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Effects of Disruption of Homocitrate Synthase Genes on Nostoc sp. Strain PCC 7120 Photobiological Hydrogen Production and Nitrogenase

机译:同质合酶基因的破坏对Nostoc sp。的影响。菌株PCC 7120光生物产氢和固氮酶

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摘要

In the case of nitrogenase-based photobiological hydrogen production systems of cyanobacteria, the inactivation of uptake hydrogenase (Hup) leads to significant increases in hydrogen production activity. However, the high-level-activity stage of the Hup mutants lasts only a few tens of hours under air, a circumstance which seems to be caused by sufficient amounts of combined nitrogen supplied by active nitrogenase. The catalytic FeMo cofactor of nitrogenase binds homocitrate, which is required for efficient nitrogen fixation. It was reported previously that the nitrogenase from the homocitrate synthase gene (nifV) disruption mutant of Klebsiella pneumoniae shows decreased nitrogen fixation activity and increased hydrogen production activity under N2. The cyanobacterium Nostoc sp. strain PCC 7120 has two homocitrate synthase genes, nifV1 and nifV2, and with the ΔhupL variant of Nostoc sp. strain PCC 7120 as the parental strain, we have constructed two single mutants, the ΔhupL ΔnifV1 strain (with the hupL and nifV1 genes disrupted) and the ΔhupL ΔnifV2 strain, and a double mutant, the ΔhupL ΔnifV1 ΔnifV2 strain. Diazotrophic growth rates of the two nifV single mutants and the double mutant were decreased moderately and severely, respectively, compared with the rates of the parent ΔhupL strain. The hydrogen production activity of the ΔhupL ΔnifV1 mutant was sustained at higher levels than the activity of the parent ΔhupL strain after about 2 days of combined-nitrogen step down, and the activity in the culture of the former became higher than that in the culture of the latter. The presence of N2 gas inhibited hydrogen production in the ΔhupL ΔnifV1 ΔnifV2 mutant less strongly than in the parent ΔhupL strain and the ΔhupL ΔnifV1 and ΔhupL ΔnifV2 mutants. The alteration of homocitrate synthase activity can be a useful strategy for improving sustained photobiological hydrogen production in cyanobacteria.
机译:在基于蓝藻的基于氮酶的光生物制氢系统中,摄取氢化酶(Hup)的失活导致制氢活性显着增加。但是,Hup突变体的高活性阶段在空气中仅持续数十小时,这种情况似乎是由活性固氮酶提供的足够数量的组合氮引起的。固氮酶的催化FeMo辅因子与纯柠檬酸盐结合,这是有效固氮所必需的。以前有报道说,来自肺炎克雷伯菌的纯柠檬酸合酶基因(nifV)破坏突变体的固氮酶在N2下显示出降低的固氮活性和增加的产氢活性。蓝细菌Nostoc sp。菌株PCC 7120具有两个纯柠檬酸合酶基因nifV1和nifV2,以及Nostoc sp。的ΔhupL变体。菌株PCC 7120作为亲本菌株,我们构建了两个单一突变体,即ΔhupLΔnifV1菌株(hupL和nifV1基因被破坏)和ΔhupLΔnifV2菌株,以及双突变体ΔhupLΔnifV1ΔnifV2菌株。与个体Δ hupL 菌株相比,两个 nifV 单突变体和双突变体的重营养生长速率分别适度和严重降低。大约2天后,Δ hupL Δ nifV1 突变体的产氢活性比亲本Δ hupL 菌株的活性高。氮的浓度降低,前者的培养活性高于后者。 N2气体的存在抑制了Δ hupL Δ nifV1 Δ nifV2 突变体中氢的产生,其抑制作用不如亲本Δ hupL < / em>菌株和Δ hupL Δ nifV1 和Δ hupL Δ nifV2 突变体。改变纯柠檬酸合酶活性可以是用于改善蓝细菌中持续的光生物产氢的有用策略。

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