Rapid Fluorescence Lifetime Imaging Reveals That TRPV4 Channels Promote Dysregulation of Neuronal Na+ in Ischemia

被引:19
作者
Meyer, Jan [1 ]
Gerkau, Niklas J. [1 ]
Kafitz, Karl W. [1 ]
Patting, Matthias [2 ]
Jolmes, Fabian [2 ]
Henneberger, Christian [3 ,4 ,5 ]
Rose, Christine R. [1 ]
机构
[1] Heinrich Heine Univ Dusseldorf, Inst Neurobiol, Fac Math & Nat Sci, D-40225 Dusseldorf, Germany
[2] PicoQuant, D-12489 Berlin, Germany
[3] Univ Bonn, Inst Cellular Neurosci, Fac Med, D-53127 Bonn, Germany
[4] German Ctr Neurodegenerat Dis, D-53175 Bonn, Germany
[5] UCL, UCL Queen Sq Inst Neurol, London WC1N 3BG, England
关键词
cell swelling; FLIM; glutamate; hippocampus; sodium; stroke; HEAT-EVOKED ACTIVATION; INTRACELLULAR CHLORIDE; ION-CHANNEL; CA2+; MECHANISMS; TEMPERATURE; PLASTICITY; MICROSCOPY; EDEMA;
D O I
10.1523/JNEUROSCI.0819-21.2021
中图分类号
Q189 [神经科学];
学科分类号
071006 ;
摘要
Fluorescence imaging is an indispensable method for analysis of diverse cellular and molecular processes, enabling, for example, detection of ions, second messengers, or metabolites. Intensity-based approaches, however, are prone to artifacts introduced by changes in fluorophore concentrations. This drawback can be overcome by fluorescence lifetime imaging (FLIM) based on time -correlated single-photon counting. FLIM often necessitates long photon collection times, resulting in strong temporal binning of dynamic processes. Recently, rapidFLIM was introduced, exploiting ultra-low dead-time photodetectors together with rapid electronics. Here, we demonstrate the applicability of rapidFLIM, combined with new and improved correction schemes, for spatiotemporal fluorescence lifetime imaging of low-emission fluorophores in a biological system. Using tissue slices of hippocampi of mice of either sex, loaded with the Na+ indicator ING2, we show that improved rapidFLIM enables quantitative, dynamic imaging of neuronal Na+ signals at a full-frame temporal resolution of 0.5 Hz. Induction of transient chemical ischemia resulted in unexpectedly large Na+ influx, accompanied by considerable cell swelling. Both Na+ loading and cell swelling were dampened on inhibition of TRPV4 channels. Together, rapidFLIM enabled the spatiotemporal visualization and quantification of neuronal Na+ transients at unprecedented speed and independent from changes in cell volume. Moreover, our experiments identified TRPV4 channels as hitherto unappreciated contributors to neuronal Na+ loading on metabolic failure, suggesting this pathway as a possible target to ameliorate excitotoxic damage. Finally, rapidFLIM will allow faster and more sensitive detection of a wide range of dynamic signals with other FLIM probes, most notably those with intrinsic low-photon emission.
引用
收藏
页码:552 / 566
页数:15
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