HepG2 and SK-N-MC: Two Human Models to Study Alpha-2 Adrenergic Receptors of the Alpha-2C Subtype

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Vol. 281, Issue 2, 983-991, 1997

HepG2 and SK-N-MC: Two Human Models to Study Alpha-2 Adrenergic Receptors of the Alpha-2C Subtype

Stéphane Schaak, Cécile Cayla, Régis Blaise, Françoise Quinchon and Hervé Paris

Institut National de la Santé et de la Recherche Médicale U.317, Institut Louis Bugnard, Toulouse, France

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

It is now clearly established that alpha-2 adrenergic receptors can be subdivided in three pharmacological subtypes (alpha-2A,alpha-2B and alpha-2C) encoded by distinct genes ( $alpha$ ₂C10, $alpha$ ₂C2and $alpha$ ₂C4, respectively, in humans). Whereas the study of the regulationof the human alpha-2A adrenergic receptor and of the promoterregion of the $alpha$ ₂C10 gene has being greatly helped by the availabilityof the colon carcinoma cell line HT29, the study of the otherhuman receptor subtypes has thus far been limited to homologousdesensitization/down-regulation in transfected cells, becauseof the lack of human cellular models constitutively expressingalpha-2B or alpha-2C adrenergic receptors. Several human celllines were thus screened, in an attempt to find such models. Radioligandbinding studies with [³H]RX821002 and [³H]MK912, reverse transcription-polymerase chain reactions andRNase mapping experiments with pairs of primers and riboprobesspecific for each subtype demonstrated that the hepatoma cellline HepG2 and the neuroblastoma cell line SK-N-MC possess alpha-2adrenergic receptors of the alpha-2C subtype. However, whereasHepG2 expresses exclusively alpha-2C receptors (55 ± 7 fmol of[³H]MK912 binding sites/mg of protein), SK-N-MC expresses both alpha-2Aand alpha-2C subtypes in fairly similar amounts (20 ± 8 and 23± 3 fmol of [³H]MK912 binding sites/mg of protein, respectively). The studyof the inhibition of ³H-labeled antagonist binding by UK14304 demonstrated that a fractionof the receptor population was coupled to pertussis toxin-sensitiveG-proteins, which were identified as G_i2 and G_i3 by immunoblotting.The alpha-2 agonist was, moreover, able to decrease forskolin-stimulatedcAMP production by 47% in HepG2 and 23% in SK-N-MC, demonstratingthat inhibition of adenylyl cyclase is one of the primary mechanismsof signal transduction in both cell lines. HepG2 and SK-N-MC arethe first human cell lines unquestionably shown to natively expressalpha-2C adrenergic receptors. The discovery of these two modelsmay be useful for future study of the regulation of $alpha$ ₂C4 geneexpression in cells of different origins and investigation ofthe reciprocal regulation of alpha-2A and alpha-2C subtype insingle cells.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

The alpha-2 adrenergic receptors constitute a group of receptors that mediate many of the physiological effects of the endogenouscatecholamines epinephrine and norepinephrine, through activationof G-proteins of the G_i or G_o class. Extensive radioligand bindingstudies and more limited functional investigations have demonstratedthe existence of three pharmacological receptor subtypes (alpha-2A,alpha-2B and alpha-2C), which can be distinguished by their affinityfor subtype-selective drugs such as oxymetazoline, prazosin, chlorpromazineand WB4101 (Bylund, 1988). The genes that encode alpha-2A, alpha-2Band alpha-2C adrenergic receptors have been cloned and were termed $alpha$ ₂C10, $alpha$ ₂C2 and $alpha$ ₂C4, respectively, on the basis of their localizationon human chromosomes (Kobilka et al., 1987; Regan et al., 1988;Lomasney et al., 1990). The physiological significance of thisdiversity of receptors is not fully understood. According to bindingdata (DeVos et al., 1992) and RNase protection experiments (Peralaet al., 1992; Berkowitz et al., 1994), the different receptorsubtypes and their RNAs exhibit distinct tissue distribution,suggesting that they may be endowed with discrete functions invivo. However, with the exception of a few situations where agiven receptor has been assigned to a particular function (Trendelenburget al., 1994; MacMillan et al., 1996; Link et al., 1996), thespecific roles of each subtype are far from clear. Recent resultsobtained in differentiated MDCK II cells transfected with constructsallowing the expression of epitope-tagged alpha-2A, alpha-2B oralpha-2C adrenergic receptors also pointed out subtype differencesin subcellular distribution and membrane targeting (Wozniak andLimbird, 1996). Finally, another major difference between receptorsubtypes may result from the fact that they are differentiallyregulated. In this respect, experiments on transfected Chinesehamster ovary cells demonstrated that short-term exposure to epinephrineresulted in a subsequent attenuation of alpha-2 agonist-inducedinhibition of adenylyl cyclase in cells expressing the alpha-2Aor alpha-2B subtype, whereas no desensitization was observed withthe alpha-2C subtype (Eason and Liggett, 1992; Kurose and Lefkowitz,1994). Moreover, alpha-2A and alpha-2B subtypes undergo down-regulationafter long-term exposure to the agonist, but alpha-2C does not(Eason and Liggett, 1992). Other experiments carried out on celllines endogenously expressing alpha-2 adrenergic receptors, however,suggest that the situation could be much more complex. Treatmentof OK cells, a model that natively expresses the alpha-2C subtype,with norepinephrine indeed results in a rapid decrease in thepotency of alpha-2 agonists to inhibit cAMP production (Joneset al., 1990). Moreover, long-term exposure to the neurotransmitterinduces a significant reduction in receptor number (Shreve etal., 1991; Pleus et al., 1993), demonstrating that both desensitizationand down-regulation of the alpha-2C adrenergic receptor subtypeoccurs in these cells. It is thus likely that the regulation ofalpha-2 adrenergic receptors is not only subtype specific butalso cell type dependent.

