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An Improved Genetically Encoded Fluorescent cAMP Indicator for Sensitive cAMP Imaging and Fast Drug Screening

Wenfeng Liu, Chang Liu, Pei‐Gen Ren, Jun Chu, Liang Wang

2022Frontiers in Pharmacology22 citationsDOIOpen Access PDF

Abstract

Cyclic adenosine 3′,5′-monophosphate (cAMP) is an important intracellular second messenger molecule downstream of many G protein-coupled receptors (GPCRs). Fluorescence imaging with bright and sensitive cAMP indicators allows not only dissecting the spatiotemporal dynamics of intracellular cAMP, but also high-content screening of compounds against GPCRs. We previously reported the high-performance circularly permuted GFP (cpGFP)-based cAMP indicator G-Flamp1. Here, we developed improved G-Flamp1 variants G-Flamp2 and G-Flamp2b. Compared to G-Flamp1, G-Flamp2 exhibited increased baseline fluorescence (1.6-fold) and larger fluorescence change (ΔF/F 0 ) (1,300% vs. 1,100%) in HEK293T cells, while G-Flamp2b showed increased baseline fluorescence (3.1-fold) and smaller ΔF/F 0 (400% vs. 1,100%). Furthermore, live cell imaging of mitochondrial matrix–targeted G-Flamp2 confirmed cytosolic cAMP was able to enter the mitochondrial matrix. G-Flamp2 imaging also showed that adipose tissue extract activated the Gi protein-coupled orphan GPCR GPR50 in HEK293T cells. Taken together, our results showed that the high-performance of G-Flamp2 would facilitate sensitive intracellular cAMP imaging and activity measurement of compounds targeting GPCR-cAMP signaling pathway during early drug development.

Topics & Concepts

G protein-coupled receptorIntracellularHEK 293 cellsSecond messenger systemCyclic adenosine monophosphateCytosolGreen fluorescent proteinFluorescenceCell biologyDrug discoveryLive cell imagingAdenosineReceptorFluorescence-lifetime imaging microscopyChemistrySignal transductionBiologyBiochemistryCellEnzymeGenePhysicsQuantum mechanicsReceptor Mechanisms and SignalingPhosphodiesterase function and regulationNeuropeptides and Animal Physiology
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