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一种改进的Akt报告基因揭示了细胞内和细胞间的信号转导异质性及振荡。

An improved Akt reporter reveals intra- and inter-cellular heterogeneity and oscillations in signal transduction.

作者信息

Norris Dougall M, Yang Pengyi, Krycer James R, Fazakerley Daniel J, James David E, Burchfield James G

机构信息

Charles Perkins Centre, School of Life and Environmental Sciences, The University of Sydney, Sydney, NSW 2006, Australia.

Charles Perkins Centre, School of Mathematics and Statistics, The University of Sydney, Sydney, NSW 2006, Australia.

出版信息

J Cell Sci. 2017 Aug 15;130(16):2757-2766. doi: 10.1242/jcs.205369. Epub 2017 Jun 29.

DOI:10.1242/jcs.205369
PMID:28663386
Abstract

Akt is a key node in a range of signal transduction cascades and play a critical role in diseases such as cancer and diabetes. Fluorescently-tagged Akt reporters have been used to discern Akt localisation, yet it has not been clear how well these tools recapitulate the behaviour of endogenous Akt proteins. Here, we observed that fusion of eGFP to Akt2 impaired both its insulin-stimulated plasma membrane recruitment and its phosphorylation. Endogenous-like responses were restored by replacing eGFP with TagRFP-T. The improved response magnitude and sensitivity afforded by TagRFP-T-Akt2 over eGFP-Akt2 enabled monitoring of signalling outcomes in single cells at physiological doses of insulin with subcellular resolution and revealed two previously unreported features of Akt biology. In 3T3-L1 adipocytes, stimulation with insulin resulted in recruitment of Akt2 to the plasma membrane in a polarised fashion. Additionally, we observed oscillations in plasma membrane localised Akt2 in the presence of insulin with a consistent periodicity of 2 min. Our studies highlight the importance of fluorophore choice when generating reporter constructs and shed light on new Akt signalling responses that may encode complex signalling information.This article has an associated First Person interview with the first author of the paper.

摘要

Akt是一系列信号转导级联反应中的关键节点,在癌症和糖尿病等疾病中发挥着关键作用。荧光标记的Akt报告基因已被用于识别Akt的定位,但这些工具在多大程度上能够重现内源性Akt蛋白的行为尚不清楚。在这里,我们观察到eGFP与Akt2融合会损害其胰岛素刺激的质膜募集及其磷酸化。用TagRFP-T取代eGFP可恢复类似内源性的反应。与eGFP-Akt2相比,TagRFP-T-Akt2提供了更高的反应幅度和灵敏度,能够在生理剂量的胰岛素作用下以亚细胞分辨率监测单细胞中的信号转导结果,并揭示了Akt生物学中两个以前未报道的特征。在3T3-L1脂肪细胞中,胰岛素刺激导致Akt2以极化方式募集到质膜。此外,我们观察到在存在胰岛素的情况下,质膜定位的Akt2会以2分钟的一致周期振荡。我们的研究强调了在构建报告基因时选择荧光团的重要性,并揭示了可能编码复杂信号信息的新的Akt信号转导反应。本文配有对该论文第一作者的第一人称访谈。

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