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小麦胚芽剪接内切核酸酶对植物前体tRNA具有高度特异性。

Wheat germ splicing endonuclease is highly specific for plant pre-tRNAs.

作者信息

Stange N, Gross H J, Beier H

机构信息

Institut für Biochemie, Bayerische Julius-Maximilians-Universität, Würzburg, FRG.

出版信息

EMBO J. 1988 Dec 1;7(12):3823-8. doi: 10.1002/j.1460-2075.1988.tb03267.x.

Abstract

Intron-containing pre-tRNAs from organisms as different as yeast, Nicotiana, Xenopus and man are efficiently spliced and processed in a HeLa cell extract. They are also correctly processed in a wheat germ extract; however, the intron is removed only from the tobacco pre-tRNA. To determine whether plant pre-tRNA introns have any specific structural and/or sequence feature we have cloned two intron-containing tRNATyr genes from the plant Arabidopsis. Comparison of these genes, of the Nicotiana tRNATyr gene and of a Glycine max tRNAMet gene reveals that plant introns from three different species have no sequence homology and are only 11 to 13 nucleotides long. Thus, short length may be one important feature of plant introns. Furthermore, the 5' and 3' splice sites are separated by 4 bp in the extended anticodon stems of these pre-tRNA structures. In contrast, yeast and vertebrate introns are rather variable in length and the splice sites are separated by 5 or 6 bp. These differences in distance and relative helical orientation of the splice sites in plant pre-tRNAs versus pre-tRNAs from other organisms are obviously tolerated by the vertebrate splicing endonuclease, but not at all by the plant enzyme.

摘要

来自酵母、烟草、非洲爪蟾和人类等不同生物体的含内含子前体tRNA在HeLa细胞提取物中能有效地进行剪接和加工。它们在小麦胚芽提取物中也能正确加工;然而,只有烟草前体tRNA中的内含子被去除。为了确定植物前体tRNA内含子是否具有任何特定的结构和/或序列特征,我们从植物拟南芥中克隆了两个含内含子的tRNATyr基因。对这些基因、烟草tRNATyr基因和大豆tRNAMet基因的比较表明,来自三个不同物种的植物内含子没有序列同源性,长度仅为11至13个核苷酸。因此,短长度可能是植物内含子的一个重要特征。此外,在这些前体tRNA结构的延伸反密码子茎中,5'和3'剪接位点相隔4个碱基对。相比之下,酵母和脊椎动物的内含子长度变化较大,剪接位点相隔5或6个碱基对。植物前体tRNA与其他生物体前体tRNA在剪接位点距离和相对螺旋方向上的这些差异显然能被脊椎动物剪接内切酶容忍,但植物酶却完全不能容忍。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d138/454960/9fa95594814a/emboj00149-0194-a.jpg

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