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Inefficient reinitiation is responsible for upstream open reading frame-mediated translational repression of the maize R gene.

机译:低效的重新初始化是导致上游开放阅读框介导的玉米R基因翻译抑制的原因。

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摘要

Maize R genes encode a small family of transcriptional activators of several structural genes in the anthocyanin biosynthetic pathway. The 5' leader region of most R genes contains a 38-codon upstream open reading frame (uORF) that previously was shown to be responsible for the repression of downstream gene expression in a transient transformation assay. In this study, we report that the 5' leader also can repress translation of the downstream luciferase gene both in the rabbit reticulocyte translation system and in transgenic rice plants. The ability to visualize the uORF peptide after in vitro translation permits quantification of both products of dicistronic mRNAs. Similarly, the construction of transgenic rice plants expressing wild-type and mutant constructs permits the quantification and correlation of steady state mRNA levels and reporter gene activities. Using these assays, we demonstrate directly that translation of the uORF is required for repression, that increasing translation of the uORF peptide decreases downstream gene expression, and that repression is unaffected by either subtle or gross changes in the uORF peptide. Rather, we find that ribosomes that translate the uORF reinitiate inefficiently and that the intercistronic sequence downstream of the uORF mediates this effect.
机译:玉米R基因编码花青素生物合成途径中几个结构基因的转录激活子的小家族。大多数R基因的5'前导区包含一个38密码子上游开放阅读框(uORF),以前在瞬态转化分析中显示,该框架负责抑制下游基因的表达。在这项研究中,我们报道了5'末端也可以抑制兔网织红细胞翻译系统和转基因水稻植株中下游荧光素酶基因的翻译。体外翻译后可视化uORF肽的能力允许对双顺反子mRNA的两种产物进行定量。类似地,表达野生型和突变体构建体的转基因水稻植物的构建允许稳态mRNA水平和报道基因活性的定量和相关性。使用这些测定法,我们直接证明了抑制需要uORF的翻译,增加uORF肽的翻译会降低下游基因的表达,并且抑制不受uORF肽的细微或总体变化的影响。而是,我们发现翻译uORF的核糖体无法有效地重新启动,并且uORF下游的顺反子序列介导了这种作用。

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  • 作者

    Wang, L; Wessler, S R;

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  • 年度 1998
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  • 正文语种 en
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