简介:目的:构建4E—BPl及其T37A、T46A、$65A、T70A突变体4E—BPl-4A基因表达的重组慢病毒载体,研究其对胃癌HGC27细胞生长的影响。方法:PCR扩增4E—BPl基因及其突变体aE—BPl-4A基因并克隆到pCDH载体,构建成pCDH-4E—BPl、pCDit一4E—BPl—4A,将其-9包装载体共转染293T细胞,包装成Lenti-4E—BPl及Lenti-4E—BPl—4A重组慢病毒载体,将此慢病毒感染胃癌HGC27细胞,Western印迹鉴定病毒载体介导的4E—BPl、4E~BPl—4A蛋白的表达,MTT、克隆形成和软琼脂方法研究过量表达4E—BPl、4E—BPl—4A对胃癌HGC27细胞生长的影响。结果:包装成Lenti-4E—BPl及Lenti-4E—BPl—4A重组慢病毒载体,并将此慢病毒载体感染胃癌HGC27细胞;MTT、克隆形成、软琼脂实验表明过量表达4E—BP!可抑制胃癌HGC27细胞的生长,过量表达4E—BP!一4A时抑制效果更明显。结论:构建了4E—BPl、4E—BPI-4A的重组慢病毒表达载体,在胃癌HGC27细胞中过量表达4E—BPl可抑制细胞生长,过量表达4E—BPl-4A的抑制效果更明显。
简介:Mammaliancelltotipotencyisasubjectthathasfascinatedscientistsforgenerations.AlonglastingquestionwhethersomeofthesomaticcellsretainstotipotencywasansweredbythecloningofDollyattheendofthe20thcentury.Thedawnofthe218thasbroughtforwardgreatexpectationsinharnessingthepoweroftotipotentcyinmedicine.Throughstemcellbiology,itispossibletogenerateanypartsofthehumanbodybystemcellengineering.Considerableresourceswillbedevotedtoharnesstheuntappedpotentialsofstemcellsintheforeseeablefuturewhichmaytransformmedicineasweknowtoday.Atthemolecularlevel,totipotencyhasbeenlinkedtoasingulartranscriptionfactoranditsexpressionappearstodefinewhetheracellshouldbetotipotent.NamedOct4,itcanactivateorrepresstheexpressionofvariousgenes.Curiously,verylittleisknownaboutOct4beyonditsabilitytoregulategeneexpression.ThemechanismbywhichOct4specifiestotipotencyremainsentirelyunresolved.Inthisreview,wesummarizerethestructureandfunctionofOct4andaddresstoOct4functioninmaintainingtotipotencyorpluripotencyofembryonicstemcels.
简介:甘薯(Ipomoeabatatas(L.)Lam.)作为世界上一种重要的粮食、饲料、工业原料及新型能源作物,从有性生殖F1选择优良实生系进行选择育种一直是甘薯育种的重要方式。为了优化甘薯杂交育种方法,合理选配杂交组合,提高育种效率,本试验利用SSR标记研究了甘薯杂交群体基于SSR标记及13个农艺性状的遗传多样性,得到了群体内的聚类图,并且筛选出了甘薯的高产株系。群体SSR标记的聚类分析结果显示,群体材料与各亲本遗传距离比较远,被聚为3类,而亲本单独聚在另外一类。13个农艺性状的聚类将亲本与部分群体材料聚在了一起,且将群体材料和亲本材料作为一个整体时,其遗传距离的变异高达30%以上,远远高于SSR标记所获得的遗传变异系数。
简介:目的:利用慢病毒载体建立稳定表达猪载脂蛋白BmRNA编辑酶催化多肽样蛋白3F(pAPOBEC3F,简称pA3F)的PK15细胞系。方法:以实验室前期构建的pBPLV-flag-pA3F质粒为模板,PCR扩增pA3F基因,克隆到pLenti-Puro-3Flag载体构建成pLenti-Puro-pA3F-3Flag质粒,Western印迹鉴定其在HEK293T细胞中的表达;将pLenti-Puro-pA3F-3Flag质粒与包装载体共转染HEK293T细胞,包装成Lenti-pA3F慢病毒并测定病毒滴度;将Lenti-pA3F慢病毒感染PK15细胞,通过嘌呤霉素压力筛选并结合有限稀释法,筛选稳定表达pA3F的细胞单克隆株,最终Western印迹检测细胞单克隆株中pA3F的表达。结果:菌落PCR和序列测定表明pLenti-Puro-pA3F-3Flag质粒构建正确,Western印迹显示该质粒可在HEK293T细胞中表达pA3F蛋白;包装了Lenti-pA3F慢病毒,滴度为1.32×10^8TU/mL,慢病毒感染PK15细胞后可检测到pA3F蛋白的表达;经Western印迹鉴定,筛选得到的单克隆细胞可稳定表达pA3F蛋白。结论:建立了稳定表达pA3F的PK15细胞单克隆株,为进一步深入研究猪内源性反转录病毒在pA3F作用下的免疫逃逸机制奠定了基础。
简介:目的:探讨氟代脱氧葡萄糖((18)F-FDG)正电子发射断层显像/X线计算机体层成像仪(PET/CT)检查在局灶早期宫颈癌中的临床应用价值。方法:53例病理确诊为早期宫颈癌的患者行全身~(18)F-FDGPET/CT检查,并在检查结束10日内行广泛性全子宫切除术+双附件切除术+盆腔淋巴结清扫术,计算(18)F-FDGPET/CT诊断宫颈原发部位肿瘤及盆腔淋巴结转移的敏感度,特异度与准确度。结果:(18)F-FDGPET/CT检查诊断的宫颈原发部位肿瘤的敏感度为79.25%,特异度为86.79%,准确度为84.9%;以病人为单位诊断盆腔淋巴结转移的准确度为85.71%,特异度为97.87%;以淋巴结为单位诊断盆腔淋巴结转移的准确度为84.61%,特异度为99.00%。结论:PET/CT显像对宫颈癌诊断,分期诊断及盆腔淋巴结转移的检出具有重要临床意义。
简介:选择适合于HAb18F(ab′)2片段抗体的冻干保护剂及其冻干工艺,是确保该生物制品的质量关键之一,对不同种类和不同浓度的保护剂进行了研究,结果表明10%蔗糖对HAb18F(ab′)2片段抗体冻干样品的剂型、外观、残水量(<3%)、复溶时间(<10s)、纯度(>95%)及稳定性没有影响.研究优化与保护剂相结合的适用于HAb18F(ab′)2片段抗体的最佳冻干工艺,为抗体片段扩大生产提供依据.
