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GeneticInformationContentsofThis?TypeofDNA?DNARepair? ?SomethingneedsDNADNAofmutation
DNAIsConstantlyChangingthroughtheProcessofMutationlevel NaturalpolymeraseEndogenousDNAROS,ExogenousDNARadiation,Chemical 中的錯(cuò)堿基配對(duì)的錯(cuò)誤頻率約為10-4-10-聚合酶本身具有校對(duì)作用:將不正確插入的核苷酸切除掉,重新加上正確的核苷酸。這樣,每摻入一個(gè)核苷酸,發(fā)生錯(cuò)誤的機(jī)會(huì)有。EndogenousDNA腺嘌呤的稀有互變異體腺嘌呤的稀有互變異體與胞嘧胸腺嘧啶的稀有互變異構(gòu)體與鳥(niǎo)嘌異異構(gòu)體間自發(fā)地相互變化形成導(dǎo)致下一世代中G-C配對(duì)取代A-T配?堿基的環(huán)外氨基有時(shí)會(huì)自發(fā)脫落,從而胞嘧啶會(huì)變成尿嘧?胞嘧啶自發(fā)脫氨基的頻率約為每個(gè)細(xì)胞每天190?堿基的環(huán)外氨基有時(shí)會(huì)自發(fā)脫落,從而胞嘧啶會(huì)變成尿嘧?胞嘧啶自發(fā)脫氨基的頻率約為每個(gè)細(xì)胞每天190OO Nitrous DeaminationofcytosinetoMutationGenerationpassedontodaughterDNAs deletionpassedontodaughter堿基修每個(gè)哺乳類(lèi)細(xì)胞每天DNA單鏈斷裂發(fā)生的頻率約為5萬(wàn)次ChemicalTypesChemicalTypesofX-raysandX-raysandγ-raysstrandbreaks;base/sugardestructionUVlightUVlightpyrimidineg紫外線引起的DNA損(cyclobutanering)連成二聚體。260nm Disruptssynthesis;goodforsterilizationofbacteria,badforskinTypesofPhysicalChemical ogs:AlkylatingIntercalatingIntercalating DNAcanIncorporate5-BU ceofNote:changesaG-CpairintoanA-Tpair(G>Aisatransition,C>Tisatransition) EthylmethaneSulfonate(EMS)AlkylatesIntercalatingInsertionsorTheadditionorlossofoneormorebasesinaDNAFrameshiftTheORFofaproteinencodedgeneischangedsothattheC-terminalsideofthemutationiscomple ychanged.ThetranscriptsisdegradedviaNonsense-mediateddecay(NMD)pathwaysifitcontainsprematuretermination(stop)codons(PTCs)EffectsofPoint3rdpositionofa Silent CodingDNAalteredCodingDNAalteredCodingDNAstopCodingDNAstoptruncated
DNAreplication-independentproductionoferroneousTumorTwoStrikeselectivegrowthselectivegrowth
Smallchange,greatsecondroundsecondroundofclonalgrowththatallowsanexpansionofcellnumberOtherdrivergenemutation gene Mut-Drivercodinggenes74-64-~50%chromatin(modification)factors:HIST1H3B,H3F3A,DNMT1,TET1…...Epi-DriverGeneticHeterogeneityofl
Thejoiningofafragmentedchromosometoanon-homologouschromosomethebreakageofachromosomeinwhich eslostduringcell
ExtracopiesofgenesaregeneratedonathebrokenchromosomesegmentisreversedandinsertedbackintothechromosomeIsochromosomescontaineithertwoshortarmsortwolongarms,derivedfromimproperdivisionofthecentromere.ChromosomeNumberAneuploidyAneuploidy:Turnermassive,complexchromosomeNatureMedicine18,1630–1638Genome-widedistributionofsomaticDNACell.2012.148(1-2):DNADNARepairCellularCellularprotectionfromDNANaturalerrors:polymerasebaseselection,proofreading,mismatchrepairEndogenous/exogenousDNAdamage:Baseexcisionrepair,Nucleotideexcisionbination(DNAdoublestrandbreak)polymerasebypass(TranslesionDNAsynthesis)ProofreadingofDNAMostDNApolymerasescontain“proofreading”activity(3’to5’exonuclease)increasesfidelityofreplicationby100X.ProkaryoticMutSbindstoDNAatmismatchsiteMutLrecruitedbyMutLactsasmat