TheL-Fucosetestkitisasimple,rapid andreliablemethod,forthemeasurementandanalysisofL-Fucoseinplantextracts,BIOLOGicalsamplesandothermaterials.Thiskitcanbeusedinthemeasurementofα-fucosidasesthatdonotactonchromogenicsubstrates. Suitableformanual,auto-analyserandmicroplateformats.Correlationofserumlevo-fucoselevelsasabioMarkerwithtumornodemetastasisstaginginoralcancerpatients.Manchil,P.R.D.,Joy,E.T.,Kiran,M.S.,Sherubin,J.E.,Khan,M.F.&Aravind,B.S.(2016).JournalofPharmacy&BioalliedSciences,8(Suppl1),S147-S150.LinktoArticleReadAbstractBackground:oralcancerisaresultofdisorderedcellularbehaviorinitiatedbyvariousstimuliwhichischaracterizedbythealterationofserumglycoproteinsconsistingofdifferentmonosaccharides.Oneoftheseislevo-fucose(L-fucose),amethylpentose.Elevatedlevelsofprotein-boundfucosehavebeenreportedinvariousmalignancies.Aim:ThepresentstudyattemptedtocorrelatelevelsofserumL-fucoseasabiomarkerwiththevarioustumornodemetastasis(TNM)stagesoforalcancer.Methodology:Thestudywascarriedouton90subjectsconsistingof30healthycontrolsand60histopathologicallyprovenoralsquamouscellcarcinoma(OSCC)cases.TheserumfucoselevelestimationwasdonebasedonthemethodadoptedbyWinzler.Statisticalanalysisincludedindependentsample"st-test,one-wayANOVAtest,Karl–Pearsoncorrelationtest,andTukey"sHSDposthoctesttoevaluatethesignificanceandvariABIlityofvaluesbetweengroups.Results:SignificantelevationinserumfucoselevelswasnoticedamongOSCCpatientswhencomparedwiththecontrolsandaprogressiveascentofL-fucoselevelswerenotedasthestageofseverityincreased.SerumfucoselevelswereindependentofhistopathologicalgrADIng,age,andsex.Conclusion:SerumL-fucoselevelswereincreasedinOSCCpatients,andapositivecorrelationwasobservedbetweenserumL-fucoselevelsandTNMstagingofOSCC.Thus,serumL-fucosecanbeusedasaneffectivediagnosticandprognosticbiomarkerinOSCCpatients.Characterizationofanα-L-fucosidasefromtheperiodontalpathogenTannerellaforsythia.Megson,Z.A.,Koerdt,A.,Schuster,H.,Ludwig,R.,Janesch,B.,Frey,A.,Naylor,K.,Wilson,I.B.H.,Stafford,G.P.,Messner,P.&Schäffer,C.(2015).Virulence,6(3),282-292.LinktoArticleReadAbstractTheperiodontalpathogenTannerellaforsythiaexpressesseveralglycosidaseswhicharelinkedtospecificgrowthrequirementsandareinvolvedintheinvasionofhosttissues.α-L-Fucosylresiduesareexposedonvarioushostglycoconjugatesand,thus,theα-L-fucosidasespredictedintheT.forsythiaATCC43037genomecouldpotentiallyserverolesinhost-pathogeninteractions.WedescribethemolecularcloningandcharacterizationoftheputativefucosidaseTfFuc1(encodedbythebfo_2737=Tffuc1gene),previouslyreportedtobepresentinanoutermembranepreparation.Intermsofsequence,this51-kDaproteinisamemberoftheglycosylhydrolasefamilyGH29.Usinganartificialsubstrate,p-nitrophenyl-α-fucose(KM 670 