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光学生物传感器为A431细胞中缓激肽B(2)受体信号传导提供了见解。

Optical biosensor provides insights for bradykinin B(2) receptor signaling in A431 cells.

作者信息

Fang Ye, Li Guangshan Gary, Peng Jinlin

机构信息

Biochemical Technologies, Science and Technology Division, Corning Incorporated, Sullivan Park, Corning, NY 14831, USA.

出版信息

FEBS Lett. 2005 Nov 21;579(28):6365-74. doi: 10.1016/j.febslet.2005.10.019. Epub 2005 Oct 25.

DOI:10.1016/j.febslet.2005.10.019
PMID:16263113
Abstract

The spatial and temporal targeting of proteins or protein assemblies to appropriate sites is crucial to regulate the specificity and efficiency of protein-protein interactions, thus dictating the timing and intensity of cell signaling and responses. The resultant dynamic mass redistribution could be manifested by label free optical biosensor, and lead to a novel and functional optical signature for studying cell signaling. Here we applied this technology, termed as mass redistribution cell assay technology (MRCAT), to study the signaling networks of bradykinin B(2) receptor in A431 cells. Using MRCAT, the spatial and temporal relocation of proteins and protein assemblies mediated by bradykinin was quantitatively monitored in microplate format and in live cells. The saturability to bradykinin, together with the specific and dose-dependent inhibition by a B(2) specific antagonist HOE140, suggested that the optical signature is a direct result of B(2) receptor activation. The sensitivity of the optical signature to cholesterol depletion by methyl-beta-cyclodextrin argued that B(2) receptor signaling is dependent on the integrity of lipid rafts; disruption of these microdomains hinders the B(2) signaling. Modulations of several important intracellular targets with specific inhibitors suggested that B(2) receptor activation results in signaling via at least dual pathways - G(s)- and G(q)-mediated signaling. Remarkably, the two signaling pathways counter-regulate each other. Several critical downstream targets including protein kinase C, protein kinase A, and epidermal growth factor receptor had been identified to involve in B(2) signaling. The roles of endocytosis and cytoskeleton modulation in B(2) signaling were also demonstrated.

摘要

蛋白质或蛋白质组装体在空间和时间上靶向至合适位点对于调节蛋白质-蛋白质相互作用的特异性和效率至关重要,从而决定细胞信号传导和反应的时机及强度。由此产生的动态质量再分布可通过无标记光学生物传感器得以体现,并产生一种用于研究细胞信号传导的新型功能性光学信号。在此,我们应用这项被称为质量再分布细胞分析技术(MRCAT)的技术来研究缓激肽B(2)受体在A431细胞中的信号网络。利用MRCAT,以微孔板形式并在活细胞中对缓激肽介导的蛋白质和蛋白质组装体的时空重新定位进行了定量监测。对缓激肽的饱和性,以及B(2)特异性拮抗剂HOE140的特异性和剂量依赖性抑制作用,表明该光学信号是B(2)受体激活的直接结果。光学信号对甲基-β-环糊精导致的胆固醇耗竭的敏感性表明,B(2)受体信号传导依赖于脂筏的完整性;这些微结构域的破坏会阻碍B(2)信号传导。用特异性抑制剂对几个重要的细胞内靶点进行调节表明,B(2)受体激活至少通过两条途径导致信号传导——G(s)介导的信号传导和G(q)介导的信号传导。值得注意的是,这两条信号传导途径相互拮抗。已确定包括蛋白激酶C、蛋白激酶A和表皮生长因子受体在内的几个关键下游靶点参与B(2)信号传导。还证明了内吞作用和细胞骨架调节在B(2)信号传导中的作用。

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