Single nuclei RNA sequencing of the rat AP and NTS following GDF15 treatment

Reiner, Benjamin C.; Crist, Richard C.; Borner, Tito; Doyle, Robert P.; Hayes, Matthew R.; Jonghe, Bart C. De

doi:10.1016/j.molmet.2021.101422

Cited by 11 publications

(5 citation statements)

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“…Bilateral NAc tissue was punched from frozen brains and nuclei suspensions were prepared, as we described previously (see supplemental methods) [13,30,31].…”

Section: Nuclei Isolation Library Preparation and Sequencingmentioning

confidence: 99%

“…As in our prior description [30], the overrepresentation of cell-type-specific DEGs in GWAS phenotypes canonical pathways, gene ontologies, hallmark gene sets, microRNA targets, and transcription factor targets was determined by comparing cluster-specific DEGs, from all clusters with at least 50 DEGs in either the acute or chronic treatment group, from both treatment groups to GWAS Catalog Molecular and Signatures Database (MsigDB) v7.0 [34] using FUMA [35] (see supplemental methods).…”

Section: Enrichment Analysesmentioning

confidence: 99%

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Single nucleus transcriptomic analysis of rat nucleus accumbens reveals cell type-specific patterns of gene expression associated with volitional morphine intake

et al. 2022

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Opioid exposure is known to cause transcriptomic changes in the nucleus accumbens (NAc). However, no studies to date have investigated cell type-specific transcriptomic changes associated with volitional opioid taking. Here, we use single nucleus RNA sequencing (snRNAseq) to comprehensively characterize cell type-specific alterations of the NAc transcriptome in rats self-administering morphine. One cohort of male Brown Norway rats was injected with acute morphine (10 mg/kg, i.p.) or saline. A second cohort of rats was allowed to self-administer intravenous morphine (1.0 mg/kg/infusion) for 10 consecutive days. Each morphine-experienced rat was paired with a yoked saline control rat. snRNAseq libraries were generated from NAc punches and used to identify cell type-specific gene expression changes associated with volitional morphine taking. We identified 1106 differentially expressed genes (DEGs) in the acute morphine group, compared to 2453 DEGs in the morphine self-administration group, across 27 distinct cell clusters. Importantly, we identified 1329 DEGs that were specific to morphine self-administration. DEGs were identified in novel clusters of astrocytes, oligodendrocytes, and D1R- and D2R-expressing medium spiny neurons in the NAc. Cell type-specific DEGs included Rgs9, Celf5, Oprm1, and Pde10a. Upregulation of Rgs9 and Celf5 in D2R-expressing neurons was validated by RNAscope. Approximately 85% of all oligodendrocyte DEGs, nearly all of which were associated with morphine taking, were identified in two subtypes. Bioinformatic analyses identified cell type-specific upstream regulatory mechanisms of the observed transcriptome alterations and downstream signaling pathways, including both novel and previously identified molecular pathways. These findings show that volitional morphine taking is associated with distinct cell type-specific transcriptomic changes in the rat NAc and highlight specific striatal cell populations and novel molecular substrates that could be targeted to reduce compulsive opioid taking.

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“…Bilateral NAc tissue was punched from frozen brains and nuclei suspensions were prepared, as we described previously (see supplemental methods) [13,30,31].…”

Section: Nuclei Isolation Library Preparation and Sequencingmentioning

confidence: 99%

Section: Enrichment Analysesmentioning

confidence: 99%

Single nucleus transcriptomic analysis of rat nucleus accumbens reveals cell type-specific patterns of gene expression associated with volitional morphine intake

et al. 2022

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“…Bilateral VTA punches were prepared on a cryostat and combined into a single sample. Nuclei were isolated from the samples as described previously 25,26 . Nuclei were processed for the 10x Genomics 3’ gene expression assay (v3.1) and sequenced per manufacturer protocols.…”

