Haraux F, de Kouchkovsky Y
Biochim Biophys Acta. 1980 Aug 5;592(1):153-68. doi: 10.1016/0005-2728(80)90122-x.
A defined ratio, gamma, of the total proton uptake to the concentration change of free internal H+ is observed for illuminated envelope-free chloroplasts (Haraux, F. and de Kouchkovsky, Y. (1979) Biochim. Biophys. Acta, 546, 455-471). Proton uptake is measured by the external pH shift, free internal H+ by 9-aminoacridine fluorescence quenching. Extension of this work leads to the following conclusions, which, in the case of 9-aminoacridine behaviour, should apply to any kind of diffusible protonizable delta pH probe: 1. The gamma constancy is preserved when the internal volume (Vi) is modulated by chlorophyll and osmolarity changes: thus, 9-aminoacridine behaves as expected from the delta pH distribution of an amine of high pK; previous doubts on this point are attributed to the lack of control of the external proton uptake. 2. With variable 9-aminoacridine concentration, however, some variation of gamma confirms the existence of slight light-induced probe-membrane interactions. 3. According to the diffuse layer theory, salts decrease the negative potential at the 'plane of closest approach' of the thylakoids, thereby releasing the excess 9-aminoacridine in this diffuse layer, which increases its fluorescence. Although of equal valency, NH4+ is more potent than K+, suggesting competition between amines for specific anionic binding sites. 4. Two categories of membrane modifications are induced by salts: in addition to the above-mentioned electrical effect, mono- and divalent cations at high concentration increase the chloroplast proton binding capacity. La3+ is only able to release the excess dye in the diffuse layer and leaves gamma unchanged. Therefore the probe-membrane interactions should have limited importance for steady-state delta pH measurement. 5. A Donnan-type dark pH difference, which could seriously bias these delta pH estimates, is found experimentally to be less than 2 (no significant gamma change when Vi varies) and even theoretically less than 1 (on the basis of the concentration of the non-diffusible internal protonizable groups). Similarly, the predictable errors of Vi and its possible light-induced variations must have a small effect on delta pH under present experimental conditions.
对于光照下无包膜的叶绿体,可观察到总质子摄取量与游离内部H⁺浓度变化的特定比率γ(Haraux, F.和de Kouchkovsky, Y. (1979) Biochim. Biophys. Acta, 546, 455 - 471)。质子摄取通过外部pH变化来测量,游离内部H⁺通过9 - 氨基吖啶荧光猝灭来测量。这项工作的拓展得出了以下结论,就9 - 氨基吖啶的行为而言,这些结论应适用于任何一种可扩散的质子化δpH探针:1. 当通过叶绿素和渗透压变化调节内部体积(Vi)时,γ的恒定性得以保持:因此,9 - 氨基吖啶的行为符合高pK胺的δpH分布预期;此前关于这一点的疑问归因于对外部质子摄取缺乏控制。2. 然而,随着9 - 氨基吖啶浓度的变化,γ会有一些变化,这证实了存在轻微的光诱导探针 - 膜相互作用。3. 根据扩散层理论,盐会降低类囊体“最接近平面”处的负电位,从而释放该扩散层中过量的9 - 氨基吖啶,这会增加其荧光。尽管NH₄⁺和K⁺具有相同的化合价,但NH₄⁺比K⁺更有效,这表明胺之间存在对特定阴离子结合位点的竞争。4. 盐会诱导两类膜修饰:除上述电效应外, 高浓度的单价和二价阳离子会增加叶绿体的质子结合能力。La³⁺仅能释放扩散层中过量的染料,而γ不变。因此,对于稳态δpH测量,探针 - 膜相互作用的重要性应有限。5. 通过实验发现,可能严重影响这些δpH估计值的唐南型暗pH差异小于2(当Vi变化时γ无显著变化),甚至从理论上讲小于1(基于不可扩散的内部可质子化基团的浓度)。同样,在当前实验条件下,Vi的可预测误差及其可能的光诱导变化对δpH的影响必定很小。
Zotero 插件