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Xenobiotic-dependent regulation of gene expression in human placental cell lines PDF

128 Pages·1996·3.1 MB·English
by  ZhangLiyan
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Preview Xenobiotic-dependent regulation of gene expression in human placental cell lines

XENOBIOTIC-DEPENDENTREGULATIONOFGENEEXPRESSIONINHUMAN PLACENTALCELLLINES BY LIYANZHANG ADISSERTATIONPRESENTEDTOTHEGRADUATESCHOOL OFTHEUNIVERSITYOFFLORIDAINPARTIALFULFILLMENT OFTHEREQUIREMENTSFORTHEDEGREEOF DOCTOROFPHILOSOPHY UNTVERSrTYOFFLORIDA 1996 ThisdissertationisdedicatedtoYukun,andalsotomyparents,brothersandsisters. ACKNOWLEDGEMENTS I would like to sincerely thank my mentor, Dr. Kathleen Shiverick, for her guidanceandpatiencethroughoutthecourseofthecompletionofthiswork. WhatIhave gained in knowledge and capability under her direction, I will carry with me into a hopefullylong-lastingcareerinscience. I also wishtorespectfully thankthe members ofmydissertationcommittee,Dr. Stephen Baker, Dr. Thomas Rowe, Dr. Jeffrey Harrison, Dr. Margaret James and Dr. RosaliaSimmen, fortheiradviceandsupport. Iwishtoalsothankthepastandpresent membersofDr. Shiverick's laboratory, includingTerryMedrano,Grantly Charles, Paul Saunders,Dr.ScottMasten,Dr.MaryVaccarello,Dr.YaraSmit,andDr.PhyllisConliffe for their help and for providing a pleasant working atmosphere. I would also like to expressmyappreciationtomyfellowgraduatestudentsandallthefacultymembersinthe DepartmentofPharmacologyfortheirhelpandfriendship. Mysincerethanksalsogoto the administrative staffof the Department ofPharmacology, especially Judy Adams, BarbaraReichert,CookieMundorff,DonnaDesmond,andPatsyMessinger. In addition, I would like to acknowledge the following people for providing materialsorinstrumentsessentialtothecompletionofthisresearch:Dr.ThomasRowe,Dr. PaulKlein, Dr. WilliamGreenlee,Dr. OliverHankinson,Dr. ChristopherBradfield, and Dr.StephenSafe. Finally,Ithankmyhusband,Yukun,forstandingbymeasIfollowedmydream, andmyparentsandparents-in-lawfortheirloveandsupport. TABLEOFCONTENTS ACKNOWLEDGEMENTS iii KEYTOABBREVIATIONS vii ABSTRACT ix CHAPTER INTRODUCTION 1: 1 HumanPlacenta:APrimaryTargetOrganofCYP1A1 Inducers 1 TheObjectiveofThisStudy 2 CulturedPlacentalCells:AnInVitroModelfortheStudyofFetoplacental Toxicity 3 GeneralCharacterizationoftheMechanismsofActionofTCDDandBaP 4 AhReceptor 4 MetabolicActivation 5 EGF Receptor: A Possible Marker of Placental Toxicity 5 TCDD-responsive Growth Control Genes 7 Trophoblast Growth Control Factors 10 TGF-a 10 TGF-pi 11 c-Myc 12 PAI-2 13 CHAPTER2:MATERIALSANDMETHODS 15 Materials 15 Chemicals and Bioreagents 15 RecombinantcDNAClones 16 AntibodiesandELISAKits 16 Methods 17 CellCultureandChemicalTreatment 17 EGF Binding Assay 17 Western Immunoblot Analysis 18 GeneralProcedure 18 CYP1A1 Protein 18 EGFReceptorProtein 18 c-MycProtein 19 RNAIsolationandNorthernBlotAnalysis 19 NuclearRun-offAssay 20 mRNAStabilizationAssay 21 ELISAforSecretedProteins 21 TGF-pi Assay 21 hCGAssay 22 CellProliferationAssay 22 MTTAssay 22 3H]ThymidineIncorporationAssay 23 [ InVitroInvasionAssay 23 ProteinAssay 24 DataAnalysis 24 CHAPTER3:EVIDENCETHATTHEHUMANPLACENTALCELLLINES BEWOANDJEG-3HAVEAFUNCTIONALAHRECEPTORSYSTEM 25 Introduction 25 Results 26 ExpressionofAhReceptorandArntmRNAinBeWoandJEG-3Cells 26 SuperinductionofCYP1A1 mRNAandStructure-ActivitySpecificity 27 InductionofCYP1A1 Protein 27 Discussion 28 CHAPTER4:EFFECTSOFTCDDANDBAPONEGFRECEPTOR EXPRESSION 34 Introduction 34 Results 35 EffectsofTCDDandBaPonSpecificBindingof125I-EGFtoBeWo andJEG-3Cells 35 Effects ofTCDD and BaP on EGF Receptor Protein 36 RelationshipbetweenCYP1A1 InductionandEGFReceptorChanges 37 EffectsofActinomycinDandCychloheximideonBaP-Mediated ChangesinEGFReceptors 38 EffectsofTCDDandBaPonSteadyStateEGFReceptormRNA Levels 38 Discussion 39 CHAPTER5:EFFECTSOFTCDDANDBAPONTGF-a,TGF-P1,C-MYC ANDPAI-2GENEEXPRESSION 56 Introduction 56 Results 57 EffectsofTCDDandBaPontheSteadyStatemRNALevelsforTGF- a,TGF-pi,PAI-2andc-myc 57 EffectsofTCDDandBaPontheRateofTGF-p1 andc-mycGene Transcription 58 EffectsofBaPon the StabilityofTGF-pl and c-myc mRNA 59 EffectsofTCDDandBaPonTGF-p1 andc-MycProteinLevels 60 Discussion 60 CHAPTER6:EVALUATIONOFTHEEFFECTSOFTCDDANDBAPON CELLULARGROWTHANDENDOCRINERESPONSESOFBEWOAND