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通过纳米颗粒辅助毒素结合延迟检测通道接近度;一项膜片钳和流式细胞术能量转移联合研究。

Detection of channel proximity by nanoparticle-assisted delaying of toxin binding; a combined patch-clamp and flow cytometric energy transfer study.

作者信息

Rubovszky Bálint, Hajdú Péter, Krasznai Zoltán, Gáspár Rezsõ, Waldmann Thomas A, Damjanovich Sándor, Bene László

机构信息

Cell Biophysics Research Group, Hungarian Academy of Sciences, Debrecen.

出版信息

Eur Biophys J. 2005 Mar;34(2):127-43. doi: 10.1007/s00249-004-0436-x.

DOI:10.1007/s00249-004-0436-x
PMID:15375639
Abstract

Gold nanoparticles of 30 nm diameter bound to cell-surface receptor major histocompatibility complex glycoproteins (MHCI and MHCII), interleukin-2 receptor alpha subunit (IL-2Ralpha), very late antigen-4 (VLA-4) integrin, transferrin receptor, and the receptor-type protein tyrosin phosphatase CD45 are shown by the patch-clamp technique to selectively modulate binding characteristics of Pi(2) toxin, an efficient blocker of K(v)1.3 channels. After correlating the electrophysiological data with those on the underlying receptor clusters obtained by simultaneously conducted flow cytometric energy transfer measurements, the modulation was proved to be sensitive to the density and size of the receptor clusters, and to the locations of the receptors as well. Based on the observation that engagement of MHCII by a monoclonal antibody down-regulates channel current and based on the close nanometer-scale proximity of the MHCI and MHCII glycoproteins, an analogous experiment was carried out when gold nanoparticles bound to MHCI delayed down-regulation of the K(v)1.3 current initiated by ligation of MHCII. Localization of K(v)1.3 channels in the nanometer-scale vicinity of the MHC-containing lipid rafts is demonstrated for the first time. A method is proposed for detecting receptor-channel or receptor-receptor proximity by observing nanoparticle-induced increase in relaxation times following concentration jumps of ligands binding to channels or to receptors capable of regulating channel currents.

摘要

采用膜片钳技术显示,直径为30纳米的金纳米颗粒与细胞表面受体主要组织相容性复合体糖蛋白(MHCI和MHCII)、白细胞介素-2受体α亚基(IL-2Rα)、极迟抗原-4(VLA-4)整合素、转铁蛋白受体以及受体型蛋白酪氨酸磷酸酶CD45结合后,可选择性调节K(v)1.3通道的有效阻滞剂Pi(2)毒素的结合特性。在将电生理数据与通过同时进行的流式细胞术能量转移测量获得的基础受体簇数据相关联后,证明这种调节对受体簇的密度和大小以及受体的位置均敏感。基于单克隆抗体与MHCII结合会下调通道电流这一观察结果,以及基于MHCI和MHCII糖蛋白在纳米尺度上的紧密接近性,当与MHCI结合的金纳米颗粒延迟由MHCII连接引发的K(v)1.3电流下调时,进行了类似实验。首次证明了K(v)1.3通道在含MHC的脂筏纳米尺度附近的定位。提出了一种通过观察配体与能够调节通道电流的通道或受体结合浓度跃变后纳米颗粒诱导的弛豫时间增加来检测受体-通道或受体-受体接近性的方法。

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本文引用的文献

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Two-dimensional receptor patterns in the plasma membrane of cells. A critical evaluation of their identification, origin and information content.细胞质膜中的二维受体模式。对其识别、起源和信息内容的批判性评估。
Biophys Chem. 1999 Dec 13;82(2-3):99-108. doi: 10.1016/s0301-4622(99)00109-x.
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Localization of ion channels to lipid Raft domains within the cardiovascular system.离子通道在心血管系统内脂质筏结构域中的定位。
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Dynamic, yet structured: The cell membrane three decades after the Singer-Nicolson model.
动态而有序:辛格-尼科尔森模型提出三十年后的细胞膜
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Ceramide inhibits the potassium channel Kv1.3 by the formation of membrane platforms.神经酰胺通过形成膜平台来抑制钾通道Kv1.3。
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T cell receptor can be recruited to a subset of plasma membrane rafts, independently of cell signaling and attendantly to raft clustering.T细胞受体可被招募至质膜筏的一个亚群,与细胞信号传导无关且伴随筏的聚集。
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GPI-microdomains (membrane rafts) and signaling of the multi-chain interleukin-2 receptor in human lymphoma/leukemia T cell lines.糖基磷脂酰肌醇微区(膜筏)与人淋巴瘤/白血病T细胞系中多链白细胞介素-2受体的信号传导
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