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在莱茵衣藻叶绿体或大肠杆菌中,叶绿体mRNA的翻译不需要类Shine-Dalgarno序列。

Shine-Dalgarno-like sequences are not required for translation of chloroplast mRNAs in Chlamydomonas reinhardtii chloroplasts or in Escherichia coli.

作者信息

Fargo D C, Zhang M, Gillham N W, Boynton J E

机构信息

Developmental, Cell and Molecular Biology Group, Department of Botany, Duke University, Durham, NC 27708, USA.

出版信息

Mol Gen Genet. 1998 Feb;257(3):271-82. doi: 10.1007/s004380050648.

Abstract

Initiation of translation in Escherichia coli and related eubacteria involves well-defined interactions between a conserved Shine-Dalgarno (SD) sequence immediately upstream of the initiation codon in the mRNA leader and an equally conserved anti-SD sequence at the 3' end of the 16S rRNA. SD-like sequences found in the leaders of many, but not all, mRNAs from cyanobacteria and chloroplasts are hypervariable in location, size, and base composition compared to those in E. coli, while anti-SD sequences in the respective 16S rRNAs remain highly conserved. We have examined the function of the SD-like sequences found in the leaders of four chloroplast genes of the green alga Chlamydomonas reinhardtii using replacement mutagenesis to eliminate complementarity with the anti-SD sequences and insertion of canonical SD sequences (GGAGG) at positions -9 to -5 relative to the initiation codon. Promoter-leader regions of the atpB, atpE, rps4, and rps7 genes representing the diversity of chloroplast SD-like sequences were fused to aadA and uidA reporter genes encoding spectinomycin resistance and GUS activity respectively. Analysis of chloroplast transformants of C. reinhardtii and transformants of E. coli carrying the wild-type and mutant reporter constructs revealed that mutagenic replacement of the putative SD sequences had no effect on the expression of either the aadA or uidA reporter genes. Chloroplast transformants with the canonical SD sequence also showed no differences in reporter gene expression, whereas expression of the reporter genes was increased by 10 to 30% in the E. coli transformants. Collectively our results suggest that even though SD-dependent initiation predominates in E. coli, this bacterium also has the capacity to initiate translation by an SD-independent mechanism. In contrast, plant chloroplasts, and very probably their cyanobacterial ancestors, appear to have adopted the SD-independent mechanism for translational initiation of most mRNAs.

摘要

在大肠杆菌及相关真细菌中,翻译起始涉及mRNA前导序列中起始密码子上游紧邻的保守的Shine-Dalgarno(SD)序列与16S rRNA 3'端同样保守的反SD序列之间明确的相互作用。与大肠杆菌中的序列相比,在蓝细菌和叶绿体的许多(但并非全部)mRNA前导序列中发现的类SD序列在位置、大小和碱基组成上具有高度变异性,而相应16S rRNA中的反SD序列则保持高度保守。我们利用置换诱变消除与反SD序列的互补性,并在相对于起始密码子的-9至-5位置插入典型的SD序列(GGAGG),研究了莱茵衣藻四个叶绿体基因前导序列中类SD序列的功能。代表叶绿体类SD序列多样性的atpB、atpE、rps4和rps7基因的启动子-前导区域分别与编码壮观霉素抗性和GUS活性的aadA和uidA报告基因融合。对莱茵衣藻叶绿体转化体以及携带野生型和突变型报告构建体的大肠杆菌转化体的分析表明,推定的SD序列的诱变置换对aadA或uidA报告基因的表达均无影响。具有典型SD序列的叶绿体转化体在报告基因表达上也未显示出差异,而在大肠杆菌转化体中报告基因的表达增加了10%至30%。总体而言,我们的结果表明,尽管在大肠杆菌中依赖SD的起始占主导,但该细菌也具有通过不依赖SD的机制起始翻译的能力。相比之下,植物叶绿体以及很可能其蓝细菌祖先似乎已采用不依赖SD的机制来起始大多数mRNA的翻译。

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