type Ti plasmid exhibit a similar activity which is not coded for by ags. Analysis of the DNA sequence of the gene encoding this activity, called agcA, showed it to be about 60% identical to T-DNA ags genes. Relatedness decreased abruptly in the 5' and 3' untranslated regions of the genes. ags is preceded by a promoter that functions only in the plant. Expression analysis showed that agcA also is preceded by its own promoter, which is active in the bacterium. Translation of agcA yielded a protein of about 45 kDa, consistent with the size predicted from the DNA sequence. Antibodies raised against the agcA product cross-reacted with the anabolic enzyme. These results indicate that the agropine system arose by a duplication of a progenitor gene, one copy of which became associated with the T-DNA and the other copy of which remained associated with the bacterium.

摘要

确保冠瘿瘤中编码参与冠瘿碱生物合成的蛋白质的Ti质粒T-DNA基因总是与赋予诱导农杆菌菌株分解该组冠瘿碱能力的Ti质粒基因相匹配的机制尚不清楚。冠瘿碱农杆碱的生物合成途径被认为需要一种由章鱼碱型Ti质粒T(R)区域中的ags基因编码的甘露碱环化酶。从农杆碱型肿瘤中制备的提取物含有一种将甘露碱环化为农杆碱的活性。含有ags发生突变的T区域的肿瘤细胞缺乏这种活性,并且不含有农杆碱。来自lac启动子的ags表达赋予大肠杆菌甘露碱内酯化活性。携带章鱼碱型Ti质粒的根癌农杆菌菌株表现出类似的活性,该活性不是由ags编码的。对编码这种活性的基因(称为agcA)的DNA序列分析表明,它与T-DNA ags基因约60%相同。基因的5'和3'非翻译区的相关性急剧下降。ags之前有一个仅在植物中起作用的启动子。表达分析表明,agcA之前也有其自身的启动子,该启动子在细菌中具有活性。agcA的翻译产生了一种约45 kDa的蛋白质,与从DNA序列预测的大小一致。针对agcA产物产生的抗体与合成代谢酶发生交叉反应。这些结果表明,农杆碱系统是由一个祖先基因的复制产生的,其中一个拷贝与T-DNA相关联,另一个拷贝仍然与细菌相关联。

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