Sevoflurane Inhibits Phorbol-Myristate-Acetate-induced Activator Protein-1 Activation in Human T Lymphocytes in Vitro : Potential Role of the p38-Stress Kinase Pathway

Author:

Loop Torsten1,Scheiermann Patrick2,Doviakue David2,Musshoff Frank3,Humar Matjaz4,Roesslein Martin5,Hoetzel Alexander5,Schmidt Rene5,Madea Burkhard6,Geiger Klaus K.7,Pahl Heike L.8,Pannen Benedikt H. J.9

Affiliation:

1. Staff Anesthesiologist.

2. Research Fellow and Medical Student.

3. Forensic Toxicologist, Institute of Legal Medicine, University of Bonn, Bonn, Germany.

4. Biologist and Postdoctoral Fellow.

5. Resident.

6. Professor of Legal Medicine.

7. Professor of Anesthesiology and Chairman, Department of Anesthesiology.

8. Professor and Head, Division of Experimental Anesthesiology, University Hospital, Freiburg, Germany.

9. Professor of Anesthesiology, Department of Anesthesiology.

Abstract

Background Modulation of immune defense mechanisms by volatile anesthetics during general anesthesia may compromise postoperative immune competence and healing reactions and affect the infection rate and the rate of tumor metastases disseminated during surgery. Several mechanisms have been suggested to account for these effects. The current study was undertaken to examine the molecular mechanisms underlying these observations. Methods Effects of sevoflurane, isoflurane, and desflurane were studied in vitro in primary human CD3 T-lymphocytes. DNA-binding activity of the transcription factor activator protein-1 (AP-1) was assessed using an electrophoretic mobility shift assay. Phorbol-myristate-acetate-dependent effects of sevoflurane on the phosphorylation of the mitogen-activated protein kinases were studied using Western blots, the trans-activating potency of AP-1 was determined using reporter gene assays, and the cytokine release was measured using enzyme-linked immunosorbent assays. Results Sevoflurane inhibited activation of the transcription factor AP-1. This effect was specific, as the activity of nuclear factor kappabeta, nuclear factor of activated T cells, and specific protein-1 was not altered and several other volatile anesthetics studied did not affect AP-1 activation. Sevoflurane-mediated suppression of AP-1 could be observed in primary CD3 lymphocytes from healthy volunteers, was time-dependent and concentration-dependent, and occurred at concentrations that are clinically achieved. It resulted in an inhibition of AP-1-driven reporter gene activity and of the expression of the AP-1 target gene interleukin-3. Suppression of AP-1 was associated with altered phosphorylation of p38 mitogen-activated protein kinases. Conclusion The data demonstrate that sevoflurane is a specific inhibitor of AP-1 and may thus provide a molecular mechanism for the antiinflammatory effects associated with sevoflurane administration.

Publisher

Ovid Technologies (Wolters Kluwer Health)

Subject

Anesthesiology and Pain Medicine

Reference56 articles.

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