In contrast to the study of the human alpha-2A adrenergic receptor, which greatly benefited from the availability of the colonadenocarcinoma cell line HT29 (Jones et al., 1990; Sakaue andHoffman, 1991; Devedjian et al., 1991), the study of other humanreceptor subtypes has been hampered by the lack of cell linesconstitutively expressing alpha-2B and/or alpha-2C subtypes. Theaim of the present work was therefore to find such models. Theanalysis of a panel of human cell lines from various origins,using RT-PCR, RPA and radioligand binding, unequivocally demonstratedthat the hepatocarcinoma cell line HepG2 and the neuroblastomacell line SK-N-MC express alpha-2 adrenergic receptors of thealpha-2C subtype.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Drugs and reagents. [³H]RX821002 (59 Ci/mmol) was from Amersham (Amersham, UK), [³H]MK912 (80.9 Ci/mmol) from New England Nuclear (Boston, MA) and[ $alpha$ -³²P]UTP from ICN (Costa Mesa, CA). Phentolamine was donated by Ciba-Geigy(Basel, Switzerland) and prazosin hydrochloride and UK14304 tartrateby Pfizer (Sandwich, UK). Oxymetazoline, forskolin, pertussistoxin, GppNHp and all other chemicals were from Sigma. Fetal calfserum was purchased from Gibco-BRL (Cergy Pontoise, France). Radioimmunoassaykits for cAMP determination were from Immunotech (Luminy, France).The antibodies generated against the common carboxyl-terminaldecapeptide of $alpha$ _i1 and $alpha$ _i2 (anti- $alpha$ _i1/ $alpha$ _i2) or against the carboxyl-terminaldecapeptide of $alpha$ _o (anti- $alpha$ _o/ $alpha$ _i3) were generously provided by Dr.B. Rouot (INSERM U.431, Université Montpellier II, Montpellier,France). The human alpha-2 adrenergic receptor genes ( $alpha$ ₂C2, $alpha$ ₂C4and $alpha$ ₂C10) were kindly provided by Dr. R. J. Lefkowitz (Duke University,Durham, NC).

Cell culture. The human cell lines HT29 and CaCo2 (colon adenocarcinoma), HepG2 and SK-Hep (hepatocarcinoma), HeLa (cervix), IMR-90 (lung),A-431 (epidermoid carcinoma) and SK-N-MC (neuroblastoma) werefrom the American Type Culture Collection (Rockville, MD). HT29,HepG2, SK-Hep, HeLa, A-431 and IMR-90 cells were grown in DMEMcontaining 25 mM glucose, 100 µg/ml streptomycin and 100 IU/mlpenicillin, supplemented with 5% (HT29) or 10% (CaCo2, HepG2,SK-Hep, HeLa and IMR-90) fetal calf serum. SK-N-MC cells werecultured in minimal essential medium containing the same concentrationsof antibiotics and supplemented with 5% fetal calf serum and 2mM glutamine.

Expression of the human alpha-2 adrenergic receptor subtypes in COS-7 cells. The plasmids that were used to express the different alpha-2 adrenergic receptor subtypes in COS-7 cells were pDP $alpha$ ₂C2, pDP $alpha$ ₂C4and pDP $alpha$ ₂C10. These expression vectors were constructed in ourlaboratory and contained the cytomegalovirus promoter, the entirecoding region of the $alpha$ ₂C2, $alpha$ ₂C4 or $alpha$ ₂C10 gene and the BamHI-XhoIfragment of rabbit $beta$ -globin genomic sequence (IVS2- $beta$ ), to increasethe stability of the transcripts. COS-7 cells were transfectedusing the DEAE-dextran method (Cullen, 1987) and were collected48 hr later.

Preparation of cellular RNAs and RT-PCR experiments. Total cellular RNAs were isolated using the guanidium isothiocyanate/phenol-chloroform extraction method (Chomczynski andSacchi, 1987). The integrity of the preparations was assessedby agarose gel electrophoresis, and the RNA concentrations weremeasured by UV spectrophotometry. Poly(A)⁺ RNAs used in RT-PCR experiments were prepared from 10 µg of cellularRNAs using the Dynabeads-oligo(dT)₂₅ kit (Dynal, Oslo, Norway).RT was performed for 1 hr at 37°C in a 20-µl reaction volume containing5 ng/µl oligo(dT)_12-18 (Pharmacia Biotech, Uppsala, Sweden),0.5 mM deoxynucleotide triphosphates and 200 U of SuperscriptIIreverse transcriptase (Gibco-BRL, Cergy Pontoise, France) in suppliedbuffer. Reaction was stopped by a 5-min treatment at 95°C. Negativecontrols were treated identically, except that reverse transcriptasewas omitted from the reaction. PCRs were carried out with 20 µlof cDNAs in a 100-µl reaction volume containing 10% dimethylsulfoxide,2.5% deionized formamide, 2.5 mM MgCl₂, 50 µM deoxynucleotidetriphosphates, 125 nM levels of each primer and 2.5 U of Taq DNApolymerase (Promega, Madison, WI). The reaction mixture was coveredwith two drops of mineral oil and subjected to incubation for3 min at 92°C and 30 cycles consisting of 1 min at 92°C, 1.5 minat 55°C and 1.5 min at 72°C, followed by a final elongation for7 min at 72°C, in a thermal cycler (Biometra, Goetingen, Germany).

