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Nucleotide sequence of an external transcribed wacer in Xenopus laevis rDNA: sequences flanking the 5' and 3' ends of 18S rRNA are non-complementary

机译:非洲爪蟾rDNA中外部转录的wacer的核苷酸序列:18S rRNA 5'和3'末端侧翼的序列是非互补的

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We have sequenced the external transcribed spacer (ETS) of a ribosomal transcription unit from Xenopus laevis, together with sections of the preceding non-transcribed spacer. Our analysis was carried out on the same cloned transcription unit as that from which the internal transcribed spacers (ITS) were previously sequenced. The ETS is approximately 712 nucleotides long and, like the ITS regions, is generally very rich in C plus G. Features of the sequence include an excess of oligo-G tracts over oligo-G tracts and a tract of 37 nucleotides consisting almost entirely of G and A residues. Parts of the sequence can give rise to stable internal secondary structures. However, in contrast to Escherichia coli, there is no potential for major basepairing between the 18S flanking regions of the ETS and ITS. Further findings are that there are no initiation (ATC) codons in the ETS and that, as in other X.laevis rDNA cloned units, the sequence preceding the ETS is duplicated, with a few changes, in the “Bam island” sequence of the non-transcribed spacer.
机译:我们已经对非洲爪蟾(Xenopus laevis)核糖体转录单位的外部转录间隔子(ETS)以及先前未转录间隔子的部分进行了测序。我们的分析是在与内部测序间隔子(ITS)先前被测序的相同克隆转录单位上进行的。 ETS大约712个核苷酸长,并且与ITS区一样,通常都非常富含C加G。该序列的特征包括,寡G片段比寡G片段和37个核苷酸的片段几乎完全由寡核苷酸组成。 G和A残基。序列的一部分可以产生稳定的内部二级结构。但是,与大肠杆菌相反,在ETS和ITS的18S侧翼区域之间没有主要碱基配对的可能性。进一步的发现是,ETS中没有起始(ATC)密码子,和其他X.laevis rDNA克隆单位一样,ETS之前的序列在Bam岛的“ Bam岛”序列中有重复,但有一些变化。非转录间隔子。

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