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Ds转座元件插入植物特异性基因导致的碧冬茄幼苗致死性。

Seedling lethality in Nicotiana plumbaginifolia conferred by Ds transposable element insertion into a plant-specific gene.

作者信息

Majira Amel, Domin Monique, Grandjean Olivier, Gofron Krystyna, Houba-Hérin Nicole

机构信息

Laboratoire de Biologie Cellulaire INRA, Versailles, France.

出版信息

Plant Mol Biol. 2002 Oct;50(3):551-62. doi: 10.1023/a:1019851913083.

Abstract

A seedling lethal mutant of Nicotiana plumbaginifolia (sdl-1) was isolated by transposon tagging using a maize Dissociation (Ds) element. The insertion mutation was produced by direct co-transformation of protoplasts with two plasmids: one containing Ds and a second with an Ac transposase gene. sdl-1 seedlings exhibit several phenotypes: swollen organs, short hypocotyls in light and dark conditions, and enlarged and multinucleated cells, that altogether suggest cell growth defects. Mutant cells are able to proliferate under in vitro culture conditions. Genomic DNA sequences bordering the transposon were used to recover cDNA from the normal allele. Complementation of the mutant phenotype with the cDNA confirmed that the transposon had caused the mutation. The Ds element was inserted into the first exon of the open reading frame and the homozygous mutant lacked detectable transcript. Phenocopies of the mutant were obtained by an antisense approach. SDL-1 encodes a novel protein found in several plant genomes but apparently missingfrom animal and fungal genomes; the protein is highly conserved and has a potential plastid targeting motif.

摘要

利用玉米解离(Ds)元件通过转座子标签法分离出了一种烟草(Nicotiana plumbaginifolia)的幼苗致死突变体(sdl-1)。插入突变是通过用两个质粒对原生质体进行直接共转化产生的:一个含有Ds,另一个含有Ac转座酶基因。sdl-1幼苗表现出几种表型:器官肿胀、在光照和黑暗条件下下胚轴短,以及细胞增大和多核,这些都表明细胞生长存在缺陷。突变细胞能够在体外培养条件下增殖。利用与转座子相邻的基因组DNA序列从正常等位基因中回收cDNA。用该cDNA对突变体表型进行互补验证,证实转座子导致了突变。Ds元件插入到开放阅读框的第一个外显子中,纯合突变体缺乏可检测到的转录本。通过反义方法获得了该突变体的拟表型。SDL-1编码一种在多个植物基因组中发现但在动物和真菌基因组中显然不存在的新型蛋白质;该蛋白质高度保守,具有潜在的质体靶向基序。

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