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Encapsula/Fluorescent-DiO Macrophage Depletion Kit/CLD-8903-
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Encapsula/Fluorescent-DiO Macrophage Depletion Kit/CLD-8903-
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Encapsula
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CLD-8903-
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Description

Macrophagedepletionkitsarecomposedoftwovials;onevialofClodrosome®(Clodronateliposomes)andonevialofEncapsome®(controlliposomescontainingnodrug).Thevolumeofthemacrophagedepletionkitrepresentsthevolumeofeachreagentindividually.Forexample,the5-mlmacrophagedepletionkitmeans5mlofClodrosome®and5mlofEncapsome®.Eachreagentinthekitcanalsobepurchasedindividually.

Clodrosome®isamultilamellarliposomesUSPensioninwhichclodronateisencapsulatedintheaqueouscompartmentsoftheliposomes.Encapsome®isformulatedandpreparedidenticallytoClodrosome®exceptthatclodronateisnotaddedtotheliposomes.Theliposomesarefilteredthrough2μmpolycarbonatemembranestoensurethatthelargerparticles,whichmaybetoxictoanimals,areremovedfromthesuspension.Botharepreparedandpackagedundersterileconditions.WhenanimalsorcellsaretreatedwithClodrosome®,phagocyticcellsrecognizetheliposomesasinvADIngforeignparticlesandproceedtoremovetheliposomesfromthelocaltissueorserumviaphagocytosis.Theliposomesthenreleaseclodronateintothecytosol,resultingincelldeath.Non-encapsulatedclodronatecannotcrossthecellmembranetoinitiatecelldeath.

Controlliposomes(Encapsome®)arerecognizedandphagocytosedbythesamemechanismasClodrosome®.Sincethecontrolliposomesdonotcontainclodronate,thephagocyticcellsarenotkilled.However,phagocytesdorespondtotheingestionofcontrolliposomesbycytokinesecretion,temporarysuspensionofphagocyticactivityandotherresponsesdescribedintheliterature.

m-Clodrosome®andm-Encapsome®aremannosylatedreagentsthatarespecificallyformulatedtoefficientlytargetthemacrophagesincentralnervoussystemsandmacrophagesthatcontainmoremannosereceptors.Formoreinformationaboutthesereagentseehere.

Fluorescentliposomes(Fluoroliposome®)suitableformacrophagetargetingandtrackingareavailable.Theycancontainfivedifferentfluorescentdyes(DiA,DiD,DiI,DiOandDiR),whichcoverstheentirespectrum.Fluorescentliposomescomeinstandardandmannosylatedform.Formoreinformationseehere.

NormalizedfluorescenceemissionspectraofDiD,DiI,DiOandDiR
MacrophageuptakeoffluorescentliposomecontainingDiO.

DownloadProductInsertDownloadSafetyDatasheet(SDS)

TechnicalInformation

Clodrosome®LiposomalClodronateSuspension

LipidCompositionConcentration(mg/ml)Concentration(mM)MolarRatioPercentage
Total23mg/ml35.1mM100
L-alpha-Phosphatidylcholine18.824.370
Cholesterol4.210.930
EncapsulatedDrugConcentration
Clodronate((Dichloro-phosphono-methyl)phosphonate),DisodiumSalt18.4*mM
*Dependingonthetypeoftheclodronatesalt,itsconcentration(mg/ml)varies.Iftetrahydratesaltisused,theconcentrationoftheencapsulateddrugwillbe~7mg/ml,andifanon-hydratedsaltisused,theconcentrationwillbe~5mg/ml.

