CB1 Cannabinoid Receptor-Mediated Cell Migration

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TETRAHYDROCANNABINOL

Vol. 294, Issue 1, 204-209, July 2000

CB1 Cannabinoid Receptor-Mediated Cell Migration¹

Zhao-Hui Song and Miao Zhong

Department of Pharmacology and Toxicology, University of Louisville School of Medicine, Louisville, Kentucky

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

Recent studies have suggested that cell migratory responses are often mediated by G_i protein-coupled receptors. Because itis known that CB1 cannabinoid receptors are coupled to pertussistoxin-sensitive G proteins, we proposed that CB1 may mediate cellmigration. To test this hypothesis, modified Boyden chamber assayswere used to investigate cell migration mediated by CB1 cannabinoidreceptors. HU-210, WIN55212-2, and anandamide, three cannabinoidagonists with distinct chemical structures, induced migrationof human embryonic kidney 293 cells stably transfected with humanCB1 gene, but not 293 cells transfected with an empty expressionvector. These migratory responses were concentration-dependent.The EC₅₀ values for HU-210, WIN55212-2, and anandamide were 0.19± 0.04, 12.2 ± 1.4, and 39.9 ± 3.7 nM, respectively. The maximalmigration index for HU-210, WIN55212-2, and anandamide were 8.9± 1.6, 9.5 ± 1.6, and 8.8 ± 1.3, respectively. Pretreating cellswith 100 ng/ml pertussis toxin eliminated the cannabinoid agonist-inducedcell migration. SR141716A, a selective antagonist for CB1, inhibitedthe cannabinoid agonist-induced migratory responses in a concentration-dependentmanner. Checkerboard analysis demonstrated that anandamide-inducedcell migrations are due to chemotaxis as well as chemokinesis.Furthermore, anandamide-induced migratory responses were inhibited,in a concentration-dependent manner, by PD098059, an inhibitorof mitogen-activated protein kinase activation, but not by 8-bromoadenosine-3',5'-cyclicmonophosphate, a cell-permeable cAMP analog. These data demonstratethat cannabinoid agonists are able to induce chemotaxis and chemokinesis,and that these migratory responses are mediated by G protein-coupled,CB1 cannabinoid receptors. In addition, these data suggest thatactivation of mitogen-activated protein kinase plays an importantrole, whereas inhibition of adenylate cyclase is probably notinvolved in the cell migration mediated byCB1.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Since the initial description that $Delta$ ⁹-tetrahydrocannabinol, the active constituent of marijuana, interacts with a specificG protein-coupled receptor (Howlett et al., 1986; Devane et al.,1988), two subtypes of cannabinoid receptors, known as CB1 andCB2, have been cloned and identified (Matsuda et al., 1990; Munroet al., 1993). CB1 is distributed in the central nervous system(Herkenham et al., 1991; Matsuda et al., 1993), as well as severalperipheral tissues, including testis and immune cells (Gerardet al., 1991; Bouaboula et al., 1993). Using cells that expressnative cannabinoid receptors and cell lines transfected with clonedcannabinoid receptors, previous studies have demonstrated thatCB1 is coupled to pertussis toxin-sensitive G proteins (Howlettet al., 1986; Felder et al., 1992). The known downstream signaltransduction pathways of CB1 include inhibition of adenylate cyclase(Howlett et al., 1986; Felder et al., 1992), activation of mitogen-activatedprotein kinase (MAPK) (Bouaboula et al., 1995), and modulationof ion channels (Mackie and Hille, 1992).

