Abstract
Opioids and cannabinoids are both associated with analgetic, psychotropic, and immunomodulatory effects. It has been suggested that both systems interact on multiple levels. We hypothesized that cannabinoids induce opioid receptors and investigated cannabinoid-dependent expression of the μ-opioid receptor subtype in a human T cell model. We report that activation of the peripheral cannabinoid receptor type 2 leads to a de novo induction of μ-opioid receptor transcription in Jurkat E6.1 cells. We show that interleukin-4 is transcriptionally induced in response to cannabinoids and that an interleukin-4 receptor antagonist blocks cannabinoid-dependent induction of μ-opioid receptors, indicating that induced expression of interleukin-4 is required in this process. Induction of interleukin-4 is blocked by decoy oligonucleotides directed against STAT5, indicating the requirement of this transcription factor. In addition, we show cannabinoid-dependent phosphorylation of STAT5. Further experiments demonstrate that interleukin-4 then induces phosphorylation of STAT6, which directly transactivates the μ-opioid receptor gene. In addition, STAT6 induces expression of the transcription factor GATA3, which also contributes to μ-opioid receptor gene transcription. The responsive promoter region of the human μ-opioid receptor gene with the binding sites for both factors was mapped to nt -1001 to -950. To demonstrate functional μ-opioid receptor proteins, morphine-mediated phosphorylation of mitogen-activated protein kinase was investigated. We show that phosphorylation of mitogen-activated protein kinase occurs only in cannabinoid-prestimulated Jurkat E6.1 cells and that it is blocked by the μ-opioid receptor antagonist d-Phe-Cys-Tyr-d-Trp-Orn-Thr-Pen-Thr-NH2. In summary, these findings provide a first example for cannabinoid-opioid-interactions in cells of the immune system.
Effects of cannabinoids are mediated by at least two types of receptors, termed CB1 and CB2, which belong to the family of Gi/Go-protein-coupled receptors. CB1 receptors are abundantly expressed in the central and peripheral nervous system. To a lesser degree, they are expressed in peripheral tissues (e.g., in cells of the immune system), where CB2 receptors predominantly are expressed (Howlett et al., 2002). Effects of opioids are mediated by receptors, which also belong to the family of Gi/Go-protein-coupled receptors. In particular, three types are distinguished, termed μ, δ, and κ, which are expressed throughout the nervous system and peripheral tissues (Pol and Puig, 2004). The μ-opioid receptor subtype is an important mediator of the analgesic effects of opioids and the main target for drugs of the morphine type. Opioid- and cannabinoid receptors are often coexpressed in cells of the nervous system (Rodriguez et al., 2001; Pickel et al., 2004); furthermore, both systems are characterized by various, sometimes synergistic interactions with respect to analgetic, psychotropic, and behavioral effects (Navarro et al., 2001; Cichewicz and McCarthy, 2003; Naef et al., 2003). In addition to central effects, agonists of both systems are well known for their modulatory effects on immune cell functions. These effects, which include modulation of T helper cell and natural killer cell functions, are similar for both opioids and cannabinoids (Sacerdote et al., 1998, 2000; Yuan et al., 2002; Klein et al., 2004; Roy et al., 2004). Whereas cannabinoid receptors are constitutively expressed in immune effector cells, μ-opioid receptors are normally not expressed in these cells but are known for their de novo inducibility. The most potent inducers of μ-opioid receptor gene expression in immune effector cells are cytokines (Kraus et al., 2001, 2003a; Borner et al., 2004a). In this study, we present cannabinoids as a novel group of substances that lead to de novo induction of μ-opioid receptor expression in the Jurkat T cell model via a CB2 receptor-mediated mechanism. We show that this effect is indirect and involves induced expression of interleukin-4. It is possible, therefore, that peripheral cannabinoids indirectly cause up-regulation of μ-opioid receptors in neuronal cells, because we have demonstrated earlier, that expression of this receptor is up-regulated by interleukin-4 in neuronal cells, as well (Kraus et al., 2001). Such a mechanism may contribute to analgesic effects of peripheral cannabinoids that have been reported recently (Ibrahim et al., 2003; Hohmann et al., 2004).
