Upchurch R G, Mortenson L E
J Bacteriol. 1980 Jul;143(1):274-84. doi: 10.1128/jb.143.1.274-284.1980.
The effects of the intracellular energy balance and adenylate pool composition on N2 fixation were examined by determining changes in the energy charge (EC) and the ADP/ATP (D/T) ratio of cells in chemostat and batch cultures of Clostridium pasteurianum, Klebsiella pneumoniae, and Azotobacter vinelandii. When cells of C. pasteurianum, K. pneumoniae, and A. vinelandii in sucrose-limited chemostats were examined, in all cases the EC increased greater than or equal to 15% when the nitrogen source was switched from N2 to NH3 and decreased greater than or equal to 15% when the nitrogen source was switched from NH3 to N2. The D/T ratio of the same cultures decreased greater than or equal to 70% when they were switched from N2 to NH3. In such cultures the adenylate pools remained constant when the cells were grown on either NH3 or N2. In nitrogen (NH3)-limited cultures, the adenylate pool was two- to threefold higher than the adenylate pool in sucrose-limited cultures, and the nitrogenase content of such cells was two- to threefold greater than the nitrogenase content of sucrose-limited N2-fixing cells. The EC and D/T ratio of cells from batch cultures of C. pasteurianum growing on NH3 in the presence of N2 were 0.82 and 0.83, respectively, but when the NH3 was consumed and the cells were switched to a nitrogen-fixing metabolism, the EC and D/T ratio changed to 0.70 and 0.90, respectively. Conversely, when NH3 was added to N2-fixing cultures the EC and D/T ratio changed within 1.5 h the EC and D/T ratio of NH3-grown cells. The nitrogen content of N2-fixing cells to which NH3 was added decreased at a rate greater could be accounted for by cell growth in the absence of further synthesis. This decay of nitrogenase activity (with a half-life about 1.2 to 1.4 h) suggests that some type of inactivation of nitrogenase occurs during repression. The nitrogenase of whole cells was estimated to be operating at about 32% of its theoretical maximum activity during steady-state N2-fixing conditions. Similarities in the data from chemostat and batch cultures of both aerobic and anaerobic N2-fixing organisms suggest that low EC and high D/T ratio are normal manifestations of an N2-fixing physiology.
通过测定巴氏梭菌、肺炎克雷伯菌和维氏固氮菌在恒化器和分批培养中的细胞能量电荷(EC)和ADP/ATP(D/T)比值的变化,研究了细胞内能量平衡和腺苷酸库组成对固氮作用的影响。当检测蔗糖限制的恒化器中巴氏梭菌、肺炎克雷伯菌和维氏固氮菌的细胞时,在所有情况下,当氮源从N₂切换到NH₃时,EC增加大于或等于15%,而当氮源从NH₃切换到N₂时,EC降低大于或等于15%。当相同培养物从N₂切换到NH₃时,其D/T比值降低大于或等于70%。在这样的培养物中,当细胞在NH₃或N₂上生长时,腺苷酸库保持恒定。在氮(NH₃)限制的培养物中,腺苷酸库比蔗糖限制培养物中的腺苷酸库高两到三倍,并且此类细胞的固氮酶含量比蔗糖限制的固氮细胞的固氮酶含量高两到三倍。在有N₂存在的情况下,在NH₃上生长的巴氏梭菌分批培养细胞的EC和D/T比值分别为0.82和0.83,但当NH₃被消耗且细胞切换到固氮代谢时,EC和D/T比值分别变为0.70和0.90。相反,当向固氮培养物中添加NH₃时,EC和D/T比值在1.5小时内发生变化,达到NH₃生长细胞的EC和D/T比值。添加NH₃的固氮细胞的氮含量以更大的速率下降,这可以由细胞在没有进一步合成的情况下生长来解释。这种固氮酶活性的衰减(半衰期约为1.2至1.4小时)表明在阻遏过程中发生了某种类型的固氮酶失活。据估计,在稳定状态的固氮条件下,全细胞的固氮酶以其理论最大活性的约32%运行。需氧和厌氧固氮生物的恒化器和分批培养数据的相似性表明,低EC和高D/T比值是固氮生理学的正常表现。
