Description:
ChromogenixS-2238™isachromogenicsubstrateforthrombin.Thesubstratehasbeenusedforthedeterminationof:
- Prothrombininplasma
- Antithrombininplasma
- Plateletfactor3inplasma
- Heparininplasma
Composition:
EachvialcontainschromogenicsubstrateS-2238™25mgandmannitol120mgasabulkingagent.StABIlity:Substance:Stableuntilexpirydateifstoredat2-8°C.Avoidexposuretolight.Thesubstanceishygroscopicandshouldbestoreddry.Solution:1mmol/LinH2Oisstableformorethan6monthsat2-8°C.
Chemicalname:H-D-Phenylalanyl-L-pipecolyl-Larginine-p-nitroanilinedihydrochloride.
Formula:H-D-Phe-Pip-Arg-pNA·2HCl
Mol.wt.:625.6
e316nm:1.27.104mol-1.L.cm-1
Solubility:>10mmol/LinH2O
Suitablestocksolution:1-2mmol/LinH2O.
ThrombinIUandEnzymeActivity:
ThecurrentInternationalStandardforthrombinistheHumana-thrombin89/588availablefromNIBSC.Thisisahighpuritypreparationofa-thrombinpreparedfromCohnfractionIIIandassayedbyaclottingtimemethodagainstthefirstInternationalStandardforthrombin,75/157.
TheNationalInstituteofHealthstandard(LotJ)isalsocommonlyusedforcalibrationandastudyconductedbyGaffneyPJetal.wasfocusedontherelationshipbetweenthetwostandards,andbetweentheInternationalUnitsandtheNIHUnits.Asaresultofthisstudy,basedbothonaclottingandachromogenicassay(withthechromogenicsubstrateS-2238™),1NIH-Ucorrespondsto1.15IU.
InanarticleitwasshownthatbovinethrombinhasahigheramidolyticactivitythanhumanthrombinwhenthesameNIH-Uarecompared.Itwasalsounderlinedthattheinfluenceofbandg-forms,thatwereprobablycontaminatingthebovineenzyme,mightbethereasonforthisdiscrepancy.
Inthesamearticleitwasconcludedthat1NIH-Ubovinethrombinwasequivalentto3.4nkatchromogenicsubstrateS-2238™,andthat1NIH-Uofhumanthrombinwasequivalentto2.7nkatchromogenicsubstrateS-2238™.
Fromanearlierpublication1NIH-Uofhumanthrombincorrespondedto 2.5nkatchromogenicsubstrateS-2238™.ThecorrespondencebetweenNIH-UorIUofthrombinandtheenzymeactivityexpressedinnkat,dependsonthesubstrate,theenzymepreparation(contentofa-,b-andg-thrombin)andtheassayconditions.
FromthearticleofFriberger,1µgthrombincorrespondsto2.2NIH-Uor5.5nkatchromogenicsubstrateS-2238™orto0.02plasmaequivalentunits.Inanotherstudy,1µgthrombincorrespondsto3.1NIH-U.
Intheexperimentsdoneby Chromogenix 1µgthrombinwasequivalentto3nkatchromogenicsubstrateS-2238™(human)or4.4nkatchromogenicsubstrateS-2238™(bovine).Itmightalsobeaddedthatifallprothrombinisactivatedin1mlofhumanplasma,about1.5nanomolesor17.5NIH-Uofthrombinareformed.
ThrombinMethod:
DeterminationofThrombininPlasmawithChromogenicSubstrateS-2238™
Reagents
- ChromogenicSubstrateS-2238™: (0.56mM)25mgArt.No.S820324.Disolve25mglyophlizedsubstratein7.14mlsterilewater=5.6mMstocksolution.