Materials and Methods
Cell Culture, Reagents and Transfection. Jurkat E6.1 cells were cultivated in RPMI-1640 medium (Cambrex Bio Science Verviers S.p.r.l., Verviers, Belgium) supplemented with 10% fetal calf serum (Biochrom, Berlin, Germany) and antibiotics (100 units/ml penicillin and 100 mg/ml streptomycin; Cambrex Bio Science). Twenty hours before stimulation experiments, cells received fresh medium with 1% fetal calf serum. Δ9-THC, R(+)-methanandamide, and cycloheximide were purchased from Sigma (Taufkirchen, Germany), AM 281, AM 630, and JWH 015 were from Tocris (Bristol, UK). The interleukin-4 antagonist IL-4[R121D,Y124D] was a kind gift from Walter Sebald (Biozentrum, Universität Würzburg, Germany) (Tony et al., 1994). Interleukin-4 (R&D Systems, Wiesbaden, Germany) was used at 5 ng/ml. Morphine and CTOP were obtained from Synopharm (Barsbüttel, Germany) and Tocris, respectively. For transfections, 5 × 106 cells were pelleted, mixed with 500 μl of transfection buffer containing 140 mM NaCl, 25 mM HEPES, 0.5 mM Na2HPO4, and 125 mM CaCl2, pH 7.15, and incubated for 20 min at room temperature. Then, 5 ml of medium was added and the cells were incubated for 16 h at 35°C and 3% CO2. After that, cells were pelleted again, resuspended in 7 ml of RPMI-1640 medium with 1% fetal calf serum and incubated for 72 h. The reporter gene product chloramphenicol acetyl transferase was assayed by enzyme-linked immunosorbent assay (Roche, Mannheim, Germany) according to the manufacturer's instructions.
Oligonucleotides. All oligonucleotides were synthesized by Metabion (Martinsried, Germany). Sequences of oligonucleotides were: STAT5, 5′-GATCGCATTTCGGAGAAGACG-3′; nSTAT5, 5′-GATCGCATTACGGAGTAGACG-3′; STAT6, 5′-CTAGTTCTTCTCAGAAGCATATGT-3′; nSTAT6, 5′-CTAGTTGATCTCAGATCCATATGT-3′; GATA3, 5′-CTAGAGGAAGTCTTCAGATAAAAAAGATAACAA-3′; nGATA3, 5′-CTAGAGGAAGTCTTCACTTAAAAAACTTAACAA-3′; STAT1/3, 5′-GATCGAGTTTACGAGAACTC-3′; AP-1, 5′-CGATTGACTCAGTACTGAGTCAATCG-3′; AP-2, 5′-TGCGGGCTCCCCGGGCTTGGGCGAGC-3′;NFκB, 5′-AAAGTTGAGGGGACTTTCCCAGGCCT-3′; NF-AT, 5′-GATCCGCCCAAAGAGGAAAATTTGTTTCATA-3′; and NF-IL-6, 5′-TGCAGATTGCGCAATCTGCA-3′.
For all oligonucleotides, only the sequences of the sense strands are given. The decoy oligonucleotide approach (final concentration of oligonucleotides, 160 nM), the efficiency and specificity of the oligonucleotides was described in detail in previous publications from our group (Kraus et al., 2003a,b; Borner et al., 2004a,b).
Reverse Transcription-Polymerase Chain Reaction. Total RNA was extracted using the Nucleospin RNA II kit from Macherey-Nagel (Düren, Germany). One microgram of total RNA was used for cDNA synthesis with Moloney murine leukemia virus reverse transcriptase, RNase H minus (Promega, Mannheim, Germany) and diluted to 50 μl. Two microliters of cDNA was used for RT-PCR reactions. The forward and reverse primers of each primer pair are located on different exons to avoid amplification of genomic DNA. Amplification of μ-opioid receptor transcripts by conventional and quantitative RT-PCR was performed as described previously (Kraus et al., 2001, 2003a). Quantitative real time RT-PCR was done according to the manufacturer's suggestions as follows: β-actin, 5′-GGTCCACACCCGCCACCAG-3′ and 5′-CAGGTCCAGACGCAGGATGG-3′ primers; preincubation, 8 min at 95°C; 50 cycles, 5 s at 95°C, 5 s at 60°C and 22 s at 72°C. Interleukin-4, 5′-GTCTCACCTCCCAACTGCTT-3′ and 5′-GTTACGGTCAACTCGGTGCA-3′ primers (located on exons 1 and 2 to avoid amplification of the splice variant interleukin-4 δ2); preincubation, 8 min at 95°C; 50 cycles, 5s at 95°C, 5 s at 68°C, and 10 s at 72°C. Interleukin-13, 5′-GCTCTCACTTGCCTTGGCGGCT-3′ and 5′-TCAGCATCCTCTGGGTCTTCTCGATG-3′ primers; preincubation, 8 min at 95°C; 50 cycles, 