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本文引用的文献

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Isoform-specific subcellular localization and function of protein kinase A identified by mosaic imaging of mouse brain.通过小鼠大脑的镶嵌成像鉴定蛋白激酶A的亚型特异性亚细胞定位和功能。
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Exploring cells with targeted biosensors.使用靶向生物传感器探索细胞。
J Gen Physiol. 2017 Jan;149(1):1-36. doi: 10.1085/jgp.201611654. Epub 2016 Dec 27.
3
Untangling ciliary access and enrichment of two rhodopsin-like receptors using quantitative fluorescence microscopy reveals cell-specific sorting pathways.利用定量荧光显微镜解析纤毛通路及两种视紫红质样受体的富集揭示细胞特异性分选途径。
Mol Biol Cell. 2017 Feb 15;28(4):554-566. doi: 10.1091/mbc.E16-07-0549. Epub 2016 Dec 14.
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Five colour variants of bright luminescent protein for real-time multicolour bioimaging.五种明亮荧光蛋白变体,可用于实时多色生物成像。
Nat Commun. 2016 Dec 14;7:13718. doi: 10.1038/ncomms13718.
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Navigating challenges in the application of superresolution microscopy.应对超分辨率显微镜应用中的挑战。
J Cell Biol. 2017 Jan 2;216(1):53-63. doi: 10.1083/jcb.201610011. Epub 2016 Dec 5.
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The Growing and Glowing Toolbox of Fluorescent and Photoactive Proteins.荧光蛋白和光活性蛋白的不断发展与功能多样的工具库
Trends Biochem Sci. 2017 Feb;42(2):111-129. doi: 10.1016/j.tibs.2016.09.010. Epub 2016 Nov 1.
7
A plasma membrane microdomain compartmentalizes ephrin-generated cAMP signals to prune developing retinal axon arbors.质膜微域将 Ephrin 产生的 cAMP 信号分隔开,以修剪发育中的视网膜轴突树突。
Nat Commun. 2016 Oct 3;7:12896. doi: 10.1038/ncomms12896.
8
The Popeye Domain Containing Genes and cAMP Signaling.含大力水手结构域的基因与环磷酸腺苷信号传导
J Cardiovasc Dev Dis. 2014 May 21;1(1):121-133. doi: 10.3390/jcdd1010121.
9
Nontrivial Effect of the Color-Exchange of a Donor/Acceptor Pair in the Engineering of Förster Resonance Energy Transfer (FRET)-Based Indicators.供体/受体对的颜色交换在基于荧光共振能量转移(FRET)的指示剂工程中的重要作用。
ACS Chem Biol. 2016 Jul 15;11(7):1816-22. doi: 10.1021/acschembio.6b00221. Epub 2016 Jun 1.
10
Intracellular tortuosity underlies slow cAMP diffusion in adult ventricular myocytes.细胞内迂曲度是成年心室肌细胞中cAMP缓慢扩散的基础。
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利用光学方法研究环磷酸腺苷信号传导。

Interrogating cyclic AMP signaling using optical approaches.

作者信息

Jiang Jason Y, Falcone Jeffrey L, Curci Silvana, Hofer Aldebaran M

机构信息

VA Boston Healthcare System and the Dept. of Surgery, Brigham & Women's Hospital and Harvard Medical School, 1400 VFW PKW, West Roxbury, MA 02132, USA.

VA Boston Healthcare System and the Dept. of Surgery, Brigham & Women's Hospital and Harvard Medical School, 1400 VFW PKW, West Roxbury, MA 02132, USA.

出版信息

Cell Calcium. 2017 Jun;64:47-56. doi: 10.1016/j.ceca.2017.02.010. Epub 2017 Mar 1.

DOI:10.1016/j.ceca.2017.02.010
PMID:28274483
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5457393/
Abstract

Optical reporters for cAMP represent a fundamental advancement in our ability to investigate the dynamics of cAMP signaling. These fluorescent sensors can measure changes in cAMP in single cells or in microdomains within cells as opposed to whole populations of cells required for other methods of measuring cAMP. The first optical cAMP reporters were FRET-based sensors utilizing dissociation of purified regulatory and catalytic subunits of PKA, introduced by Roger Tsien in the early 1990s. The utility of these sensors was vastly improved by creating genetically encoded versions that could be introduced into cells with transfection, the first of which was published in the year 2000. Subsequently, improved sensors have been developed using different cAMP binding platforms, optimized fluorescent proteins, and targeting motifs that localize to specific microdomains. The most common sensors in use today are FRET-based sensors designed around an Epac backbone. These rely on the significant conformational changes in Epac when it binds cAMP, altering the signal between FRET pairs flanking Epac. Several other strategies for optically interrogating cAMP have been developed, including fluorescent translocation reporters, dimerization-dependent FP based biosensors, BRET (bioluminescence resonance energy transfer)-based sensors, non-FRET single wavelength reporters, and sensors based on bacterial cAMP-binding domains. Other newly described mammalian cAMP-binding proteins such as Popdc and CRIS may someday be exploited in sensor design. With the proliferation of engineered fluorescent proteins and the abundance of cAMP binding targets in nature, the field of optical reporters for cAMP should continue to see rapid refinement in the coming years.

摘要

用于环磷酸腺苷(cAMP)的光学报告分子代表了我们在研究cAMP信号动态能力方面的一项重大进展。这些荧光传感器可以测量单个细胞或细胞内微区中cAMP的变化,这与其他测量cAMP的方法所需要的整个细胞群体不同。第一代光学cAMP报告分子是基于荧光共振能量转移(FRET)的传感器,利用蛋白激酶A(PKA)纯化的调节亚基和催化亚基的解离,由钱永健(Roger Tsien)在20世纪90年代初引入。通过创建可以通过转染引入细胞的基因编码版本,这些传感器的实用性得到了极大提高,其中第一个于2000年发表。随后,使用不同的cAMP结合平台、优化的荧光蛋白和定位于特定微区的靶向基序,开发出了改进的传感器。如今使用最普遍的传感器是围绕交换蛋白直接激活因子(Epac)骨架设计的基于FRET的传感器。这些传感器依赖于Epac结合cAMP时显著的构象变化,改变了位于Epac两侧的FRET对之间的信号。还开发了其他几种光学检测cAMP的策略,包括荧光易位报告分子、基于二聚化依赖荧光蛋白的生物传感器、基于生物发光共振能量转移(BRET)的传感器、非FRET单波长报告分子以及基于细菌cAMP结合结构域的传感器。其他新描述的哺乳动物cAMP结合蛋白,如Popdc和CRIS,也许有一天会被用于传感器设计。随着工程荧光蛋白的大量涌现以及自然界中cAMP结合靶点的丰富,cAMP光学报告分子领域在未来几年应该会继续快速发展。