- Buffer:50nMTris,|0.15,pH8.3with0.2%BSA(10mlbuffer+100µl20%BSA)
Assay
Dilutetoasuitablesampleconcentration(0.5–1.0nkat/mlafterdilutionwithbuffer)
| Sampleofbuffer | 100µl |
| Incubateat37°C | 4 min |
| S-2238™ | 100µl |
| Incubateat37°C | 3 min |
| AceticAcid,20% | 50µl |
Usebufferasablankandsubtractfromsampleabsorbances
AntithrombinMethod:
DeterminationofAntithrombinActivityinPlasmawithChromogenicSubstrateS-2238™
MeasurementPrinciple
Theantithrombinactivityinplasmaismeasuredafteradditionofanexcessofheparin,toformanAT•Heparincomplex.Anexcessofthrombinisthenaddedandallowedtoreactquantitativelyina1:1stoichiometricrelationshipwiththeATHeparincomplexpresent.Theresidualthrombinsplitsoffp-nitroaniline(pNA)fromthechromogenicsubstrateH-D-Phe-Pip-Arg-pNA(S-2238™).TherateatwhichpNAisreleasedismeasuredphotometricallyat405nm.Thiscanbefollowedonarecorder(initialratemethod)orreadafterstoppingthehydrolysiswithacid(acidstoppedmethod).Thecorrelationbetweenthechangeinabsorbanceperminute(ΔA/min)orabsorbance(A)andtheATactivityislinearandinverselyproportionalinthe5-125%rangeofnormalplasma.
| AT+Heparin(excess) |  | [AT·Heparin] |
| [AT·Heparin]+Thrombin(excess) | | [AT·Heparin·Thrombin] +Thrombin(residual) |
| H-D-Phe-Pip-Arg-pNA+H2O | Thrombin(residual) | H-D-Phe-Pip-Arg-OH+pNA |
Reagents
- ChromogenicSubstrateS-2238™,25mgArt.No.S820324
ReconstitutethesubstrateS-2238™(MW:625.6)in53mlofdistilledwater.Note:Polybrene®canbeaddedtothechromogenicsubstratesolutionatafinalconcentrationof0.33mg/ml. - Thrombin,53nkat,Art.No.DPGBT-10
Reconstitutewith1.5mlsterilewater.Thesolutionisstablefor4weeksat2-8°C. - Buffer–Tris/Heparin,pH8.4(25°C)
- Tris6.1g(50mmol/l)
NaCl10.2g(175mmol/l)
Na2EDTA-2H2O2.8g(7.5mmol/l)
Distilledwater800ml
AdjustthepHto8.4at25°Cbyaddinganappropriateamount(approx.22ml)of1mol/lHCl.Add3000IUofheparin.Fillupto1000mlwithdistilledwater.Thebuffer,ifnotcontaminated,willremainstablefortwomonthsat2-8°C. - Aceticacid20%
Aceticacidisusedintheacid-stoppedmethod.
Specimencollection
Ninepartsoffreshlydrawnvenousbloodarecollectedintooneparttrisodiumcitrate.
Centrifugation:2000xgfor10-20minat20-25°C.
Standardcurve
Normalplasmahasanantithrombinactivityof100%.Twostandards(e.g.25%and100%)madeupfreshshouldbeincludedineachtestrun.CheckwhetherΔA/minorAforthetwostandardscorrespondwiththestoredstandardcurve.Thetolerancelimitis±0.1absorbanceunits.Preparethestandardsaccordingtothetablebelow:
| Antithrombin% | Normalplasmaml | Tris/Heparinbufferml |
| 0 | – | 400 |
| 25 | 100 | 300 |
| 50 | 200 | 200 |
| 75 | 300 | 100 |
| 100 | 400 | – |
Method
Dilutesamplesandstandardsasfollows:
Tris/HeparinBuffer:3000µl
Testplasmaorstandard:50µl
| Initialratemethod | |
| Dilutedtestplasmaorstandard | 400µl |
| Incubateat37°C | 3-6min |
| Thrombin(20-25°C) | 100µl |
| Mixandincubateat37°C | 30sec |
| Substrate | 300µl |
Transferimmediatelytoa1cmsemi-microcuvette(preheatedto37°C)formeasurementoftheabsorbancechangeinaphotometerat405nmandat37°C,calculateΔA/min.
| Acidstopped method | |
| Dilutedtestplasmaorstandard | 400µl |
| Incubateat37°C | 3-6min |
| Thrombin(20-25°C) | 100µl |
| Mixandincubateat37°C | 30sec |
| Substrate | 300µl |
| Incubateat37°C | 30sec |
| Aceticacid20% | 300µl |
Readtheabsorbance(A)ofthesampleagainstdistilledwaterat405nmwithin4hours.
