# Live imaging analyses of the mechanisms required for coordinated urinary tract peristalsis in lower-order and higher-order mammalian species

> **NIH NIH R21** · WEILL MEDICAL COLL OF CORNELL UNIV · 2020 · $211,875

## Abstract

ABSTRACT
Proximal-to-distal peristaltic contractions of the upper urinary tract (UUT) smooth muscle coat propel waste
from the kidney to the bladder. Defects in the peristaltic process are highly prevalent and clinically significant.
For example, impaired urine outflow from the kidney causes pressure mediated dilation of renal tissues, or
hydronephrosis. Hydronephrosis is the most commonly observed abnormality in children, detected in 1% of
newborns, and is a leading cause of pediatric kidney failure. The overall goal of this project is to better
understand the normal physiology and pathophysiology of the UUT. Indeed, despite the high morbidity
associated with urinary tract dysfunctions, the mechanisms underlying renal pacemaker activity that triggers
UUT peristalsis have remained elusive. To study this process, we have developed novel live imaging
techniques to record the propagation of electrical and contractile excitation throughout the intact UUT. Results
of our studies have revealed that hyperpolarization activate cation (HCN) channels are highly expressed and
localized to renal pacemaker tissues of the murine UUT. HCN channel inhibition abolishes UUT pacemaker
activity, and results in a loss of coordinated peristalsis. Instead of the proximal-to-distal contractile and
electrical excitation observed in control UUTs, HCN inhibited explants exhibit near-simultaneous electrical
activation throughout the UUT and twitch-like contractile activity. Thus, we have demonstrated ex-vivo that
HCN+ cells of the UUT are renal pacemakers that set the origin and coordinate UUT peristalsis. Moreover, we
have recently discovered that HCN channel expression is conserved to renal pacemaker tissues of the porcine
and human urinary tracts, which share a unique anatomy and physiology. In Aim 1 of this proposal we will use
a novel mouse model of hydronephrosis that lacks HCN+ cells in the UUT. We will use the live imaging
techniques we have developed to determine if loss of HCN+ cells in vivo results in aberrant UUT peristalsis that
underlies hydronephrosis. Aim 1 will also include mechanistic studies to begin to elucidate the transcriptional
networks regulating HCN+ pacemakers. For Aim 2, we have recently developed a novel explant system to
directly visualize the electrical and contractile properties of peristalsis in the porcine UUT. We will use this
explant system to determine if HCN channel conductance is required for coordinated UUT peristalsis in a close
homolog to humans. Results of these studies will provide much needed insight into the mechanisms underlying
normal and aberrant UUT peristalsis in both lower-order and higher-order mammalian species. Long term
translational implications of the studies include the development of novel treatments and diagnostics for
uropathies such as hydronephrosis.

## Key facts

- **NIH application ID:** 9850965
- **Project number:** 5R21DK116171-03
- **Recipient organization:** WEILL MEDICAL COLL OF CORNELL UNIV
- **Principal Investigator:** Romulo Hurtado
- **Activity code:** R21 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $211,875
- **Award type:** 5
- **Project period:** 2018-03-01 → 2024-02-29

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/9850965

## Citation

> US National Institutes of Health, RePORTER application 9850965, Live imaging analyses of the mechanisms required for coordinated urinary tract peristalsis in lower-order and higher-order mammalian species (5R21DK116171-03). Retrieved via AI Analytics 2026-05-22 from https://api.ai-analytics.org/grant/nih/9850965. Licensed CC0.

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