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Asian Pacific Journal of Cancer Prevention, Vol 13, 2012 1349

DOI:http://dx.doi.org/10.7314/APJCP.2012.13.4.1349 Up-regulation of Thy-1 Promotes Invasion and Metastasis of Hepatocarcinomas

Asian Pacific J Cancer Prev, 13, 1349-1353

Introduction

Hepaticarcinoma is the fifthmost common cancerandoneoftheleadingcausesofcancerdeathworldwide.EspeciallywithquickdevelopmentofliverdiseaseduetohepatitisBvirusinfection,incidenceofhepaticarcinomahasbeenontheriseandearlierrecurrenceafteroperationorlivertransplantiscommon.Theunderlyingrootcauseistheexistenceofcancerstemcells(CSCs)(Shupeetal.,2005;Selletal.,2008;Alisonetal.,2009;Chibaetal.,2009;Leeetal.,2009),which,despitetheirsmallnumber,play amajor role in tumor origination, development,invasionandearliermetastasis(Reyaetal.,2001;Couzinetal.,2003).Ovalcellsarethestemcellsofliver(Birdetal.,2008;Strick-Marchandetal.,2008;Okabeetal.,2009;Shupeetal.,2009).Recentlyagreatdealofresearchsuggestedapositiverelationshipbetweenitsproliferationand the incidence of hepaticarcinoma (Alison et al.,2005;Alisonetal.,2006;Wuetal.,2006).Thy-1,asamarkerproteinofovalcells,hasrecentlybeensuggestedtoplayaroleinpotentiallivercancerstemcells(Dahlkeetal.,2003;Ceafalanetal.,2005;Massonetal.,2006;Yang et al., 2008;Yang et al., 2008;Xu et al., 2009).As a gene expressed during embronic period or underpathologicstate,AFP(alphafetoprotein)participatesinDepartment of Hepatology Center, Fuzhou General Hospital, Nanjing Military Area Command, Fuzhou, China *For correspondence: [email protected]

Abstract

Increasing evidence has revealed that thy-1 was a potential stem cell marker of liver cancer, but no data have been shown on how thy-1 regulates the pathophysiology of liver cancer, such as proliferation, apoptosis, invasion and migration. We previously demonstrated that thy-1 was expressed in about 1% of hepg2 cells, thy-1+ hepg2 cells, but not thy-1-, demonstrating high tumorigenesis on inoculation 0.5x105 cells per BACA/LA mouse after 2 months. In the present study, our results showed that higher expression of thy-1 occurs in 72% (36/50 cases) of neoplastic hepatic tissues as compared to 40% (20/50 cases) of control tissues, and the expression of thy-1 is higher in poorly differentiated liver tumors than in the well-differentiated ones. In addition, thy-1 expression was detected in 85% of blood samples from liver cancer patients, but none in normal subjects or patients with cirrhosis or hepatitis. There was a significant negative correlation between thy-1expression and E-cadherin expression (a marker of invasion and migraton), but not between thy-1 expression and AFP expression in all the liver cancer and blood samples. We further investigated the relationship between thy-1 and E- cadherin in liver cancer hepg2 cell line which was transfected with pReceiver-M29/thy-1 eukaryotic expression vector followed by aspirin treatment. Lower expression of E- cadherin but higher expressions of thy-1 were detected in hepg2 cells transfected with pReceiver-M29/thy-1. Taken together, our study suggested that thy-1 probably regulates liver cancer invasion and migration. Keywords: Invasion-migration-thy-1-hepatocarcinomas

RESEARCHCOMMUNICATION

Up-regulation of Thy-1 Promotes Invasion and Metastasis of HepatocarcinomasBian-Qiao Cheng, Yi Jiang*, Dong-Liang Li, Jing-Jing Fan, Ming Ma

embryonicdevelopmentandcelldivisionprocess(Kanget al., 2006).Recent research suggested (Kuhlmann etal., 2006)AFPpossessed stem cell characteristics andcouldberegardedasanidealmarkerpredictingearlierliver cancer recurrence after operation.However, theshortcoming ofAFP loss expression in some samplesrequiredamoreaccurateandspecificmarkertopredictlivercanceroccurrenceandrecurrenceindependentoforincombinationwithAFPmarker.E-cadherin,amemberofcadherinfamily,mediatescell-celladhesionsanditslossoffunctioncouldcausebreakdownofcell-cellconjunctions.It is therefore commonlyused to predict invasion andmetastasis of variouskindsofmalignant tumor.Basedonfindingsabove,thisarticlewasaimedtoinvestigatetherelationshipbetweenthy-1,AFPandE-cadherinandtounravelthefunctionofthy-1inhepaticarcinoma.