Cell migration plays important roles in many physiological and pathological processes, including embryogenesis, angiogenesis,metastasis, inflammation, and wound healing (Lauffenburger andHorwitz, 1996). Many chemoattractants are ligands for G protein-coupledreceptors. Pertussis toxin-sensitive G proteins are thought tobe crucial for the cell migration mediated by chemokine receptors(Gerard and Gerard, 1996). Recent studies have suggested thatthe ability to mediate cell migration may be shared by many receptorsthat are coupled to G_i proteins (Arai et al., 1997; Neptune andBourne, 1997). Because it is known that CB1 is coupled to pertussistoxin-sensitive G proteins, we postulated CB1 may mediate cellmigratory responses. To test this hypothesis, the abilities ofcannabinoid agonists to induce cell migration were examined inhuman embryonic kidney 293 cells stably transfected with humanCB1 gene. Cell migration can be classified into three categories:1) random, 2) chemokinesis, and 3) chemotaxis (Lauffenburger andHorwitz, 1996; Mitchison and Cramer, 1996). Random migrationsof cells occur in the absence of a stimulus. Chemokinesis is randommotion that is affected by a chemical stimulus. Chemotaxis isdirected motion of cells toward a gradient of a chemical stimulus.In this study, checkerboard analysis was performed to study whetherthe cannabinoid agonist-induced cell migration is due to eitherchemokinesis or chemotaxis. Currently, the cellular and molecularmechanisms for cell migration have not been completely understood.It is generally believed that G_i proteins are important in mediatingcell migration (Gerard and Gerard, 1996; Arai et al., 1997; Neptuneand Bourne, 1997). However, it is not clear which downstream targetsof G_i proteins are crucial in cell migration. In this study, theinvolvement of G protein-coupled CB1 in cell migration was examinedwith pertussis toxin and with a selective CB1 antagonist. Furthermore,the roles of adenylate cyclase inhibition and MAPK activation,two known signal transduction pathways for CB1, were investigatedusing a cell-permeable analog of cAMP and an inhibitor of MAPKactivation.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials. Adenovirus-transformed 293 cells were obtained from American Type Culture Collection (Rockville, MD). Tissue culture reagentswere purchased from Biowhittaker (Walkersville, MD). WIN55212-2,anandamide, and SR141716A were obtained from RBI (Natick, MA).HU-210 was purchased from Tocris (Balwin, MO). The stock solutionsof cannabinoids were made by dissolving cannabinoids in dimethylsulfoxide. BSA, mouse collagen type I, pertussis toxin, 8-bromoadenosine3',5'-cyclic monophosphate (8-Br-cAMP), and PD098059 were purchasedfrom Sigma (St. Louis, MO). The 48-well modified Boyden chamberand polycarbonate membranes with 10-µm pore size were purchasedfrom Neuro Probe Inc. (Bethesda,MD).

Cell Culture. Human embryonic kidney 293 cells stably transfected with human CB1 gene were used (Song and Bonner, 1996). The CB1 cannabinoidreceptors expressed in these cells have a B_max value of 1217.6± 221.9 fmol/mg of protein. It has been shown that these cellsdo not express CB2, and the CB1 expressed in these cells are functional(Song and Bonner, 1996). The 293 cell system is an appropriatemodel system for studying the roles of G protein-coupled receptorsin cell migration. This has been shown by other investigatorswith known inducers of migration, e.g., interleukin-8 receptors(Neptune and Bourne, 1997). Cells were maintained in Dulbecco'smodified Eagle's medium (DMEM) supplemented with 10% fetal calfserum, 100 U/ml penicillin, 100 µg/ml streptomycin, and 20 mML-glutamine. Cells were grown at 37°C in a humidified 5% CO₂incubator.

Cell Migration Assays. In vitro cell migration assays were performed using a modified 48-well Boyden chamber as described previously (Falk et al.,1980). Briefly, cells were washed twice with PBS and harvestedfrom the culture dish into a 50-ml centrifuge tube with EDTA-trypsin(Biowhittaker). Subsequently, the cells were washed with DMEMsupplemented with 0.2% BSA, centrifuged at 500g, and cell pelletswere resuspended in the same medium with a final cell concentrationof 1.0 × 10⁶ cell/ml. Chemoattractant solutions were made by diluting cannabinoidagonists in DMEM supplemented with 0.2% BSA. Polycarbonate membranes(polyvinylpyrrolidone-free, pore size 10.0 µm) were coated overnightat 4°C with 50 µg/ml mouse collagen type I. After loading chemoattractantsolutions in the lower chamber, a sheet of polycarbonate membranewas placed on top of the chemoattractant solution, the upper chamberwas properly assembled, and aliquots of 50-µl cell suspensionswere placed in the upper chamber. The chamber was incubated for5 h in a 37°C incubator with humidified air and 5% CO₂. At theend of the incubation period, the polycarbonate membrane was removed,nonmigrated cells were carefully removed by scraping against awiper, and the membrane was stained with a HEMA 3 staining kit(Fisher Scientific Inc., Houston, TX). For each well in the Boydenchamber, the number of cells migrating through to the undersideof the membrane was counted in six nonoverlapping low power field(×100) using a light microscope equipped with an ocular micrometer.The results were expressed as a migration index, which was definedas: mean number of cells per low power field for test substances/meannumber of cells per low power field for medium control (DMEM supplementedwith 0.2% BSA). Experiments were performed in triplicate and wererepeated threetimes.

