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铁还原酶A对于反硝化副球菌有效获取铁至关重要。

Ferric reductase A is essential for effective iron acquisition in Paracoccus denitrificans.

作者信息

Sedláček Vojtěch, van Spanning Rob J M, Kučera Igor

机构信息

Department of Biochemistry, Faculty of Science, Masaryk University, Czech Republic, CZ-611 37 Brno, Czech Republic.

Department of Molecular Cell Physiology, Faculty of Earth and Life Science, VU University Amsterdam, NL-1081 HV Amsterdam, The Netherlands.

出版信息

Microbiology (Reading). 2009 Apr;155(Pt 4):1294-1301. doi: 10.1099/mic.0.022715-0.

Abstract

Based on N-terminal sequences obtained from the purified cytoplasmic ferric reductases FerA and FerB, their corresponding genes were identified in the published genome sequence of Paracoccus denitrificans Pd1222. The ferA and ferB genes were cloned and individually inactivated by insertion of a kanamycin resistance marker, and then returned to P. denitrificans for exchange with their wild-type copies. The resulting ferA and ferB mutant strains showed normal growth in brain heart infusion broth. Unlike the ferB mutant, the strain lacking FerA did not grow on succinate minimal medium with ferric 2,3-dihydroxybenzoate as the iron source, and grew only poorly in the presence of ferric sulfate, chloride, citrate, NTA, EDTA and EGTA. Moreover, the ferA mutant strain was unable to produce catechols, which are normally detectable in supernatants from iron-limited wild-type cultures. Complementation of the ferA mutation using a derivative of the conjugative broad-host-range plasmid pEG400 that contained the whole ferA gene and its putative promoter region largely restored the wild-type phenotype. Partial, though significant, restoration could also be achieved with 1 mM chorismate added to the growth medium. The purified FerA protein acted as an NADH : FMN oxidoreductase and catalysed the FMN-mediated reductive release of iron from the ferric complex of parabactin, the major catecholate siderophore of P. denitrificans. The deduced amino acid sequence of the FerA protein has closest similarity to flavin reductases that form part of the flavin-dependent two-component monooxygenases. Taken together, our results demonstrate an essential role of reduced flavins in the utilization of exogenous ferric iron. These flavins not only provide the electrons for Fe(III) reduction but most probably also affect the rate of siderophore production.

摘要

根据从纯化的细胞质铁还原酶FerA和FerB获得的N端序列,在反硝化副球菌Pd1222已发表的基因组序列中鉴定出它们相应的基因。将ferA和ferB基因克隆并通过插入卡那霉素抗性标记分别使其失活,然后将其导入反硝化副球菌以与野生型拷贝进行交换。所得的ferA和ferB突变株在脑心浸液肉汤中生长正常。与ferB突变株不同,缺乏FerA的菌株在以2,3-二羟基苯甲酸铁为铁源的琥珀酸基本培养基上不能生长,并且在硫酸铁、氯化铁、柠檬酸铁、NTA、EDTA和EGTA存在的情况下生长也很差。此外,ferA突变株无法产生儿茶酚,而在铁限制的野生型培养物的上清液中通常可以检测到儿茶酚。使用包含整个ferA基因及其推定启动子区域的接合广宿主范围质粒pEG400的衍生物对ferA突变进行互补,在很大程度上恢复了野生型表型。向生长培养基中添加1 mM分支酸也可以实现部分但显著的恢复。纯化的FerA蛋白作为NADH:FMN氧化还原酶,催化FMN介导的从反硝化副球菌的主要儿茶酚盐铁载体副杆菌素的铁络合物中还原释放铁。FerA蛋白的推导氨基酸序列与作为黄素依赖性双组分单加氧酶一部分的黄素还原酶最相似。综上所述,我们的结果证明了还原黄素在利用外源三价铁中的重要作用。这些黄素不仅为Fe(III)还原提供电子,而且很可能还影响铁载体的产生速率。

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