Fluoroliposome®-DiO

LipidCompositionConcentration(mg/ml)Concentration(mM)MolarRatioPercentage
Total23mg/ml35.1mM100
L-alpha-Phosphatidylcholine18.824.370
Cholesterol4.210.930
FluorescentDyeExcitation/Emission(nm)Concentration(mg/ml)Concentration(mM)
3,3"-DilinoleyloxacarbocyaninePerchlorate(DiO)484/5010.06250.071
BufferandLiposomeSizeSpecification
BufferPhosphateBufferedSaline
pH7.4
LiposomeSize1.5-2µm

TechnicalNotes

  • TheissuewithfluorescentClodrosome®hastodowiththepotentialforinaccurateand/oruninterpretabledatabeinggeneratedbylabelledClodrosome®.WhenClodrosome®inducesmacrophageapoptosis,thefluorescentlipidincorporatedintotheClodrosome®thatisdisruptedandmetabolizedinthephagolysosomewillbedispersedamongtheresidualapoptoticbodieswhicharesubsequentlyphagocytosedbyothermacrophages.Therefore,fluorescentlipidmaybedetectedinphagocyticcellswhichneverphagocytosedClodrosome®especiallywhenFACSorfluoroscopyareutilizedtodetectfluorescentcells(FACS)orfluorescencelevelsinatissuehomogenate(fluoroscopy).Anotherpotentialartifactarisesfromfluorescentlipidremainingintheextracellular“garbage”,whichhasnotyetbeenclearedbyotherphagocytes,generatingahighbackgroundfluorescence.However,experiencedconfocalmicroscopistmaybeabletodifferentiatebetweenthepunctatefluorescenceresultingfromfluorescentintactliposomesversusthemorediffusefluorescencecharacteristicofdisruptedliposomesandsomehavesuccessfullyusedfluorescentclodronateliposomestovisualizethecellularlocationoftheseliposomesbyconfocalmicroscopyinvivo[1].Afurthercomplicatingfactoristhatpublisheddatavarieswidelyastoexactlywhenclodronateliposomesbegintoinduceapoptosisinmacrophages.Mönkönnnen etal.showthatmacrophagedeathismeasurablewithinthefirsthourafterclodronateliposometreatmentonRAW264cellsinvitro[2],whilemanyothershavereportednosignsofmacrophageapoptosisuntilseveralhoursaftertreatmentinvivo.ThevariABIlityinthedataislikelyduetodifferentliposomalformulationsofclodronateaswellasthevastlydifferentexperimentalconditions.Therefore,aswithmostBIOLOGicalstudies,especiallythoseinvolvingliposomes,theamountoftimebetweentreatingtheanimalorcellswithclodronateliposomesandtheonsetofapoptosiswillneedtobeestablishedineachexperimentalmodel.IfthenatureoftheresearchdemandsthatClodrosome®betrackedratherthanthecontrol,EncapsulacanprovideDiI-labelledClodrosome®uponrequest,andassumingthattheClodrosome®distributioncandefinitivelybeassessedpriortotheonsetofapoptosis,clearandvaliddataonthebiodistributionoffluorescentClodrosome®shouldbeobtainable.Still,formostpurposes,Fluoroliposome®(fluorescentcontrolliposomes)willprovidetherequireddatawithfarfewerpotentialartifacts.
  • Whenmonitoringmonocyteuptakeinvivoinnormalanimals,thecirculatingmonocytesmay“disappear”orshowreducedcountswithinthefirst2hpost-injectionduetomarginationofthemonocytespost-liposomephagocytosis.Thesecellswillre-enterthecirculationwithinafewhours.Sunderkötter etal.demonstratethisphenomenonanddiscussthebehaviorindetail.Alsoconsiderthatcirculatingmonocyteshavealifetimeofabout24hsolabeledmonocyteswillbecontinuallyleavingthecirculation,eveninnormalanimals,duetoagingofthemonocytes[3].