Materials and Methods

Cell lines Thehumancelllinehepg2(ATCC,American)wasmaintainedinRPMI1640medium(Hyclone,American)containing10%fetalbovineserum(Hyclone,American)and1%penicillinat37°Cinahumidifiedincubatorwith5%CO2.

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Patients and sample collection Fifty paraffin-embedded tissueswith liver cancerwho had undergone laparotomy (46/50 had curativehepaticresectionand4/50hadlivertransplation;18/50well-differentiated and 32/50 poorly differentiated)were included in the study. Pathology diagnosiswasmade according to the histology of tumor specimensand examinations were performed by experiencedpathologists.Fiftycorrespondingperi-tumoroushealthytissueswere used as controlswhichwere confirmedaccordingtopathologicaldiagnosis.ThemajorityofHCC(53cases)andcirrhosisorhepatitispatients(36cases)werepositiveforserumhepatitisBsurfaceantigen.AllthebloodsamplestudieswereapprovedbytheInstitutionalReviewBoardofthefuzhougeneralhospital.

Immunohistochemistry and Immunocytochemistry Immunohistochemical evaluation on 4mm-thintissue sections from formalin-fixed and paraffin-embeddedsampleswasperformedforthy-1(sc-53456,dilution1:200; SantaCruzBiotechnology Inc., SantaCruzCA),AFP(sc-51506, dilution1:200; SantaCruzBiotechnologyInc.,SantaCruzCA;),E-cadherin(sc-8426,dilution1:200; SantaCruzBiotechnology Inc., SantaCruzCA).Thestainingreactionswereinterpretedinthepresenceoftissuemastcellsinportalfieldsoftheliverasinternalcontrols,whileAFPandE-cadherinasexternalcontrolsforembryonictissuesandbreastductcarcinomarespectively. Stainingwasperformedaccordingaspermanufacturer’sinstructions of vltrasensitiveTMS-P (mouse/rabbit) kit(Maixin, Fujian China). Briefly, paraffin-embeddedsectionswere deparaffinized and rehydrated throughgraded alcohols to phosphate buffered saline (PBS).0.01Mcitratebuffersolution(pH6.0)wasusedinantigenrecovery.Aftersequentialincubationwith3%endogenousperoxidaseblockingsolutionand1%normalnonimmuneserum, 10min for each at room temperature, primaryantibodieswereincubatedovernightat4°C.Anti-mouseIgGwasusedinsteadofprimaryantibodyasadditionalcontrol.Other negative controls included theomissionof either primaryor secondary antibodies.Nonspecificreactionsweredetectedinthenegativecontrols.AccordingtoFromowitzscorestandard,whenthereweredifferentdifferentiationdegreeinthesamesample,predominateareawasselected(Fromowitzetal.,1987)accordingtopositivestainingpercent,scorewasclassifiedasfollows:0: ≤ 25%; 1: 26%~50%; 2: 51%~75%; 3: > 75%. Inaddition, staining intensitywas rated as 0 (negative),1 (weakly positive), 2 (intermediate) and 3 (stronglypositive).Finally,asummationofthetwoscoresabovewas furtherclassified into:0:negative;1~2:“+”;3~4:“++”;5~6:“+++”(Jawharietal.,1997).

Immunocytochemistry HepG2 cellswere plated at 100,000 cells perwellonenightbeforetheexperiment.BreastcarcinomacelllineDBA-DA231 andun-transfected hepg2 cellswereused as positive and negative controls respectively.Hepg2cellswere transfectedwithpReceiver-M29/ thy-1expressionvectorandtreatedwithAspirininthetest

group according to themanufacturer’s instructions ofvltrasensitiveTMS-P(mouse/rabbit)kit(Maixin,FujianChina).Briefly,cellswerefixedin4%paraformaldehydefor10minandpermeabilizedwith0.3%Triton-100for10min.Thefollowingstepswereperformedinthesamewayasimmunohistochemistry.

