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RNA editing in six mitochondrial ribosomal protein genes of Didymium iridis

机译:鸢尾线虫六个线粒体核糖体蛋白基因的RNA编辑

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摘要

Similarity searches with Didymium iridis mitochondrial genomic DNA identified six possible ribosomal protein-coding regions, however, each region contained stop codons that would need to be removed by RNA editing to produce functional transcripts. RT-PCR was used to amplify these regions from total RNA for cloning and sequencing. Six functional transcripts were verified for the following ribosomal protein genes: rpS12, rpS7, rpL2, rpS19, rpS3, and rpL16. The editing events observed, such as single C and U nucleotide insertions and a dinucleotide insertion, were consistent with previously observed editing patterns seen in D. iridis. Additionally, a new form of insertional editing, a single A insertion, was observed in a conserved region of the rpL16 gene. While the majority of codons created by editing specify hydrophobic amino acids, a greater proportion of the codons created in these hydrophilic ribosomal proteins called for positively charged amino acids in comparison to the previously characterized hydrophobic respiratory protein genes. This first report of edited soluble mitochondrial ribosomal proteins in myxomycetes expands upon the RNA editing patterns previously seen; there was: a greater proportion of created codons specifying positively charged amino acids, a shift in the codon position edited, and the insertion of single A nucleotides.
机译:与鸢尾线粒体线粒体基因组DNA的相似性搜索确定了六个可能的核糖体蛋白编码区,但是,每个区都包含终止密码子,需要通过RNA编辑将其去除以产生功能性转录本。 RT-PCR用于从总RNA扩增这些区域,以进行克隆和测序。验证了以下核糖体蛋白基因的六个功能转录本:rpS12,rpS7,rpL2,rpS19,rpS3和rpL16。观察到的编辑事件,例如单个C和U核苷酸插入和一个二核苷酸插入,与以前在iridis D.中观察到的编辑模式一致。此外,在rpL16基因的保守区中观察到一种新的插入编辑形式,即一个A插入。尽管通过编辑产生的大多数密码子都指定了疏水性氨基酸,但是与先前表征的疏水性呼吸蛋白质基因相比,在这些亲水核糖体蛋白中产生的密码子中有更大比例的需要带正电荷的氨基酸。粘菌丝中可编辑的可溶性线粒体核糖体蛋白的第一个报道扩展了先前见过的RNA编辑模式。有:更大比例的创建密码子指定带正电荷的氨基酸,编辑的密码子位置发生变化以及单个A核苷酸的插入。

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