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鉴定大肠杆菌中菠萝泛菌番茄红素环化酶(crtY)基因的一个替代翻译起始位点及其进化保守性。

Identification of an alternative translation initiation site for the Pantoea ananatis lycopene cyclase (crtY) gene in E. coli and its evolutionary conservation.

作者信息

Kim Sung-Woo, Jung Woo-Hyuk, Ryu Ji-Myung, Kim Jae-Bum, Jang Hyung-Wook, Jo Young-Bae, Jung Joon-Ki, Kim Jung-Hoe

机构信息

AceBiotech Co., Ltd., #114 Bio-Venture Center, KRIBB, Yuseong, Daejeon 305-806, Republic of Korea.

出版信息

Protein Expr Purif. 2008 Mar;58(1):23-31. doi: 10.1016/j.pep.2007.11.004. Epub 2007 Nov 19.

Abstract

Previous sequence analyses of the lycopene cyclase gene (crt Y) from Pantoea ananatis revealed that translation of its protein product in Escherichia coli began at the ATG start codon. We found, however, that this enzyme could also be produced in E. coli without the ATG start codon present. Results of experiments using crt Y mutants revealed that a GTG (Val) sequence, located in-frame and 24 bp downstream of the ATG, could act as a potential start codon. Additionally, a point-mutated GTA (Val), replaced from alternative GTG start codon, also displayed its potential as a start codon although the strength as a translation initiation codon was considerably weak. This finding suggests that non-ATG codons, especially one base pairing with the anticodon (3'-UAC-5') in fMet-tRNA, might be also able to function as start codon in translation process. Furthermore, amino acid sequence alignment of lycopene cyclases from different sources suggested that a Val residue located within the N-terminus of these enzymes might be used as an alternative translation initiation site. In particular, presence of a conserved Asp, located in-frame and 12 bp upstream of potential start codon, supports this assumption in view of the fact that Asp (GAT or GAC) can function as part of the Shine-Dalgano sequence (AGGAGG).

摘要

先前对菠萝泛菌番茄红素环化酶基因(crtY)的序列分析表明,其蛋白质产物在大肠杆菌中的翻译起始于ATG起始密码子。然而,我们发现,在没有ATG起始密码子的情况下,这种酶也能在大肠杆菌中产生。使用crtY突变体的实验结果表明,位于ATG下游24 bp且读码框内的GTG(Val)序列可作为潜在的起始密码子。此外,从替代GTG起始密码子替换而来的点突变GTA(Val),尽管作为翻译起始密码子的强度相当弱,但也显示出其作为起始密码子的潜力。这一发现表明,非ATG密码子,尤其是与fMet-tRNA中的反密码子(3'-UAC-5')配对的一个碱基,在翻译过程中也可能作为起始密码子发挥作用。此外,不同来源的番茄红素环化酶的氨基酸序列比对表明,这些酶N端内的一个Val残基可能用作替代的翻译起始位点。特别是,鉴于Asp(GAT或GAC)可作为Shine-Dalgarno序列(AGGAGG)的一部分发挥作用,在潜在起始密码子上游12 bp且读码框内存在保守的Asp支持了这一假设。

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