5s at 95°C, 5 s at 70°C, and 11 s at 72°C. GATA3, 5′-AACTGTCAGACCACCACAACCACAC-3′ and 5′-GGATGCCTTCCTTCTTCATAGTCAGG-3′ primers; preincubation, 8 min at 95°C; 50 cycles, 5 s at 95°C, 5 s at 70°C, and 8 s at 72°C. δ-Opioid receptor, 5′-ACGTGCTTGTCATGTTCGGCATCGT-3′ and 5′-ATGGTGAGCGTGAAGATGCTGGTGA-3′ primers; preincubation, 8 min at 95°C; 40 cycles, 5 s at 95°C, 5 s at 63°C, and 13 s at 72°C. CB1, 5′-CACCTTCCGCACCATCACCAC-3′ and 5′-GTCTCCCGCAGTCATCTTCTCTTG-3′ primers; preincubation, 8 min at 95°C; 40 cycles, 5 s at 95°C, 5 s at 68°C, and 10 s at 72°C. CB2, 5′-CATGGAGGAATGCTGGGTGAC-3′ and 5′-GAGGAAGGCGATGAACAGGAG-3′ primers; preincubation, 8 min at 95°C; 40 cycles, 5 s at 95°C, 5 s at 70°C, and 24 s at 72°C. Interleukin-5, 5′-GAGGATGCTTCTGCATTTGAGTTTG-3′ and 5′-GTCAATGTATTTCTTTATTAAGGACAAG-3′ primers; preincubation, 8 min at 95°C; 40 cycles, 5 s at 95°C, 5 s at 65°C, and 20 s at 72°C.
Reporter Gene Plasmids. All reporter plasmids are based on the pBLCAT2/pBLCAT3 vector system. The construction of the human μ-opioid receptor promoter containing reporter genes -2624, -1854, -1372, -779, -1372Δ-1001/-950, -2624/-2291, -2229/-1854, and -1854/-1227 has been described in previous publications (Kraus et al., 2001, 2003a; Borner et al., 2002, 2004a). Insertion of oligonucleotides into pBLCAT2 was performed according to a method described previously (Kang and Inouye, 1993). All plasmids were sequenced from both sides to ensure correct orientations and sequences of the inserts.
Western Blot Analysis. Cells (2 × 106) were seeded in RPMI-1640 medium without serum. After 18 h, cells were treated with 500 nM Δ9-THC, 5 ng/ml interleukin-4 (R&D Systems, Wiesbaden, Germany), or vehicle. After stimulation, cells were pelleted and lysed with 80°C sample buffer. Cell lysis, blotting and antibody incubations were performed as suggested in the “Western immunoblotting protocol” from Santa Cruz Biotechnology (Heidelberg, Germany). Aliquots of 20 μl were separated on a 7% polyacrylamide gel. Primary phospho-STAT-specific (P-STAT5(Tyr694)-R, P-STAT6-(Tyr641)-R) and primary antibodies against unphosphorylated STAT proteins were obtained from Santa Cruz Biotechnology and used in a 1:200 dilution. Phospho-p44/42-MAPK antibody (E10; Cell Signaling Technology, Frankfurt, Germany) and ERK 2 antibody (C-14; Santa Cruz Biotechnology) were used in 1:2500 and 1:2000 dilutions, respectively. Secondary antibodies [Anti-rabbit and anti-mouse Ig from GE Healthcare (Braunschweig, Germany)] were used in a 1:2500 dilution.
Statistical Analysis. For statistical evaluation Student's t tests were performed. Stars indicate significantly different values (*, p < 0.05; **, p < 0.01; ***, p < 0.001).
Results
Cannabinoids Induce μ-Opioid Receptor mRNA via CB2 Receptors. μ-Opioid receptors are normally not expressed in Jurkat E6.1 cells. However, stimulation of cells with Δ9-THC markedly induced μ-opioid receptor gene transcription (Fig. 1A). To determine the cannabinoid receptor type mediating this induction, CB1 and CB2 receptor agonists and antagonists were used (Fig. 1B). The combination of Δ9-THC with the CB1-specific antagonist AM 281 did not influence the induction of μ-opioid receptor mRNA. In contrast, the combination of Δ9-THC with the CB2-specific antagonist AM 630 inhibited μ-opioid receptor mRNA induction, indicating a CB2-mediated mechanism. Supporting this idea was that the CB1-specific agonist R-(+)-methanandamide did not cause μ-opioid receptor mRNA up-regulation, whereas the CB2-specific agonist JWH 015 markedly induced μ-opioid receptor mRNA. The protein translation inhibitor cycloheximide prevented the Δ9-THC-mediated μ-opioid receptor induction, indicating that protein synthesis is needed for μ-opioid receptor induction.