betweenMutSandMutHMutHcreatesanick5’totheunmethylatedGATCsiteExonucleasedegradessectionofthestrandcontainingRecognizescorrectstrandbecauseitisunmethylatedGapinDNAisPhotoactivationRepairinPREbondbetweenPhotoreactivation(theenzymeDNApotolyasecapturesenergyfromlightDirectDirectTypesTypesoflesionsrepairedbyOxidativelesions;8-oxo-G,highlymutagenic,mispairswithA,producingGC-->TADeoxyuracil(dU):frommisincorporationofdUordeaminationofdC-->dU,Spontaneousdepurination(esp.G)yieldabasicsitesthatarerepairedbysecondhalfofBERRecognitionofunusualthrough“base out”recognizedbyDNAglycosylaseDNAglycosylaseleision-andhumancellshave8DNAglycosylaseswithdifferentBaseExcisionAPIfadamagedbaseisnotremovedbybaseexcisionbeforeDNAreplicationAfail-safeNucleotideExcisionNucleotideExcisionRecognitionofdoublehelixEnzymescleavedamagedDNAoneithersideofthelesionDNApolymeraseandligasefillinthegap.ModelforEukaryoticNucleotideExcisionRepair:XerodermaPigmentosum(XP) 性干皮病NERenzymeincludingXPA,XPC,XPDandXPFisassociatedwithbinationbinationTranslesionDNAsynthesis:CatalyzedbyaspecializedclassofDNApolymerasesthatsynthesizeDNAdirectilyacrossthesiteofthedamageCharacteristicsCharacteristicsoflesionbypassinresponsetoDNAdamageTheactivationofbinationPost-ReplicationRecA:交換DNA鏈EmergencyDNAEmergencyDNARepairforDoublestrand TheexchangeofhomologousregionsbetweentwoDNADeleteriousmutationswouldn’taccumulateineachbinationgeneratesgeneticdiversity;Criticalforantigenicvariation.Diploideukaryotes:crossingMitoticand binationcanoccurbothduringmitosisandmeiosisOnlymeiotic binationservestheimportantroleofreassortinggenes binationmaybeimportantforrepairofmutationsinoneofapairofsisterchromatidsThecross-strandHollidaystructureisanintermediatein bination(partI)Thecross-strandHollidaystructureisanintermediatein bination(partII) lian RecBCDexonuclease:opensRecBCDRecBCDexonuclease:opens3’Uponrecognitionofχ,the3’to5’nucleaseactivityisattenuated,aweaker5’to3’nucleaseactivityisactivatedontheoppositeTheundegraded3’end
RecA:neededtoformRecA:neededtoformtriple cedstrandbindstooriginalcomplementarystrandoftheinvasivestrandtocreateHollidayHollidayEfficientbranchmigrationrequiresRuvAandEfficientbranchmigrationrequiresRuvAand-resultantstructurebetterabletoundergobranchmigrationandRuvB:formsahexamericringaroundtheDNADNAispumpedthroughtheringusingATPcleavagetodrivethethesynapseis dto RuvC:RuvC:specificallycuttingtheHollidayRuvCisaspecializedresolvethecrossedtheHollidayBreakRepair3’ssDNAGeneGeneTLoxP:34bp:8-bpTLoxP:34bp:8-bpsequenceflankedby13-bpinvertedDeletionofloxP-flankedTissue-SpecificTissuespecific ConditionalKnockoutTissuespecific Silencingthe3rd21#chromosomeusingNature,2013(500):296-clusteredregularlyinterspacedshortpalindromicrepeats(CRISPR)/CRISPR-associated(Cas)systemsNature,2013(495,)GN(20) MovingMcClintock,1983NobelPrizeinMedicineor geneticelementsfoundinIStransposasegeneflankedbyashortinvertedterminalrepeatsTn:transpositionelementsandadditionalshortinvertedterminalrepeatsCutandPasteTranspositionDuplicative like
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