Limitationsoftheprocedure
Insomepathologicalstates(DIC,sepsis)plasmaalonemayhydrolysethechromogenicsubstrateS-2238™.Thisinterferingreactionmaybedeterminedbyassayofatestsampleintheabsenceofaddedthrombin.Thisactivityrarelycorrespondstomorethan1%ofthatoftheaddedthrombin.Toimprovethevalidityoftheassaythevalueobtainedintheabsenceofaddedthrombincanbesubtractedfromthesamplevalue.Bilirubin,haemoglobinandplasmafromhyperlipaemicpatientsinterfereinabsorbancereADIng.Patientsplasmablanksarenecessaryintheseinstancesfortheacidstoppedmethodonly.Atconcentrationsbelow25%ATitisrecommendedtodoubletheplasmaconcentration(100µlplasma+3mlbuffer).Theresultisthendividedbytwo.
Calculation
PlotAorΔA/minforthestandardsagainsttheirknownantithrombinactivity.
PercentofnormalATactivityisdeterminedbyplottingtheAorΔA/minforthetestsampleonthestandardcurveandreadingthecorrespondingATvalue.
BIBLiography
- OdegardORetal.Heparincofactoractivitymeasuredwithanamydolyticmethod.ThrombRes6,287-294(1975).
- OdegardORetal.Evaluationofanamidolyticheparincofactormethod.ThrombRes7,351-360(1975).
- AbildgaardUetal.Antithrombin(heparincofactor)assaywithnewchromogenicsubstrates.ThrombRes11,549-553(1977).
- KahléLHetal.AntithrombinIII,EvaluationofanautomatedantithrombinIIImethod.ThrombRes12,1003-1014(1975).
HeparinMethod:
DeterminationofHeparininPlasmawithChromogenicSubstrateS-2238™
MeasurementPrinciple
Heparinisanalysedasacomplexwithantithrombin(AT)presentinthesample.TheconcentrationofthiscomplexisdependentontheavailabilityofAT.InordertoobtainamoreconstantconcentrationofAT,purifiedATisaddedtothetestplasma.Thrombininexcessisneutralizedinproportiontotheamountofheparin,whichdeterminestheamountofheparin-ATcomplex.TheremainingamountofthrombinhydrolysesthechromogenicsubstrateH-D-Phe-Pip-Arg-pNA(ChromogenicSubstrateS-2238™)thusliberatingthechromophoricgroup,pNA.Thecoloristhenreadphotometricallyat405nm.
| Heparin+AT | | [Heparin·AT] |
| [Heparin·AT]+Thrombin(excess) | | [Heparin·AT·Thrombin]+Thrombin(residual) |
| H-D-Phe-Pip-Arg-pNA+H2O | Thrombin(residual) | H-D-Phe-Pip-Arg-OH+pNA |
Reagents
- ChromogenicSubstrateS-2238™,25mgArt.No.S820324
ReconstitutethesubstrateS-2238™(MW:625.6)with40mlofdistilledwater. - Thrombin
Humanthrombinorbovinethrombincanbeusedin0.15mol/lNaClsolution.
Theactivityofthesolutionshouldbe14nkat/ml(about6NIH-U/ml).
Ifbovinethrombin53nkatfromDiapharma (Art.No.DPGBT-10)isused,dissolvethecontentofonevialwith3.8mlsaline. - Antithrombin10IUArtNo.B820720
Reconstitutewith5mlwatertoobtainaconcentrationof2IU/ml. - TrisBuffer,pH8.4(25°C)
Tris6.1g(50mmol/l)
NaCl10.2g(175mmol/l)
Na2EDTA2.8g(7.5mmol/l)
Distilledwater800ml
AdjustthepHto8.4at25°Cbyaddinganappropriateamount(approx.22ml)of1mol/lHCl.Fillupto1liter. - Normalplasma
Bloodshouldbetakenfromnormaldonors.10-30mlofcitratedblood(9volbloodand1vol0.1mol/lsodiumcitrate)aretakenfromeachdonor.Thefirstmlofbloodisdiscardedandthetubeiskeptinanicebath.Plasmaispreparedbycentrifugationat2000xgfor20minutesat4°C.Equalamountsofplasmafromthedonorsaremixedanddispensedinsmallvolumes.Thenormalplasmaisstablefor3monthsat-20°Corbelow.Thawat37°Candthenkeeponice. - Aceticacid20%
Aceticacidisusedintheacid-stoppedmethod.