Oligonucleotides. Three sets of primers were used in PCR experiments. The sense and antisense primer pairs for $alpha$ ₂C2 and $alpha$ ₂C4 gene were identicalto those used by Eason and Liggett (1993). The $alpha$ ₂C2 primers 5 $'$ -CCTGGCCTCCAGCATCGGAT-3 $'$ (sense) and 5 $'$ -CAGAGCACAAAAACGCCAAT-3 $'$ (antisense) amplified a630-bp fragment corresponding to nucleotides 519 to 1148 of the $alpha$ ₂C2 ORF. The digestion of this product by PstI gives two fragmentsof 465 and 165 bp. The $alpha$ ₂C4 primers 5 $'$ -GTGGTGATCGCCGTGCTGAC-3 $'$ (sense) and 5 $'$ -CGTTTTCGGTAGTCGGGGAC-3 $'$ (antisense) amplified a574-bp fragment corresponding to nucleotides 214 to 787 of the $alpha$ ₂C4 ORF. BstXI digestion of this product gives three fragments,of 271, 225 and 78 bp. The $alpha$ ₂C4/10 primers 5 $'$ -AAACCTCTTCCTGGTGTCTCT-3 $'$ (sense) and 5 $'$ -GTGCGCTTCAGGTTGTACTC-3 $'$ (antisense) allow amplificationof either a 233-bp fragment corresponding to nucleotides 259 to491 of the $alpha$ ₂C4 ORF or a 234-bp fragment corresponding to nucleotides204 to 437 of the $alpha$ ₂C10 ORF. The product from $alpha$ ₂C10 amplificationbut not that from $alpha$ ₂C4 amplification contains a BglII restrictionsite, generating two fragments of 117 bp each. Conversely, theproduct from $alpha$ ₂C4 amplification but not that from $alpha$ ₂C10 amplificationcontains a SacI restriction site, generating two fragments of153 and 80 bp.

Preparation and synthesis of the subtype-specific riboprobes. The antisense riboprobes for detection of $alpha$ ₂C2, $alpha$ ₂C4 and $alpha$ ₂C10 mRNAs were obtained by subcloning regions of the three genesinto pBluescriptII KS+ (pKS+; Stratagene, La Jolla, CA). The plasmidpKSC2-221 contained a 221-bp fragment (BamHI-HindIII) correspondingto nucleotides 1311 to 1531 of the $alpha$ ₂C2 sequence. The plasmidpKSC4-370 contained a 370-bp fragment (SmaI-MaeIII) correspondingto nucleotides 1014 to 1382 of the $alpha$ ₂C4 sequence. The plasmidpKSC10-352 contained a 352-bp fragment (PstI-PstI) correspondingto nucleotides 1041 to 1392 of the $alpha$ ₂C10 gene. For synthesis ofthe radiolabeled probes, the plasmids were linearized with theappropriated restriction enzyme and antisense RNAs were synthesizedin the presence of [³²P]UTP, using T3 RNA polymerase (Promega).

RPA. RPAs were performed as previously described but with slight modifications (Devedjian et al., 1991). Two hundred microgramsof lyophilized cellular RNAs were taken up in 30 µl of hybridizationbuffer [80% deionized formamide, 0.4 M NaCl, 1 mM EDTA, 40 mMpiperazine-N,N $'$ -bis(2-ethanesulfonic acid), pH 6.7] containingan excess of ³²P-labeled riboprobe. The samples were heated to 95°C for 5 minand then immediately placed at 55°C for 14 hr. Nonhybridized probewas eliminated by the addition of 0.3 ml of RNase A (40 µg/ml)and RNase T₁ (2 µg/ml), in 300 mM NaCl, 5 mM EDTA, 10 mM Tris-HCl(pH 7.5). After 2 hr at 37°C, digestion was stopped by additionof 5 µl of proteinase K (10 mg/ml) and the samples were furtherincubated for 15 min at 37°C. Carrier tRNA (10 µg) and 0.3 mlof solution D (4 M guanidinium thiocyanate, 25 mM sodium citrate,pH 7.0, 0.1 M 2-mercaptoethanol, and 0.5% sarkosyl) were addedto each tube, and protected hybrids were precipitated with isopropylalcohol. After washing with 70% ethanol, RNA pellets were dissolvedin 10 µl of sample buffer (97% deionized formamide, 0.1% sodiumdodecyl sulfate, 10 mM Tris-HCl, pH 7.0) and loaded onto a 5%acrylamide/7 M urea gel. The gels were exposed for 48 hr, at $-$ 80°C,to X-ray film (Hyperfilm; Amersham), with intensifying screens.The quantification of the amounts of radiolabeled antisense probeprotected by mRNA was performed using a PhosphorImager (MolecularDynamics, Sunnyvale, CA).

Receptor quantification. The quantification of alpha-2 adrenergic receptors was performed on crude membrane preparations using the selective alpha-2adrenergic antagonists [³H]RX821002 (Devedjian et al., 1994) and [³H]MK912 (Pettiborne et al., 1989). Frozen cells were harvestedin 5 ml of TE buffer (50 mM Tris-HCl, 5 mM EDTA, pH 7.5), disruptedusing a Dounce homogenizer and centrifuged at 39,000 × g for 10min. The particulate fraction was washed in TE buffer, and thefinal crude membrane pellet was taken up in the appropriate volumeof TM buffer (50 mM Tris-HCl, 0.5 mM MgCl₂, pH 7.5) for immediateuse. The protein concentration was determined using the Coomassieblue method (Bradford, 1976). Total binding was measured by incubating100 µl of cell membrane with the radioligand in a total volumeof 400 µl of TM buffer. After a 45-min incubation at 25°C, boundradioactivity was separated from free by filtration through GF/CWhatman filters, using a Millipore manifold sampling unit. Filterswere rapidly washed with ice-cold TM buffer, and membrane-boundradioactivity was determined by liquid scintillation counting.Specific binding was defined as the difference between total andnonspecific binding measured in the presence of 10 µM phentolamine.For saturation studies, the final concentrations of radioligandranged from 0.25 to 22 nM for [³H]RX821002 and from 0.04 to 8 nM for [³H]MK912. For inhibition studies, the indicated concentrationsof competitor were added to the incubation mixture before additionof the membrane suspension. Saturation isotherms and inhibitioncurves were analyzed using the EBDA-LIGAND computer programs (McPherson,1985).