µM),theenzymewasdeterminedtohaveapHoptimumof9.0andtobecompetitivelyinhibitedbyfucoseanddeoxyfuconojirimycin.TfFuc1wasshownheretobeauniqueα(1,2)-fucosidasethatalsopossessesα(1,6)specificityonsmallunbranchedsubstrates.Itisactiveonmucinaftersialidase-catalyzedremovalofterminalsialicacidresiduesandalsoremovesfucosefrombloodgroupH.Followingknock-outoftheTffuc1geneandanalyzingbiofilmformationandcellinvasion/adhesionofthemutantincomparisontothewild-type,itismostlikelythattheenzymedoesnotactextracellularly.BiochemicallyinterestingasthefirstfucosidaseinT.forsythiatobecharacterized,thebiologicalroleofTfFuc1maywellbeinthemetabolismofshortoligosaccharidesintheperiplasm,therebyindirectlycontributingtothevirulenceofthisorganism.TfFuc1isthefirstglycosylhydrolaseintheGH29familyreportedtobeaspecificα(1,2)-fucosidase.Cloning,characterization,andproductionofthreeα‐L‐fucosidasesfromClostridiumperfringensATCC13124.Fan,S.,Zhang,H.,Chen,X.,Lu,L.,Xu,L.&Xiao,M.(2015).JournalofBasicMicrobiology,56(4),347-357.LinktoArticleReadAbstractα-L-Fucosidasesarekeyenzymesforthedegradationofintestinalglycansbygutmicrobes.Inthiswork,threeputativeα-L-fucosidases(Afc1,Afc2,andAfc3)genesfromClostridiumperfringensATCC13124wereclonedandexpressedinEscherichiacoli.Afc1hadtheα-L-fucosidasedomainofglycosidehydrolase(GH)29familybutshowednoenzymeactivitytowardallthesubstratesexamined.Theputativeacid/baseresidueofAfc1,Ser205,wasreplacedbyaglutamicacidwhichisconservedinGH29-Bα-L-fucosidases.However,themutantAfc1-S205Estillfailedtoshowenzymeactivity.Afc2andAfc3weredeterminedtobe1,3-1,4-α-L-fucosidaseofGH29-Bsubfamilyand1,2-α-L-fucosidaseofGH95family,respectively,andbothofthemcouldreleasefucosefromporcinegastricmucin(PGM).WhenC.perfringensATCC13124grewwiththepresenceofPGM,thetranscriptionofafc1decreasedslightly,whilethoseofafc2andafc3increasedto2.2-foldand1.4-fold,respectively,andtheenzymeactivitiesofAfc2andAfc3inthecultureincreasedto2.2-foldand2.6-fold,respectively.TheseresultssuggestthatAfc2andAfc3areinvolvedinthedegradationofintestinalfucosylglycansbyC.perfringensATCC13124.UV-methodforthedeterminationofL-Fucoseinplantmaterial,polysaccharides,pharmaceuticalsandothermaterialsPrinciple:          (L-fucosedehydrogenase)(1)L-Fucose+NADP+→L-fucono-1,5-lactone+NADPH+H+Kitsize:  * 100assays(manual)/1000(microplate)                                         /1020(auto-analyser)* Thenumberofmanualtestsperkitcanbedoubledifallvolumesarehalved. ThiscanbereadilyaccommodatedusingtheMegaQuantTM WaveSpectrophotometer(D-MQWAVE).Method:                          Spectrophotometricat340nmReactiontime:                 ~10minDetectionlimit:                0.68mg/LApplicationexamples:L-Fucoseispresentasthemaincomponentinfucoidan(amarinepolysaccharide),foods,pharmaceuticalsandothermaterials(e.g.biologicalsamples,etc.)Methodrecognition:  NovelmethodAdvantagesVerycosteffective Allreagentsstablefor>2yearsafterpreparation Onlyenzymatickitavailable Simpleformat Rapidreactiontime(~10min) Mega-Calc™softwaretoolisavailablefromourwebsiteforhassle-freerawdataprocessing Standardincluded Suitableformanual,microplateandauto-analyserformats

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