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切除一个古老重复插入片段对康氏立克次体鸟苷酸激酶活性的影响。

Impact of the excision of an ancient repeat insertion on Rickettsia conorii guanylate kinase activity.

作者信息

Abergel Chantal, Blanc Guillaume, Monchois Vincent, Renesto Patricia, Sigoillot Cécile, Ogata Hiroyuki, Raoult Didier, Claverie Jean-Michel

机构信息

Information Génomique & Structurale, CNRS UPR 2589, IBSM, Marseille cedex, France.

出版信息

Mol Biol Evol. 2006 Nov;23(11):2112-22. doi: 10.1093/molbev/msl082. Epub 2006 Aug 4.

DOI:10.1093/molbev/msl082
PMID:16891376
Abstract

The genomic sequencing of Rickettsia conorii revealed a new family of Rickettsia-specific palindromic elements (RPEs) capable of in-frame insertion in preexisting open reading frames (ORFs). Many of these altered ORFs correspond to proteins with well-characterized or essential functions in other microorganisms. Previous experiments indicated that RPE-containing genes are normally transcribed and that no excision of the repeat occurs at the mRNA level. Using mass spectrometry, we now confirmed the retention of the RPE-derived amino acid residues in 4 proteins successfully expressed in Escherichia coli, raising the general question of the consequences of this common insertion event on the fitness of Rickettsia enzymes. The predicted guanylate kinase activity of the R. conorii gmk gene product was measured both on the RPE-containing and RPE-excised recombinant proteins. We show that the 2 proteins are active but exhibit substantial differences in their affinity for adenosine triphosphate, guanosine monophosphate, and catalytic constants. The distribution of the RPEgmk insert among Rickettsia species indicates that the insertion event is ancient and occurred after the divergence of Rickettsia felis and R. conorii but before that of Rickettsia helvetica and R. conorii. We found no evidence that the gmk gene fixed adaptive changes to compensate the RPE peptide insertion. Furthermore, the analysis of the rates of divergence in 23 RPE-containing genes indicates that coding RPE repeats tend to evolve under weak selective constraint, at a rate similar to intergenic noncoding RPE sequences. Altogether, these results suggest that the insertion of RPE-encoded "selfish peptides," although respecting the original fold and activity of the host proteins, might be slightly detrimental to the enzyme efficiency within limits tolerable for slow-growing intracellular parasites such as Rickettsia.

摘要

康氏立克次体的基因组测序揭示了一个新的立克次体特异性回文元件(RPEs)家族,它们能够在已有的开放阅读框(ORFs)中进行框内插入。许多这些改变的ORF对应于在其他微生物中具有明确特征或基本功能的蛋白质。先前的实验表明,含有RPE的基因通常会转录,并且在mRNA水平上不会发生重复序列的切除。通过质谱分析,我们现在证实了在大肠杆菌中成功表达的4种蛋白质中保留了RPE衍生的氨基酸残基,这引发了一个普遍问题,即这种常见的插入事件对立克次体酶适应性的影响。对含有RPE和切除RPE的重组蛋白都测定了康氏立克次体gmk基因产物的预测鸟苷酸激酶活性。我们发现这两种蛋白质都有活性,但在对三磷酸腺苷、单磷酸鸟苷的亲和力和催化常数方面表现出显著差异。RPEgmk插入序列在立克次体物种中的分布表明,插入事件是古老的,发生在猫立克次体和康氏立克次体分化之后,但在瑞士立克次体和康氏立克次体分化之前。我们没有发现gmk基因固定适应性变化以补偿RPE肽插入的证据。此外,对23个含有RPE的基因的分歧率分析表明,编码RPE重复序列倾向于在弱选择约束下进化,其速率与基因间非编码RPE序列相似。总之,这些结果表明,RPE编码的“自私肽”的插入,尽管保留了宿主蛋白的原始折叠和活性,但对于像立克次体这样生长缓慢的细胞内寄生虫来说,在可容忍的限度内可能会对酶的效率略有不利影响。

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