Immunoblotting of G_i-protein $alpha$ -subunits. Immunoblotting was carried out as described previously (Homburger et al., 1987). After electrophoresis on 10% sodium dodecylsulfate-polyacrylamide gels, proteins were electrotransferredto nitrocellulose membranes (16 hr at 150 mA). To minimize nonspecificprotein binding, the nitrocellulose sheet was treated with Tris-salinebuffer (10 mM Tris-HCl, 500 mM NaCl, pH 7.5) containing 2% gelatin.The blots were incubated overnight at room temperature in thesame buffer supplemented with 1% gelatin and containing anti- $alpha$ _i1/ $alpha$ _i2or anti- $alpha$ _o/ $alpha$ _i3 (1/250 dilution). After three washes in 50 mM Tris-HCl,500 mM NaCl, 0.05% Tween 20, the blots were incubated for 1 hrwith ¹²⁵I-protein A (0.14 µCi/ml) in 50 mM Tris-HCl, 500 mM NaCl, 0.02%NaN₃. After extensive washing in Tris-HCl buffer containing 500mM NaCl and 0.05% Tween 20, blots were dried and autoradiographedas indicated above.

Determination of cAMP content. Cells were detached in phosphate-buffered saline containing 0.6 mM EDTA and were collected by gentle centrifugation (400 ×g for 5 min at 37°C). The pellet was suspended in DMEM bufferedwith 25 mM Hepes (pH 7.4). Aliquots of the cell suspension (180µl, corresponding to 0.4 mg of total protein) were incubated ina 200-µl final volume of Hepes-buffered DMEM containing 0.2 mM3-isobutyl-1-methylxanthine and the indicated concentration ofthe drug to be tested. After 15 min at 37°C, the reaction wasstopped by adding 1.8 ml of methanol/formic acid (95:5, v/v).The cell lysate was centrifuged (3000 × g for 10 min at 4°C),and an aliquot of supernatant was evaporated. The dry sampleswere taken up in acetate buffer containing 0.1% NaN₃, and theircAMP content was determined by radioimmunological assay (Steineret al., 1972).

	Results

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RT-PCR experiments. The aim of the present work was to search for human cell lines expressing alpha-2 adrenergic receptors of subtypes other thanalpha-2A. The RT-PCR approach was chosen as a primary screen becauseit allowed us to rapidly test a large panel of cell types andbecause of its high sensitivity. As a first step, the specificityof each primer pair was assessed on DNase-treated RNAs preparedfrom COS-7 cells transfected with pDP $alpha$ ₂C2, pDP $alpha$ ₂C4 and pDP $alpha$ ₂C10.As can be seen in figure 1, the $alpha$ ₂C2 and the $alpha$ ₂C4 primer pairsallowed amplification of a single fragment of the expected molecularsize (630 and 574 bp, respectively) only in cells transfectedwith the corresponding gene. On the other hand, the $alpha$ ₂C4/C10 primersworked as well on RNA from cells transfected with pDP $alpha$ ₂C4 as onthat from cells transfected with pDP $alpha$ ₂C10 and allowed amplificationof two fragments of indistinguishable size (233 and 234 bp, respectively;see "Materials and Methods" for additional comments).

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Fig. 1. Specificity of the oligonucleotide primers used in RT-PCR experiments. RT-PCRs were performed as described in "Materials andMethods," using $alpha$ ₂C2 primers (left), $alpha$ ₂C4 primers (middle) or $alpha$ ₂C4/C10 primers (right). The specificity of the different oligonucleotidepairs was validated on DNase-treated RNAs prepared from COS-7cells transfected with pDP $alpha$ ₂C2 (C2), pDP $alpha$ ₂C4 (C4) or pDP $alpha$ ₂C10(C10). Fragments of the expected molecular size were amplifiedonly in reactions where the primer pair corresponding to the transfectedgene was used. Lane M, 100-bp ladder.

