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光合磷酸化的初始阶段。使用饱和短闪光激发的研究。

The initial stages of photophosphorylation. Studies using excitation by saturating, short flashes of light.

作者信息

Harris D A, Crofts A R

出版信息

Biochim Biophys Acta. 1978 Apr 11;502(1):87-102. doi: 10.1016/0005-2728(78)90134-2.

Abstract
  1. Photophosphorylation was studied in spinach chloroplasts on illumination, from the dark state, with saturating short ("single turnover") flashes of light. 2. At rapid flash rates (100 Hz), phosphorylation began within the first five flashes. The ATPase inhibitor protein appeared to be displaced from its inhibitory site on the ATPase also within five flashes, as deduced from the flash-induced ATPase activity. 3. At slower flash rates, or if the rate of electron transfer were reduced with 3-(3,4-dichlorophenyl)-1,1-dimethyl urea (DCMU), phosphorylation began only after a larger number (50--60) of flashes. The displacement of the ATPase inhibitior protein was similarly delayed. 4. Partial displacement of the inhibitor protein from its inhibitory site on the ATPase (by pretreatment with dithioerythritol) allowed phosphorylation to proceed without a perceptible lag, even in the presence of DCMU. It was concluded that the ATPase inhibitor protein must be displaced on the ATPase before phosphorylation can begin, and that this process is energy dependent. 5. During the flash regime used, release of inhibitor from its inhibitory site seemed to be governed largely by the membrane potential. The light-induced pH gradient seemed to have little effect under these conditions. Our results are not compatible with a direct conformational interaction between the electron transfer chain and the ATPase causing displacement of the inhibitor. 6. The maximal rate of photophosphorylation induced by less than 200 flashes was 0.12--0.15 mol ATP made/mol ATPase per flash. This rate seemed to be limited not be the supply of energy to the ATPase molecules, nor by the maximal turnover capacity of the ATP synthesising system, but by the number of ATPase molecules which were active in synthesis, i.e., which lacked the inhibitor protein. 7. The bound nucleotides of the coupling ATPase exchanged with added nucleotides during single turnover flashes. At high flash rates, exchange began within 5 flashes. The average amount of nucleotide exchanged per flash over 100 flashes was about one tenth the amount of ATP synthesised in each flash. 8. It is concluded that, during phosphorylation, a steady state level of active coupling ATPases is set up. The energy-dependent displacement of the inhibitor protein, and its (energy-independent) relaxation back on to the inhibitory site are the two opposing factors involved in this steady state.
摘要
  1. 在菠菜叶绿体中,于黑暗状态下用光饱和的短(“单次周转”)闪光照射,研究了光合磷酸化作用。2. 在快速闪光频率(100赫兹)下,磷酸化作用在前五次闪光内开始。从闪光诱导的ATP酶活性推断,ATP酶抑制蛋白似乎也在五次闪光内从其在ATP酶上的抑制位点被置换。3. 在较慢的闪光频率下,或者如果用3-(3,4-二氯苯基)-1,1-二甲基脲(DCMU)降低电子传递速率,磷酸化作用仅在大量(50 - 60次)闪光后才开始。ATP酶抑制蛋白的置换同样延迟。4. 用二硫苏糖醇预处理使抑制蛋白从其在ATP酶上的抑制位点部分置换,即使在存在DCMU的情况下,也能使磷酸化作用无明显延迟地进行。得出的结论是,在磷酸化作用开始之前,ATP酶抑制蛋白必须从ATP酶上被置换,并且这个过程是能量依赖的。5. 在所用的闪光模式期间,抑制蛋白从其抑制位点的释放似乎在很大程度上受膜电位控制。在这些条件下,光诱导的pH梯度似乎影响很小。我们的结果与电子传递链和ATP酶之间直接的构象相互作用导致抑制蛋白置换不相符。6. 少于200次闪光诱导的光合磷酸化的最大速率为每次闪光0.12 - 0.15摩尔ATP生成/摩尔ATP酶。这个速率似乎不是受ATP酶分子的能量供应限制,也不是受ATP合成系统的最大周转能力限制,而是受参与合成的、即缺乏抑制蛋白的ATP酶分子数量限制。7. 在单次周转闪光期间,偶联ATP酶结合的核苷酸与添加的核苷酸进行交换。在高闪光频率下,交换在5次闪光内开始。在100次闪光中每次闪光平均交换的核苷酸量约为每次闪光合成的ATP量的十分之一。8. 得出的结论是,在磷酸化过程中,建立了活性偶联ATP酶的稳态水平。抑制蛋白的能量依赖置换及其(能量独立)回到抑制位点的松弛是参与这个稳态的两个相反因素。

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