Dataset DOI: 10.5061/dryad.7wm37pw71

PS & ICC Ca²⁺ Imaging and Electrophysiology Dataset

This dataset contains summary data analyses of calcium imaging, gene expression, and electrophysiological experiments in interstitial cells of Cajal (ICC) and pyloric sphincter (PS) muscles in mice. All data files are provided as GraphPad Prism (.prism) files. Supplemental movies illustrating calcium imaging experiments are also included.

Prism Data Files

Fig_1ICC_Ca2__imaging_in_the_whole_murine_stomach._Calcium_waves_freq_and_propagation.prism

Calcium waves across the whole stomach (corpus to antrum) in ICC GCaMP mice. ST maps were generated using Fiji/ImageJ; duration and propagation velocity of each wave were measured and analyzed with GraphPad Prism 10.

Fig_2-ICC_Ca2__signals_pyloric_sphincter._Frequency_and_duration_of_PS_imaging.prism

ICC cells in the PS were imaged to measure calcium transients, and the frequency and duration were quantified using Fiji/ImageJ and normalized to control wells before analysis with GraphPad Prism.

Fig_3-Effects_of_Ca2_-free_solution_and_SERCA_inhibitors_on_the_spatio-temporal_(ST)_analysis_of_Ca2__transients_in_the_PS.prism

Calcium activation signals in PS ICC were imaged. Spatio-temporal (ST) maps were generated using Fiji/ImageJ, and the frequency of each wave was measured and analyzed with GraphPad Prism.

Fig_4-Effects_of_T-type_Ca2__channel_blocker_(Z944)on_the_spatio-temporal(ST)_analysis_of_Ca2__transients_in_the_PS..prism

PS ICC cells were treated with the T-type Ca²⁺ channel blocker Z944. Calcium transients were analyzed using spatio-temporal (ST) maps generated with Fiji/ImageJ, normalized to control conditions, and the frequency, duration, and propagation velocity of each wave were quantified using GraphPad Prism.

Fig_5_The_quantitative_transcriptional_analysis_of_possible_Ca2__influx_gene_candidates_and_immunohistochemistry_of_ICC_and_ANO1_in_the_PS.__.prism

Transcriptional analysis of Ano1 and voltage-gated Ca²⁺ channel genes was performed in isolated ICC of the PS. Expression of c-kit and ANO1 was confirmed by immunohistochemistry.

Fig_6-Fig_6._Effects_of_Ani9_on_mechanical_tone_and_membrane_potential_of_the_PS_muscle_strips..prism

PS muscle strips were treated with Ani9 to assess contractile tone and resting membrane potential. Contractile responses, including AUC and resting membrane potential, were measured. Additionally, in the presence of Ani9, electrically evoked contractions were recorded, and both the on-response and post-stimulus contraction (PSC) were quantified. All data were analyzed using GraphPad Prism.

 
Fig_7-LNNA_Ani9_and_atropine_on___off_response-of_muscle_contraction.prism

Ongoing contractile activity of PS muscle strips was recorded in the presence of TTX. Additionally, contractile responses and EFS under LNNA + Ani9 and LNNA + atropine treatments were quantified. The area under the curve (AUC) of these responses was analyzed using Clampfit, and all data were further analyzed with GraphPad Prism.

Supplemental Movies

movie1.avi

Supplemental Movie 1. Use of Ca²⁺ imaging to monitor slow wave propagation in mouse stomach.

Calcium imaging to monitor slow wave propagation in mouse stomach was performed, fluorescence intensity measured across stomach regions, and data are included for visualization.

movie2.avi

Supplemental Movie 2. Ca²⁺ transients in ICC within the pyloric sphincter (PS). 

Calcium transients in ICC within the pyloric sphincter were recorded, fluorescence intensity measured across ICC clusters, and data are included for visualization.