RT-PCR experiments were thus carried out on RNAs extracted from various human cell lines. Whatever the pair of primers used,no signal was obtained when RT-PCRs were performed with RNAs fromHeLa, SK-Hep, IMR90, A-431 or CaCo2 cells (data not shown). Incontrast, fragments were amplified when RNAs from HepG2, SK-N-MCor HT29 cells were assayed (fig. 2). It is unlikely that theseproducts came from amplification of contaminating traces of genomicDNA, because no signal was observed in reactions where reversetranscriptase was omitted. The $alpha$ ₂C4 and $alpha$ ₂C4/C10 primers but notthe $alpha$ ₂C2 primers allowed amplification of fragments in HepG2 andSK-N-MC cells. In both cell lines, BstXI digestion of the 630-bpproduct obtained with the $alpha$ ₂C4 primers generated three fragmentsof the expected sizes (271, 225 and 78 bp). According to the cellline considered, BglII and SacI digestion of the product amplifiedwith the $alpha$ ₂C4/C10 primers gave different patterns. Whereas this233/234-bp fragment was digested by SacI but not BglII in HepG2cells, it was cut by both enzymes in SK-N-MC cells. These resultssuggested that HepG2 contains exclusively $alpha$ ₂C4 transcripts andthat $alpha$ ₂C4 and $alpha$ ₂C10 mRNAs are represented in SK-N-MC cells. Notonly the $alpha$ ₂C4/C10 primers but also the $alpha$ ₂C2 primers generateda signal in HT29 cells. Digestion of the $alpha$ ₂C2 primer product byPstI gave two fragments (465 and 165 bp), verifying that it trulycorresponded to $alpha$ ₂C2 amplification. Conversely to HepG2, the productgenerated with the $alpha$ ₂C4/C10 primers was cut by BglII but not SacI,indicating that it corresponded only to $alpha$ ₂C10 amplification. Thisconclusion was confirmed by the absence of amplification whenthe specific $alpha$ ₂C4 primers were used. According to these results,it appears that HT29 cells contain both $alpha$ ₂C10 and $alpha$ ₂C2 mRNAs.Such a result was unexpected, because this cell line is generallyconsidered to express exclusively receptors of the alpha-2A subtype(Bouscarel et al., 1985

; Bylund, 1988

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Fig. 2. RT-PCR experiments on RNAs from HepG2, SK-N-MC and HT29 cells. Upper, poly(A)⁺ RNAs were prepared from HepG2 (left), SK-N-MC (middle) and HT29(right) cells. RT-PCRs were performed as described in "Materialsand Methods," using $alpha$ ₂C2 primers ( $alpha$ ₂C2), $alpha$ ₂C4 primers ( $alpha$ ₂C4) or $alpha$ ₂C4/C10 primers ( $alpha$ ₂C4/C10). Lanes $-$ , reactions where reversetranscriptase was omitted. Lower, restriction analysis of RT-PCRproducts. The fragments resulting from the amplification with $alpha$ ₂C2 primers ( $alpha$ ₂C2) and $alpha$ ₂C4 primers ( $alpha$ ₂C4) were digested withPstI (P) and BstXI (X), respectively. The fragments resultingfrom the amplification with $alpha$ ₂C4/C10 primers ( $alpha$ ₂C4/C10) were digestedwith either BglII (B) (which cuts $alpha$ ₂C10 product) or SacI (S) (whichcuts $alpha$ ₂C4 product). Lanes $-$ , undigested products. Lanes M, 100-bpladder.

RPAs. Because our RT-PCR conditions were not quantitative, RPAs were performed, to yield a better estimation of the respective amountsof the three RNA species in the three cell lines that gave positiveresults in RT-PCR experiments. The subtype specificity of theriboprobes used in these experiments has been demonstrated inprevious work (Valet et al., 1993), and assays were performedwith 200 µg of cellular RNAs, to detect weak signals. Qualitatively,the results from RPA (fig. 3) agreed fully with those from RT-PCRexperiments; however, the amounts of the different receptor RNAsappeared to vary widely, according to the cells considered. HepG2was found to express exclusively $alpha$ ₂C4 and contains large amountsof this gene transcript. In agreement with binding data (Devedjianet al., 1994) and with previous results from RPAs (Devedjian etal., 1991), the predominant alpha-2 adrenergic receptor mRNA speciesin HT29 is the $alpha$ ₂C10 mRNA. A very weak $alpha$ ₂C2 mRNA signal was alsodetected, and its quantification indicated that it represented<1% of the amount of $alpha$ ₂C10 in this cell line. SK-N-MC cells containedfairly similar amounts of $alpha$ ₂C4 and $alpha$ ₂C10 mRNA but, in contrastto conclusions from RT-PCR, the amounts of $alpha$ ₂C4 and $alpha$ ₂C10 transcriptswere much lower than that of $alpha$ ₂C4 in HepG2 cells and than thatof $alpha$ ₂C10 in HT29 cells. Together, the results from RT-PCR andRPA definitively show that HepG2 and SK-N-MC contain $alpha$ ₂C4 mRNAs.Previous studies carried out with SK-N-MC and HepG2 have demonstratedthat both cell lines also contain alpha-1 adrenergic receptormRNAs. However, although the presence of transcripts was followedby alpha-1 adrenergic receptor expression in SK-N-MC (Esbenshadeet al., 1995), no receptor was detected in HepG2 (Kost et al.,1992). Binding experiments were thus conducted to verify thatthe presence of $alpha$ ₂C4 transcripts was accompanied by alpha-2C adrenergicreceptor expression.

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Fig. 3. RPA of RNAs from HepG2, SK-N-MC and HT29 cells. Two hundred micrograms of RNAs prepared from HepG2, SK-N-MC and HT29 cellswere hybridized with an excess of $alpha$ ₂C2-221 (left), $alpha$ ₂C4-370 (middle)or $alpha$ ₂C10-352 (right) ³²P-labeled riboprobe. Samples were digested with a mixture of RNasesA and T1. The resistant hybrids were electrophoresed and gelswere autoradiographed as described in "Materials and Methods."Lanes P, undigested probes; lanes $-$ , hybridization with 5 µg ofRNA from untransfected COS-7 cells; lanes C2, C4 and C10, hybridizationwith 5 µg of RNA from COS-7 cells transfected with pDP $alpha$ ₂C2, pDP $alpha$ ₂C4and pDP $alpha$ ₂C10, respectively.