Immunosorbent assay Thy-1,AFPandE-cadherinELISA.wereperformedusingELISAkit(R&D)aspermanufacturer’sinstructions.Briefly,50µlstandardor50µlof1:5dilutedsampleswasdispensedtostandardorsamplewells,respectively.Thrityminutesaftertheadditionof50µlenzymelabelreagentat37°C,chromogenicagentAandBwereaddedtoreactfor10minat37°Cwithprotectionfromlight,followingwhichstopbufferwasadded.Thereafter,theabsorbanceat450nmwasmeasuredwithanenzyme-labelinginstrument(ELX-800type).

RT-PCR Experiments were performed using RT-PCR kit(TakaRa,code:DRRO14A).TotalRNAwasisolatedwithtrizol reagent (Invitrogen,Cat: 15596-026) accordingto themanufacturer’s instructionsusing1ml trizol per1*107 cells.TotalRNA concentrationwas quantifiedwith eppendorf Bio photometer. The cDNAsweregenerated from 5 µg of totalRNAper sample using20µl reaction containing 1µl random6 primers, 1µldNTPmixture,0.5µlprimeScripTMRtaseand0.5µlRNaseinhibitor.Gene-specificprimesforthy-1(primerA:5’-AAGGTGACCAGCCTAACGG-3’,primerB:5’-CCCTCGTCCTTGCTAGTGAA-3’),forβ-actin(primerA: 5’-GGAAATCGTGCGTGACATT -3’, primerB:5’-CGTCATACTCCTGCTTGCTG-3’),andforE-cadherin(primerA:5’-CGCCGACGAGAGCTACACGTTCA-3’,primerB:5’-CCCAGGCGTAGACCAAGAAA-3’)weredesignedusing the primer 3 software and synthesized(ShanghaiBiologiccompany,China).

Statistical analysis Descriptive statistics, t-test, χ2 test andOne-wayANOVAwithLSDmultiplecomparisonwereperformed.Fisherpreciseprobabilisticmethodwasusedtoanalyzeexpressionintensity,Spearmanforcorrelationanalysis.SPSS software (version 11.5 forWindows; spss Inc.,Chicago,IL)wasusedforallstatisticalanalyses.Pvaluelessthan0.05wasconsideredsignificant.

Results

Altered expression pattern of thy-1,AFP andE-cadherin in liver cancers. Immunohistochemicalstainingshowedreactivitiesofthy-1,AFPandE-cadherinin 40%, 20%, and30%of peritumoral normal tissues,whereas72%,76%and64%ofneopastic liver tissuesrespectively.Staining intensities for thy-1 andAFPin normal peritumoral samples were significantlyweaker than in tumorsamples,butE-cadherinstainingshowedtheoppositeresults(Figure1).Inaddition,wedetectedasignificantcorrelationbetweenthedegreeofdifferentiationofhepatocarcinomasandtheexpressionof



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Figure 1. Immunohistochemical Staining of Thy-1, AFP and E-cadherin in Hepatocarcinoma and Peritumoral Normal Liver Samples. (a) Peritumoral normal tissuesdemonstratingweakAFP reactivity (magnification 200x).(b)Hepatocarcinoma exhibiting strong expression ofAFP(magnification200x). (c)Hepatocarcinoma exhibiting strongexpression of thy-1 (magnification 200x). (d) Peritumoralnormal liver tissues revealing intermediate thy-1 expression(magnification 100x). (e) Liver cancer cells demonstratingweaker expressionofE-cadherin (black arrow) compared tohigherexpressioninnormaltissues(redarrow)(magnification200x).(f)BreastcancerascontrolexhibitingstrongexpressionofE-cadherin(magnification200x)

Figure 2. RT-PCR Analysis of Thy-1 mRNA and E-cadherin mRNA Expression. (a)Expressionofthy-1wasincreasedinpReceiver-M29/Thy-1transfectedhepg2cellsbutdramaticallyreducedaftertreatmentwithAspirin.(b)E-cadherinexpressionwaslowestininpReceiver-M29/Thy-1transfectedhepg2cellsbutslightincreasedwithAspirintreatment

