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大肠杆菌谷氨酰胺合成酶的级联调控。PII蛋白的纯化、性质及其结构基因的核苷酸序列

Cascade control of Escherichia coli glutamine synthetase. Purification and properties of PII protein and nucleotide sequence of its structural gene.

作者信息

Son H S, Rhee S G

出版信息

J Biol Chem. 1987 Jun 25;262(18):8690-5.

PMID:2885322
Abstract

A procedure was developed to purify large quantities of PII protein from an Escherichia coli strain which contains a multicopy plasmid harboring the structural gene of PII (the glnB gene). Ultraviolet spectra of uridylylated and unuridylylated PII were obtained using the purified PII and empirical formulas to calculate the concentration of protein and the average number of uridylylated subunits per molecule were derived. A continuous fluorometric assay for the measurement of uridylylated PII (PIID) and adenylyltransferase (ATase) was also established. Rate measurements at various concentrations of PIID and at a fixed concentration of ATase showed that a tetrameric PIID molecule interacts with only one ATase molecule at a time. The complete nucleotide sequence of the glnB gene was determined and parts of the deduced amino acid sequence were confirmed by the results of amino acid sequence analysis of peptides. The PII subunit consists of 103 amino acids (Mr = 11,580). Two tyrosines reside at positions 46 and 51, where Tyr51 is the site of uridylylation. Nucleotide sequence analysis of the upstream region showed no obvious sites for the binding of RNA polymerase, indicating that the glnB gene is a part of an as yet unidentified operon.

摘要

已开发出一种从大肠杆菌菌株中纯化大量PII蛋白的方法,该菌株含有携带PII结构基因(glnB基因)的多拷贝质粒。使用纯化的PII获得了尿苷酰化和未尿苷酰化PII的紫外光谱,并推导了用于计算蛋白质浓度和每个分子尿苷酰化亚基平均数的经验公式。还建立了一种用于测量尿苷酰化PII(PIID)和腺苷酰转移酶(ATase)的连续荧光测定法。在不同浓度的PIID和固定浓度的ATase下进行速率测量表明,四聚体PIID分子一次仅与一个ATase分子相互作用。确定了glnB基因的完整核苷酸序列,并通过肽段氨基酸序列分析结果证实了推导的氨基酸序列的部分内容。PII亚基由103个氨基酸组成(Mr = 11,580)。两个酪氨酸位于第46和51位,其中Tyr51是尿苷酰化位点。上游区域的核苷酸序列分析未显示RNA聚合酶结合的明显位点,表明glnB基因是一个尚未确定的操纵子的一部分。

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