Binding experiments. Alpha-2 adrenergic receptors were quantified using the radiolabeled antagonists [³H]RX821002 and [³H]MK912. The Scatchard plots obtained by transformation of saturationbinding data for HT29, SK-N-MC and HepG2 cell membranes using[³H]RX821002 are depicted in figure 4. Under the conditions used,[³H]RX821002 labeled a single class of high-affinity binding sitesin HT29 and HepG2 membrane preparations, and statistical analysisof the data indicated that a two-site model did not give a betterfit than the one-site model. On the other hand, Scatchard transformationof [³H]RX821002 binding on SK-N-MC yielded curvilinear plots, and inthis case data were better fitted by a two-component model thanby a one-component model (P < .002). The results obtained underthe same conditions but with [³H]MK912 as radioligand are reported in figure 5. Like [³H]RX821002, this molecule appears to label a single class of bindingsites in HT29 and HepG2 membrane preparations, whereas it revealsan heterogeneous population of binding sites in SK-N-MC. Again,in contrast to observations for HT29 and HepG2, binding of [³H]MK912 on SK-N-MC membranes was significantly better fitted bya two-site model (P < .001). Table 1 summarizes the results fromthe computer-assisted analysis of the data obtained from severalexperiments. It also allows us to compare the binding parametersof [³H]RX821002 and [³H]MK912 with membranes from the three cell lines with those obtainedwith membranes from COS-7 cells transfected with the $alpha$ ₂C2, $alpha$ ₂C4or $alpha$ ₂C10 gene. As expected, HT29 cells expressed only one classof binding sites, with K_d values for [³H]RX821002 (1.01 ± 0.24 nM) and [³H]MK912 (0.64 ± 0.27 nM) that match those found in COS-7 cellstransfected with the $alpha$ ₂C10 gene (1.37 ± 0.33 and 0.71 ± 0.31 nM,respectively). The sites labeled in HepG2 cells displayed a moderateaffinity for [³H]RX821002 (K_d = 3.5 ± 0.4 nM) and a remarkably high affinityfor [³H]MK912 (K_d = 0.08 ± 0.02 nM), which is characteristic of the $alpha$ ₂C4-adrenergic receptor subtype. SK-N-MC exhibited fairly similaramounts of two binding site populations with different affinitiesfor [³H]RX821002 and [³H]MK912. Given the relative selectivity of the two radioligandsfor the different receptor subtypes, it is obvious that the receptorsubpopulation displaying high affinity for [³H]RX821002 corresponds to alpha-2A, whereas that having high affinityfor [³H]MK912 corresponds to the alpha-2C subtype. According to theradioligand used, the alpha-2A receptor fraction represented 32to 46% of the whole receptor population. The pharmacological propertiesof these receptors were further studied by comparing the abilityof the subtype-selective drugs oxymetazoline and prazosin to inhibit³H-labeled antagonist binding to membrane preparations from HT29,HepG2 and SK-N-MC cells (table 2). Whereas oxymetazoline wasseveral orders of magnitude more potent than prazosin in preventing[³H]RX821002 binding to HT29 receptors (K_i ratio = 470), these twocompounds exhibited similar potencies for inhibiting [³H]MK912 binding at HepG2 receptors (K_i ratio = 0.55). In agreementwith the conclusion from saturation data, inhibition curves for[³H]RX821002 binding to SK-N-MC receptors were clearly biphasicand allowed two sites, with distinct affinities for oxymetazolineor prazosin, to be distinguished. Based on the known selectivityof the two compounds, sites having high affinity for oxymetazolineand low affinity for prazosin correspond to the alpha-2A subtypereceptor population, whereas those having fairly similar affinitiesfor the two compounds represent alpha-2C receptors.

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Fig. 4. Scatchard plots of [³H]RX821002 binding to membranes of HepG2, SK-N-MC and HT29 cells. Membranes prepared from HepG2 (left),SK-N-MC (middle) and HT29 (right) cells were incubated in thepresence of various concentrations of radioligand. The amountof specifically bound [³H]RX821002 was determined using 10⁵ M phentolamine to estimate nonspecific binding. The presenteddata are from a typical experiment, and each point representsthe mean of duplicates.

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Fig. 5. Scatchard plots of [³H]MK912 binding to membrane of HepG2, SK-N-MC and HT29 cells. Membranes prepared from HepG2 (left), SK-N-MC(middle) and HT29 (right) cells were incubated in the presenceof various concentrations of radioligand. The amount of specificallybound [³H]MK912 was determined using 10⁵ M phentolamine to estimate nonspecific binding. The presenteddata are from a typical experiment, and each point representsthe mean of duplicates.

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TABLE 1
Binding parameters of [³H]RX821002 and [³H]MK912
Membranes prepared from HepG2, SK-N-MC, HT29 and COS-7 cells transfected with pDP $alpha$ ₂C2, pDP $alpha$ ₂C4 or pDP $alpha$ ₂C10 were incubatedin the presence of increasing concentrations of [³H]RX821002 or [³H]MK912, and specific binding was determined as described in "Materialsand Methods." Computer analysis of the binding data indicatedthat the two radioligands labeled a single class of binding sitesin HepG2, HT29 and transfected COS cells. In contrast, two receptorpopulations were distinguishable in SK-N-MC cells. The maximumnumber of binding sites (B_max) and the dissociation constant value(K_d) were calculated by nonlinear regression analysisof the data according to a one- or two-component model. Reportedvalues are the means ± S.E.M. from n (in parentheses) determinations.

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TABLE 2
Inhibition of radioligand binding by oxymetazoline and prazosin
Inhibition studies were performed as described in "Materials and Methods." The concentrations of radioligand used in theseexperiments were 4 nM [³H]RX821002 for HT29, 0.7 nM [³H]MK912 for HepG2 and 12 nM [³H]RX821002 for SK-N-MC. Data were analyzed using computer programsallowing curve fitting to a one-site (HT29 and HepG2) or two-site(SK-N-MC) inhibition model (McPherson, 1985

). Reported valuesare means ± S.E. of three determinations.