Specimencollection
Blood(9vol)ismixedwithsodiumcitrate(1vol)cooledto0°Cwithiceandcentrifugedat2000xgfor20minat4°C.
Diluteplasma1:5withTrisBufferpH8.4.
Standardcurve
Thesameheparinasisusedforthepatientisdilutedto1IU/mlwithsaline0.9%.Then100µldilutionisfurtherdilutedwith1.9mlbuffertoobtainaconcentrationof0.05IU/ml.
| Standard IU/ml | Buffer ml | AT ml | Plasmadil1:5 ml | Heparin0.05IU/ml ml |
| 0.00 | 800 | 100 | 100 | 0 |
| 0.25 | 700 | 100 | 100 | 100 |
| 0.50 | 600 | 100 | 100 | 200 |
| 0.75 | 500 | 100 | 100 | 300 |
| 0.10 | 400 | 100 | 100 | 400 |
Method
| Initialratemethod | TubeNo.1 |
| Buffer | 800µl |
| AT | 100µl |
| Testplasma | 100µl |
| Mix | |
| TubeNo.2 | |
| StandardortubeNo.1 | 200µl |
| Incubateat37°C | 3-4min |
| Thrombin | 100µl |
| Incubateat37°C | 30sec |
| Substrate(37°C) | 200µl |
| Mix |
Transfersampleimmediatelytoa1cmmicro-cuvette(preheatedat37°C)formeasurementoftheabsorbancechangeat405nm.CalculateΔA/min.Readtheabsorbanceagainstanormalplasmablankinaphotometerat405nm.
| Acidstoppedmethod | TubeNo.1 |
| Buffer | 100µl |
| AT | 100µl |
| Testplasma | 100µl |
| Mix | |
| TubeNo.2 | |
| StandardortubeNo.1 | 200µl |
| Incubateat37°C | 3-4min |
| Thrombin | 100µl |
| Incubateat37°C | 30sec |
| Substrate(37°C) | 200µl |
| Incubateat37°C | 60sec |
| Aceticacid20% | 300µl |
| Blanksforacidstopped method | Normal plasmablank | Test plasmablank |
| Standard0IU/ml | 200µl | – |
| SamplefromtubeNo.1 | – | 200µl |
| Aceticacid | 300µl | 300µl |
| Mix | ||
| Distilledwater | 300µl | 300µl |
| Mix |
Note:Asaruleanormalplasmablankorevenwaterisusedasablank.Ifbilirubinexceeds100mmol/lorthetestplasmaisopaque,readthetestplasmasampleagainstitsownblank.
Calculation
PlotAorΔA/minforthestandardsagainsttheirknownheparinconcentration.
HeparinconcentrationisdeterminedbyplottingtheAorΔA/minforthetestsampleonthestandardcurveandreadthecorrespondingheparinvalue.
Bibliography
- BhargavaASetal.Characterizationofanewpotentheparin.2ndcommunication:chemicalanalysisofthecarbohydratecontentanddeterminationoftheBIOLOGicalactivityofanewpotentheparinpreparationinvitro,usingprotaminenutralizationandamidolyticmethodsforfactorXaandthrombin.Arzneimittelforschung30,1071-1074(1980).
- SacheEetal.Studiesonahighlyactiveanticoagulantfractionofhighmolecularweightisolatedfromporcinesodiumheparin.ThrombRes25,443-458(1982).
- VanPuttenJetal.Determinationoflowmolecularweightheparininclinicallaboratory.Haemostasis14,205-210(1984).
- VanPuttenJetal.Automatedspectrophotometricheparinassays.Comparisonofmethods.Haemostasis14,195-204(1984).
- BerryCNetal.Effectsofthesyntheticthrombininhibitorargatrobanonfibrin-orclot-incorporatedthrombin:comparisonwithheparinandrecombinanthirudin.ThrombHaemost72,381-386(1994).
