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Unitary TRPA1‐Mediated Ca2+ Influx Events in Primary Cerebral Artery Endothelial Cells

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The sole member of the ankyrin subfamily of transient receptor potential channels, TRPA1, is a Ca 2+ permeable, non‐selective cation channel involved in endothelium‐dependent cerebral artery vasodilation. Total Internal Reflection Fluorescence microscopy (TIRFM) was utilized to investigate the biophysical properties and regulation of TRPA1‐mediated Ca 2+ influx in primary cerebral artery endothelial cells (EC). Rat basilar arteries were cut open and placed intima side down on Matrigel‐coated plates. EC were allowed to proliferate (≤14 days), loaded with Fluo 4‐AM, and imaged in situ using TIRFM. Localized, transient Ca 2+ influx events (mean amplitude (F‐F 0 ) of 0.17±0.02, duration of 0.21±0.03 s, and spatial spread of 2.09±0.29 μm 2 ) were detected at a whole‐cell frequency of 0.04±0.02 Hz (n = 24) under basal conditions. Mean event frequency and duration greatly increased with addition of the TRPA1 agonist allyl isothiocyanate (AITC) (0.23±0.08 Hz, 1.64±0.10 s, n = 25). These increases were attenuated in the presence of the selective TRPA1 antagonist HC‐030031 (0.03±0.02 Hz, 0.65±0.16 s, n = 10 cells). Histogram analysis of AITC‐invoked event amplitudes indicates that these Ca 2+ signals display quantal separation. Similar events were recorded from HEK 293 cells overexpressing TRPA1. Together, these data suggest that quantal, TRPA1‐mediated Ca 2+ influx can be recorded from EC using TIRFM. RO1HL091905.
Title: Unitary TRPA1‐Mediated Ca2+ Influx Events in Primary Cerebral Artery Endothelial Cells
Description:
The sole member of the ankyrin subfamily of transient receptor potential channels, TRPA1, is a Ca 2+ permeable, non‐selective cation channel involved in endothelium‐dependent cerebral artery vasodilation.
Total Internal Reflection Fluorescence microscopy (TIRFM) was utilized to investigate the biophysical properties and regulation of TRPA1‐mediated Ca 2+ influx in primary cerebral artery endothelial cells (EC).
Rat basilar arteries were cut open and placed intima side down on Matrigel‐coated plates.
EC were allowed to proliferate (≤14 days), loaded with Fluo 4‐AM, and imaged in situ using TIRFM.
Localized, transient Ca 2+ influx events (mean amplitude (F‐F 0 ) of 0.
17±0.
02, duration of 0.
21±0.
03 s, and spatial spread of 2.
09±0.
29 μm 2 ) were detected at a whole‐cell frequency of 0.
04±0.
02 Hz (n = 24) under basal conditions.
Mean event frequency and duration greatly increased with addition of the TRPA1 agonist allyl isothiocyanate (AITC) (0.
23±0.
08 Hz, 1.
64±0.
10 s, n = 25).
These increases were attenuated in the presence of the selective TRPA1 antagonist HC‐030031 (0.
03±0.
02 Hz, 0.
65±0.
16 s, n = 10 cells).
Histogram analysis of AITC‐invoked event amplitudes indicates that these Ca 2+ signals display quantal separation.
Similar events were recorded from HEK 293 cells overexpressing TRPA1.
Together, these data suggest that quantal, TRPA1‐mediated Ca 2+ influx can be recorded from EC using TIRFM.
RO1HL091905.

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