Identification of the Δ9-THC-Inducible Promoter Region of the Human μ-Opioid Receptor Gene. To characterize the promoter region responsible for the induction of the μ-opioid receptor gene by Δ9-THC, transfection experiments in Jurkat E6.1 cells were performed with reporter gene constructs containing various lengths of the 5′-flanking region of the gene (Fig. 2). The longest μ-opioid receptor promoter construct -2624 and consecutive 5′-deletions of it up to nt -1372 were inducible by Δ9-THC, whereas construct -779 showed no induction. Contrasting with construct -1372, a reporter gene with an internal deletion (-1372Δ-1001/-950) was not Δ9-THC-inducible. Constructs -2624/-2291, -2229/-1854, and -1854/-1227, which contain upstream promoter parts in front of the heterologous thymidine kinase promoter of the Herpes simplex virus, were not responsive, and the reporter gene vector pBLCAT2 alone was not responsive, suggesting that the region between nt -1001 and nt -950 is responsible for the induction of the μ-opioid receptor gene by Δ9-THC. We demonstrated previously that this region also confers interleukin-4-responsiveness of the gene and contains a binding site for the transcription factor STAT6 at nt -997 (Kraus et al., 2001). In addition, the experiments with cycloheximide (Fig. 1B) indicate that novel gene expression is needed for μ-opioid receptor regulation. Therefore, a possible role of interleukin-4 expression in the cannabinoid-mediated μ-opioid receptor induction was investigated next.
An Interleukin-4 Antagonist Inhibits the Induction of μ-Opioid Receptor mRNA by Δ9-THC. Jurkat E6.1 cells were incubated with Δ9-THC and the interleukin-4 antagonist IL-4[R121D,Y124D], and relative amounts of μ-opioid receptor mRNA were determined. The interleukin-4 antagonist dose dependently decreased the Δ9-THC induced up-regulation of μ-opioid receptor mRNA, suggesting that expression of interleukin-4 and binding to its receptor is necessary (Fig. 3). The antagonist is known to bind to the interleukin-4Rα receptor subunit (Tony et al., 1994). Thus, interleukin-13 signaling, which is also dependent on this receptor subunit, is blocked as well. To address the question of which of the two cytokines might mediate the Δ9-THC-induced up-regulation of μ-opioid receptor, the mRNA levels for interleukin-4 and interleukin-13 were determined (Fig. 4). Interleukin-4 mRNA was significantly induced by Δ9-THC. Furthermore, experiments using cycloheximide demonstrated that this induction is independent of protein synthesis. In contrast, interleukin-13 mRNA levels were not significantly influenced by Δ9-THC.
GATA3 is an important transcription factor in the biology of T cells and is up-regulated by interleukin-4. Its mRNA was therefore assayed as well. An induction of GATA3 mRNA by Δ9-THC was indeed observed, and this induction was suppressed by the interleukin-4 antagonist, indicating that this cytokine is a stimulus for GATA3 induction in this scenario.
Identification of Transcription Factors Involved. The transcription factor decoy oligonucleotide approach was used to address the question of which transcription factors participate in the Δ9-THC regulation in Jurkat E6.1 cells (Fig. 5A). In general, double-stranded decoy oligonucleotides with specific binding sequences for transcription factors are brought into living cells to selectively disrupt the function of these factors. The functional inactivation of the transcription factors is due to their interaction with the excess of specific decoy oligonucleotides instead of binding to the natural regulatory motifs of genes. Induction of μ-opioid receptor mRNA by Δ9-THC was strongly inhibited by STAT5 and STAT6 decoy oligonucleotides and significantly reduced by GATA3 decoy oligonucleotides, indicating that these factors are involved in the regulatory events. In addition, we tested decoy oligonucleotides specific for the transcription factors STAT1, STAT3, AP-1, AP-2, NFκB, NF-AT and NF-IL-6, which, however, did not interfere with induction of μ-opioid receptor transcription (data not shown). Δ9-THC-induced up-regulation of interleukin-4 mRNA was inhibited only by STAT5 decoy oligonucleotides but was not influenced by STAT6 and GATA3 decoy oligonucleotides, indicating that STAT5 is needed for interleukin-4 induction and that the latter two factors are required downstream of interleukin-4 induction for μ-opioid receptor gene trans-activation. GATA3 mRNA up-regulation by Δ9-THC was reduced by STAT5 and STAT6 decoy oligonucleotides, indicating that STAT6 not only transactivates the μ-opioid receptor gene directly, as shown previously (Kraus et al., 2001), but also trans-activates GATA3. As negative controls, nSTAT5, nSTAT6, and nGATA3 decoy oligonucleotides were used in which the specific transcription factor binding sites were destroyed by mutations. GATA3 belongs to the group of transcription factors that are upregulated during activation, as shown above. In contrast, STAT factors are phosphorylated for activation. Thus, phosphorylation of STAT factors was investigated next in our model (Fig. 5B). A robust phosphorylation of both STAT5 and STAT6 was observed after stimulation of Jurkat E6.1 cells with Δ9-THC. In response to interleukin-4, however, only phosphorylation of STAT6 was observed, whereas STAT5 remained unphosphorylated, strengthening our hypothesis that STAT5 acts upstream of the interleukin-4 induction (Fig. 5C).