Checkerboard Analysis. Chemical-induced increases in cell mobility could be attributed to either chemotaxis or chemokinesis. To distinguish chemotaxisfrom chemokinesis, checkerboard assays were performed (Zigmondand Hirsch, 1973; Wilkinson, 1998). Briefly, various concentrationsof anandamide, an endogenous cannabinoid agonist, were placedin upper wells, lower wells, or both upper and lower wells ofthe chemotaxis chamber to determine whether the number of migratedcells was greater with a positive gradient, no gradient, or anegative gradient of anandamide. According to the definition ofchemotaxis and chemokinesis, cell migration toward a positivegradient represents chemotaxis, whereas drug-stimulated randomcell migration (toward no gradient or a negative gradient) representschemokinesis.

Cell Pretreatment. To study the involvement of pertussis toxin-sensitive G proteins, cells were pretreated for 16 h with 100 ng/ml pertussistoxin in DMEM medium containing 10% fetal calf serum, 100 U/mlpenicillin, 100 µg/ml streptomycin, and 20 mM L-glutamine at 37°C,95% air, 5% CO_2. The cells were washed and resuspended after pertussistoxin treatment. To study the effects of CB1 antagonist SR141716A,cell-permeable cAMP analog 8-Br-cAMP, and MAPK activation inhibitorPD098059, cell suspensions were pretreated with these agents for30 min in DMEM supplemented with 0.2% BSA before being subjectedto cell migrationassays.

Data Analysis. The data presented in the table and figures represent mean ± S.E. The data were analyzed and the concentration-response curveswere generated with the use of GraphPad Prizm software. The EC₅₀and maximal migration index values were determined through nonlinearregression analysis performed with GraphPad Prizm. One-way ortwo-way ANOVA was used to compare the data of different treatmentgroups. The level of significance was chosen as P < .05.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Effects of Cannabinoid Agonists on Cell Migration. HU-210, WIN55212-2, and anandamide, three cannabinoid agonists that belong to three different chemical classes (Mechoulamet al., 1988; Compton et al., 1992; Devane et al., 1992), increasedthe migration of 293 cells stably transfected with human CB1 genefrom the upper chamber to the underside of the membrane (Fig.1). The effects of cannabinoid agonists on cell migration wereconcentration-dependent (P < .05 by ANOVA). The EC₅₀ values forHU-210, WIN55212-2, and anandamide were 0.19 ± 0.04, 12.2 ± 1.4,and 39.9 ± 3.7 nM, respectively. Approximately 30 to 50 cellsmigrated in the absence of drugs. The maximal migration indexvalues for HU-210, WIN55212-2, and anandamide were 8.9 ± 1.6,9.5 ± 1.6, and 8.8 ± 1.3, respectively. In contrast, cannabinoidagonists did not affect the migration of 293 cells transfectedwith an empty RC/CMV expression (P > .05 by ANOVA) (Fig. 1).

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Fig. 1. Effects of HU-210 (A), WIN55212-2 (B), and anandamide (C) on migration of 293 cells stably transfected with human CB1 gene. Cells were pretreated with 100 ng/ml pertussis toxin (PTX, open symbols) or vehicle (solid symbols) overnight before they were subject to cell migration assays. Data on vector-transfected 293 cell controls (×) were also shown. Results are expressed as migration index as described in Experimental Procedures. Data represent mean ± S.E. of three separate assays, each conducted in triplicate.