  • WhenanimalsorcellsaretreatedwithClodrosome®,phagocyticcellsrecognizetheliposomesasinvadingforeignparticlesandproceedtoremovetheliposomesfromthelocaltissueorserumviaphagocytosis.Theliposomesthenreleaseclodronateintothecytosolresultingincelldeath.Unencapsulatedclodronatecannotcrossthecellmembranetoinitiatecelldeath.
  • Encapsome®controlliposomesarerecognizedandphagocytosedbythesamemechanismasClodrosome®.Sincethecontrolliposomesdonotcontainclodronate,thephagocyticcellsarenotkilled.However,phagocytesdorespondtotheingestionofthecontrolliposomesbycytokinesecretion,temporarysuspensionofphagocyticactivityandotherresponsesdescribedintheliterature.
  • Theproductmustberemovedfromthevialusingsteriletechnique.Donotuseifsterilityiscompromised.Thisisparticularlyimportantifasinglevialisaccessedmultipletimesoverseveralweeks.Theproductshouldnotbeusedmorethan60daysafterreceipt,evenifunopened.
  • Liposomesmaysettlewhenleftundisturbedformorethanafewhours.Immediatelypriortouse,inordertoensureahomogeneousliposomesuspension,slowlyinvertthevialseveraltimesuntilthesuspensionappearshomogeneousbyvisualinspection.Vigorousorerraticshakingwillnotdamagetheliposomesbutmayinducefoamingandbubbleformationmakingitmoredifficulttoaccuratelymeasurethedesireddosage.
  • Ifthepersonnelperformingintravenousinjectionsarenotexperiencedinorfamiliarwith,precautionsforinjectinglargervolumes(~10%animalweightinml),viscousliquidsorparticulatesuspensions,considerhavingextraanimalsavailableincaseseriousinjection-relatedadverseeventsoccur.Dosecontrolanimalsfirsttobecomefamiliarwithlargevolumeinjections.
  • WithinhoursaftersystemicadmiNISTrationofClodrosome®,animalsbegintoloseimportantcomponentsoftheirimmunesystem.Standardanimalhandlingandhousingprotocolsarenotsuitableforimmunocompromisedanimals.Evenwhensuchprecautionsaretaken,monitorthegeneralhealthofeachanimalforopportunisticinfectionsunrelatedtotheexperimentalprotocol.Thereisnoinherenttoxicitytotheproductattherecommendeddoselevels.
  • Whendosingintravenously,usestandardprecautionsfordosinglargervolumestoanimalsincludingthefollowing:a)Warmproducttoroomtemperaturepriortodosing.b)Ensurethatallairbubblesareremovedfromthesyringepriortodosing;intravenousinjectionofairbubblesmayresultinairemboliwhichcankillorseriouslyinjureanimals.c)Injectproductataslow,steadyrateofnomorethan1ml/min;decreaseinfusionrateifanimalsdisplayanyatypicalreactionssuchasunusualagitation.
  • Infusion-relatedadversereactionsusuallyinvolvetheanimalgaspingforairorotherseizure-likemovements.Animalsoftenrecoverwithnoapparentpermanentinjury,butanypotentialeffectsonexperimentalresultsmustbeassessedbytheresearcher.
  • Liposomesshouldbekeptat4°CandNEVERbefrozen.

