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首页> 外文期刊>Neuroscience: An International Journal under the Editorial Direction of IBRO >Live-cell imaging of aquaporin-4 diffusion and interactions in orthogonal arrays of particles.
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Live-cell imaging of aquaporin-4 diffusion and interactions in orthogonal arrays of particles.

机译:Aquaporin-4扩散和粒子正交阵列中相互作用的活细胞成像。

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摘要

Orthogonal arrays of particles (OAPs) have been visualized for many years by freeze-fracture electron microscopy. Our laboratory discovered that aquaporin-4 (AQP4) is the protein responsible for OAP formation by demonstrating OAPs in AQP4-transfected cells and absence of OAPs in AQP4 knockout mice. We recently developed live-cell, single-molecule imaging methods to study AQP4 diffusion and interactions in OAPs. The methods include single particle tracking of quantum-dot labeled AQP4, and total internal reflection fluorescence microscopy of green fluorescent protein (GFP) and small fluorophore-labeled AQP4. The full-length (M1) form of AQP4 diffuses freely in membranes and does not form OAPs, whereas the shorter (M23) form of AQP4 forms OAPs and is nearly immobile. Analysis of a series of AQP4 truncations, point mutants and chimeras revealed that OAP formation by AQP4-M23 is stabilized by hydrophobic tetramer-tetramer interactions involving N-terminus residues, and that absence of OAPs in AQP4-M1 results from blocking of this interaction by residues just upstream from Met23. These biophysical methods are being extended to identify the cellular site of AQP4 assembly, AQP4 isoform interactions, OAP size and dynamics, and the determinants of regulated OAP assembly.
机译:多年以来,通过冷冻断裂电子显微镜观察了颗粒的正交阵列(OAP)。我们的实验室发现水通道蛋白4(AQP4)是负责OAP形成的蛋白,它通过证明AQP4转染的细胞中的OAP和AQP4基因敲除小鼠中不存在OAP来实现。我们最近开发了活细胞单分子成像方法来研究AQP4在OAP中的扩散和相互作用。该方法包括对量子点标记的AQP4进行单粒子跟踪,以及绿色荧光蛋白(GFP)和小荧光团标记的AQP4的全内反射荧光显微镜检查。 AQP4的全长(M1)形式在膜中自由扩散,不形成OAP,而较短的(M23)形式的AQP4形成OAP,几乎不动。对一系列AQP4截短,点突变体和嵌合体的分析表明,AQP4-M23的OAP形成通过涉及N末端残基的疏水四聚体-四聚体相互作用而得以稳定,并且AQP4-M1中不存在OAP是由于通过阻断该相互作用而导致的。残留在Met23上游。这些生物物理方法正在扩展,以识别AQP4组装的细胞部位,AQP4同工型相互作用,OAP大小和动力学以及受调控的OAP组装的决定因素。

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