Section: Methodsmentioning

confidence: 99%

An endogenous GLP-1 circuit engages VTA GABA neurons to regulate mesolimbic dopamine neurons and attenuate cocaine seeking

Merkel,

Hernandez,

Weir

et al. 2024

Preprint

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Recent studies show that systemic administration of a glucagon-like peptide-1 receptor (GLP-1R) agonist is sufficient to attenuate the reinstatement of cocaine-seeking behavior, an animal model of relapse. However, the neural mechanisms mediating these effects and the role of endogenous central GLP-1 signaling in cocaine seeking remain unknown. Here, we show that voluntary cocaine taking decreased plasma GLP-1 levels in rats and that chemogenetic activation of GLP-1-producing neurons in the nucleus tractus solitarius (NTS) that project to the ventral tegmental area (VTA) decreased cocaine reinstatement. Single nuclei transcriptomics and FISH studies revealed GLP-1Rs are expressed primarily on GABA neurons in the VTA. Usingin vivofiber photometry, we found that the efficacy of a systemic GLP-1R agonist to attenuate cocaine seeking was associated with increased activity of VTA GABA neurons and decreased activity of VTA dopamine neurons. Together, these findings suggest that targeting central GLP-1 circuits may be an effective strategy toward reducing cocaine relapse and highlight a novel functional role of GABAergic GLP-1R-expressing midbrain neurons in drug seeking.

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“…Data from our prior studies were used to phenotype DVC cell populations relevant to this study (NCBI GEO GSE 167981). Briefly, nuclei were isolated from frozen Sprague Dawley AP and NTS punches as previously described [ 32 , 33 ]. Nuclei capture and library preparation was performed at the Children’s Hospital of Philadelphia Center for Applied Genomics using the 10× Genomics Chromium Single Cell 3′ GEM, Library and Gel Bead Kit v3.1.…”

Section: Methodsmentioning

confidence: 99%

GPR-160 Receptor Signaling in the Dorsal Vagal Complex of Male Rats Modulates Meal Microstructure and CART-Mediated Hypophagia

et al. 2023

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The g-protein coupled receptor GPR-160, recently identified as a putative receptor for the cocaine and amphetamine-regulated transcript (CART) peptide, shows abundant expression in the energy-balance control nuclei, including the dorsal vagal complex (DVC). However, its physiological role in the control of food intake has yet to be fully explored. Here, we performed a virally mediated, targeted knockdown (KD) of Gpr160 in the DVC of male rats to evaluate its physiological role in control of feeding. Our results indicate that DVC Gpr160 KD affects meal microstructure. Specifically, DVC Gpr160 KD animals consumed more frequent, but shorter meals during the dark phase and showed decreased caloric intake and duration of meals during the light phase. Cumulatively, however, these bidirectional effects on feeding resulted in no difference in body weight gain. We next tested the role of DVC GPR-160 in mediating the anorexigenic effects of exogenous CART. Our results show that DVC Gpr160 KD partially attenuates CART’s anorexigenic effects. To further characterize Gpr160+ cells in the DVC, we utilized single-nucleus RNA sequencing data to uncover abundant GPR-160 expression in DVC microglia and only minimal expression in neurons. Altogether, our results suggest that DVC CART signaling may be mediated by Gpr160+ microglia, which in turn may be modulating DVC neuronal activity to control food intake.

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Single nuclei RNA sequencing of the rat AP and NTS following GDF15 treatment

Cited by 11 publications

References 50 publications

Single nucleus transcriptomic analysis of rat nucleus accumbens reveals cell type-specific patterns of gene expression associated with volitional morphine intake

Single nucleus transcriptomic analysis of rat nucleus accumbens reveals cell type-specific patterns of gene expression associated with volitional morphine intake

An endogenous GLP-1 circuit engages VTA GABA neurons to regulate mesolimbic dopamine neurons and attenuate cocaine seeking

GPR-160 Receptor Signaling in the Dorsal Vagal Complex of Male Rats Modulates Meal Microstructure and CART-Mediated Hypophagia

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