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论文题目川芎嗪衍生物TBN的HPLC含量测定方法
学院
国际学院
学系
药学系
专业
药学
姓名
学号
指导教师
2008年5月25日
StatementofOriginality
Iherebydeclarethatthethesispresentedistheresultofresearchperformedbymepersonally,underguidancefrommysupervisor.Thisthesisdoesnotcontainanycontent(otherthanthosecitedwithreferences)thathasbeenpreviouslypublishedorwrittenbyothers,nordoesitcontainanymaterialpreviouslypresentedtoothereducationalinstitutionsfordegreeorcertificatepurposetothebestofmyknowledge.Ipromisethatallfactspresentedinthisthesisaretrueandcreditable.
Signed:
_________________Date:
25-05-2009
QuantitativeHPLCanalyticalmethodfortetramethylpyrazine
derivativeTBN
Abstract:
Ahigh-performanceliquidchromatography(HPLC)methodforanewtetramethylpyrazinederivative,TBN,wasdeveloped.Analyticalperformanceparameterssuchaslinearity,precision,accuracy,specificity,limitofdetection(LOD)andlimitofquantification(LOQ)weredeterminedundertheguidelineofInternationalConferenceonHarmonizationQ2B[1].TBNwasanalyzedbyRP-HPLCwithC18columnusingmethanol-water(35:
65)asmobilephase.Theflowrateis0.8ml/minandthedetectorwassetto295nm.Thelinearityofcalibrationcurveisgood(r2>
0.999)andtheLODandLOQwere12.096ng/mland40.32ng/mlrespectively.Therelativestandarddeviation(RSD)ofprecisionandaccuracywere0.1245%and0.6895%,respectively,andthesamplerecoverywas99.08%(RSD:
0.40%).ThismethodisreliableandeasyforTBNanalysis.
KeyWords:
tetramethylpyrazinederivative,TBN,HPLC
川芎嗪衍生物TBN的HPLC含量测定方法
摘要:
目的:
建立川芎嗪衍生物(TBN)高效液相含量测定方法。
方法:
选用C-18色谱柱;
甲醇-水(35:
65);
流速:
0.8ml/min;
检测波长为295nm。
结果:
TBN在12.42-310.5g/ml范围内线性关系良好(r2>
0.999);
定量限和检测限分别为12.096ng/ml及40.32ng/ml;
精密度及准确度RSD分别为0.1245%及0.6895%;
加样回收率结果为99.08%(RSD:
0.40%)。
结论:
本方法简便可靠,可作为TBN之定量分析方法。
关键词:
川芎嗪衍生物,TBN,高效液相
Contents
1.Introduction1
2.Materials2
2.1.Chemicals2
2.2.Apparatus3
3.ExperimentalMethod3
3.1.TBNstandardpreparation3
3.1.1.ColumnchromatographyforTBNpurification4
3.1.2.Semi-preparativecolumnchromatography5
3.2.DevelopmentofHPLCmethodforTBN5
3.2.1.maxdetermination5
3.2.2.OptimizationofHPLCconditionsforTBN6
3.3.ValidationofHPLCmethod7
3.3.1.Specificity7
3.3.2.Linearity7
3.3.3.Precision7
3.3.4.LimitofQuantificationandLimitofDetection7
3.3.5.Range7
3.3.6.Accuracy7
3.3.7.Stability7
3.3.8.Recovery7
3.3.9.ContentAssay7
4.ResultsandDiscussion7
5.Conclusion7
Acknowledgement7
References7
1.Introduction
TBNisanovelcompounddevelopedbytheInstituteofNewDrugResearchatthePharmacyCollege,JinanUniversity.TBNhasbeenshowntobeantioxidativeandthrombolytic,andisunderdevelopmentasatreatmentforischemicstroke[2].
TBNisaderivativeof2,3,5,6-tetramethylpyrazine(TMP),whichisthemainactiveingredientofLigusticumwallichiiFranchat(ChuanXiong),formedbyconjugatingTMPandanitronemoiety(seeFigure1).
TMPisusedtotreatischemicstrokeinChinaformanyyearswhichwasfoundbeneficialininhibitingplateletaggregation[3],lysingbloodclots[4],blockingcalciumentry[5]andscavengingreactiveoxygenspecies(ROS)[6].WhileretainingthethrombolyticactivityofTMP,thenitroneaddedtoTMP(i.e.TBN)hadbeenprovedtoprovideastrongantioxidativeactivity.Nitronesareusefulastherapeuticagentsforneuralandsystemicdiseasessuchasatherosclerosis,septicemia,stroke,andAlzheimer’sdisease[7].
(1)
(2)
(3)
Figure1StructureofTMP
(1);
Nitrone
(2);
TBN(3)
Asapotentialnewdrug,seriesofresearcheslikepharmacology,toxicology,pharmacokinetics,pharmacodynamicsareneeded.Therefore,qualityanalysisandcontrolonTBNisnecesary.Firstofall,aquantitativemethodofTBNhadtobedeveloped.
HPLCmethodforanalyzingchemicalcompoundisquick,simpleandreliable.ThereforewechoseitastheanalyzingmethodforTBN.AreliableHPLCmethodshouldbeabletoseparatethesamplefromitsimpuritiescompletelyandcanbevalidatedproperly,socalledtheMethodology.
ThevalidationofdevelopedHPLCmethod[1,8]includedseveralpartswhicharelinearity,precision,range,limitofquantificationandlimitofdetection,accuracy,stability,specificity,andrecovery.Thecontentassaywouldbedoneafterthevalidationofmethod.However,referencestandardofthesubstancetobetestedisneededinsomeitemsoftheHPLCmethodvalidation.