Dosage

ClickheretoloadthisCaspio

Appearance

Clodrosome®isawhitemilkysuspension,andFluoroliposome®-DiOisayellowliquidsuspension,bothmadeoflargemicrosizemultilamellarliposomes.Duetotheirlargesize,someliposomesmightsettletothebottomofthevial.Ifleftsittingidleintherefrigerator,Fluoroliposome®-DiOwillphaseseparateandformpelletsinthebottomofthevial,leavingaclearsolutionontop.Clodrosome®mightdothesameonlynotasseverely. Therefore,bothshouldbegentlyshakennottoformbubblesbuttoformahomogeneoussolutionpriortouse.

EducationalVideos

Ordering/ShippingInformation

  • Allliposomebasedformulationsareshippedonblueiceat4°Cininsulatedpackagesusingovernightshippingorinternationalexpressshipping.
  • LiposomesshouldNEVERbefrozen.Icecrystalsthatforminthelipidmembranecanrupturethemembrane,changethesizeoftheliposomesandcausetheencapsulateddrugtoleakout.Liposomesinliquidformshouldalwaysbekeptintherefrigerator.
  • ClientswhoorderfromoutsideoftheUnitedStatesofAmericaareresponsIBLefortheirgovernmentimporttaxesandcustomspaperwork.EncapsulaNanoSciencesisNOTresponsibleforimportationfeestocountriesoutsideoftheUnitedStatesofAmerica.
  • WestronglyencouragetheclientsinJapan,Korea,TaiwanandChinatoorderviaadistributor.Toughcustomsclearanceregulationsinthesecountrieswillcausedelayincustomclearanceoftheseperishableformulationsifordereddirectlythroughus.Distributorscaneasilyclearthepackagesfromcustoms.Toseethelistofthedistributorsclickhere.
  • ClientsorderingfromuniversitiesandresearchinstitutesinAustraliashouldkeepinmindthattheliposomeformulationsaremadefromsyntheticmaterialandtheformulationsdonotrequirea“permittoimportquarantinematerial”.LiposomesareNOTbiologicalproducts.
  • Ifyouwouldlikeyourinstitute’sFedExorDHLaccounttobechargedforshipping,thenpleaseprovidetheaccountnumberatthetimeofordering.
  • EncapsulaNanoScienceshasnocontroloverdelaysduetoinclementweatherorcustomsclearancedelays.YouwillreceiveaFedExorDHLtrackingnumberonceyourorderisconfirmed.ContactFedExorDHLinadvanceandmakesurethatthepaperworkforcustomsisdoneontime. AllsubsequentshippinginquiriesshouldbedirectedtoFederalExpressorDHL.

StorageandShelfLife

Storage

Clodrosome®and Fluoroliposome® shouldalwaysbestoredatinthedarkat4°C,exceptwhenbroughttoroomtemperatureforbriefperiodspriortoanimaldosing.DONOTFREEZE.Ifthesuspensionisfrozen,clodronatecanbereleasedfromtheliposomesthuslimitingitseffectivenessindepletingmacrophages.ENSisnotresponsibleforresultsgeneratedbyfrozenproduct.

ShelfLife

Clodrosome®andFluoroliposome® aremadeondailybasis.Thebatchthatisshippedismanufacturedonthesameday.Itisadvisedtousetheproductswithin60daysofthemanufacturingdate.

Referencesandbackgroundreading

1.PolflietMM,GoedePH,vanKesteren-HendrikxEM,vanRooijenN,DijkstraCD,vandenBergTK.Amethodfortheselectivedepletionofperivascularandmeningealmacrophagesinthecentralnervoussystem.J.Neuroimmunol.2001Jun1;116(2):188–95.

2.MönkkönenJ,LiukkonenJ,TaskinenM,HeathTD,UrttiA.Studiesonliposomeformulationsforintra-articulardeliveryofclodronate.JournalofControlledRelease.1995Aug;35(2–3):145–54.

3.SunderkötterC,NikolicT,DillonMJ,vanRooijenN,StehlingM,DrevetsDA,LeenenP.SubpopulationsofMouseBloodMonocytesDifferinMaturationStageandInflammatoryResponse.JImmunol.2004Apr1;172(7):4410–7.

4.HinsonSR,CliftIC,LuoN,KryzerTJ,LennonVA.Autoantibody-inducedinternalizationofCNSAQP4waterchannelandEAAT2glutamatetransporterrequiresastrocyticFcreceptor.ProceedingsoftheNationalAcademyofSciences.2017May23;114(21):5491-6.

5.DhupkarP,GordonN,StewartJ,KleinermanES.Anti‐PD‐1therapyredirectsmacrophagesfromanM2toanM1phenotypeinducingregressionofOSlungmetastases.CancerMedicine.2018May7.

6.XiongY,PageJC,NarayananN,WangC,JiaZ,YueF,ShiX,JinW,HuK,DengM,ShiR.Peripheralneuropathyandhindlimbparalysisinamousemodelofadipocyte-specificknockoutofLkb1.EBioMedicine.2017Oct1;24:127-36.

