# TRANSCRIPTIONAL DYSREGULATION OF T-TYPE CALCIUM CHANNELS IN CHILDHOOD ABSENCE EPILEPSY

> **NIH NIH F31** · BAYLOR COLLEGE OF MEDICINE · 2022 · $46,752

## Abstract

PROJECT SUMMARY/ABSTRACT
The goal of my research is to identify pathophysiological mechanisms of Childhood Absence Epilepsy (CAE)
using transgenic mouse models. CAE is the most common pediatric epilepsy, and over one-third of cases are
pharmaco-resistant. While clinical absence episodes are non-convulsive, the generalized 3-5 Hz spike-wave
seizures (SWs) are accompanied by partial loss of consciousness and behavioral arrest, occur hundreds of
times per day, and are linked to significant attention and cognitive deficits. This is not a benign disorder.
Electrophysiological evidence in human and mouse models show SWs are generated within the
thalamocortical circuit of the brain, where elevated T-type calcium currents have a well-characterized role in
rebound burst firing activity that is thought to drive CAE seizure activity. Data from several monogenic mouse
models of CAE, beginning with the P/Q-type calcium channel mutant tottering, support the hypothesis that
abnormal synaptic input onto thalamic neurons elevates low threshold T-currents prior to SWs onset. However,
the molecular mechanisms mediating the downstream remodeling of T-channel activity in thalamic neurons are
not yet clearly defined. The experiments proposed in this application will dissect the roles of specific T-channel
isoforms within the thalamocortical circuit that lead to hyperexcitability and spike-wave seizures. I will test three
hypotheses that defective synaptic release due to P/Q-type calcium channel mutations elevate T-currents in
postsynaptic thalamic cells by altering 1) transcription of T-type subunit genes, 2) their splice form ratios,
and/or 3) transcription of auxiliary genes for T-type channels that encode functionally interacting proteins that
regulate T-channel expression. To achieve these goals, I propose the following 2 research aims: 1) Determine
the level and pattern of thalamic Cacna1g and Cacna1h channel isoform expression in Cacna1a mutant model
tottering, and 2) Investigate the role of an established T-channel modifier gene, Stac1, in T-current elevation
and SWs. The first aim will investigate the T-channel isoform expression patterns within identified
thalamocortical circuit neurons and determine whether they have expression ratio abnormalities before and
after seizure onset in tottering mice. The second aim will investigate whether Stac1 contributes to SWs activity,
whether Stac1 deletion modifies thalamic T-channel expression in vivo, and whether deletion of Stac1 will
modify or prevent seizures in tottering mice. In preliminary studies, I have obtained quantitative evidence using
the sensitive, single cell resolution RNAscope in situ hybridization method that mRNA for Cacna1g, the
predominant T-type channel alpha-subunit expressed in thalamic relay nuclei, is elevated in tottering thalamus
in concordance with electrophysiological evidence. I have also identified that deletion of Stac1, a modifier of
surface expression of T-type channel subtype expresse...

## Key facts

- **NIH application ID:** 10448262
- **Project number:** 5F31NS124345-02
- **Recipient organization:** BAYLOR COLLEGE OF MEDICINE
- **Principal Investigator:** SAMANTHA Jane THOMPSON
- **Activity code:** F31 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2022
- **Award amount:** $46,752
- **Award type:** 5
- **Project period:** 2021-07-06 → 2024-07-05

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10448262

## Citation

> US National Institutes of Health, RePORTER application 10448262, TRANSCRIPTIONAL DYSREGULATION OF T-TYPE CALCIUM CHANNELS IN CHILDHOOD ABSENCE EPILEPSY (5F31NS124345-02). Retrieved via AI Analytics 2026-05-23 from https://api.ai-analytics.org/grant/nih/10448262. Licensed CC0.

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