Requirement of STAT6 and GATA3 for the Induction of the μ-Opioid Receptor Gene. Transfection experiments demonstrated that the promoter region between nt -1001 and nt -950 is responsible for the induction of the μ-opioid receptor gene by Δ9-THC (Fig. 2). Furthermore, the experiments with transcription factor decoy oligonucleotides indicated that STAT6 and GATA3 are involved in this effect (Fig. 5). The involvement of STAT6 in the direct transactivation of the μ-opioid receptor gene was demonstrated previously, and a binding site for this factor (nt -997) was identified (Kraus et al., 2001; Fig. 5C). Sequence comparisons indicated that two putative GATA3 binding sites (at nt -962 and nt -953) are located within the Δ9-THC-responsive μ-opioid receptor gene promoter region, as well (Fig. 6A). To characterize the involvement of STAT6 and GATA3 in the trans-activation of the μ-opioid receptor gene by Δ9-THC, mutational analysis was performed (Fig. 6B). The wild-type sequence was fully responsive to Δ9-THC. In contrast, mutation of the STAT6 element completely abolished inducibility of the reporter gene, indicating that STAT6 is essential for the induction of the μ-opioid receptor gene by Δ9-THC and that GATA3 alone cannot trans-activate the gene. However, mutations in the putative GATA3 binding sites significantly reduced Δ9-THC-inducibility, indicating that GATA3 additionally contributes to Δ9-THC induction of the gene.
Functionality of Δ9-THC Induced μ-Opioid Receptors in Jurkat E6.1 Cells. It was reported previously that opioids mediate phosphorylation of MAPK in various cell types, including immunocytes (Chuang et al., 1997; Schmidt et al., 2000). If this effect of opioids occured also in the Jurkat E6.1 model, it was used to demonstrate functional expression of μ-opioid receptor proteins after induction by cannabinoids. As shown in Fig. 7, morphine-mediated phosphorylation of MAPK was observed only in cells pretreated with Δ9-THC, but not in unstimulated cells, indicating that the cannabinoid-induced μ-opioid receptor mRNA is correctly translated into functional receptor proteins. In addition, the μ-opioid receptor-specific antagonist CTOP blocked the effect, indicating that it is indeed mediated by this receptor type.