Effects of Pertussis Toxin on Cannabinoid Agonist-Induced Cell Migration. To study the involvement of pertussis toxin-sensitive G proteins in cannabinoid agonist-induced cell migration, cells werepretreated with 100 ng/ml pertussis toxin for 16 h. As demonstratedin Fig. 1, pretreatment of cells with pertussis toxin blockedthe cell migration induced by HU-210, WIN55212-2, and anandamide(P < .05 by two-way ANOVA). Pertussis toxin pretreatment at thesame concentration was able to block cannabinoid-induced inhibitionof forskolin-stimulated cAMP accumulation (data notshown).

Effects of a CB1 Antagonist on Cannabinoid Agonist-Induced Cell Migration. SR141716A, a selective CB1 antagonist (Rinaldi-Carmona et al., 1994), was used to test whether cannabinoid agonist-inducedcell migration is mediated by specific CB1 receptors. In a concentration-dependentmanner, SR141716A inhibited the cell migration induced by HU-210,WIN55212-2, and anandamide. The concentration-response curveswere shifted parallel to the right by SR141716A (P < .05 by two-wayANOVA) (Fig. 2, A, B, and C). The pA₂ values for SR141716A againstHU-210, WIN55212-2, and anandamide were 7.81 ± 0.20, 8.09 ± 0.04,and 7.92 ± 0.02, respectively. SR141716A by itself had no significanteffect on the cell migration (Fig. 2D).

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Fig. 2. Effects of SR141716A on cell migration induced by HU-210 (A), WIN55212-2 (B), and anandamide (C). Cells were pretreated with various concentrations of SR141716A for 30 min before they were subject to cell migration assays. Effects of SR141716A alone on cell migration are shown in (D). Results are expressed as migration index as described in Experimental Procedures. Data represent mean ± S.E. of three separate assays, each conducted in triplicate.

Checkerboard Analysis of Anandamide-Induced Cell Migration. Checkerboard analysis was performed to examine the degree to which the migratory responses of cells are due to chemotacticor chemokinetic effects (Wilkinson, 1998; Zigmond and Hirsch,1973). The results of checkerboard analysis are shown in Table1. The underlined values along the diagonal reflect migratoryresponses to uniform concentrations of anandamide on both sidesof the chamber (chemokinesis). The values below the diagonal reflectresponses to a positive gradient (chemotaxis), whereas the valuesabove the diagonal represent responses to a negative gradient(chemokinesis). When equal concentrations of anandamide were presentin the upper and lower chambers, the migration indexes were increasedwith increasing concentrations of anandamide (P < .05 by ANOVA).The migration indexes were increased with an increase in positivegradient of anandamide (P < .05 by ANOVA). These data demonstratethat anandamide induced both chemokinesis and chemotaxis, withchemotaxis stimulated to a greater extent (maximum of 7.79/1.12= 7-fold increase over the background compared with a 5.54/1.12= 5-fold increase for chemokinesis).

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TABLE 1
Checkerboard analysis of anandamide-induced migration of 293 cells stably transfected with human CB1 gene
Results are expressed as migration index as described in Experimental Procedures. Data represent mean ± S.E. of three separate assays, each conducted in triplicate.

Effects of a Cell-Permeable Analog of cAMP on Anandamide-Induced Cell Migration. To study whether the anandamide-induced cell migration is a result of inhibition of adenylate cyclase, thereby a decreasein intracellular cAMP levels, the cells were pretreated with 8-Br-cAMPfor 30 min before being subject to migration assays. As shownin Fig. 3A, this pretreatment did not block the migratory responsesinduced by anandamide. At 1 and 3 mM, 8-Br-cAMP might have enhancedcell migration. However, analysis by ANOVA demonstrated no significantdifferences (P > .05) between the data points in Fig. 3A. In theabsence of cannabinoids, 8-Br-cAMP by itself had no significanteffect (P > .05 by ANOVA) on the cell migration (Fig. 3B). Inour control experiments, 8-Br-cAMP was active in that it enhancedthe activation of MAPK by cannabinoids as previously demonstrated(Bouaboula et al., 1995) (data not shown).

