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Phospholamban Oligomerization Quaternary Structure and Sarco(endo)plasmic Reticulum Calcium ATPase Binding Measured by Fluorescence Resonance Energy Transfer in Living Cells

机译：Phospholamban低聚四级结构和荧光测定肌质膜内质网钙ATP酶的结合生活中的共振能量转移细胞

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Phospholamban (PLB) oligomerization, quaternary structure, and sarco(endo)plasmic reticulum calcium ATPase (SERCA) binding were quantified by fluorescence resonance energy transfer (FRET) in an intact cellular environment. FRET between cyan fluorescent protein-PLB and yellow fluorescent protein-PLB in AAV-293 cells showed hyperbolic dependence on protein concentration, with a maximum efficiency of 45.1 ± 1.3%. The observed FRET corresponds to a probe separation distance of 58.7 ± 0.5Å, according to a computational model of intrapentameric FRET. This is consistent with models of the PLB pentamer in which cytoplasmic domains fan out from the central bundle of transmembrane helices. An I40A mutation of PLB did not alter pentamer conformation but increased the concentration of half-maximal FRET (KD) by >4-fold. This is consistent with the previous observation that this putatively monomeric mutant still oligomerizes in intact membranes but forms more dynamic pentamers than wild type PLB. PLB association with SERCA, measured by FRET between cyan fluorescent protein-SERCA and yellow fluorescent protein-PLB, was increased by the I40A mutation without any detectable change in probe separation distance. The data indicate that the regulatory complex conformation is not altered by the I40A mutation. A naturally occurring human mutation (L39Stop) greatly reduced PLB oligomerization and SERCA binding and caused mislocalization of PLB to the cytoplasm and nucleus. Overall, the data suggest that the PLB pentamer adopts a “pinwheel” shape in cell membranes, as opposed to a more compact “bellflower” conformation. I40A mutation decreases oligomerization and increases PLB binding to SERCA. Truncation of the transmembrane domain by L39Stop mutation prevents anchoring of the protein in the membrane, greatly reducing PLB binding to itself or its regulatory target, SERCA.

机译：在完整的细胞环境中，通过荧光共振能量转移（FRET）定量分析了磷脂酰肌醇（PLB）的低聚，四级结构和肌质网钙蛋白酶（SERCA）的结合。 AAV-293细胞中青色荧光蛋白-PLB和黄色荧光蛋白-PLB之间的FRET对蛋白质浓度呈双曲线依赖性，最大效率为45.1±1.3％。根据内部五聚体FRET的计算模型，观察到的FRET对应于探针间隔距离为58.7±0.5Å。这与PLB五聚体的模型一致，在PLB五聚体的模型中，胞质域从跨膜螺旋的中央束呈扇形散开。 PLB的I40A突变不会改变五聚体构象，但会使半最大FRET（KD）的浓度增加> 4倍。这与以前的观察结果一致，即该推测的单体突变体仍在完整膜中低聚，但形成比野生型PLB更多的动态五聚体。 I40A突变增加了蓝绿色荧光蛋白-SERCA和黄色荧光蛋白-PLB之间通过FRET测得的PLB与SERCA的关联，但探针未检测到任何变化分离距离。数据表明监管复杂 I40A突变不会改变构象。自然人突变（L39Stop）大大降低了PLB寡聚和SERCA结合，导致PLB在细胞质和细胞核中的定位错误。总体而言，数据建议PLB五角体在单元格中采用“风车”形状膜，而不是更紧凑的“风铃草”构象。 I40A突变减少寡聚并增加PLB与SERCA的结合。 L39Stop突变截短跨膜结构域可阻止锚定膜中蛋白质的含量，大大减少了PLB与其自身或其结合的结合监管目标，SERCA。

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期刊名称 The Journal of Biological Chemistry
作者
Eileen M. Kelly; Zhanjia Hou; Julie Bossuyt; Donald M. Bers; Seth L. Robia;
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年(卷),期 2008(283),18
年度 2008
页码 12202–12211
总页数 10
原文格式 PDF
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中图分类分子生物学;
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专利

1. Phospholamban and sarcolipin: Are they functionally redundant or distinct regulators of the Sarco(Endo)Plasmic Reticulum Calcium ATPase? [J] . Shaikh Sana A., Sahoo Sanjaya K., Periasamy Muthu Journal of Molecular and Cellular Cardiology . 2016,第Null期

机译：Phospholamban和sarcolipin：它们在功能上是否是Sarco（Endo）血浆网状钙ATPase的功能冗余或不同的调节剂？
2. Sarcolipin regulates sarco(endo)plasmic reticulum Ca2+-ATPase (SERCA) by binding to transmembrane helices alone or in association with phospholamban. [J] . Asahi M, Sugita Y, Kurzydlowski K, Proceedings of the National Academy of Sciences of the United States of America . 2003,第9期

机译：Sarcolipin通过单独或与phosphorlamban结合跨膜螺旋来调节sarco（endo）质网Ca2 + -ATPase（SERCA）。
3. Green fluorescent protein-tagged sarco(endo)plasmic reticulum Ca2+-ATPase overexpression in Paramecium cells: isoforms, subcellular localization, biogenesis of cortical calcium stores and functional aspects. [J] . Hauser K, Pavlovic N, Klauke N, Molecular Microbiology . 2000,第4期

机译：草履虫细胞中绿色荧光蛋白标记的肌（内）质网Ca2 + -ATPase过表达：同工型，亚细胞定位，皮质钙存储的生物发生和功能方面。
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. Mechanisms of calcium-dependent inactivation of L-type calcium channels revealed by fluorescence resonance energy transfer in living cells. [D] . Erickson, Michael Gustaf. 2003

机译：荧光共振能量转移在活细胞中揭示了钙依赖的L型钙通道失活的机制。
6. Characterizing phospholamban to sarco(endo)plasmic reticulum Ca2+-ATPase 2a (SERCA2a) protein binding interactions in human cardiac sarcoplasmic reticulum vesicles using chemical cross-linking. [O] . Brandy L. Akin, Larry R. Jones 2014

机译：使用化学交联表征磷酸lamban与肌（内）肌浆网Ca2 + -ATPase 2a（SERCA2a）蛋白结合相互作用的人类心脏肌浆小泡中。
7. Phospholamban Oligomerization, Quaternary Structure, and Sarco(endo)plasmic Reticulum Calcium ATPase Binding Measured by Fluorescence Resonance Energy Transfer in Living Cells* [O] . Kelly, Eileen M., Hou, Zhanjia, Bossuyt, Julie, 2008

机译：Phospholamban低聚，四级结构和荧光测定肌质膜内质网钙ATP酶的结合生活中的共振能量转移细胞*

Phospholamban Oligomerization Quaternary Structure and Sarco(endo)plasmic Reticulum Calcium ATPase Binding Measured by Fluorescence Resonance Energy Transfer in Living Cells

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