- ByunYetal.EffectoffibronectinonthebindingofantithrombinIIItoimmobilizedheparin.JBiomedMaterRes30,95-100(1996).
ProthrombinActivityMethod:
DeterminationofprothombinactivityinplasmawithChromogenixS-2238™
Background
Anumberofstudiesduringthelastfewyearssupportthenotionthatvenousthromboembolism(VTE)isamultifactorialdiseasemostoftentriggeredbycircumstantialriskfactors(trauma,surgery,pregnancy,oralcontraceptives,immobilizationandage)incombinationwithoneormoregeneticoracquiredcoagulationdisorders(seeref.1ofareview).
Elevatedactivityofprothrombinintheabsenceofaknownunderlyinggeneticdisorderisalsoassociatedwithanincreasedthromboticrisk2.
AmutationG→Aintheuntranslated3’-regionoftheprothrombingeneatnucleotideposition20210constitutesariskfactorforVTEwithanoddsratioof3-52-10.About90%ofthecarriersofthismutationhaveelevatedlevels(>115%)ofprothrombinactivity2,7,8.Levelsabovetheupperlimitofthenormalrange(75–130%)arecommonlyhetero-andhomozygotes2,7-9.
Sofar,thereisnoexplanationwhyacomparativelymildincreaseofprothrombinactivityconstitutesariskfactorforthrombosisandthisisthereforeanareaofactiveclinicalandbiochemicalresearch.Chromogenicmethodsforaccuratedeterminationofelevatedactivitiesofprothrombinandothercoagulationfactors,suchasfactorVIII11,12areimportanttoolsforassessingtheriskforVTEinpatientsandfamilymembers.
MeasurementPrinciple
ProthrombinisactivatedtomeizothrombinbythesnakevenomenzymeEcarinfromEchisCarinatus.
Afteracertainincubationtime,theamountofmeizothrombinformedismeasuredwiththethrombinselectivesubstrateChromogenixS-2238™,whichalsoiscleavedbymeizothrombin.
Theabsorbancerecordedat405nmisproportionaltotheprothrombinactivityinthesample.
| Prothrombin | Ecarin | Meizothrombin |
| S-2238™ | Meizothrombin | pNA+Peptide |
Reagents
- TrisBSABuffer(catalog#TB031-20)Bufferforsampledilution,containing0.5mol/lTrisHClpH7.3,I=2.0withNaCland2%bovineserumalbumin.Beforeuse,dilutethestocksolution1+9withsterilewatertoobtainabufferworkingsolution.Thebufferworkingsolutionispreparedandusedwithinthesameday.
- EcarinDiluent(catalog#ED0413-20)BufferfordilutionofEcarin,containing0.05mol/lTrisHClpH7.6,I=0.15withNaCl,bovineserumalbumin,polyethyleneglycolandafibrinpolymerizationinhibitor.
- Ecarin(catalog#ECARIN50B)ReconstitutewithsterilewateraccordingtotheEcarinpackageinsert.Freezeinsuitablealiquotsat-20°Corat-70°C.Stablefor3monthsatbothstoragetemperatures.Beforeuse,dilutewithProthrombinActivatorDiluenttoobtainaconcentrationof2.4U/ml.Stablefor8hoursat20-25°Candfor1weekat2-8°C.Note:EchisCarinatuscrudevenomcanalsobeused.Asuitablefinalconcentrationofthisreagentisapproximately5µg/ml;however,thismayvarybetweendifferentsources.10-20%lossofactivitymayoccuruponfreezingat-20°C.
- S-2238™(catalog#S820324)Reconstitutewith13mlofsterilewatertoobtaina3mmol/lsolution.
SpecimenCollection
Blood(9volumes)ismixedwith0.1mol/lsodiumcitrate(1volume)andcentrifugedat2000xgfor20minat20-25°C.Separateplasmacarefullyfrombloodcells.Performtheanalysiswithin24hourswhenplasmaisstoredat2-25°C.Alternatively,freezealiquots≤1mlat-20°Corbelow.Performtheanalysisoffrozensampleswithintwomonthswhenstoredat-20°Corwithinoneyearwhenstoredat-70°Corbelow.Nosignificantlossofprothrombinactivityoccursuponfreezingonce,providedfreezingismadeinsmallaliquots(<1ml)andthawingisperformedinawaterbathorinanelectricheaterat25-37°C.
