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光诱导核苷酸在菠菜叶绿体类囊体中与偶联因子1的交换。

Light-induced exchange of nucleotides into coupling factor 1 in spinach chloroplast thylakoids.

作者信息

Magnusson R P, McCarty R E

出版信息

J Biol Chem. 1976 Dec 10;251(23):7417-22.

PMID:63460
Abstract

The method of centrifugation of chloroplast thylakoids through silicone fluid, previously used to estimate the uptake of solutes by thylakoids, is shown to be an excellent method for measuring binding of nucleotides to thylakoids. This binding, which is probably an exchange (Harris, D. A. and Slater, E. C. (1975) Biochim. Biophys. Acta 387, 335-348), is enhanced by light and is sensitive to uncoupling. Half-maximal binding of adenosine 5'-triphosphate (ATP) or adenosine 5'-diphosphate (ADP) at 10 mjM was reached within less than 0.1 s. With illumination times sufficient to elicit maximal binding, saturation of the site(s) is approached at 20 muM nucleotide and dissociation constants of 5 muM and 7 muM were calculated for ADP and ATP, respectively. At saturation, the binding corresponds to 1 mol/mol of coupling factor 1 or less. Although the light-dependent binding of ADP does not require Mg2+, that of ATP is markedly enhanced by Mg2+. A 10-fold molar excess of guanosine di- or triphosphate or adenyl-5'-yl imidodiphosphate had little effect on the binding. Adenosine 5'-phosphosulfate, a competitive inhibitor of phosphorylation with respect to ADP, decreases the binding. Thylakoids, previously illuminated in the absence of added nucleotides, retain the capacity to bind ADP or ATP in the dark long after the H+ electrochemical gradient has decayed. The conformation of coupling factor 1 in darkened thylakoids following illumination in the absence of added nucleotides may thus differ from that in thylakoids either illuminated in the presence of nucleotides or kept in the dark. Approximately 20% of the ADP bound to coupling factor 1 in thylakoids is converted to ATP by a 2-s illumination. Bound inorganic phosphate, derived either from ATP or from inorganic phosphate itself, serves as the phosphoryl donor. Bound ADP may, therefore, be of catalytic significance in the mechanism of phosphorylation.

摘要

以前用于估计类囊体对溶质吸收的通过硅油对叶绿体类囊体进行离心的方法,被证明是一种测量核苷酸与类囊体结合的出色方法。这种结合可能是一种交换(哈里斯,D.A.和斯莱特,E.C.(1975年)《生物化学与生物物理学报》387卷,335 - 348页),受光增强且对解偶联敏感。在10 mM时,腺苷5'-三磷酸(ATP)或腺苷5'-二磷酸(ADP)的半最大结合在不到0.1秒内达到。在足以引发最大结合的光照时间下,在20 μM核苷酸时接近位点饱和,分别计算出ADP和ATP的解离常数为5 μM和7 μM。在饱和时,结合量相当于每摩尔偶联因子1或更少。虽然ADP的光依赖性结合不需要Mg2 +,但ATP的光依赖性结合在Mg2 +存在下明显增强。鸟苷二磷酸或三磷酸或腺苷 - 5'-亚氨基二磷酸的10倍摩尔过量对结合影响很小。腺苷5'-磷酸硫酸酯,一种相对于ADP的磷酸化竞争性抑制剂,会降低结合。以前在不添加核苷酸的情况下光照的类囊体,在H +电化学梯度衰减很久之后,在黑暗中仍保留结合ADP或ATP的能力。因此,在不添加核苷酸的情况下光照后,黑暗中类囊体中偶联因子1的构象可能与在有核苷酸存在下光照或一直处于黑暗中的类囊体中的构象不同。通过2秒光照,类囊体中与偶联因子1结合的约20%的ADP会转化为ATP。结合的无机磷酸,要么来自ATP,要么来自无机磷酸本身,作为磷酰基供体。因此,结合的ADP在磷酸化机制中可能具有催化意义。

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