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Fig. 3. Effects of 8-Br-cAMP on anandamide-induced cell migration (A). Cells were pretreated with various concentrations of 8-Br-cAMP or vehicle for 30 min before they were subject to the cell migration assays. Results are expressed as the percentage of anandamide-induced cell migration with 8-Br-cAMP pretreatment versus with vehicle pretreatment. Effects of 8-Br-cAMP alone on cell migration are shown in (B). Results are expressed as migration index as described in Experimental Procedures. Data represent the mean ± S.E. of three separate assays, each conducted in triplicate.

Effects of an Inhibitor of MAPK Activation on Anandamide-Induced Cell Migration. MAPK, i.e., extracellular signal-regulated kinase (ERK)-1 and ERK-2, are a group of serine/threonine-specific protein kinasesthat are activated by various cell surface receptors, includingreceptor tyrosine kinases, receptors coupled to cytoplasmic tyrosinekinases, and G protein-coupled receptors (Hill and Treisman, 1995;Seger and Krebs, 1995). PD98059 is an inhibitor of MEK (MAPK orERK kinase), a dual specific kinase that activates both ERK-1and ERK-2 by phosphorylation at specific threonine and tyrosineresidues (Alessi et al., 1995). PD098059 was used to study therole of MAPK activation in anandamide-induced cell migration.In a concentration-dependent manner, PD098059 inhibited the anandamide-inducedcell migration, with an IC₅₀ value of 8.6 ± 1.3 µM (Fig. 4A) (P< .05 by ANOVA). In the absence of cannabinoids, PD098059 by itselfhad no significant effect on the cell migration (Fig. 4B) (P >.05 by ANOVA). In our control experiments, PD098059 was able toinhibit cannabinoid-induced MAPK activity as expected (Alessiet al., 1995) (data not shown).

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Fig. 4. Effects of PD098059 on anandamide-induced cell migration (A). Cells were pretreated with various concentrations of PD098059 or vehicle for 30 min before they were subject to the cell migration assays. Results are expressed as percentage of anandamide-induced cell migration with PD098059 pretreatment versus with vehicle pretreatment. Effects of PD098059 alone on cell migration are shown in (B). Results are expressed as migration index as described in Experimental Procedures. Data represent the mean ± S.E. of three separate assays, each conducted in triplicate.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

In this study, HU-210, WIN55212-2, and anandamide, three cannabinoid agonists with distinct chemical structures, were foundto cause the migration of 293 cells stably transfected with humanCB1 gene. In contrast, these cannabinoid agonists did not causethe migration of 293 cells stably transfected with an empty expressionvector. The cannabinoid-induced cell migrations were concentration-dependent,with a rank order of potency of HU-210 > WIN55212-2 > anandamide.The concentration-response curves of cannabinoid agonists wereshifted parallel to the right by SR141716A, a selective antagonistfor CB1. These data indicate that the cannabinoid agonist-inducedcell migratory responses are mediated by specific CB1 receptorsexpressed in thesecells.

The cannabinoid-induced migratory responses were impaired in this study by pretreatment of cells with 100 ng/ml pertussistoxin. These results demonstrate that pertussis toxin-sensitiveG proteins are crucial for cannabinoid agonist-induced cell migration.These results are consistent with the previous reports that functionalCB1s are coupled to G_i proteins (Howlett et al., 1986; Felderet al., 1992). These data also support the notion suggested byArai et al. (1997) and Neptune and Bourne (1997) that the abilityto mediate cell migration is shared by G_i-coupledreceptors.

To identify the type of cell migration induced by anandamide, checkerboard analyses were carried out in this study. Our experimentsdemonstrated that anandamide is able to induce both chemotaxisand chemokinesis; however, chemotaxis was induced to a greaterextent.

One of the known mechanisms of signal transduction for CB1 is inhibition of adenylate cyclase (Howlett et al., 1986; Felderet al., 1992). However, in this study we found 8-Br-cAMP, a cell-permeableanalog of cAMP, did not attenuate cannabinoid agonist-inducedcell migration. These results indicate that cell migration isnot mediated by a decrease of intracellular cAMP level inducedby anandamide. This conclusion is consistent with the previousfindings that cAMP is not a critical intracellular mediator ofcell migration (Neptune and Bourne, 1997).

