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T-DNA介导的翻译型β-葡萄糖醛酸酶基因融合分析

Analysis of T-DNA-mediated translational beta-glucuronidase gene fusions.

作者信息

Kertbundit S, Linacero R, Rouzé P, Galis I, Macas J, Deboeck F, Renckens S, Hernalsteens J P, De Greve H

机构信息

Laboratorium Genetische Virologie, Vrije Universiteit Brussel, Sint-Genesius-Rode, Belgium.

出版信息

Plant Mol Biol. 1998 Jan;36(2):205-17. doi: 10.1023/a:1005902730810.

Abstract

Three random translational beta-glucuronidase (gus) gene fusions were previously obtained in Arabidopsis thaliana, using Agrobacterium-mediated transfer of a gus coding sequence without promoter and ATG initiation site. These were analysed by IPCR amplification of the sequence upstream of gus and nucleotide sequence analysis. In one instance, the gus sequence was fused, in inverse orientation, to the nos promoter sequence of a truncated tandem T-DNA copy and translated from a spurious ATG in this sequence. In the second transgenic line, the gus gene was fused to A. thaliana DNA, 27 bp downstream an ATG. In this line, a large deletion occurred at the target site of the T-DNA. In the third line, gus is fused in frame to a plant DNA sequence after the eighth codon of an open reading frame encoding a protein of 619 amino acids. This protein has significant homology with animal and plant (receptor) serine/threonine protein kinases. The twelve subdomains essential for kinase activity are conserved. The presence of a potential signal peptide and a membrane-spanning domain suggests that it may be a receptor kinase. These data confirm that plant genes can be tagged as functional translational gene fusions.

摘要

之前通过农杆菌介导转移无启动子和ATG起始位点的gus编码序列,在拟南芥中获得了三个随机的翻译型β-葡萄糖醛酸酶(gus)基因融合体。通过对gus上游序列进行反向PCR扩增和核苷酸序列分析对其进行了分析。在一个实例中,gus序列以反向方向与截短的串联T-DNA拷贝的nos启动子序列融合,并从该序列中的一个假ATG起始翻译。在第二个转基因系中,gus基因与拟南芥DNA融合,位于一个ATG下游27 bp处。在这个系中,T-DNA的靶位点发生了大片段缺失。在第三个系中,gus与一个编码619个氨基酸的蛋白质的开放阅读框的第八个密码子后的植物DNA序列读框内融合。该蛋白质与动物和植物(受体)丝氨酸/苏氨酸蛋白激酶具有显著同源性。激酶活性所必需的十二个亚结构域是保守的。潜在信号肽和跨膜结构域的存在表明它可能是一种受体激酶。这些数据证实植物基因可以被标记为功能性翻译基因融合体。

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