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玉米的En/Spm转座元件在末端含有剪接位点,可从A2基因中的dSpm元件产生一个新的内含子。

The En/Spm transposable element of Zea mays contains splice sites at the termini generating a novel intron from a dSpm element in the A2 gene.

作者信息

Menssen A, Höhmann S, Martin W, Schnable P S, Peterson P A, Saedler H, Gierl A

机构信息

Max-Planck-Institut für Züchtungsforschung, Molekulare Pflanzengenetik, Köln, FRG.

出版信息

EMBO J. 1990 Oct;9(10):3051-7. doi: 10.1002/j.1460-2075.1990.tb07501.x.

Abstract

The A2 locus of Zea mays, identified as one of the genes affecting anthocyanin biosynthesis, was cloned using the transposable elements rcy and dSpm as gene tags. The A2 gene encodes a putative protein of 395 amino acids and is devoid of introns. Two a2-m1 alleles, containing dSpm insertions of different sizes, were characterized. The dSpm element from the original state allele has perfect termini and undergoes frequent transposition. The element from the class II state allele is no longer competent to transpose. It has retained the 13 bp terminal inverted repeat but has lost all subterminal sites at the 5' end, which are recognized by tnpA protein, the most abundant product of the En/Spm transposable element system. The relatively high A2 gene expression of one a2-m1 allele is due to removal of almost all dSpm sequences by splicing. The slightly altered A2 enzyme is still functional as shown by complementation of an a2 mutant with the corresponding cDNA. The 5' and 3' splice sites are constituted by the termini of the dSpm element; it therefore represents a novel intron of the A2 gene.

摘要

玉米的A2基因座被鉴定为影响花青素生物合成的基因之一,利用转座元件rcy和dSpm作为基因标签进行克隆。A2基因编码一个由395个氨基酸组成的推定蛋白,且不含内含子。对两个含有不同大小dSpm插入片段的a2-m1等位基因进行了表征。来自原始状态等位基因的dSpm元件具有完美的末端,并频繁发生转座。来自II类状态等位基因的元件不再具有转座能力。它保留了13bp的末端反向重复序列,但在5'端失去了所有被En/Spm转座元件系统中最丰富的产物tnpA蛋白识别的亚末端位点。一个a2-m1等位基因相对较高的A2基因表达是由于通过剪接去除了几乎所有的dSpm序列。如用相应的cDNA对a2突变体进行互补所显示的,略有改变的A2酶仍然具有功能。5'和3'剪接位点由dSpm元件的末端构成;因此它代表了A2基因的一个新内含子。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/05e8/552029/1d14cc3d1bdc/emboj00237-0037-a.jpg

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