Figure 3. Immuocytochemical Staining for E-cadherin in Hepg2 Cells after Differenct Treatments. (a)E-cadherinstaininginnon-transfectedhepg2cells(magnification200x).(b)ObviouslyweakerstainingforE-cadherininhepg2cells transfectedwith pReceiver-M29/thy-1 (magnification200x). (c) Slightlyweaker staining in pReceiver-M29/thy-1hepg2 transfected cells treatedwithAspirin (magnification200x).(d)E-cadherinstaininginbreastcancerDAB-DA231cells(magnification200x)

Table 2 Correction Between thy-1 and AFP, E-cadherin by Immunohistochemistry Proteinofinterest Thy-1 rs p + _

AFP + 27 7 0.116 0.421 _ 11 5 E-cadherin + 18 16 -0.336 0.117 _ 14 2

Table 1 Immunohistochemical Reactivity in Liver Cancers and Peritumoral Nomal Tissues proteinofinterest tumorperitumousWellPoorly -differentiateddifferentiated (n=50)(n=50)(n=18)(n=32)

Thy-1 36 20 7 26AFP 38 10 7 22E-cadherin 32 15 15 17

Table 3 Correction Between thy-1 and AFP, E-cadherin by ELISA groups Serum(U/ml)rsp

Thy-1 3.694 2.961 E-cadherin 1.591 -0.334 0.027 0.696 AFP 3.121 0.046 0.746 1.965

thy-1,AFPandE-cadherin,wherebypoorlydifferentiatedhepatocarcinomasweremorelikelytoexpressthy-1andAFP but less likely to expressE-cadherin thanwell-differentiated ones (poorly differentiated: thy-1,AFPandE-cadherinexpressed in81.2%,68.8%and53.1%ofsamplesrespectively;well-differentiated:thy-1,AFPandE-cadherinexpressedin38.8%,38%and83.3%ofsamplesrespectively)(Table1). Lack of correlation between thy-1 andAFP, butnegative correlation between thy-1 and E-cadherin.

Bothpositiveexpressionsamplesornegativefor thy-1andAFPwas 27or 5, Positive expression samples forthy-1of7casesbutnegative1forAFPandnegative11forthy-1butpositiveforAFPwasalsoobserved,therewas no significant difference between them (rs=0.116,p=0.421).Both positive expression samples for thy-1andE-cadherinwas18,bothnegative for themwas2,positive for thy-1was 16 but negative forE-cadherinwas14,negativecorrelationwasdetectedbetweenthem(rs=-0.336,p=0.017)(Table2).Inaddition,from53livercancerserumsamples,levelsofthy-1,AFPandE-cadherindetectedwere3.6942.961,3.1211.965,and1.5910.696respectively.No correlationwas found betweenAFPandthy-1(rs=0.046,p=0.746),buttherewasanegativecorrelation between thy-1 andE-cadherin (rs=-0.334,p=0.027)(Table3). EnhancedThy-1 expression reduces E-cadherinlevel. In order to further understand the relationship

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betweenThy-1 andE-cadherin,we transfected hepg2cellswith pReceiver-M29/thy-1 expressionvector andlookedforchangesinexpressionofE-cadherinandthy-1usingRT-PCR.Immunocytochemistryrevealedhigherexpressionof thy-1but lowerexpressionofE-catherinin pReceiver-M29/thy-1 transfected hepg2 cells ascomparedtonon-transfectedhepg2cellsanddifferencesinexpressionlevelswerestatisticallysignificant(p



early invasion/metastasis of liver cancer are complexprocesses.Therefore, understanding detailed actionsof thy-1 inhepatocarcinomaanddesigning therapeuticstrategies such asRNAi or gene knock-out directedtowardsthy-1wouldholdpromiseforfuturelivercancertherapy.

Acknowledgements

ThebreastcarcinomaDAB-DA231cellswerekindlyprovidedbyQiao-JiaHuangofDepartmentofLaboratoryInstitute, FuzhouGeneralHospital,NanjingMilitaryDistrict,Fuzhou,China.

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