简介:InteractionbetweencytotoxicTlymphocyte-associatedantigen-4(CTLA4,CD152)andB7molecules(B7-1andB7-2)isofimportanceinthecellulareventsoflymphocyte,includingantigen-specificT-cellactivationandinductionofautoreactiveT-cell.WedescribehaerethefirstintroductionofamurinesolubleCTLA4gene,CTLA4Ig,toMm1cells,amacrophagiccellline.CTLA4IgwassuccessfullyexpressedonMm1cellsandtheexpressedCTLA4IgwasfoundtobefunctionallyactiveintheirbindingtoB7moleculesbyflowcytometryandimmunofluorescencestudies.ThebiologicalactivityofCTLA4IgfromthetransfectedMm1cellswasstudiedandshowedinhibitoryactivityonmixedlymphocyteculture.AhighCTLA4Igproducingmacrophagiccelllinewasobtained.AsMm1cellswereregardedasdifficultforgenetransfectionandtherehassofarbeennoreportonexpressionofCTLA4IggeneonMm1cells,theseresultssuggestedthattheCELA4IgexpressingMm1cellscouldbeusefulforanalysisofCTLA4andB8moleculeinteractioninbothmacrophageandT-cell.
简介:Trichosanthin(TCS)isapotentallergentomice.Accordingtoourpreviousexperiments,itcouldbringouttheIgEresponsetoovabumin(OVA)ifTCSwasgivenonedaybeforeOVAimmunization,whileOVAalonecouldnotinduceIgEtoit.Inthiswork,thekineticsofinterleukin4(IL-4)andinterferonγ(IFN-γ)geneexpressioninthemesentericlymphnode(MLN)ofTCS-immunizedmicewasinvestigatedusingasemi-quantitativeRT-PCRmethod.ItindicatedthatTCSinducedsignificantIL-4geneexpressionandthepeaksofIL4geneexpressionwereondayoneafterTCSimmunizationinbothprimaryandsecondaryresponse.Incontrast,theIFN-γgeneexpressionwassuppressed.Furthermor,theIL-4geneexpressioninthesecondaryresponsewaslowerthanthatintheprimaryresponse.ThusthepresenceofIgEmemoryBcellswerestudied.ResultsshowedthattheamountofmatureIgEmRNAarosesignificantlyandrapidlyonedayafterTCSrestimulation,whileintheMLNofthemiceprimed30daysbeforeandwithoutboost,itwasalmostasthesameamountoftheunimmunizedcontrol.ThesefindingssuggesttheexistenceoftheIgEmemoryBcellsinthemiceaftertheprimaryTCSimmunization.
简介:报道了内蒙古白粉菌4个新记录种,分别是寄生在白桦Betulaplatyphylla上的桦木白粉菌Erysiphebetulina、大果榆Ulmusmacrocarpa上的榆白粉菌原变种Erysipheulmivar.ulmi、刺果茶藤Ribesburejense上的醋栗单囊白粉菌Podosphaeramors-uvae和栾树Koelreuteriapaniculata上的栾树叉钩丝壳Sawadaeakoelreuteriae。其中,白桦Betulaplatyphylla和刺果茶蔗子Ribesburejense为上述白粉菌的国内新记录寄主,文中提供了详细的形态描述和线条图。引证标本保存在赤峰学院菌物标本室(CFSZ)。
简介:Asimplemethodtocreateachromosome-specificDNAlibrqaryofrice,includingmicrodissection,amplification,charterizationandcloning,isdescribed.Ricechromosome4fromametaphasecellhasbeenisolatedandamplifiedbytheLinkerAdapterPCR(LA-PCR).ThePCRproductswerelabeledasprobeswithDIG-11-dUTPusingtherandomprimingmethod.SouthernblotanalysiswithricegenomicDNAandspecificRFLPmarkersdemonstratedthatthePCRproductswerederivedfromricechromosome4.Alargelibrarycomprisingover100,000recombinantplasmidmicroclonesfromricechromosome4wasconstructed.Colonyhybridizationshowedthat58%oftheclonescontainedsingleorlow-copysequencesand42%containedrepetitivesequences.ThesizeofinsertsgeneratedbyPCRrangedfrom140bpto500bp.ThismethodwillfacilitatecloningofthespecificchromosomeDNAmarkersandimportantgenesofrice.