Receptor coupling, identification of G_i-proteins and inhibitory effect of UK14304 on cAMP production. The degree of receptor coupling to G-proteins was estimated by studying the inhibition of ³H-antagonist binding by the alpha-2 agonist UK14304, in the absenceor presence of GppNHp/Na. For all cell lines considered (fig.6), agonist-inhibition curves obtained under control conditionsexhibited a Hill coefficient value significantly different from1 and were better fitted by a multicomponent model. The additionof GppNHp/Na to the binding medium resulted in a rightward shiftand in a significant increase in the slope of the curves, reflectingthe conversion of the whole receptor population into a low-affinitystate for the agonist. From computer-assisted analysis of thedata, it was calculated that the percentage of receptors in thehigh-affinity state for UK14304 was 43 ± 11% in HepG2 and 29 ±7% in SK-N-MC. Similar observations were made when membranes weretreated with pertussis toxin and the G_i/G_o-proteins expressedby the cells were identified by immunoblotting using either anti- $alpha$ _o/ $alpha$ _i3or anti- $alpha$ _i1/ $alpha$ _i2 antibody. As shown in figure 7, each of theseantibodies recognized a single band in HepG2 and SK-N-MC. Comparisonof the relative mobility of these proteins with those labeledin rat brain membranes indicated that the two cell lines expressG_i2 and G_i3. In a final series of experiments, the biologicalefficacy of the receptor was tested by measuring the extent ofthe inhibitory effect of UK14304 on the intracellular cAMP accumulationinduced by forskolin. The alpha-2 agonist caused a significantreduction of forskolin-induced cAMP accumulation in both celllines (table 3). On the basis of 18 determinations in three independentexperiments, it was calculated that the extent of the inhibitoryeffect of UK14304 reached 47% in HepG2 and 23% in SK-N-MC. Thiseffect was dose-dependent and was abolished by addition of anexcess of yohimbine or by prior treatment of the cells with pertussistoxin (data not shown).

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Fig. 6. Inhibition of ³H-labeled antagonist binding by UK14304. Binding studies were performed as described in "Materials and Methods."Concentrations of [³H]MK912 and [³H]RX821002 were 0.7 nM (HepG2) and 8 nM (SK-N-MC), respectively.Inhibition of radioligand binding by UK14304 were measured inthe absence ( $square$ ) or presence ( $open circle$ ) of GppNHp (100 µM) plus NaCl (100mM). The presented data are from a typical experiment, and eachpoint represents the mean of duplicates.

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Fig. 7. Identification of G_i-protein $alpha$ -subunits by immunoblotting. Membrane proteins from rat brain (RB) and HepG2 and SK-N-MC cellswere separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresisand transferred to nitrocellulose membranes. Immunoblottings wereperformed as described in "Materials and Methods," with eitheranti- $alpha$ _i1/ $alpha$ _i2 antibody (left) or anti- $alpha$ _o/ $alpha$ _i3 antibody (right).

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TABLE 3
Effect of UK14304 on forskolin-induced accumulation of intracellular cAMP
HepG2 or SK-N-MC cells were detached by treatment with phosphate-buffered saline-EDTA, resuspended and incubated for 15 minat 37°C in 200 µl of Hepes-buffered DMEM containing either vehicle(basal), 1 µM forskolin or 1 µM forskolin plus 10 µM UK14304.Concentrations of cAMP were measured as described in "Materialsand Methods." Results are expressed as picomoles of cAMP per milligramof cellular protein and are means ± S.E. of 18 determinations.Statistical analysis was performed using the Student's t test.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

The existence of three subtypes of alpha-2 adrenergic receptors (namely, alpha-2A, alpha-2B and alpha-2C) was initially proposedon the basis of the pharmacological profiles of receptors expressedin various species tissues and was then confirmed by the cloningof $alpha$ ₂C10, $alpha$ ₂C2 and $alpha$ ₂C4 genes in humans. The prototypical celllines expressing each of these subtypes are so far consideredto be the colon adenocarcinoma cell line HT29 for alpha-2A, theneuroblastoma-glioma hybrid cell line NG108-15 for alpha-2B andthe epithelial kidney cell line OK for alpha-2C (Bylund, 1988).One of the major limitations to the use of NG108-15 and OK cellsfor the study of the regulation of alpha-2B and alpha-2C adrenergicreceptors results from the fact that they are not of human origin.NG108-15 is a mouse-rat hybrid cell line and expresses a receptorpopulation that may be a mixture of the products from two differentgenes, RNG and RG10 (Hu et al., 1993), which are the rodent homologsof human $alpha$ ₂C2 and $alpha$ ₂C4, respectively. On the other hand, OK cellsare derived from American opossum and express a receptor for whichthe amino acid sequence exhibits large divergences from human $alpha$ ₂C4 (Blaxall et al., 1994). Major differences between the twopolypeptides are located in the third intracellular loop, a regionparticularly important in receptor regulation. On the basis ofbinding data, the retinoblastoma Y79 line was proposed to representa model of human cells expressing alpha-2C adrenergic receptors(Gleason and Hieble, 1992). However, another study assigned theY79 receptor to the alpha-2A subtype (Kazmi and Mishra, 1989),and definitive demonstration that the receptor expressed in thiscell line is encoded by $alpha$ ₂C4 is missing. One of the consequencesof the lack of human models clearly established as expressingalpha-2B and/or alpha-2C is that the study of the regulation ofthese two human receptor subtypes has thus far been restrictedto homologous regulation in transfected cells (Eason and Liggett,1992; Kurose and Lefkowitz, 1994).

