# GLP1R neurons in the subfornical organ and integration of thirst and satiety cues

> **NIH NIH K01** · YALE UNIVERSITY · 2020 · $156,568

## Abstract

Project Summary
Discoveries made in sensory biology not only shape the way we live, but also have important repercussions for
human health. My long-term career goal is to better understand how environmental cues are detected and
encoded in the periphery, and communicated with the brain to control physiology and behavior in health and
disease. My current objective described in this proposal is to investigate how GLP-1 communicates centrally
with the subfornical organ to control water intake and body fluid homeostasis. Maintaining fluid homeostasis is
crucial for health and disease. Elevation of circulatory osmolarity by high glucose causes polydipsia in diabetic
patients. Incretin therapies that involve mimicry or stabilization of glucagon-like peptide 1 (GLP-1) provide a
strategy for treatment of type 2 diabetes. As an incretin, GLP-1 not only controls insulin release and feeding
behavior but also regulates blood pressure, renal excretion of sodium, and fluid intake to coordinately promote
digestion at a systematic level after meal. Intriguingly, acute GLP-1 administration elicits hypodipsia and
effectively reduces water consumption in both healthy subjects and diabetic patients, suggesting an alternative
strategy for alleviating polydipsia in diabetic patients. Among the many sites that express the receptor for GLP-
1 (GLP1R), the subfornical organ is a major brain center that controls water intake and fluid homeostasis. My
central hypothesis is that SFO GLP1R neurons integrate satiety signals after meal to control fluid intake
through specific signaling cascades and central neural circuits. I will test this hypothesis through three specific
aims: to determine the effect of SFO GLP1R neuron stimulation on fluid intake (Specific Aim 1), to decipher
GLP1R signaling pathways in these cells (Specific Aim 2), and to scrutinize their anatomical and functional
connectivity (Specific Aim 3). For the training necessary for Specific Aim 2, I will continue to greatly benefit
from the guidance of my mentor Prof. Liberles, who has incredible knowledge and understanding in GPCR
signaling pathways. To carry out Specific Aim 1 and 3, I will also need to broaden my knowledge and skills to
include mouse behavior and neurocircuit mapping, such as stereotaxic brain surgeries, brain slice
electrophysiology, and chemogenetics. Such knowledge and skills will be obtained from training with my co-
mentor, Prof. Bradford Lowell. I have received tremendous guidance from Prof. Lowell and his lab members in
the past, with generation of Glp1r-ires-Cre mice and brain stereotaxic injection. I will continue to learn brain
slice recording, rabies virus-based tracing, channelrhodopsin-assisted circuit mapping (CRACM), and
DREADD-involved behavioral experiments under the guidance of Prof. Lowell. Particularly regarding the
anatomical tracing of SFO GLP1R neurons (Specific Aim 3) that requires very extensive knowledge of brain
anatomy, I will collaborate with Prof. Clifford Saper, ...

## Key facts

- **NIH application ID:** 9893863
- **Project number:** 5K01DK113047-05
- **Recipient organization:** YALE UNIVERSITY
- **Principal Investigator:** RUI CHANG
- **Activity code:** K01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $156,568
- **Award type:** 5
- **Project period:** 2017-04-01 → 2021-03-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/9893863

## Citation

> US National Institutes of Health, RePORTER application 9893863, GLP1R neurons in the subfornical organ and integration of thirst and satiety cues (5K01DK113047-05). Retrieved via AI Analytics 2026-05-23 from https://api.ai-analytics.org/grant/nih/9893863. Licensed CC0.

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