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一种阴离子泵的分子特性。arsA基因产物是一种受亚砷酸盐(锑酸盐)刺激的ATP酶。

Molecular characterization of an anion pump. The arsA gene product is an arsenite(antimonate)-stimulated ATPase.

作者信息

Rosen B P, Weigel U, Karkaria C, Gangola P

机构信息

Department of Biological Chemistry, University of Maryland School of Medicine, Baltimore 21201.

出版信息

J Biol Chem. 1988 Mar 5;263(7):3067-70.

PMID:2449436
Abstract

The products of the arsenical resistance operon of resistance plasmid R733 form an efflux system for arsenicals. Detoxification results from active efflux of the oxyanions, preventing their concentration from reaching toxic levels. The largest polypeptide encoded by the ars operon was purified. From N-terminal sequencing the purified protein, termed the ArsA protein, was shown to correspond to the product of the arsA gene. The purified protein was demonstrated to bind ATP by two methods. First, a photoadduct of the protein with [alpha-32P]ATP was formed by irradiation at 254 nm. Second, the purified protein bound a fluorescent ATP analogue, 2',3'-o-(2,4,6)trinitrophenyl ATP, with a half-maximal affinity of 2 microM. By both assays competition was observed with ATP or ADP, but not with AMP, GTP, CTP, or UTP. In both nucleotide binding assays, Mg2+ was required, but neither arsenite nor antimonate had any affect. In contrast, the ArsA protein exhibited an ATPase activity which was dependent on the presence of arsenite or antimonate. The results suggest that the ArsA protein is the catalytic subunit of an oxyanion-translocating ATPase.

摘要

抗性质粒R733的抗砷操纵子产物形成了一个砷排出系统。解毒作用源于氧阴离子的主动排出,可防止其浓度达到有毒水平。对ars操纵子编码的最大多肽进行了纯化。通过对纯化蛋白进行N端测序,该蛋白被称为ArsA蛋白,结果显示它与arsA基因的产物相对应。通过两种方法证明纯化后的蛋白能结合ATP。第一,在254nm波长下照射,可使该蛋白与[α-32P]ATP形成光加合物。第二,纯化后的蛋白能结合一种荧光ATP类似物2',3'-O-(2,4,6)三硝基苯基ATP,其半最大亲和力为2μM。在这两种检测方法中,均观察到ATP或ADP存在竞争,但AMP、GTP、CTP或UTP不存在竞争。在这两种核苷酸结合检测中,均需要Mg2+,但亚砷酸盐和锑酸盐均无任何影响。相反,ArsA蛋白表现出一种依赖于亚砷酸盐或锑酸盐存在的ATP酶活性。结果表明,ArsA蛋白是一种氧阴离子转运ATP酶的催化亚基。

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