Neuroscience

Stimulation of VTA dopamine inputs to LH upregulates orexin neuronal activity in a DRD2-dependent manner

Masaya Harada
Laia Serratosa Capdevila
Maria Wilhelm
Denis Burdakov
Tommaso Patriarchi author has email address

Institute of Pharmacology and Toxicology, University of Zürich, Zürich, Switzerland;
Neuroscience Center Zürich, University and ETH Zürich, Zürich, Switzerland;
Department of Health Sciences and Technology, ETH Zürich, Zürich, Switzerland

https://doi.org/10.7554/eLife.90158.2

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Figures and data

A. Preparation for opto-Pavlovian task combined with dLight recordings in the NAc. Scale bar; 1mm. White dashed lines indicate fiber tracts. B. Schematic for opto-Pavlovian task. One cue was associated with the laser delivery while the other cue was not. C. dLight recordings in the NAc of a representative mouse around the laser-paired cue presentation at session (left) and grouped data (middle). dLight recordings of non laser-paired trials are also shown (right) at session 1. D. dLight signals at session 1 during laser stimulation. The signals during non-laser trials are shown also. E. The signals of a representative mice around laser-paired cue (left), grouped data (middle) and signals around non-laser paired cue presentation (right) at session 10. F. Area under the curve (AUC) of dLight signal in the NAc around the cue presentations (0-1.5 seconds) across sessions. Laser-paired cue triggered bigger transient than non-laser paired cue. 2-way repeated measures ANOVA. Session, F_{9, 27} = 3.339, P=0.0072. Cue, F_{1, 3} = 3.997, P=0.139. Interaction, F_{9, 27} = 5.287, P=0.0003. Tukey’s multiple comparison, *p<0.05, **p<0.01,***p<0.001 and ***p<0.0001. n=4 mice.

A. Schematic for the omission sessions. Two thirds of laser associated cue was followed by the laser stimulation while the other one third of the laser associated cue failed to trigger the laser stimulation. B.dLight recordings of a representative mouse during omission sessions. dLight signal around the laser-paired cue presentation is shown here. White asterisks indicate omission trials, while in the other trials, the laser stimulation was delivered. D. dLight recordings in the NAc during stimulation trials and during omission trials(C). A dip of dLight signals was observed. One sample t test; t=4.176, df=3.P= 0.0250. n=4 mice.

A. Schematic for the dLight recording in the LH while stimulating dopamine neurons in the VTA (left). Coronal image of the LH of a mouse infected with AAV-hSyn-DIO-Chrimson-tdTomato in the VTA and AAV-hSyn-dLight1.3b in the LH (right). White dashed lines indicate fiber tracts. Scale bar; 1mm. B. dLight signal in the LH during dopaminergic stimulation in the VTA at several number of pulses (20Hz, 10ms duration for each pulse). C. dLight recordings during the laser-paired cue presentation of a representative mouse at session 1. D. dLight recordings around the laser-paired cue presentation (left) and non-laser-paired cue presentation (right) at session 1. E. dLight recordings during the laser-paired cue presentation of a representative mouse at session 10. F. dLight recordings around the laser-paired cue presentation (left) and non-laser-paired cue presentation (right) at session 10. G. Area under the curve (AUC) of dLight signal in the LH around the cue presentations (0-1.5 seconds) across sessions. Laser-paired cue triggered bigger transient than non-laser paired cue. 2-way repeated measures ANOVA. Session, F_{9, 27} = 3.814, P=0.0033. Cue, F_{1, 3} = 5.818, P=0.0948. Interaction, F_{9, 27} = 3.923, P=0.0027. Tukey’s multiple comparison, *p<0.05, **p<0.01,***p<0.001 and ***p<0.0001. H. dLight recordings in the LH during omission trials. A dip of dLight signals was observed. One sample t test; t=3.193, df=3.P= 0.0496. n=4 mice.

A. Schematic of the preparation for opto-Pavlovian task combined with orexin promoter GCaMP recordings in the LH. B. Coronal image of a mouse brain slice infected with AAV-hSyn-DIO-ChrimsonR-tdTomato in the VTA and AAV1-hOX-GcaMP6S in the LH (left. Scale Bar; 1mm). White dashed lines indicate fiber tracts. Zoom of infected LH with AAV1-hOX-GcaMP6s and co-localization orexin IR and GcaMP6s (right. Scale Bars; 50 μm). C. Orexin promoter GcaMP recordings in the LH of a representative mouse around the laser-paired cue presentation at session 1 (left), grouped data (middle) and recordings during non laser-paired trial (right). D. Orexin promoter GcaMP recordings in the LH of a representative mouse around the laser-paired cue presentation at session 10 (left), grouped data (middle) and recordings during non laser trial (right). E. Area under the curve (AUC) of hOX-GcaMP signal in the LH around the cue presentations (0-1.5 seconds) across sessions. Laser-paired cue triggered bigger transient than non-laser paired cue. 2-way repeated measures ANOVA. Session, F_{9, 27} = 4.438, P=0.0012. Cue, F_{1, 3} = 25.41, P=0.0151. Interaction, F_{9, 27} = 4.125, P=0.0020. Tukey’s multiple comparison, *p<0.05, **p<0.01,***p<0.001 and ***p<0.0001. F. Orexin promoter GCaMP recordings during stimulation trials (left) and omission trials (middle and right). AUC around the omission was higher than baseline. One sample t test; t=4.693, df=3.P= 0.0183. n=4 mice.

A. Schematic for the orexin promoter GCaMP recording in the LH while stimulating dopamine terminals in the LH. B. Orexin promoter GCaMP signals of a representative mouse. Recordings were performed while mice were freely moving (top) and anesthetized with isoflurane (bottom). Red bars indicate the stimulation. (20Hz, 100 pulses, 10 ms duration). C. Orexin promoter GCaMP signals around the stimulation of dopamine terminals in the LH while animals were freely moving (left) and anesthetized (right). D. AUC at 0 to 20 seconds was not significantly different between freely moving and anesthetized conditions. Paired t test, t=1.923 df=2.P= 0.1944. n=3 mice.E. In freely moving condition, recordings were performed after mice received the intraperitoneal injection of vehicle (left), SCH 23390 (1mg/kg, middle), and raclopride (1mg/kg, right). F. Area under the curve (AUC) at 0-5 seconds. Black line indicates the mean for each condition and grey lines show individual mice. The administration of raclopride decreased the AUC significantly while SCH 23390 did not change the AUC. One-way analysis of variance; F (3, 6) = 5.305, P=0.04. Tukey’s multiple comparison test. vehicle vs. SCH 23390; P= 0.8145. vehicle vs. raclopride; P= 0.0476. n=4 mice.

dLight recordings in the NAc during non-laser-paired cue delivery at session 1 (left) and 10(right).

A.
dLight recordings in the NAc (top) and LH (bottom) during optical stimulation of VTA dopamine neurons. B. Derivative of panel A. C. quantification of zero-crossing point in panel B after the initiation of laser stimulation. Unpaired t-test; t=21.69, df=6. p<0.0001. D. dLight recordings in the NAc (top) and LH (bottom) during omission trials. E. Derivative of panel D. F. Quantification of first (top, point A) and second (bottom, point B) zero-crossing points after the initiation of the cue in panel E. Top, unpaired t-test. T=2.920, df=6. p=0.0266. bottom, unpaired t- test. T=2.614, df=6. p=0.0399. Note that panels A and D are shown in the main figures also. They are displayed for comparison purposes.

Orexin-promoter GCaMP recording (left) and dLight recording during stimulation at session 1.

Individual traces for Figure 5E.

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