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北方爪蟾和非洲爪蟾的28S核糖体DNA以及这两个物种完整的40S核糖体前体RNA编码单元。

Xenopus borealis and Xenopus laevis 28S ribosomal DNA and the complete 40S ribosomal precursor RNA coding units of both species.

作者信息

Ajuh P M, Heeney P A, Maden B E

机构信息

Department of Biochemistry, University of Liverpool, U.K.

出版信息

Proc Biol Sci. 1991 Jul 22;245(1312):65-71. doi: 10.1098/rspb.1991.0089.

Abstract

We have determined the nucleotide sequence of Xenopus borealis 28S ribosomal DNA (rDNA) and have revised the sequence of Xenopus laevis 28S rDNA (Ware et al., Nucl. Acids Res. 11, 7795-7817 (1983)). In the regions encoding the conserved structural core of 28S rRNA (2490 nucleotides) there are only four differences between the two species, each difference being a base substitution. In the variable regions, also called eukaryotic expansion segments (ca. 1630 nucleotides) there are some 61 differences, due to substitutions, mini-insertions and mini-deletions. Thus, evolutionary divergence in the variable regions has been at least 20-fold more rapid than in the conserved core. A search for intraspecies sequence variation has revealed minimal heterogeneity in X. laevis and none in X. borealis. At three out of four sites where heterogeneity was found in X. laevis (all in variable regions) the minority variant corresponded to the standard form in X. borealis. Intraspecies heterogeneity and interspecies divergence in the 28S variable regions are much less extensive than in the transcribed spacers. The 28S sequences are from the same clones that were used previously for sequencing the 18S genes and transcribed spacers. The complete sequences of the 40S precursor regions of the two reference clones are given.

摘要

我们已经测定了北方爪蟾28S核糖体DNA(rDNA)的核苷酸序列,并对非洲爪蟾28S rDNA的序列进行了修订(Ware等人,《核酸研究》11,7795 - 7817(1983))。在编码28S rRNA保守结构核心的区域(2490个核苷酸),这两个物种之间只有四处差异,每处差异都是一个碱基替换。在可变区域,也称为真核生物扩展片段(约1630个核苷酸),由于替换、小插入和小缺失,大约有61处差异。因此,可变区域的进化分歧速度比保守核心区域至少快20倍。对种内序列变异的搜索显示,非洲爪蟾的异质性极小,而北方爪蟾则没有异质性。在非洲爪蟾中发现异质性的四个位点中的三个(均在可变区域),少数变体与北方爪蟾的标准形式相对应。28S可变区域的种内异质性和种间分歧比转录间隔区要小得多。28S序列来自先前用于对18S基因和转录间隔区进行测序的相同克隆。给出了两个参考克隆的40S前体区域的完整序列。

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