首页> 美国卫生研究院文献>Journal of Bacteriology >Bradyrhizobium japonicum delta-aminolevulinic acid dehydratase is essential for symbiosis with soybean and contains a novel metal-binding domain.
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Bradyrhizobium japonicum delta-aminolevulinic acid dehydratase is essential for symbiosis with soybean and contains a novel metal-binding domain.

机译:日本慢生根瘤菌δ-氨基乙酰丙酸脱水酶对于与大豆共生是必不可少的并且含有一个新的金属结合域。

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摘要

The Bradyrhizobium japonicum hemA gene product delta-aminolevulinic acid (ALA) synthase is not required for symbiosis of that bacterium with soybean. Hence, the essentiality of the subsequent heme synthesis enzyme, ALA dehydratase, was examined. The B. japonicum ALA dehydratase gene, termed hemB, was isolated and identified on the basis of its ability to confer hemin prototrophy and enzyme activity on an Escherichia coli hemB mutant, and it encoded a protein that was highly homologous to ALA dehydratases from diverse organisms. A novel metal-binding domain in the B. japonicum ALA dehydratase was identified that is a structural composite of the Mg(2+)-binding domain found in plant ALA dehydratases and the Zn(2+)-binding region of nonplant ALA dehydratases. Enzyme activity in dialyzed extracts of cells that overexpressed the hemB gene was reconstituted by the addition of Mg2+ but not by addition of Zn2+, indicating that the B. japonicum ALA dehydratase is similar to the plant enzymes with respect to its metal requirement. Unlike the B. japonicum hemA mutant, the hemB mutant strain KP32 elicited undeveloped nodules on soybean, indicated by the lack of nitrogen fixation activity and plant hemoglobin. We conclude that the hemB gene is required for nodule development and propose that B. japonicum ALA dehydratase is the first essential bacterial enzyme for B. japonicum heme synthesis in soybean root nodules. In addition, we postulate that ALA is the only heme intermediate that can be translocated from the plant to the endosymbiont to support bacterial heme synthesis in nodules.
机译:该细菌与大豆的共生不需要日本根瘤菌(Bradyrhizobium japonicum)hemA基因产物δ-氨基乙酰丙酸(ALA)合酶。因此,检查了随后的血红素合成酶,ALA脱水酶的必要性。分离的日本血吸虫ALA脱水酶基因hemB是根据其赋予大肠杆菌hemB突变体血红素原营养和酶活性的能力而分离和鉴定的,它编码的蛋白质与多种生物的ALA脱水酶高度同源。确定了一种新的金属结合结构域,在日本芽孢杆菌ALA脱水酶中,它是在植物ALA脱水酶和非植物ALA脱水酶的Zn(2+)结合区中发现的Mg(2+)结合结构域的结构复合物。通过添加Mg2 +而不是通过添加Zn2 +来重构过表达hemB基因的细胞透析提取物中的酶活性,这表明日本芽孢杆菌ALA脱水酶在金属需求方面与植物酶相似。与日本血吸虫hemA突变体不同,hemB突变株KP32在大豆上引起未发育的根瘤,这表明缺乏固氮活性和植物血红蛋白。我们得出的结论是,hemB基因是根瘤发育所必需的,并提出日本根瘤菌ALA脱水酶是大豆根瘤中日本根瘤菌血红素合成的第一种必需细菌酶。此外,我们假设ALA是唯一可以从植物转移到内共生体以支持结节中细菌血红素合成的血红素中间体。

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