Based on data from mRNA identification by RT-PCR and RPA and on the results from binding experiments with [³H]RX821002 and [³H]MK912, the present work unequivocally demonstrates that thehuman hepatoma cell line HepG2 and the human neuroblastoma cellline SK-N-MC both contain alpha-2 adrenergic receptors of thealpha-2C subtype. HepG2 expresses exclusively this receptor subtype,at a density of 55 fmol/mg of protein. The receptor is coupledto pertussis toxin-sensitive G-proteins (G_i2 and/or G_i3), andits stimulation by the alpha-2 agonist UK14304 efficiently reducescAMP production, indicating that inhibition of adenylyl cyclaseis one of the primary mechanisms of signal transduction in thesecells. The presence of alpha-2C adrenergic receptors in HepG2was rather unexpected. This cell line, which is commonly usedin many laboratories, was apparently never examined in this respect.It would be interesting to determine whether the presence of alpha-2Cadrenergic receptors corresponds to ectopic expression in a giventransformed cell or whether it reflects the situation in normalhuman hepatocytes. The lack of alpha-2 adrenergic receptors inthe other human hepatoma cell line, SK-Hep, and the failure toidentify noradrenaline-displaceable [³H]idazoxan binding sites in membranes from human liver (Tessonet al., 1991) support to the first alternative. However, the factthat $alpha$ ₂C4 transcripts were found in human liver (Berkowitz etal., 1994; H. Paris and S. Schaak, personal observation), togetherwith the fact that alpha-2 adrenergic receptors negatively coupledto adenylyl cyclase were identified in rat liver membranes (Hoffmanet al., 1981; Jard et al., 1981), supports the second possibility.The application of the techniques used in the current work tofreshly isolated human hepatocytes may bring a definitive answerto this question. According to previous observations made withcells transfected with the $alpha$ ₂C4 gene (Wozniak and Limbird, 1996)or with its mouse homolog M $alpha$ ₂-4H (Von Zastrow et al., 1993), intracellularlocalization is a peculiar feature of the alpha-2C adrenergicreceptor subtype. Whether this is true in HepG2 would also meritexamination. Whatever the answers to these questions, HepG2 cannow be considered as the first human cell line unequivocally demonstratedas expressing the alpha-2C adrenergic receptor. The future useof this model may yield valuable information on the mechanismsof regulation of alpha-2C receptor expression and $alpha$ ₂C4 gene transcription.

The presence of alpha-2 adrenergic receptors in SK-N-MC is less surprising, because other human neuroblastoma cell lines,such as SH-SY5Y (Kazmi and Mishra, 1989) and SK-N-SH (Baron andSiegel, 1989), were previously shown to exhibit alpha-2 adrenergicreceptors. In addition to being a second model expressing thealpha-2C subtype, SK-N-MC has the very interesting characteristicof coexpressing the alpha-2A subtype, making this cell line asuitable system to investigate the parallel regulation of thesetwo receptor subtypes in a single cell line of neural origin.According to estimations of the number of [³H]MK912 binding sites, the two subtypes are expressed in fairlysimilar amounts (20 ± 8 fmol/mg of protein for alpha-2A and 23± 3 fmol/mg of protein for alpha-2C). The results from the measurementof cAMP did not allow estimation of the respective contributionsof the two receptor populations to inhibition of cAMP production,but it is likely that both subtypes participate in this process.In comparisons of the results obtained in the three cell lines,it is also obvious that there is no direct correlation betweenthe amounts of mRNA for the different receptors and their respectivelevels of expression. Quantitative analysis of the data from RPAexperiments indicates, for example, that the amount of $alpha$ ₂C4 mRNAin SK-N-MC is about 100-fold lower than in HepG2, whereas bindingdata show that the alpha-2C receptor number in SK-N-MC is onlyhalf that in HepG2. In the same manner, the amount of $alpha$ ₂C10 transcriptsin HT29 is approximately 200 times higher than that in SK-N-MC,whereas the number of alpha-2A receptors is 10 to 15 times higher.The reasons for these differences were not investigated, but differencesin the translation efficacy and/or in the degradation rate ofthe receptor proteins may be at the origin of this apparent discrepancy.

With the exception of HT29 cells, which contain a small amount of $alpha$ ₂C2 gene transcripts but express none or undetectable tracesof the protein, our search for a human cell line expressing alpha-2Badrenergic receptors has been unsuccessful. In spite of this failure,surely due to the relatively limited number of cell types screenedin the current study, our work provides two new human models,which will certainly be valuable systems for the study of homologousand heterologous regulation of the alpha-2C adrenergic receptorsubtype in vitro.

	Footnotes

Accepted for publication January 6, 1997.

Received for publication September 20, 1996.

Send reprint requests to: Dr. Hervé Paris, INSERM U317, Institut Louis Bugnard, CHU Rangueil, Bat. L3, 31054 Toulouse Cedex, France.

	Abbreviations

bp, base pair(s); cAMP, cyclic AMP; DMEM, Dulbecco's modified Eagle's medium; GppNHp, 5 $'$ -guanylylimidodiphosphate; Hepes, 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid; MK912, (2S,12bS)-1 $'$ ,3 $'$ -dimethylspiro(1,3,4,5 $'$ ,6,6 $'$ ,7,12b-octahydro-2H-benzo[b]furo[2,3-a]quinazoline)-2,4 $'$ -pyrimidin-2 $'$ one; ORF, open reading frame; PCR, polymerase chain reaction; RT, reverse transcription; RPA, RNase protection assay; RX821002, 2-(2-methoxy-1,4-benzodioxan-2-yl)-2-imidazoline.

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