JEG-3 CELLS 77 Introduction 77 Results 77 EffectsofTCDDandBaPonCellProliferationasMeasuredbythe MTTConversionAssay 77 EffectsofTCDDandBaPonJEG-3CellProliferationasMeasuredby 3H]Thymidine Incorporation and Cell Number Changes 78 Effe[ctsofTCDDandBaPonBeWoCellProliferationasMeasuredby 3H]Thymidine Incorporation 79 [ EffectsofTCDDandBaPonSecretionoftheHormonehCG 79 DifferentialEffectsofTCDDandBaPonJEG-3Cell Invasiveness 80 Discussion 80 CHAPTER 7: CONCLUSIONS AND FUTURE DIRECTIONS 95 LISTOFREFERENCES 103 BIOGRAPHICALSKETCH 115 KEYTOABBREVIATIONS AD actinomycinD Ah arylhydrocarbon AhR arylhydrocarbonreceptor Arnt arylhydrocarbonreceptornucleartranslocator oc-NF a-naphthoflavone BaP benzo(a)pyrene BPDE benzo(a)pyrene-7,8-diol-9,10-epoxide BSA bovineserumalbumin c-myc celluarmycgeneorribonucleicacid c-Myc c-myconcoprotein cDNA complementarydeoxyribonucleicacid CHX cycloheximide CYP1A1 cytochromeP450 1Al DMSO dimethylsulfoxide DNA deoxyribonucleicacid DRE/XRE dioxinresponsiveelement/xenobioticresponsiveelement DTT dithiothreitol ECM extracellularmatrix EGF epidermalgrowthfactor EGFR epidermalgrowthfactorreceptor ELISA enzyme-linkedimmunosorbentassay FBS fetalbovineserum HCB 2,2',4,4',5,5'-hexachlorobiphenyl hCG humanchorionicgonadotropin hi hours IGF-II insulin-likegrowthfactorII IGFBP insulin-likegrowthfactorbindingprotein kb kilobases kd dissociationconstant kDa kilodaltons MMP matrixmetalloproteinase MNF 3'-methoxy-4'-nitroflavone mRNA messengerribonucleicacid PAI plasminogenactivatorinhibitor PBS phosphate-bufferedsaline PCB polychlorinatedbiphenyl PCDF polychlorinateddibenzofurans PDGF platelet-derivedgrowthfactor PMSF phenyl-methylsulfonylfluoride RNA ribonucleicacid SE standarderror SDS-PAGE sodiumdodecylsulfatepolyacrylamidegelelectrophoresis TCB 3,3',4,4'-tetrachlorobiphenyl TCDD 2,3,7,8-tetrachlorodibenzo-p-dioxin TGF transforminggrowthfactor TIMP tissueinhibitorofmetalloproteinases t-PA tissueplasminogenactivator u-PA urokinaseplasminogenactivator AbstractofDissertationPresentedtotheGraduateSchool oftheUniversityofFloridainPartialFulfillmentofthe RequirementsfortheDegreeofDoctorofPhilosophy XENOBIOTIC-DEPENDENTREGULATIONOFGENEEXPRESSIONINHUMAN PLACENTALCELLLINES By LiyanZhang December1996 Chairman: KathleenT.Shiverick MajorDepartment: PharmacologyandTherapeutics This study evaluated the usefulness of human placental trophoblastic choriocarcinoma cell lines BeWo and JEG-3 to study the effects of the prototype environmental chemicals on the expression ofimportant trophoblast growth regulatory genes. The environmental chemicals studied are the aryl hydrocarbon (Ah) receptor agonists, 2,3,7,8-tetrachlorodibenzo-/>-dioxin (TCDD) andbenzo(a)pyrene (BaP). The placentalgenesunderstudyincludethegrowthfactors,transforminggrowthfactor(TGF)- a, TGF-fjl and the epidermal growth factor (EGF) receptor, the proteinase inhibitor, plasminogenactivatorinhibitor(PAI)-2,andtheprotooncogene,c-myc. Thisstudy first demonstratedthatbothcelllinespossessafunctionalAhreceptorsystemasevidencedby CYP1A1 inductionfollowingTCDDandBaPexposure. Secondly,inductionofCYP1A1 does not appearto be directly linked with loss ofEGF receptor. BaP decreased EGF receptorbinding and protein in both cell lines, without affecting EGF receptor mRNA level. TCDD,however,wasnotfoundtoaltertheEGFreceptorexpressionineithercell line. Thirdly, significant dysregulation of TGF-p"1 and c-myc gene expression was observedwithBaPbutnotTCDDinJEG-3cells. BeWocellsprimarilyshowedeffectsof both chemicals on hCG secretion, BaP on TGF-[}1 and TCDD on TGF-a expression. Finally, BaPhasbeen shown toinhibitchoriocarcinomacell proliferation andinvasion, whereasTCDDincreasedcellinvasionwithoutaffectingcellproliferation. In summary, BaP-mediated changes in EGF receptor, TGF-pM and c-myc expressionwerecorrelatedwithalteredtrophoblastproliferationandinvasiveness. These alteredprocessesmayunderliemechanismsbywhichxenobioticssuchasthosefoundin cigarettesmokedisruptplacentalfunctionandleadtofetalgrowthretardation. Dataalso indicatethatTCDDandBaPproduceplacentaltoxicitythroughdifferentmechanisms. In addition, this study supports the feasibility ofusing the BeWo and JEG-3 cell lines to investigatebiomarkersandmechanismsofplacentaltoxicity.

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