SampleandStandardDilutions
Standards
Calibratednormalplasmaisdiluted1:23–1:160toprovidestandardconcentrationsof25-175%.Thefollowingtableprovidesasuggestionofstandarddilutions.
| StandardDilution | ProthrombinActivity |
| 1:18 | 167% |
| 1:22 | 136% |
| 1:30 | 100% |
| 1:60 | 50% |
| 1:120 | 25% |
Samples
Plasmasamplesarediluted1:40inTrisBSABufferworkingsolutionforapplicationonmicroplateanddiluted1:80forapplicationonACL(seebelow).
MicroplateAssayProcedure
| Standard/Sampledilution | 50μl |
| Incubateat37°C | 2-4min |
| EcarinorEchisCarinatus(37°C) | 50μl |
| Incubateat37°C | 3min |
| Substrate(37°C) | 50μl |
| Readkineticallyorincubateat37°C | 2min |
| Aceticacid,20% | 50μl |
DeterminetheabsorbancedifferenceA405nm-490nmforthestandarddilutionandthesamples.Drawastandardcurvefromtheabsorbancesobtainedforthestandarddilutions.Readtheprothrombinactivityforthesamplesfromthestandardcurve.
Fig.1.Standardcurvewiththemicroplatemethod.
ApplicationonACL
Usetheplasminogenchannelprogram.Prepareastandarddilution1:40,whichcorrespondstoanominalprothrombinactivityof100%(seeaboveregardingcalibration).Standarddilutionscorrespondingto25%and50%arethenautomaticallypreparedbytheinstrument.Inordertoallowdeterminationofprothrombinactivityupto200%,sampleplasmashouldbediluted1:80andtheobtainedresultshouldbemultipliedwithtwo.
Fig.2.StandardcurvewiththeACLmethod
Expectedvalues13
Thenormalrangeis75–130%(mean102%2SD)asdeterminedfromanalysisinmicroplateandontheACL300of101healthyindividuals(49menand52women;agerange20–68years).Analysisofplasmafrom42carriersoftheG20210Amutation,whowerenotonoralanticoagulanttreatmentatthetimeofbloodsampling,resultedinanactivityrangeof94–164%(mean128%2SD).
InterferenceandLimitations
Noinfluenceintheassayisobtainedfromvariationofantithrombinactivityintherange50–150%ofnormal.Sincemeizothrombinisformedandmeasured,noinfluenceintheassayisobtainedfromheparinlevels≤1IU/mlplasma.SinceEcarinalsoactivatesdecarboxyprothrombin,whichisproducedduringoralanticoagulanttherapywithanti-vitaminKdrugs,plasmafrompatientsundergoingsuchtreatmentshouldnotbeanalysedwiththismethod.
Repeatability
Theimprecision,expressedasCV,withinandbetweenseries(7series,5replicatesineachseries)is≤4%at50%and100%prothrombinactivity.
Bibliography
- LaneDA,MannucciPM,BauerKA,BertinaRM,BochkovNP,BoulyjenkovV,ChandyM,DahlbäckB,GinterEK,MiletichJp,RoosendaalFR,SelingsohnU.
InheritedThrombophilia:part1.
ThrombHaemost76,651-662(1996) - PoortSR,RoosendaalFR,ReitsmaPH,BertinaRM.Acommongeneticvariationinthe3’-untranslatedregionoftheprothrombingeneisassociatedwithelevatedplasmaprothrombinlevelsandanincreaseinvenousthrombosis.
Blood88,3698-3703(1996) - HillarpA,ZöllerB,SvenssonPJ,DahlbäckB.
The20210alleleoftheprothrombingeneisacommonriskfactoramongSwedishout-patientswithverifieddeepvenousthrombosis.
ThrombHaemost78,990-992(1987) - CummingAM,KeeneyS,SaldenA,BhavnaniM,ShweRH,HayCRM.TheprothrombingeneG20210Avariant:prevalenceinaUKanticoagulantclinicpopulation.