The well known roles of MAPK are their involvement in the signal transduction between the plasma membrane receptors and thenucleus (Hill and Treisman, 1995; Seger and Krebs, 1995). ForG_i protein-coupled receptors, it has been shown that the activationof MAPK pathway is mediated by $beta$ $gamma$ subunit stimulation of Ras (Crespoet al., 1994; Koch et al., 1994). However, in certain cell types,G_i proteins use a novel $beta$ $gamma$ - and Ras-independent pathway to activateMAPK (Hedin et al., 1999). At present, the roles of MAPK in cellmigratory responses mediated by G protein-coupled receptors havenot been established, and existing reports are controversial.For example, Kuroki and O'Flaherty (1997) reported that PD098059blocks neutrophil chemotaxis induced by several chemoattractants.In contrast, Knall et al. (1997) reported that MAPK activationis not important in interleukin-8-induced chemotaxis. It has beenestablished that activation of CB1 cannabinoid receptor increasesthe activity of MAPK (Bouaboula et al., 1995). In this study,PD098059 inhibited concentration dependently anandamide-inducedcell migration. The effective concentrations of PD098059 in inhibitingcell migration are within the concentration range for this drugto inhibit MAPK activation (Alessi et al., 1995). Thus, thesedata suggest that activation of MAPK may play an important rolein anandamide-induced cell migration. Currently, it is not clearhow the MAPK activation is involved in anandamide-induced cellmigration. Cytoskeletal regulation is a critical step in cellmigration (Lauffenburger and Horwitz, 1996; Mitchison and Cramer,1996). MAPK has been reported to regulate cytoskeleton and cellmotility by phosphorylating and enhancing myosin light chain kinaseactivity (Klemke et al., 1997). Because it is known that anandamidecan activate MAPK (Wartmann et al., 1995), one possible mechanismfor anandamide-induced cell migration may be anandamide-inducedactivation of MAPK, and subsequent cytoskeletal regulation byMAPK. In this study, the inhibition by PD098058 was not complete.This suggests that in addition to MAPK, there might be other pathwaysthat are involved in cannabinoid-induced cellmigration.

After demonstrating the involvement of CB1 in cannabinoid-induced migration with three different agonists, we focused on anandamidebecause it is an endogenous cannabinoid agonist. We expect similarmechanisms for HU-210 and WIN55212-2 because it is well knownthat both of these ligands activate similar second messenger systemsthroughCB1.

In summary, to our knowledge this is the first report that cannabinoid agonists can induce cell migration. These migratoryresponses are concentration-dependent, antagonized by SR141716A,a selective antagonist for the CB1, and blocked by pertussis toxinpretreatment. These results indicate that these migratory responsesare mediated by G protein-coupled, CB1 cannabinoid receptors.Furthermore, anandamide-induced migratory responses are blockedby PD098059, an inhibitor of MAPK activation, but not by 8-Br-cAMP,a cell-permeable analog of cAMP. These data suggest that activationof MAPK, but not inhibition of adenylate cyclase, are crucialfor the cell migration mediated by CB1. The detailed cellularand molecular mechanisms underlying the CB1-mediated cell migratoryresponses warrant additionalinvestigation.

	Footnotes

Accepted for publication March 22, 2000.

Received for publication November 15, 1999.

¹ This work was supported in part by National Institutes of Health Grant DA-11551.

Send reprint requests to: Z. H. Song, Ph.D., Department of Pharmacology and Toxicology, University of Louisville School of Medicine, Louisville, KY 40292. E-mail: zhsong{at}louisville.edu

	Abbreviations

MAPK, mitogen-activated protein kinase; 8-Br-cAMP, 8-bromoadenosine-3',5'-cyclic monophosphate; DMEM, Dulbecco's modified Eagle's medium; ERK, extracellular signal-regulated kinase.

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CB1 Cannabinoid Receptor-Mediated Cell Migration1

CB1 Cannabinoid Receptor-Mediated Cell Migration¹