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Influence of the stacking potential of the base 3 of tandem shift codons on -1 ribosomal frameshifting used for gene expression.

机译:串联移位密码子的碱基3的堆积潜力对用于基因表达的-1核糖体移码的影响。

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摘要

Translating ribosomes can shift reading frame at specific sites with high efficiency for gene expression purposes. The most common type of shift to the -1 frame involves a tandem realignment of two anticodons from pairing with mRNA sequence of the form X XXY YYZ to XXX YYY Z where the spaces indicate the reading frame. The predominant -1 shift site of this type in eubacteria is A AAA AAG. The present work shows that in Escherichia coli the identity of the 6 nt 3' of this sequence can be responsible for a 14-fold variation in frameshift frequency. The first 3' nucleotide has the primary effect, with, in order of decreasing efficiency, U > C > A > G. This effect is independent of other stimulators of frameshifting. It is detected with other X XXA AAG sequences, but not with several other heptameric -1 shift sites. Pairing of E. coli tRNALYS with AAG is especially weak at the third codon position. We propose that strong stacking of purines 3' of AAG stabilizes pairing of tRNALys, diminishing the chance of codon:anticodon dissociation that is a prerequisite for the realignment involved in frameshifting.
机译:为了基因表达目的,翻译核糖体可以高效地在特定位点移动阅读框。移至-1帧的最常见类型涉及两个反密码子的串联重排,配对形式为X XXY YYZ至XXX YYY Z,其中空格表示阅读框。在真细菌中,这种类型的主要-1移位位点是A AAA AAG。目前的工作表明,在大肠杆菌中,该序列的6 nt 3'的身份可能导致移码频率发生14倍的变化。第一个3'核苷酸具有主要作用,按照效率递减的顺序,U> C> A>G。该作用独立于移码的其他刺激物。它可以用其他X XXA AAG序列检测到,但不能用其他几个七聚体-1移位位点检测到。大肠杆菌tRNALYS与AAG的配对在第三个密码子位置特别弱。我们提出,AAG嘌呤3'的强堆积可以稳定tRNALys的配对,从而减少密码子:反密码子解离的机会,这是移码所涉及的重新排列的前提。

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