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Changes in the sarcoplasmic reticulum membrane profile induced by enzyme phosphorylation to E1 approximately P at 16 A resolution via time-resolved x-ray diffraction.

机译：通过时间分辨的X射线衍射在16 A的分辨率下酶磷酸化为E1引起的肌质网膜轮廓的变化约为P。

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摘要

Time-resolved x-ray diffraction studies of the isolated sarcoplasmic reticulum (SR) membrane have provided the difference electron density profile for the SR membrane for which the Ca2+ ATPase is transiently trapped exclusively in the first phosphorylated intermediate state, E1 approximately P, in absence of detectable enzyme turnover vs. that before ATP-initiated phosphorylation of the enzyme. These diffraction studies, which utilized the flash-photolysis of caged ATP, were performed at temperatures between 0 and -2 degrees C and with a time-resolution of 2-5 s. Analogous time-resolved x-ray diffraction studies of the SR membrane at 7-8 degrees C with a time resolution of 0.2-0.5 s have previously provided the difference electron density profile for the SR membrane for which the Ca2+ ATPase is only predominately in the first phosphorylated intermediate state under conditions of enzyme turnover vs. that before enzyme phosphorylation. The two difference profiles, compared at the same low resolution (approximately 40 A), are qualitatively similar but nevertheless contain some distinctly different features and have therefore been analyzed via a step-function model analysis. This analysis was based on the refined step-function models for the two different electron density profiles obtained independently from x-ray diffraction studies at higher resolution (16-17 A) of the SR membrane before enzyme phosphorylation at 7.5 and -2 degrees C. The step-function model analysis indicated that the low resolution difference profiles derived from both time-resolved x-ray diffraction experiments arise from a net movement of Ca2+ ATPase protein mass from the outer monolayer to the inner monolayer of the SR membrane lipid bilayer. The conserved redistribution of this protein mass is however somewhat different for the two cases, especially at the extravesicular membrane surface containing the Ca2+ATPase "headpiece." However, the conserved redistribution of protein mass within the SR membrane lipid bilayer common to both cases is clearly due to E1~P formation.

机译：对分离的肌质网（SR）膜的时间分辨X射线衍射研究提供了SR膜的差电子密度分布图，其中Ca2 + ATPase仅在第一个磷酸化的中间态E1约P的情况下瞬时被捕获ATP引发的酶磷酸化之前可检测到的酶转化率的变化。这些利用笼状ATP的快速光解的衍射研究是在0到-2摄氏度之间的温度下进行的，时间分辨率为2-5 s。 SR膜在7-8摄氏度，时间分辨率为0.2-0.5 s的情况下，类似的时间分辨X射线衍射研究以前提供了SR膜的差电子密度分布图，其中Ca2 + ATPase仅主要存在于Ca2 + ATPase中。与酶磷酸化之前相比，在酶转换条件下的第一个磷酸化中间状态在相同的低分辨率（约40 A）下进行比较的两个差异曲线在质量上相似，但仍包含一些明显不同的特征，因此已通过阶跃函数模型分析进行了分析。该分析基于两个不同电子密度曲线的精细阶梯函数模型，该模型独立于SR膜在7.5和-2摄氏度下进行磷酸化之前以较高的分辨率（16-17 A）通过X射线衍射研究获得。阶跃函数模型分析表明，两个时间分辨的X射线衍射实验得出的低分辨率差异图谱是由Ca2 + ATPase蛋白质量从SR膜脂质双层的外单层向内单层的净运动引起的。但是，在两种情况下，此蛋白质质量的保守重分布有些不同，尤其是在包含Ca2 + ATPase“头戴式耳机”的囊外膜表面。然而，两种情况下常见的SR膜脂质双层内蛋白质质量的保守重新分布显然是由于E1〜P的形成。

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期刊名称 Biophysical Journal
作者
D. Pascolini; L. G. Herbette; V. Skita; F. Asturias; A. Scarpa; J. K. Blasie;
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年(卷),期 1988(54),4
年度 1988
页码 679–687
总页数 9
原文格式 PDF
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中图分类生物物理学 ;
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专利

1. Calcium dependence of Pi phosphorylation of sarcoplasmic reticulum Ca2+-ATPase at low water content: water dependence of the E2-->E1 conversion. [J] . Sodre CL, Barrabin H, Scofano HM Biochimica et biophysica acta: international journal of biochemistry and biophysics . 1999 ,第1期

机译：低水含量下肌质网Ca2 + -ATPase的Pi磷酸化的钙依赖性：E2-> E1转化的水依赖性。
2. Quantifying bond distortions in transient enzyme species by a combination of density functional theory calculations and time-resolved infrared difference spectroscopy. Implications for the mechanism of dephosphorylation of the sarcoplasmic reticulum Ca2+-ATPase (SERCA1a) [J] . Barth Andreas Biochimica et biophysica acta. Bioenergetics . 2015 ,第10期

机译：结合密度泛函理论计算和时间分辨红外差光谱法定量分析瞬时酶中的键畸变。对肌浆网Ca2 + -ATPase（SERCA1a）的去磷酸化机制的意义
3. Rearrangement of domain elements of the Ca-ATPase in cardiac sarcoplasmic reticulum membranes upon phospholamban phosphorylation. [J] . Negash S, Huang S, Squier TC Biochemistry . 1999 ,第25期

机译：磷酸lamban磷酸化后，心肌肌浆网膜中Ca-ATPase的域元素重排。
4. TIME-RESOLVED FLUORESCENCE ENERGY TRANSFER MEASUREMENTS BETWEEN SITE-SPECIFIC PROBES ON THE CA-ATPASE OF SARCOPLASMIC RETICULUM IN DIFFERENT ENZYMATIC STATES [C] . Thomas C. Squier, Diana J. Bigelow, Jorge Garcia de Ancos, Fluorescence Science and Technology . 2000

机译：不同酶促态在肌肉网状术中CA-ATP酶的定位探针之间的时间分辨荧光能量转移测量
5. Phosphorylation kinetics of the sarcoplasmic reticulum calcium ion-ATPase following exercise. [D] . McCarthy, John Joseph. 1995

机译：运动后肌质网钙离子ATPase的磷酸化动力学。
6. Changes in the profile structure of the sarcoplasmic reticulum membrane induced by phosphorylation of the Ca2+ ATPase enzyme in the presence of terbium: a time-resolved x-ray diffraction study. [O] . F J Asturias, R F Fischetti, J K Blasie 1994

机译：2存在下Ca2 + ATPase酶磷酸化引起的肌质网膜轮廓结构的变化：时间分辨X射线衍射研究。
7. Changes in the sarcoplasmic reticulum membrane profile induced by enzyme phosphorylation to E1 approximately P at 16 A resolution via time-resolved x-ray diffraction. [O] . Pascolini, D., Herbette, L. G., Skita, V., 1988

机译：通过时间分辨的X射线衍射，以16 A的分辨率将酶磷酸化为E1引起的肌质网膜轮廓的变化。
8. Cyclic AMP Stimulation of Membrane Phosphorylation and Ca(2+)-Activated, Mg(2+)-Dependent ATPase in Cardiac Sarcoplasmic Reticulum. [R] . Wray, H. L., Gray, R. R. 1976

机译：环磷酸腺苷对心肌肌浆网中膜磷酸化和Ca（2 +）激活的mg（2+）依赖性aTp酶的刺激作用。

Changes in the sarcoplasmic reticulum membrane profile induced by enzyme phosphorylation to E1 approximately P at 16 A resolution via time-resolved x-ray diffraction.

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