Forthiscase,TBNisanewcompoundanditsreferencestandardisunavailable.Therefore,inthispaper,arelativelypuresamplewasusedasareferencestandard.Hence,toobtainarelativelypureTBNsample,apurificationofTBNwasalsodoneinthisresearch.
ThetargetofthisresearchistoestablishaneasyandreliableHPLCmethodforTBNanalysis,usedinroutinequalitycontrolofitsrelatedstudies.AftertheestablishmentofTBNreferencestandard,thisHPLCmethodcanbeapplieddirectlytoquantifyTBNcontent.
Inthisresearch,therewerethreemainparts:
TBNstandardpreparation,HPLCmethodestablishment,andMethodvalidation.
2.Materials
2.1.Chemicals
TBN,preparedbytheInstituteofNewDrugResearchatPharmacyCollege,JinanUniversity;
Petroleumether,ethylacetate,acetoneanddichloromethane(Analyticalreagents)purchasedfromFUYURefinedChemicalProductsLtd.;
Reagentgradedsilicagel(200-300mesh)purchasedfromBranchofQingdaoHaiyangChemicalPlant;
Methanol(HPLCgrade)purchasedfromJiangsuHanbonSci.&
Tech.Co.,Ltd.;
Double-distilledwaterprovidedbytheInstitute;
Sodiumdihydrogenphosphateanddisodiumhydrogenphosphate(Analyticalreagents),purchasedfromGuangzhouChemicalReagentFactory.
2.2.Apparatus
GlassChromatographiccolumn;
Thinlayerchromatographicsilicagelplates;
RotaryEvaporator(EYELAN-1001)andDigitalWaterBath(EYELASB1000);
Vacuumdryingoven(DZF-6050);
UltrasonicCleaners(KQ-250E);
MeltingPointMeasuringInstrument(SGWX-4);
ShimadzuUV-VISSpectrophotometers(UV-2450)
Shimadzu-10ATHPLCandSPD-10AVPUV-VISDetector;
LUBEXKromasilC18column(5100Å
250mm4.6mm);
semipreparativeHPLCcolumn(VYDACRPC1890APHARMACEUTICAL);
Electronicbalance(ACCULABALC110.4);
Otherapparatus:
volumetricflasks,conicalflasks,pipette,microfiltersandmembranes(0.45m).
3.ExperimentalMethod
3.1.TBNstandardpreparation
TBNisawhitecrystalwhichiswatersoluble,withmolecularweightof221g/mol.Duetothedifferenceinpuritybetweeneachbatchesofproduction,thephysicalpropertiesofTBNsamplesarevariedfromoneanother.
Inthispart,relativelypureTBNsamplewouldbepreparedandthenusedinthevalidationofHPLCmethodasreferencestandard.
3.1.1.ColumnchromatographyforTBNpurification
(1)TLCmethod
UseethylacetateasthesolventtodissolveTBNsample,separatethesamplecomponentswithdifferentmobilephases.
A.Thecontinuousseparatingcondition:
petroleumether-ethylacetate(1:
1)
B.Modifiedcondition1:
petroleumether-ethylacetate(4:
C.Modifiedcondition2:
petroleumether-acetone(5:
Figure2TLCofTBNwithdifferentmobilephase(fromlefttoright:
A,B,C)
(2)Columnchromatography
FromtheresultsofTLC,methodBandCwereimplementedincolumn.About300mgofTBNwereusedineachmethod.FormethodB,yellowsemisolidwasobtained.VerypaleyellowsolidwasobtainedinmethodC.Hence,methodCwaschosen.
Batch2008.10.11TBN(4.26g)wasputincolumnchromatographywiththemobilephasepetroleumether-acetone(5:
1)and2.88gofpurifiedTBNwasyielded.Meltingpointwastested77℃.
3.1.2.Semi-preparativecolumnchromatography
SincethereweretraceamountofimpuritiesinthepurifiedTBNfrom3.1.1,semi-preparativecolumnchromatographywasperformedforfurtherpurification.
OnehundredmgofTBNwasusedthistime,andamethanol-water(35:
65)systemwasusedasamobilephase.However,Shimadzu-10ATHPLCisnotdesignedforsemi-preparativecolumn,toomuchsolventwasusedandtoofewTBNhavebeenpurified.ThismethodisnotfeasibleforproducingsufficientpurifiedTBN.AndfortheTBNpurified,sincetherewastoomuchwaterinthemobilephasethatwasdifficulttodry,onlytraceamountofTBNwasobtainedwhichwasnotenoughforexperimentaluse.
Withtheresult,theTBNpurifiedfrom3.1.1wasusedasreferencestandard.
3.2.DevelopmentofHPLCmethodforTBN
3.2.1.maxdetermination
BeforetheprocedureofHPLC,themaxofTBNshouldbedetermined.WiththeUV-VISSpectrophotometer,theTBNsamplesolutionwasscannedin200-400nmforthedeterminationofmax.
Method:
TBN(0.01g)from3.1.1wasweightedandwasdissolvedin10mlvolumetricflaskwithmethanol.Dilutethesolutionto50g/mlbyusingpipetteandvolumetricflasks.
ScanthesamplesolutionwiththeUV-VISSpectrophotometerandrecordtheresult.
Figure3UVspectrogramforTBN
Fromtheaboveresult,295nmwaschoseforTBNdetection.
3.2.2.OptimizationofHPLCconditionsforTBN
LUBEXKromasilC18column(5100Å
250mm4.6mm)wasusedinthisresearchwhichissuitableformostorganiccompound.
Differentratioofmobilephase,flowrate,pH,havebeenusedtodeterminethemostsuitableHPLCmethodforTBN.WiththeaimofseparatingtheTBNfromitsimpurities,TBNsamplewithoutpurification(Batch200
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