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绿针假单胞菌B23中腈水合酶基因簇的转录调控

Transcriptional regulation of the nitrile hydratase gene cluster in Pseudomonas chlororaphis B23.

作者信息

Sakashita Toshihide, Hashimoto Yoshiteru, Oinuma Ken-ichi, Kobayashi Michihiko

机构信息

Institute of Applied Biochemistry, and Graduate School of Life and Environmental Sciences, The University of Tsukuba, 1-1-1 Tennodai, Tsukuba, Ibaraki 305-8572, Japan.

出版信息

J Bacteriol. 2008 Jun;190(12):4210-7. doi: 10.1128/JB.00061-08. Epub 2008 Apr 11.

Abstract

An enormous amount of nitrile hydratase (NHase) is inducibly produced by Pseudomonas chlororaphis B23 after addition of methacrylamide as the sole nitrogen source to a medium. The expression pattern of the P. chlororaphis B23 NHase gene cluster in response to addition of methacrylamide to the medium was investigated. Recently, we reported that the NHase gene cluster comprises seven genes (oxdA, amiA, nhpA, nhpB, nhpC, nhpS, and acsA). Sequence analysis of the 1.5-kb region upstream of the oxdA gene revealed the presence of a 936-bp open reading frame (designated nhpR), which should encode a protein with a molecular mass of 35,098. The deduced amino acid sequence of the nhpR product showed similarity to the sequences of transcriptional regulators belonging to the XylS/AraC family. Although the transcription of the eight genes (nhpR, oxdA, amiA, nhpABC, nhpS, and acsA) in the NHase gene cluster was induced significantly in the P. chlororaphis B23 wild-type strain after addition of methacrylamide to the medium, transcription of these genes in the nhpR disruptant was not induced, demonstrating that nhpR codes for a positive transcriptional regulator in the NHase gene cluster. A reverse transcription-PCR experiment revealed that five genes (oxdA, amiA, nhpA, nhpB, and nhpC) are cotranscribed, as are two other genes (nhpS and acsA). The transcription start sites for nhpR, oxdA, nhpA, and nhpS were mapped by primer extension analysis, and putative -12 and -24 sigma(54)-type promoter binding sites were identified. NhpR was found to be the first transcriptional regulator of NHase belonging to the XylS/AraC family.

摘要

在以甲基丙烯酰胺作为唯一氮源添加到培养基中后,氯代绿针假单胞菌B23可诱导产生大量腈水合酶(NHase)。研究了氯代绿针假单胞菌B23的NHase基因簇在向培养基中添加甲基丙烯酰胺后的表达模式。最近,我们报道NHase基因簇由七个基因(oxdA、amiA、nhpA、nhpB、nhpC、nhpS和acsA)组成。对oxdA基因上游1.5 kb区域的序列分析揭示了一个936 bp的开放阅读框(命名为nhpR)的存在,该阅读框应编码一种分子量为35,098的蛋白质。nhpR产物的推导氨基酸序列与属于XylS/AraC家族的转录调节因子的序列相似。尽管在向培养基中添加甲基丙烯酰胺后,氯代绿针假单胞菌B23野生型菌株中NHase基因簇中的八个基因(nhpR、oxdA、amiA、nhpABC、nhpS和acsA)的转录被显著诱导,但nhpR缺失突变体中这些基因的转录未被诱导,这表明nhpR编码NHase基因簇中的一个正转录调节因子。逆转录PCR实验表明,五个基因(oxdA、amiA、nhpA、nhpB和nhpC)是共转录的,另外两个基因(nhpS和acsA)也是如此。通过引物延伸分析确定了nhpR基因、oxdA基因、nhpA基因和nhpS基因的转录起始位点,并鉴定了推定的-12和-24 σ⁵⁴型启动子结合位点。发现NhpR是属于XylS/AraC家族的NHase的第一个转录调节因子。

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