BrJHaematol98,353-355(1997) - BrownK,LuddingtonR,WilliamsonD,BakerP,BaglinT.
RiskofvenousthromboembolismassociatedwithaGtoAtransitionatposition20210inthe3’-untranslatedregionoftheprothrombingene.
BrJHaematol98,907-909(1997) - MakrisM,PrestonFE,BeuchampNJ,HamptonKK,DalyME,CooperP,BaylissP,PeakeIR.Co-inheritanceofthe20210Aalleleoftheprothrombingeneincreasesthethromboticriskinsubjectswithfamilialthrombophilia.
ThrombHaemost78,Suppl.,165(1997) - FerraresiP,MarchettiG,LegnaniC,CavallariE,CastoldiE,MascoliF,ArdissinoD,PalaretiG,BernardiF.Theheterozygous20210G/Aprothrombingenotypeisassociatedwithearlyvenousthrombosisininheritedthrombophiliasandisnotincreasedinfrequencyinarterydisease.
ArteriosclThrombVascBiol17,2418-2422(1997) - KapurRK,MillsLA,SpitzerSG,HultinMB.Aprothrombingenemutationissignificantlyassociatedwithvenousthrombosis.
ArteriosclThrombVascBiol17,2875-2879(1997) - HowardTE,MarusaM,ChannelC,DuncanA.Apatienthomozygousforamutationintheprothrombingene3’-untranslatedregionassociatedwithmassivethrombosis.
BloodCoagFibrinol8,316-319(1997) - MartinelliI,SacchiE,LandiG,TaioliE,DucaF,MannucciPM.Highriskofcerebral-veinthrombosisincarriersofaprothrombin-genemutationandinusersoforalcontraceptives.
NewEnglJMed338,1793-1797(1998) - KosterT,BlannAD,BriëtE,VanenbrouckeJP,RoosendaalFR.RoleofclottingfactorVIIIineffectofvonWillebrandfactoronoccurrenceofdeep-veinthrombosis.
TheLancet345,151-155(1995) - D’OnnelJ,TuddenhamEGD,ManningR,Kemball-CookG,JohnsonD,LaffanM.HighprevalenceofelevatedfactorVIIIlevelsinpatientsreferredforthrombophiliascreening:roleofincreasedsynthesisandrelationshiptotheacutephasereaction.
ThrombHaemost77,825-828(1997) - RosénS,AnderssonM,GhoshR.Anewchromogenicprothombinmethodprovidingaccuratedeterminationofelevatedprothombinactivityinplasmasamples.
ISTH1999,Abstract269
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通过解答,教会我,谢谢
请问下有无同学需要H37RA的?我是做EAE模型的,上个月购买了BDDifco公司的H37RA(货号),因为购买的时候只能整盒6支购买,但我们用不了那么多,所以想问问有无同学需要的,100mg/支,800元/支或用等价试剂交换。地址广州。有需要的请私信,谢谢!
(1)优级纯试剂 亦称保证试剂,为一级品,纯度高,杂质极少,主要用于精密分析和科学研究,常以GR表示。
(2)分析纯试剂 亦称分析试剂,为二级品,纯度略低于优级纯,杂质含量略高于优级纯,适用于重要分析和一般性研究工作,常以AR表示。
(3)化学纯试剂 为三级品,纯度较分析纯差,但高于实验试剂,适用于工厂、学校一般性的分析工作,常以CP表示。
(4)实验试剂 为四级品,纯度比化学纯差,但比工业品纯度高,主要用于一般化学实验,不能用于分析工作,常以 LR表示。
以上按试剂纯度的分类法已在我国通用。根据化学工业部颁布的“化学试剂包装及标志”的规定,化学试剂的不同等级分别用各种不同的颜色来标志,见表1。
表1 我国化学试剂的等级及标志
刚入这行,谢谢大家
我想检测血管组织中的钙离子浓度,不知道哪个公司有试剂盒
A.H2SO4Na2SO4AgNO3BaCl2.
B.NaOHNa2CO3NaHSO4MgCl2
C.CaCl2NaNO3MgSO4BaCl2
D.HNO3KOHKClK2CO3
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