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. 2015 Dec;39(12):2302-12.
doi: 10.1111/acer.12892. Epub 2015 Nov 18.

The Effect and Underlying Mechanism of Ethanol on Intracellular H(+) -Equivalent Membrane Transporters in Human Aorta Smooth Muscle Cells

Shih-Hurng Loh  1 Chung-Yi Lee  2 Gunng-Shinng Chen  3   4   5 Ching-Hsia Wu  1 Chan-Jun Tsao  1 Shou-Jou Shih  1 Chi-Chung Chou  1 Chien-Sung Tsai  2   6 Yi-Ting Tsai  2   6   7
Affiliations

The Effect and Underlying Mechanism of Ethanol on Intracellular H(+) -Equivalent Membrane Transporters in Human Aorta Smooth Muscle Cells

Shih-Hurng Loh et al. Alcohol Clin Exp Res. 2015 Dec.

Erratum in

  • Erratum.
    [No authors listed] [No authors listed] Alcohol Clin Exp Res. 2016 Aug;40(8):1793. doi: 10.1111/acer.13058. Epub 2016 Mar 14. Alcohol Clin Exp Res. 2016. PMID: 27453192 No abstract available.

Abstract

Background: The presence of intracellular pH (pHi ) regulators, including Na(+) -H(+) exchanger (NHE), Na(+) -HCO3- co-transporter (NBC), Cl(-) /OH(-) exchanger (CHE), and Cl(-) /HCO3- exchanger (AE), have been confirmed in many mammalian cells. Alcohol consumption is associated with increased risk of cardiovascular disorder. The aims of the study were to identify the possible transmembrane pHi regulators and to explore the effects of ethanol (EtOH) (10 to 300 mM) on the resting pHi and pHi regulators in human aorta smooth muscle cells (HASMCs).

Methods: HASMCs were obtained from patients undergoing heart transplant. The pHi was measured by microspectrofluorimetry with the pH-sensitive dye, BCECF-AM.

Results: The following results are obtained. (i) In cultured HASMCs, the resting pHi was 7.19 ± 0.04 and 7.13 ± 0.02 for HEPES- and CO2 /HCO3--buffered solution, respectively. (ii) Two different Na(+) -dependent acid-equivalent extruders, including NHE and Na(+) -coupled HCO3- transporter, functionally coexisted. (iii) Two different Cl(-) -dependent acid loaders (CHE and AE) were functionally identified. (iv) EtOH induced a biphasic, concentration-dependent change in resting pHi (+0.25 pH unit at 100 mM but only +0.05 pH unit at 300 mM) in bicarbonate-buffered solution, while caused a concentration-dependent decrease in resting pHi (-0.06 pH unit at 300 mM) in HEPES-buffered solution. (v) The effect of EtOH on NHE activity was also biphasic: increase of 40% at lower concentration of 10 mM, followed by decrease of 30% at higher concentration of 300 mM. (vi) The increase in Na(+) -coupled HCO3- transporter activity by EtOH was concentration dependent. (vii) The effect of EtOH on CHE and AE activities was both biphasic: increase of ~25% at 30 mM, followed by decrease of 10 to 25% at 100 mM, and finally increase of 15 to 20% at 300 mM.

Conclusions: This study demonstrated that 2 acid extruders and 2 acid loaders coexisted functionally in HASMCs and that EtOH induced a biphasic, concentration-dependent change in resting pHi by altering the activity of the 2 acid extruders, NHE and Na(+) -coupled HCO3- transporter, and the 2 acid loaders, CHE and AE.

Keywords: Alcohol/Ethanol; Cl−/HCO3− Exchanger (AE); Human Aorta Smooth Muscle Cells; Intracellular pH (pHi) Regulators; Na+-H+ Exchanger.

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