Azorhizobium caulinodans uses both cytochrome bd (quinol) and cytochrome cbb3 (cytochrome c) terminal oxidases for symbiotic N2 fixation.

P A Kaminski; C L Kitts; Z Zimmerman; R A Ludwig

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Azorhizobium caulinodans uses both cytochrome bd (quinol) and cytochrome cbb3 (cytochrome c) terminal oxidases for symbiotic N2 fixation.

机译：固氮假单胞菌同时使用细胞色素bd（喹诺尔）和细胞色素cbb3（细胞色素c）末端氧化酶进行共生N2固定。

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Azorhizobium caulinodans employs both cytochrome bd (cytbd; quinol oxidase) and cytcbb3 (cytc oxidase) as terminal oxidases in environments with very low O2 concentrations. To investigate physiological roles of these two terminal oxidases both in microaerobic culture and in symbiosis, knockout mutants were constructed. As evidenced by visible absorbance spectra taken from mutant bacteria carrying perfect gene replacements, both the cytbd- and cytcbb3- mutations were null alleles. In aerobic culture under 2% O2 atmosphere, Azorhizobium cytbd- and cytcbb3- single mutants both fixed N2 at 70 to 90% of wild-type rates; in root nodule symbiosis, both single mutants fixed N2 at 50% of wild-type rates. In contrast, Azorhizobium cytbd- cytcbb3-double mutants, which carry both null alleles, completely lacked symbiotic N2 fixation activity. Therefore, both Azorhizobium cytbd and cytcbb3 oxidases drive respiration in environments with nanomolar O2 concentrations during symbiotic N2 fixation. In culture under a 2% O2 atmosphere, Azorhizobium cytbd- cytcbb3- double mutants fixed N2 at 70% of wild-type rates, presumably reflecting cytaa3 and cytbo (and other) terminal oxidase activities. In microaerobic continuous cultures in rich medium, Azorhizobium cytbd- and cytcbb3- single mutants were compared for their ability to deplete a limiting-O2 sparge; cytbd oxidase activity maintained dissolved O2 at 3.6 microM steady state, whereas cytcbb3 oxidase activity depleted O2 to submicromolar levels. Growth rates reflected this difference; cytcbb3 oxidase activity disproportionately supported microaerobic growth. Paradoxically, in O2 limited continuous culture, Azorhizobium cytbd oxidase is inactive below 3.6 microM dissolved O2 whereas in Sesbania rostrata symbiotic nodules, in which physiological, dissolved O2 is maintained at 10 to 20 nM, both Azorhizobium cytbd and cytcbb3 seem to contribute equally as respiratory terminal oxidases.

机译：在含氧量非常低的环境中，阿布鲁霍单胞菌藻类同时使用细胞色素bd（cytbd;喹诺醇氧化酶）和cytcbb3（cytc氧化酶）作为末端氧化酶。为了研究这两个末端氧化酶在微有氧培养和共生中的生理作用，构建了敲除突变体。如从携带完美基因替代物的突变细菌中获得的可见吸收光谱所证明的，cytbd-和cytcbb3-突变均为无效等位基因。在2％的O2气氛下进行有氧培养时，偶氮假单胞菌cytbd-和cytcbb3-单个突变体都将N2固定为野生型率的70％至90％。在根瘤共生中，两个单个突变体都将N2固定为野生型发生率的50％。相反，携带两个无效等位基因的满生偶氮cytbd-cytcbb3-double突变体完全缺乏共生N2固定活性。因此，在共生N2固定过程中，氮杂偶氮菌的cytbd和cytcbb3氧化酶都可在具有纳摩尔O2浓度的环境中驱动呼吸。在2％O2气氛下的培养中，假单胞菌cytbd-cytcbb3-双突变体将N2固定为野生型率的70％，大概反映了cytaa3和cytbo（和其他）末端氧化酶的活性。在丰富培养基中的微需氧连续培养中，比较了满江红假单胞菌cytbd-和cytcbb3-单个突变体消耗有限O2的能力。 cytbd氧化酶活性将溶解的O2保持在3.6 microM的稳态，而cytcbb3氧化酶活性则将O2消耗至亚微摩尔水平。增长率反映了这种差异; cytcbb3氧化酶的活性不成比例地支持了有氧微生物的生长。矛盾的是，在O2有限的连续培养中，低于3.6 microM的溶解态O2时，固氮假单胞菌氧化酶失活，而在Sesbania rostrata共生结节中，生理性溶解的O2维持在10至20 nM，Azorhizobium cytbd和cytcbb3似乎与呼吸作用相同末端氧化酶。

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《Journal of bacteriology》 |1996年第20期|共6页
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P A Kaminski; C L Kitts; Z Zimmerman; R A Ludwig;
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6. Azorhizobium caulinodans uses both cytochrome bd (quinol) and cytochrome cbb3 (cytochrome c) terminal oxidases for symbiotic N2 fixation. [O] . P A Kaminski, C L Kitts, Z Zimmerman, 1996

机译：固氮假单胞菌同时使用细胞色素bd（喹诺尔）和细胞色素cbb3（细胞色素c）末端氧化酶进行共生N2固定。
7. Azorhizobium caulinodans uses both cytochrome bd (quinol) and cytochrome cbb3 (cytochrome c) terminal oxidases for symbiotic N2 fixation. [O] . Kaminski, P A, Kitts, C L, Zimmerman, Z, 1996

机译：固氮假单胞菌同时使用细胞色素bd（喹诺尔）和细胞色素cbb3（细胞色素c）末端氧化酶进行共生N2固定。

Azorhizobium caulinodans uses both cytochrome bd (quinol) and cytochrome cbb3 (cytochrome c) terminal oxidases for symbiotic N2 fixation.

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