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构建用于过表达氧阴离子转运ATP酶的嵌合ArsA-ArsB蛋白。

Construction of a chimeric ArsA-ArsB protein for overexpression of the oxyanion-translocating ATPase.

作者信息

Dou D, Owolabi J B, Dey S, Rosen B P

机构信息

Department of Biochemistry, Wayne State University, School of Medicine, Detroit, Michigan 48201.

出版信息

J Biol Chem. 1992 Dec 25;267(36):25768-75.

PMID:1281474
Abstract

Resistance to toxic oxyanions of arsenic and antimony in Escherichia coli is conferred by the conjugative R-factor R773, which encodes an ATP-driven anion extrusion pump. The ars operon is composed of three structural genes, arsA, arsB, and arsC. Although transcribed as a single unit, the three genes are differentially expressed as a result of translational differences, such that the ArsA and ArsC proteins are produced in high amounts relative to the amount of ArsB protein made. Consequently, biochemical characterization of the ArsB protein, which is an integral membrane protein containing the anion-conducting pathway, has been limited, precluding studies of the mechanism of this oxyanion pump. To overexpress the arsB gene, a series of changes were made. First, the second codon, an infrequently used leucine codon, was changed to a more frequently utilized codon. Second, a GC-rich stem-loop (delta G = -17 kcal/mol) between the third and twelfth codons was destabilized by changing several of the bases of the base-paired region. Third, the re-engineered arsB gene was fused 3' in frame to the first 1458 base pairs of the arsA gene to encode a 914-residue chimeric protein (486 residues of the ArsA protein plus 428 residues of the mutated ArsB protein) containing the entire re-engineered ArsB sequence except for the initiating methionine. The ArsA-ArsB chimera has been overexpressed at approximately 15-20% of the total membrane proteins. Cells producing the chimeric ArsA-ArsB protein with an arsA gene in trans excluded 73AsO2- from cells, demonstrating that the chimera can function as a component of the oxyanion-translocating ATPase.

摘要

大肠杆菌对砷和锑的毒性含氧阴离子的抗性由接合性R因子R773赋予,该因子编码一种ATP驱动的阴离子外排泵。ars操纵子由三个结构基因arsA、arsB和arsC组成。尽管这三个基因作为一个单一单元转录,但由于翻译差异,它们的表达存在差异,因此相对于所产生的ArsB蛋白量,ArsA和ArsC蛋白的产量较高。因此,作为包含阴离子传导途径的整合膜蛋白的ArsB蛋白的生化特性研究受到限制,这妨碍了对这种含氧阴离子泵机制的研究。为了过量表达arsB基因,进行了一系列改变。首先,将第二个密码子(一个不常用的亮氨酸密码子)改为一个更常用的密码子。其次,通过改变碱基配对区域的几个碱基,使第三和第十二个密码子之间富含GC的茎环(ΔG = -17千卡/摩尔)不稳定。第三,将重新设计的arsB基因在框架内与arsA基因的前1458个碱基对融合,以编码一个914个残基的嵌合蛋白(486个ArsA蛋白残基加上428个突变的ArsB蛋白残基),该蛋白包含除起始甲硫氨酸外的整个重新设计的ArsB序列。ArsA-ArsB嵌合体已在总膜蛋白的约15-20%水平上过量表达。用arsA基因反式产生嵌合ArsA-ArsB蛋白的细胞将73AsO2-从细胞中排出,这表明该嵌合体可以作为含氧阴离子转运ATP酶的一个组分发挥作用。

相似文献

1
Construction of a chimeric ArsA-ArsB protein for overexpression of the oxyanion-translocating ATPase.构建用于过表达氧阴离子转运ATP酶的嵌合ArsA-ArsB蛋白。
J Biol Chem. 1992 Dec 25;267(36):25768-75.
2
Molecular characterization of an anion pump. The ArsB protein is the membrane anchor for the ArsA protein.一种阴离子泵的分子特征。ArsB蛋白是ArsA蛋白的膜锚定蛋白。
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The plasmid-encoded arsenical resistance pump: an anion-translocating ATPase.质粒编码的抗砷泵:一种阴离子转运ATP酶。
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Membrane topology of the ArsB protein, the membrane subunit of an anion-translocating ATPase.阴离子转运ATP酶的膜亚基ArsB蛋白的膜拓扑结构。
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Molecular analysis of an ATP-dependent anion pump.一种ATP依赖型阴离子泵的分子分析
Philos Trans R Soc Lond B Biol Sci. 1990 Jan 30;326(1236):455-63. doi: 10.1098/rstb.1990.0024.
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Dual mode of energy coupling by the oxyanion-translocating ArsB protein.氧阴离子转运蛋白ArsB的双模式能量偶联
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A plasmid-encoded anion-translocating ATPase.一种质粒编码的阴离子转运ATP酶。
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Mutagenesis of a nucleotide-binding site of an anion-translocating ATPase.
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引用本文的文献

1
The proteins encoded by the rbs operon of Escherichia coli: II. Use of chimeric protein constructs to isolate and characterize RbsC.大肠杆菌rbs操纵子编码的蛋白质:II. 利用嵌合蛋白构建体分离和鉴定RbsC
Protein Sci. 1996 Jun;5(6):1100-7. doi: 10.1002/pro.5560050612.
2
Arsenic efflux governed by the arsenic resistance determinant of Staphylococcus aureus plasmid pI258.由金黄色葡萄球菌质粒pI258的砷抗性决定因素所调控的砷流出
J Bacteriol. 1993 Jun;175(11):3480-5. doi: 10.1128/jb.175.11.3480-3485.1993.
3
Dual mode of energy coupling by the oxyanion-translocating ArsB protein.氧阴离子转运蛋白ArsB的双模式能量偶联
J Bacteriol. 1995 Jan;177(2):385-9. doi: 10.1128/jb.177.2.385-389.1995.