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荧光标记的蛋白激酶B的p21激活激酶结合结构域和PH结构域在小鼠中性粒细胞趋化过程中的表达与转位

Expression and translocation of fluorescent-tagged p21-activated kinase-binding domain and PH domain of protein kinase B during murine neutrophil chemotaxis.

作者信息

Magalhães Marco A O, Zhu Fei, Sarantis Helen, Gray-Owen Scott D, Ellen Richard P, Glogauer Michael

机构信息

CIHR Group in Matrix Dynamics and Dental Research Institute, Faculty of Dentistry, University of Toronto, 241 Fitzgerald Building, 150 College Street, Toronto, Canada M5S 3E2.

出版信息

J Leukoc Biol. 2007 Sep;82(3):559-66. doi: 10.1189/jlb.0207126. Epub 2007 May 29.

Abstract

Neutrophils are key cells of the innate immune system; they are terminally differentiated and therefore difficult to genetically manipulate and study in vitro. In the present study, we describe a protocol to transiently express two fluorescent markers, the PH domain of protein kinase B fused to red fluorescent protein and the p21-activated kinase-binding domain fused to a yellow fluorescent protein, in primary neutrophils. Using this approach, we are able to achieve a transfection efficiency of approximately 30%. The expression of the transfected probes occurred within 2 h and allowed for real-time monitoring of intermediates in key neutrophil activation pathways at the leading edge of migrating cells. We describe here a transfection protocol for primary neutrophils, which preserves fMLP-mediated cell polarization and cytoskeleton reorganization with simultaneous accumulation of PI-3K products and active Rac at the leading edge. The visualization and analysis of transfected fluorescent markers in primary neutrophils are a powerful technique to monitor chemotaxis signaling pathways in real time.

摘要

中性粒细胞是先天性免疫系统的关键细胞;它们是终末分化细胞,因此难以进行基因操作和体外研究。在本研究中,我们描述了一种在原代中性粒细胞中瞬时表达两种荧光标记物的方法,即与红色荧光蛋白融合的蛋白激酶B的PH结构域和与黄色荧光蛋白融合的p21激活激酶结合结构域。使用这种方法,我们能够实现约30%的转染效率。转染探针的表达在2小时内发生,并允许在迁移细胞前沿实时监测中性粒细胞关键激活途径中的中间体。我们在此描述了一种原代中性粒细胞的转染方案,该方案保留了fMLP介导的细胞极化和细胞骨架重组,同时PI-3K产物和活性Rac在前缘积累。原代中性粒细胞中转染荧光标记物的可视化和分析是实时监测趋化信号通路的强大技术。

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