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An octopine synthase enhancer element directs tissue-specific expression and binds ASF-1 a factor from tobacco nuclear extracts.

机译:章鱼碱合酶增强子元件指导组织特异性表达并结合ASF-1(一种来自烟草核提取物的因子)。

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摘要

We have investigated the expression pattern conferred by a cis-regulatory element (-212 to -154) from the upstream region of the octopine synthase (ocs) gene in transgenic tobacco plants. Analysis of beta-glucuronidase expression driven by the ocs regulatory element revealed a pattern that is tissue-specific and developmentally regulated. In young seedlings, expression is confined primarily to root tips. In older seedlings, expression is stronger and becomes apparent also in the shoot apex. Insertion of a 16-base pair palindromic sequence (-193 to -178), which is included in the regulatory element, into an rbcS promoter results in the expression of rbcS in roots. The 16-base pair palindrome binds activation sequence factor (ASF)-1, a factor from tobacco nuclear extracts that interacts with the sequence between -83 to -63, designated as activation sequence (as)-1, of the cauliflower mosaic virus 35S promoter [Lam et al. (1989). Proc. Natl. Acad. Sci. USA 86, in press]. The in vivo expression patterns and in vitro binding properties of the ocs palindromic sequence are remarkably similar to those of the as-1 element of the cauliflower mosaic virus 35S promoter. These results suggest the involvement of ASF-1 in the transcriptional regulation of the ocs promoter and the 35S promoter.
机译:我们已经研究了从转基因烟草植物中章鱼碱合酶(ocs)基因上游区域的顺式调控元件(-212至-154)赋予的表达模式。由ocs调节元件驱动的β-葡萄糖醛酸苷酶表达的分析揭示了一种组织特异性和发育受调节的模式。在幼苗中,表达主要限于根尖。在较老的幼苗中,表达更强并且在茎尖也变得明显。将包含在调控元件中的16个碱基对的回文序列(-193至-178)插入rbcS启动子,导致rbcS在根中表达。 16个碱基对的回文结合了激活序列因子(ASF)-1,该因子来自烟草核提取物,与花椰菜花叶病毒35S的-83至-63之间的序列相互作用,称为激活序列(as)-1启动子[La​​m等。 (1989)。程序Natl。学院科学USA 86,印刷中]。 ocs回文序列的体内表达模式和体外结合特性与花椰菜花叶病毒35S启动子的as-1元件非常相似。这些结果表明ASF-1参与了ocs启动子和35S启动子的转录调控。

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