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Phylogeny of related functions: the case of polyamine biosynthetic enzymes

机译:相关功能的系统发育:多胺生物合成酶的情况

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Genome annotation requires explicit identification of gene function. This task frequently uses protein sequence alignments with examples having a known function. Genetic drift, co-evolution of subunits in protein complexes and a variety of other constraints interfere with the relevance of alignments. Using a specific class of proteins, it is shown that a simple data analysis approach can help solve some of the problems posed. The origin of ureohydrolases has been explored by comparing sequence similarity trees, maximizing amino acid alignment conservation. The trees separate agmatinases from arginases but suggest the presence of unknown biases responsible for unexpected positions of some enzymes. Using factorial correspondence analysis, a distance tree between sequences was established, comparing regions with gaps in the alignments. The gap tree gives a consistent picture of functional kinship, perhaps reflecting some aspects of phylogeny, with a clear domain of enzymes encoding two types of ureohydrolases (agmatinases and arginases) and activities related to, but different from ureohydrolases. Several annotated genes appeared to correspond to a wrong assignment if the trees were significant. They were cloned and their products expressed and identified biochemically. This substantiated the validity of the gap tree. Its organization suggests a very ancient origin of ureohydrolases. Some enzymes of eukaryotic origin are spread throughout the arginase part of the trees: they might have been derived from the genes found in the early symbiotic bacteria that became the organelles. They were transferred to the nucleus when symbiotic genes had to escape Muller’s ratchet. This work also shows that arginases and agmatinases share the same two manganese-ion-binding sites and exhibit only subtle differences that can be accounted for knowing the three-dimensional structure of arginases. In the absence of explicit biochemical data, extreme caution is needed when annotating genes having similarities to ureohydrolases.
机译:基因组注释需要显式鉴定基因功能。该任务经常使用蛋白质序列对齐与具有已知功能的示例。遗传漂移,蛋白质复合物中亚基的共同演变和各种其他约束干扰了对准的相关性。使用特定类别的蛋白质,表明简单的数据分析方法可以帮助解决构成的一些问题。通过比较序列相似性树木,最大化氨基酸对准守恒来探讨乌雷水溶酶的来源。树木将来自氨基酶的毒素分离,但表明存在未知偏见的偏见,这对某些酶的意外位置负责。使用阶乘对应分析,建立了序列之间的距离树,将区域与距离中的间隙进行比较。间隙树给出了功能性血缘关系的一致图,也许反映了系统发育的一些方面,其中包含编码两种类型的乌雷水(Gmatinase和Aginase)的酶的透明结构域和与uReoHoldolase不同但不同的活性。如果树木显着,则几种注释基因似乎对应于错误的分配。他们被克隆,他们的产品表达并鉴定了生物化学上。这证实了差距树的有效性。它的组织表明乌雷水上的古老起源。一些真核原子的酶在整个树木的整个氨基酶部分中涂布:它们可能是从成为有机细胞的早期共生细菌中发现的基因。当共生基因不得不逃避Muller的棘轮时,它们被转移到细胞核中。这项工作还表明,氨基酶和毒素酶共享相同的两个锰 - 离子结合位点,并且只能占知道酶学酶的三维结构的微妙差异。在没有明确的生化数据的情况下,当注释与乌雷水溶酶相似的基因时需要极度小心。

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