Time-dependent Inhibition of G Protein–coupled Receptor Signaling by Local Anesthetics

Author:

Hollmann Markus W.1,Herroeder Susanne2,Kurz Katrin S.2,Hoenemann Christian W.3,Struemper Danja4,Hahnenkamp Klaus4,Durieux Marcel E.5

Affiliation:

1. Research Assistant Professor.

2. Medical Student, Department of Anesthesiology and Intensive Care Medicine, University Hospital Heidelberg.

3. Chief, Department of Anesthesiology, Marienhospital.

4. Research Fellow, Department of Anesthesiology and Intensive Care Medicine, University Hospital Muenster.

5. Professor, Department of Anesthesiology and Pain Therapy, University Hospital Maastricht, and Department of Anesthesiology, University of Virginia.

Abstract

Background Several beneficial effects of local anesthetics (LAs) were shown to be due to inhibition of G protein-coupled receptor signaling. Differences in exposure time might explain discrepancies in concentrations of LAs required to achieve these protective effects in vivo and in vitro (approximately 100-fold higher). Using Xenopus oocytes and human neutrophils, the authors studied time-dependent effects of LAs on G protein-coupled receptor signaling and characterized possible mechanisms and sites of action. Methods Measurement of agonist-induced Ca2+-activated Cl currents, using a two-electrode voltage clamp technique, and determination of superoxide anion production by cytochrome c assay were used to assess the effects of LAs on G protein-coupled receptor signaling in oocytes and primed and activated human neutrophils, respectively. Antisense knockdown of G alpha q protein and inhibition of various proteins within the signaling pathway served for defining mechanisms and sites of action more specifically. Results LAs attenuated G protein-coupled receptor signaling in both models in a time-dependent and reversible manner (lidocaine reduced lysophosphatidic acid signaling to 19 +/- 3% after 48 h and 25 +/- 2% after 6 h of control response in oocytes and human neutrophils, respectively). Whereas no effect was observed after extracellularly applied or intracellularly injected QX314, a lidocaine analog, using G alpha q-depleted oocytes, time-dependent inhibition also occurred after intracellular injection of QX314 into undepleted oocytes. Inhibition of phosphatases or protein kinases and agonist-independent G-protein stimulation, using guanosine 5'-O-3-thiotriphosphate or aluminum fluoride, did not affect time-dependent inhibition by LAs. Conclusion Inhibition of G protein-coupled receptor signaling by LAs was found to be time dependent and reversible. Critically requiring G alpha q-protein function, this effect is located downstream of guanosine diphosphate-guanosine triphosphate exchange and is not dependent on increased guanosine triphosphatase activity, phosphatases, or protein kinases.

Publisher

Ovid Technologies (Wolters Kluwer Health)

Subject

Anesthesiology and Pain Medicine

Reference24 articles.

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