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豌豆根瘤菌蚕豆生物型氢化酶的宿主依赖性表达在豆科植物根瘤中受转录和转录后水平的控制。

Host-dependent expression of Rhizobium leguminosarum bv. viciae hydrogenase is controlled at transcriptional and post-transcriptional levels in legume nodules.

作者信息

Brito Belén, Toffanin Annita, Prieto Rosa-Isabel, Imperial Juan, Ruiz-Argüeso Tomás, Palacios Jose M

机构信息

Departamento de Biotecnología, Escuela Técnica Superior Ingenieros Agrónomos, Universidad Politécnica de Madrid (UPM), Spain.

出版信息

Mol Plant Microbe Interact. 2008 May;21(5):597-604. doi: 10.1094/MPMI-21-5-0597.

Abstract

The legume host affects the expression of Rhizobium leguminosarum hydrogenase activity in root nodules. High levels of symbiotic hydrogenase activity were detected in R. leguminosarum bacteroids from different hosts, with the exception of lentil (Lens culinaris). Transcription analysis showed that the NifA-regulated R. leguminosarum hydrogenase structural gene promoter (P(1)) is poorly induced in lentil root nodules. Replacement of the P(1) promoter by the FnrN-dependent promoter of the fixN gene restored transcription of hup genes in lentil bacteroids, but not hydrogenase activity. In the P(fixN)-hupSL strain, additional copies of the hup gene cluster and nickel supplementation to lentil plants increased bacteroid hydrogenase activity. However, the level of activity in lentil still was significantly lower than in pea bacteroids, indicating that an additional factor is impairing hydrogenase expression inside lentil nodules. Immunological analysis revealed that lentil bacteroids contain reduced levels of both hydrogenase structural subunit HupL and nickel-binding protein HypB. Altogether, results indicate that hydrogenase expression is affected by the legume host at the level of both transcription of hydrogenase structural genes and biosynthesis or stability of nickel-related proteins HypB and HupL, and suggest the existence of a plant-dependent mechanism that affects hydrogenase activity during the symbiosis by limiting nickel availability to the bacteroid.

摘要

豆科宿主影响根瘤中豆科根瘤菌氢化酶活性的表达。在来自不同宿主的豆科根瘤菌类菌体中检测到高水平的共生氢化酶活性,但小扁豆(兵豆)除外。转录分析表明,受NifA调控的豆科根瘤菌氢化酶结构基因启动子(P(1))在小扁豆根瘤中诱导程度很低。用fixN基因的依赖FnrN的启动子替换P(1)启动子可恢复小扁豆类菌体中hup基因的转录,但不能恢复氢化酶活性。在P(fixN)-hupSL菌株中,hup基因簇的额外拷贝以及向小扁豆植株补充镍可提高类菌体氢化酶活性。然而,小扁豆中的活性水平仍显著低于豌豆类菌体中的活性水平,这表明还有一个额外因素在损害小扁豆根瘤内氢化酶的表达。免疫分析显示,小扁豆类菌体中氢化酶结构亚基HupL和镍结合蛋白HypB的水平均降低。总之,结果表明氢化酶表达在氢化酶结构基因转录以及镍相关蛋白HypB和HupL的生物合成或稳定性水平上受到豆科宿主的影响,并提示存在一种植物依赖性机制,该机制通过限制类菌体可利用的镍来影响共生期间的氢化酶活性。

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