7.CriderA,FengT,PandyaCD,DavisT,NairA,AhmedAO,BabanB,TureckiG,PillaiA.Complementcomponent3areceptordeficiencyattenuateschronicstress-inducedmonocyteinfiltrationanddepressive-likebehavior.Brain,behavior,andimmunity.2018Mar5.

8.KocherT,AsslaberD,ZaborskyN,FlenadyS,DenkU,ReinthalerP,AblingerM,GeisbergerR,BauerJW,SeiffertM,HartmannTN.CD4+Tcells,butnotnon-classicalmonocytes,aredispensableforthedevelopmentofchroniclymphocyticleukemiaintheTCL1-tgmurinemodel.Leukemia.2016Jun;30(6):1409.

9.ZhuZ,DingJ,MaZ,IwashinaT,TredgetEE.Systemicdepletionofmacrophagesinthesubacutephaseofwoundhealingreduceshypertrophicscarformation.WoundRepairandRegeneration.2016Jul1;24(4):644-56.

10.HaqueMR,LeeDY,AhnCH,JeongJH,ByunY.Localco-deliveryofpancreaticisletsandliposomalclodronateusinginjectablehydrogeltopreventacuteimmunereactionsinatype1diabetes.Pharmaceuticalresearch.2014Sep1;31(9):2453-62.

11.MayoL,CunhaAP,MadiA,BeynonV,YangZ,AlvarezJI,PratA,SobelRA,KobzikL,LassmannH,QuintanaFJ.IL-10-dependentTr1cellsattenuateastrocyteactivationandamelioratechroniccentralnervoussysteminflammation.Brain.2016May31;139(7):1939-57.

12.KermanizadehA,ChauchéC,BalharryD,BrownDM,KanaseN,BoczkowskiJ,LanoneS,StoneV.TheroleofKupffercellsinthehepaticresponsetosilvernanoparticles.Nanotoxicology.2014Aug31;8(sup1):149-54.

13.NandiB,ShapiroM,SamurMK,PaiC,FrankNY,YoonC,PrabhalaRH,MunshiNC,GoldJS.StromalCCR6drivestumorgrowthinamurinetransplantablecoloncancerthroughrecruitmentoftumor-promotingmacrophages.Oncoimmunology.2016Aug2;5(8):e1189052.

