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嗜水气单胞菌编码气溶素及其调控区的aerCaerA区域的核苷酸序列和转录分析。

Nucleotide sequence and transcriptional analysis of the aerCaerA region of Aeromonas sobria encoding aerolysin and its regulatory region.

作者信息

Husslein V, Huhle B, Jarchau T, Lurz R, Goebel W, Chakraborty T

机构信息

Institut für Genetik und Mikrobiologie, Universität Würzburg, FRG.

出版信息

Mol Microbiol. 1988 Jul;2(4):507-17. doi: 10.1111/j.1365-2958.1988.tb00057.x.

Abstract

The nucleotide sequence of a 2510 base pair chromosomal fragment containing the aerolysin gene aerA, and its regulatory region aerC, from a clinical isolate of Aeromonas sobria was determined. The aerolysin gene coded for a 54.5 kD polypeptide and had a G + C content of 59%, indicating that it is endogenous to the genus Aeromonas. In contrast, the aerC region was characterized by its high A + T content (61%) and the presence of a core motif, aATAAAa, repeated eight times within 300 base pairs. A 12 base pair repeat, 5'AATAAAACCGGG3', present within this region occurred as a direct repeat 544 base pairs away, within the coding region of aerolysin. RNA polymerase binding studies and S1 mapping allowed the detection of two divergent non-overlapping promoters within aerC. Despite having identical transcriptional start sites in both A. sobria and Escherchia coli, the amount of aerolysin transcript produced in E. coli is 30-40 times less than that found in A. sobria. The signal peptide of preproaerolysin was shown by deletion to be essential for export of the toxin to the external medium. The mature toxin is a hydrophilic protein with no hydrophobic stretches long enough to cross a membrane. A search for similarities to the primary sequence of aerolysin revealed that the toxin may share a functional similarity to haemolysin (hlyA) of E. coli.

摘要

测定了来自温和气单胞菌临床分离株的一个包含气溶素基因aerA及其调控区域aerC的2510个碱基对染色体片段的核苷酸序列。气溶素基因编码一种54.5 kD的多肽,其G + C含量为59%,表明它是气单胞菌属的内源基因。相比之下,aerC区域的特征是其高A + T含量(61%)以及存在一个核心基序aATAAAa,该基序在300个碱基对内重复八次。该区域内存在的一个12个碱基对的重复序列5'AATAAAACCGGG3',在气溶素编码区域内与之相距544个碱基对处呈正向重复。RNA聚合酶结合研究和S1图谱分析使得能够在aerC内检测到两个不同的非重叠启动子。尽管在温和气单胞菌和大肠杆菌中具有相同的转录起始位点,但在大肠杆菌中产生的气溶素转录本数量比在温和气单胞菌中少30 - 40倍。前气溶素原的信号肽经缺失实验表明对于毒素分泌到细胞外培养基中至关重要。成熟毒素是一种亲水蛋白,没有足够长的疏水片段来穿过细胞膜。对气溶素一级序列相似性的搜索表明,该毒素可能与大肠杆菌的溶血素(hlyA)具有功能相似性。

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