Publication | Open Access
Fluorescence-activated cell sorting to reveal the cell origin of radioligand binding
48
Citations
48
References
2019
Year
Fluorescence-activated CellMolecular BiologyCellular PhysiologyNeuroinflammationPositron Emission TomographyAlzheimer's DiseaseCell InteractionMolecular SortingNeurologyBrain PathologyNeuropathologyNeuroimmunologyCell SignalingMolecular ImagingBiochemistryCell TraffickingBrain-immune InteractionNeuroimagingTspo BindingCerebral Blood FlowPharmacologyCell BiologyMicroglial Tspo BindingNeuroimaging BiomarkersSignal TransductionNeurophysiologyNatural SciencesRadioligand BindingNeuroscienceMedicineCell Origin
Many studies have explored the role of TSPO (18 kDa translocator protein) as a marker of neuroinflammation using single-photon emission computed tomography (SPECT) or positron emission tomography (PET). In vivo imaging does not allow to determine the cells in which TSPO is altered. We propose a methodology based on fluorescence-activated cell sorting to sort different cell types of radioligand-treated tissues. We compared left/right hippocampus of rats in response to a unilateral injection of lipopolysaccharide (LPS), ciliary neurotrophic factor (CNTF) or saline. We finally applied this methodology in human samples (Alzheimer's disease patients and controls). Our data show that the pattern of TSPO overexpression differs across animal models of acute neuroinflammation. LPS induces a microglial expansion and an increase in microglial TSPO binding. CNTF is associated with an increase in TSPO binding in microglia and astrocytes in association with an increase in the number of microglial binding sites per cell. In humans, we show that the increase in CLINDE binding in Alzheimer's disease concerns microglia and astrocytes in the presence of a microglial expansion. Thus, the cellular basis of TSPO overexpression is condition dependent, and alterations in TSPO binding found in PET/SPECT imaging studies cannot be attributed to particular cell types indiscriminately.
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