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古细菌、真细菌和真核生物中L10等效核糖体蛋白和L12等效核糖体蛋白的序列比对及进化比较。

Sequence alignment and evolutionary comparison of the L10 equivalent and L12 equivalent ribosomal proteins from archaebacteria, eubacteria, and eucaryotes.

作者信息

Shimmin L C, Ramirez C, Matheson A T, Dennis P P

机构信息

Department of Biochemistry, University of British Columbia, Vancouver, Canada.

出版信息

J Mol Evol. 1989 Nov;29(5):448-62. doi: 10.1007/BF02602915.

Abstract

The genes corresponding to the L10 and L12 equivalent ribosomal proteins (L10e and L12e) of Escherichia coli have been cloned and sequenced from two widely divergent species of archaebacteria, Halobacterium cutirubrum and Sulfolobus solfataricus. The deduced amino acid sequences of the L10e and L12e proteins have been compared to each other and to available eubacterial and eucaryotic sequences. We have identified the human P0 protein as the eucaryotic L10e. The L10e proteins from the three kingdoms were found to be colinear. The eubacterial L10e protein is much shorter than the archaebacterial-eucaryotic proteins because of two large deletions, one internal and one at the carboxy terminus. The archaebacterial and eucaryotic L12e proteins were also colinear; the eubacterial protein is homologous to the archaebacterial and eucaryotic L12e proteins, but has suffered rearrangement through what appear to be gene fusion events. Intraspecies comparisons between L10e and L12e sequences indicate the archaebacterial and eucaryotic L10e proteins contain a partial copy of the L12e protein fused to their carboxy terminus. In the eubacteria most of this fusion has been removed by the carboxy terminal deletion. Within the L12e-derived region, a 26-amino acid-long internal modular sequence reiterated thrice in the archaebacterial L10e, twice in the eucaryotic L10e, and once in the eubacterial L10e was discovered. This modular sequence also appears to be present as a single copy in all L12e proteins and may play a role in L12e dimerization, L10e-L12e complex formation, and the function of L10e-L12e complex in translation.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

已从两种差异很大的古细菌——深红嗜盐菌和嗜热栖热菌中克隆并测序了与大肠杆菌L10和L12等效核糖体蛋白(L10e和L12e)相对应的基因。已将L10e和L12e蛋白推导的氨基酸序列相互比较,并与现有的真细菌和真核生物序列进行了比较。我们已确定人类P0蛋白为真核生物的L10e。发现来自三个王国的L10e蛋白是共线的。由于两个大的缺失,一个在内部,一个在羧基末端,真细菌的L10e蛋白比古细菌 - 真核生物蛋白短得多。古细菌和真核生物的L12e蛋白也是共线的;真细菌蛋白与古细菌和真核生物的L12e蛋白同源,但通过似乎是基因融合事件发生了重排。L10e和L12e序列的种内比较表明,古细菌和真核生物的L10e蛋白在其羧基末端融合了L12e蛋白的部分拷贝。在真细菌中,这种融合的大部分已被羧基末端缺失去除。在源自L12e的区域内,发现了一个26个氨基酸长的内部模块化序列,在古细菌L10e中重复三次,在真核生物L10e中重复两次,在真细菌L10e中重复一次。这个模块化序列似乎也以单拷贝形式存在于所有L12e蛋白中,并且可能在L12e二聚化、L10e - L12e复合物形成以及L10e - L12e复合物在翻译中的功能中发挥作用。(摘要截短于250字)

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