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烟草I类几丁质酶基因启动子中乙烯应答区域的鉴定

Identification of an ethylene-responsive region in the promoter of a tobacco class I chitinase gene.

作者信息

Shinshi H, Usami S, Ohme-Takagi M

机构信息

Molecular Biology Department, National Institute of Bioscience and Human-Technology, Ibaraki, Japan.

出版信息

Plant Mol Biol. 1995 Mar;27(5):923-32. doi: 10.1007/BF00037020.

Abstract

The Chn48 gene is a representative of a family of tobacco class I basic chitinase genes, and the expression is induced by the stress hormone ethylene. To investigate the molecular basis for transcriptional regulation by ethylene we have examined the Chn48 promoter to identify cis-elements and trans-acting factors that are involved in the chitinase gene expression. In transgenic tobacco plants, a chimeric gene construct containing a 2 kb Chn48 promoter fused to a beta-glucuronidase reporter gene was induced by ethylene in leaf tissues. Deletion analysis indicated that a positive ethylene-responsive region is located between nucleotides -503 and -358 relative to the transcription initiation site. This 146 bp sequence was found to confer ethylene-responsive reporter gene expression when inserted in either orientation upstream of the heterologous promoter, indicating that the sequence functions as a regulatory enhancer. The ethylene-responsive region contains two copies of a GCC-box (TAAGAGCCGCC), which is conserved in a number of ethylene-responsive defense genes. The sequences within this ethylene-responsive region that are necessary for ethylene-responsive transcription were further localized to the 71 bp sequence between positions -480 and -410 containing two copies of the GCC-box by loss-of-function analysis. Gel mobility-shift experiments showed the presence of leaf nuclear factors that interact with the DNA sequences included in the ethylene-responsive region.

摘要

Chn48基因是烟草I类碱性几丁质酶基因家族的代表,其表达受应激激素乙烯的诱导。为了研究乙烯转录调控的分子基础,我们检测了Chn48启动子,以鉴定参与几丁质酶基因表达的顺式元件和反式作用因子。在转基因烟草植株中,一个包含与β-葡萄糖醛酸酶报告基因融合的2 kb Chn48启动子的嵌合基因构建体在叶片组织中受乙烯诱导。缺失分析表明,相对于转录起始位点,一个正向乙烯响应区域位于核苷酸-503至-358之间。当以任一方向插入异源启动子上游时,发现这个146 bp的序列可赋予乙烯响应报告基因表达,这表明该序列起调控增强子的作用。乙烯响应区域包含两个GCC-box(TAAGAGCCGCC)拷贝,这在许多乙烯响应防御基因中是保守的。通过功能缺失分析,乙烯响应转录所需的乙烯响应区域内的序列进一步定位到-480至-410位之间的71 bp序列,该序列包含两个GCC-box拷贝。凝胶迁移率变动实验表明存在与乙烯响应区域中包含的DNA序列相互作用的叶片核因子。

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