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用哪家公司的免疫组化试剂盒好一些?打算用SABC染色的,其他方法也行。
实验进度比较紧,近期急求dako公司的envision试剂盒免疫组化非生物素二抗系统,需要做50张片子,但官方最小的版本是做500张片子,供应商要价13000,所以求助大家,是否曾经购置此试剂,愿购买或交换相关资源,谢谢!谢谢!
如能成功,愿追加50个或更多蚁豆,麻烦大家帮忙~~
即用型快捷免疫组化 MaxVision TM 试剂盒是根据聚合物技术把过氧化物酶与抗鼠或/和抗兔IgG分子结合在多聚物上形成多聚物分子。
我做肉瘤的免疫组化一抗用的ABCom,二抗和DAB用的博士德,但是做了几次都没有任何染色。由于烘箱60度烤片我只烤了20分钟,可能时间短了,但苏木素可以染上,是否说明烤片、脱蜡已足够。
用双氧水去除过氧化物酶时,我是自己配的3%双氧水滴到片上而非将片浸入双氧水,这样可否?
用博士德的DAB染色,配制方法为:1mlH20中加入DAB、H2O2、TBS各一滴,我配制的时候发现将DAB加入H20时很容易沉淀,要震荡才能混匀,且将配好的DAB滴到玻片上时,DAB会结为很小块的微颗粒悬浮在液体中但并不染色,是否DAB有问题?
现在打算换中衫的试剂盒,代理商说中衫的试剂盒包括了二抗和DAB,想请教一下该试剂盒的具体内容有些什么?
万分感谢!
各位战友大家好!我目前在做SD大鼠腹主动脉球囊损伤模型,模型刚刚建成,需要检验模型是否建成功。需要做一个免疫组化。可是咨询了几家试剂公司,都没有PCNA免疫组化的试剂盒。想咨询各位战友们,有谁知道哪家有卖SD大鼠血管PCNA免疫组化试剂盒的,请指点一二,哪家的试剂盒比较好。我的联系方式是463843267@qq.com。谢谢!
EnVision是DAKO公司推出的一种两步法免疫组化技术,又称为ELPS法。EnVision比SP,ABC一般的显色比较:1 要敏感很多,定位比较好:EnVision系统是将二抗和酶联接成一个多聚体(即EnVision)直接放大信号40-50倍,再与已经结合的一抗反应,最后显色剂显色。采用该法可将一抗稀释度提高1~2倍,尤其对抗原表达较弱组织。也有人说SP法敏感度比EnVision高1-2倍,但SP法毕竟不宜用于富含亲生物素物质的组织。2 非特异性背景少: EnVision法是多聚物上连接二抗和酶,在组织中不含有这种多聚物,从而避免了组织中生物素的干扰。在含生物素较丰富的组织中,用EnVision法比较好。除血细胞较丰富的组织和坏死组织外,其实可省略内源性过氧化物封闭步骤。3 比较省时:染色步骤为两步,且第二抗体孵育时较短。EnVision程序:1) 脱蜡、水化组织切片。2) 预处理组织切片3) 蒸馏水漂洗,置于TBS中。4) 阻断内源性过氧化物酶(仅用于EnVision TM)5) 蒸馏水漂洗,置于TBS,10分钟6) 一抗孵育10-30分钟7) TBS漂洗10分钟8) EnVisionTM孵育10-30分钟9) TBS漂洗10分钟10) 色源底物溶液孵育10分钟11) 蒸馏水漂洗12) 复染及封片
elisa试剂盒抗体一般不能用于免疫组化。

一、免疫组化试剂盒一般包括:
1、特异性的一抗
2、免疫组化检测系统。
3、有的同时还具备显色系统。
二、不同的公司内容有差别,所以购买时一定了解清楚:
1、一抗是做人的还是兔、鼠的组织;
2、检测系统是ABC/SP/非生物素/其他;
3、试剂盒的内容都有什么?有没有显色系统?
4、如果没有,自己根据前面的检测系统需配哪个显色系统。(其他的辅助试剂如PBS缓冲液、抗原修复液等一般另卖或自配)
三、免疫组化抗体即指特异性一抗,是用来标记的指标,免疫组化过程的其他试剂一律另外配备。
另外:做实验时,如遇出结果困难,记得做阳性片对照,敢于怀疑检测系统或显色系统的问题。
最近想用免疫组化鉴定干细胞原代细胞,想了解国内哪家公司的免疫组化试剂盒做得最好、最专业?
福州迈新和北京康为相比,哪个比较好?还有博士德、中杉金桥都怎么样?
不管报价,只要品质,国产IHC试剂盒中最好的,请各位大侠不吝指教,谢谢!
免疫组化试剂盒检测标本的数量和你盒子大小有直接关系,盒子大的检测的就多!
免疫组化试剂盒是通用的吗?比如我要做小鼠MMp-9的,是买一种含兔抗鼠一抗的就行,还是必须要买MMP-9的兔抗鼠一抗才可以?
免疫组化试剂盒,有国产的和进口的
上海好多的供应商的,具体还是看你选择了,其实试剂盒产品都差不多,什么远慕生物,古朵生物...好多的额
本人是新手,近来要做大鼠肝脏α-SMA免疫组化,是否单单购买α-SMA免疫组化试剂盒就够了,试剂盒里面是否就包含一抗二抗等?是否需要购买其他试剂?还是一抗、二抗分开来买?谢谢!