Discussion
We have shown that μ-opioid receptor expression is induced by cannabinoids in Jurkat E6.1 cells via a CB2-dependent mechanism. Cannabinoids first induce expression of interleukin-4, which requires STAT5. Interleukin-4 then activates the transcription factors GATA3 and STAT6, which both trans-activate the μ-opioid receptor gene (see Fig. 5C). As an early step in the process, the transcription factor STAT5 is phosphorylated in response to cannabinoids. In general, activation of STAT members by G-protein-coupled receptors is increasingly recognized (Pelletier et al., 2003; Lo and Wong, 2004; Mazarakou and Georgoussi, 2005). Because cannabinoid and opioid receptors are structurally similar, it is interesting to mention that a recent report demonstrated STAT5 phosphorylation in response to μ-opioid receptor agonists (Mazarakou and Georgoussi, 2005). However, exact molecular mechanisms are largely unknown and need to be elucidated also for our model. In addition, we demonstrated a direct requirement of STAT5, STAT6, and GATA3 by decoy oligonucleotides. These specifically disrupt the function of a chosen transcription factor and, by attenuating downstream effects, directly demonstrate the necessity of a given transcription factor in a specific process. From the phylogenetic point of view, it may be interesting that the μ-opioid receptor gene is trans-activated by STAT6 and GATA3, because these transcription factors are typical for type 2 T helper cells. Moreover, immunomodulatory effects of opioids and cannabinoids, which are often similar for both substances, include, for example, T helper cell regulation. Thus, opioids (Sacerdote et al., 2000; Wang et al., 2003; Roy et al., 2004) as well as cannabinoids direct the balance between T helper cells from the type 1 to the type 2 phenotype. Thus far, inhibition of interferon-γ by cannabinoids is well described (Klein et al., 2000, 2004; Yuan et al., 2002). Cannabinoid-induced inter-leukin-4 and downstream factors such as STAT6 and GATA3 may not only be key players in the induction of the μ-opioid receptor gene but may also play a central role in T helper cell regulation by cannabinoids. In this context, it would be interesting to see whether other typical T helper cell type 2 genes are induced by cannabinoids via an interleukin-4-dependent pathway. Preliminary data indicate that cannabinoids regulate not only μ-opioid receptors in Jurkat cells but also other genes. Whereas mRNA for interleukin-13 (Fig. 4) and interleukin-5 (data not shown), which are typical for T helper cells type 2, and for CB2 (data not shown) were not changed at the 48-h time point, increased mRNA levels were found not only for interleukin-4 and GATA3, but also for δ-opioid receptors and CB1 receptors (data not shown). Thus, cannabinoids do not specifically induce μ-opioid receptors. Mechanisms for regulatory events on other genes will be topics of future reports. It is a general question, with regard to mRNA data, whether changes in mRNA really reflect changes in functional protein levels. Using phosphorylation of MAPK, which is a typical effect of opioids in various cell types including immunocytes (Chuang et al., 1997; Schmidt et al., 2000), we demonstrated that cannabinoids indeed induce functional μ-opioid receptor proteins. In general, regulation of μ-opioid receptor mRNA in immunocytes may thus cause changes in the efficacy of opioids modulating immune functions.
We reported previously that interleukin-4 induces μ-opioid receptor transcription not only in various immune effector cells but also in primary neuronal cells (Kraus et al., 2001). It would be worthwhile to investigate whether peripheral cannabinoids, via an interleukin-4-dependent mechanism, induced μ-opioid receptor expression in neuronal cells, as well. Although not unequivocally established, an up-regulation of antinociceptive receptors in neurons may enhance analgetic effects, as indicated by reports investigating the role of μ-opioid receptors in inflammation (Brack et al., 2004) and after viral transduction into dorsal root ganglia (Xu et al., 2003). In theory, an up-regulation of μ-opioid receptors in neuronal cells by cannabinoids might thus contribute to synergistic effects of cannabinoids and opioids (Cichewicz and McCarthy, 2003; Yesilyurt et al., 2003; Tham et al., 2005) and to antinociceptive effects of CB2 agonists (Ibrahim et al., 2003; Hohmann et al., 2004).
Acknowledgments
We thank Walter Sebald (Biozentrum, Universität Würzburg, Germany) for generously providing the interleukin-4 antagonist IL-4[R121D,Y124D].
Footnotes
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Supported by grants from the Doktor-Robert-Pfleger-Stiftung (J.K.) and the Deutsche Forschungsgemeinschaft (KR 1740) (J.K.).
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ABBREVIATIONS: Δ9-THC, Δ9-tetrahydrocannabinol; AM 281, 1-(2,4-dichlorophenyl)-5-(4-iodophenyl)-4-methyl-N-4-morpholinyl-1H-pyrazole-3-carboxamide; AM 630, 6-iodo-2-methyl-1-[2-(4-morpholinyl)ethyl]-1H-indol-3-yl(4-methoxyphenyl) methanone; JWH 015, (2-methyl-1-propyl-1H-indol-3-yl)-1-naphthalenylmethanone; IL, interleukin; MAPK, mitogen-activated protein kinase; RT-PCR, reverse transcriptase-polymerase chain reaction; STAT, signal transducer and activator of transcription; AP, activator protein; NFκB, nuclear factor κB; NF-AT, nuclear factor of activated T cells; nt, nucleotide(s); CTOP, d-Phe-Cys-Tyr-d-Trp-Orn-Thr-Pen-Thr-NH2.
- Received August 19, 2005.
- Accepted January 24, 2006.
- The American Society for Pharmacology and Experimental Therapeutics