快报
欢迎光临蚂蚁淘在线! 请登录 免费注册
商品
品牌
文章
热门搜索:
快报
品牌首页 品牌新闻 品牌简介 产品中心 品牌咨询 联系我们
品牌分类
品牌咨询
联系方式
公司地址
苏州工业园区生物纳米园A4#216
联系电话
4000-520-616 / 18915418616
传真号码
0512-67156496
电子邮箱
info@ebiomall.com
公司网址
https://www.ebiomall.com
蚂蚁淘在线 / 品牌中心 / Everest Biotech / 珠穆朗玛峰生物技术/Ki67免疫组织化学试剂盒10张载玻片/3100010105/10张载玻片

珠穆朗玛峰生物技术/Ki67免疫组织化学试剂盒10张载玻片/3100010105/10张载玻片

价格
¥3473.60
货号:3100010105
浏览量:127
品牌:Everest Biotech
服务
全国联保
正品保证
正规发票
签订合同
商品描述

Ki67antigenistheprototypiccellcyclerelatednuclearprotein,expressedbyproliferatingcellsinallphasesoftheactivecellcycle(G1,S,G2andMphase).Itisabsentinresting(G0)cells.Ki67antibodiesareusefulinestablishingthecellgrowingfractioninnormal,neoplasticandregenerativetissues.

Imageshowsimmunohistochemicalstainingofparaffin‐embeddedhumanglioblastomaxenografttumorsectionstainedwithKi67antibodyusingtheEtonBio’sKi67IHCKit(CatNo.3100010105).Ki67(darkbrown)displaysanuclearlocalizationpatternwhichcorrelatesitsfunctionincycleprogression(20X,counterstainedwithhematoxylin).

KitContents

Reagentsprovidedinthekit

Thematerialslistedaresufficientfor20tests.Thenumberoftestsisbasedontheuseof200μLeachofreadytousereagentperslide.

PositiveControlSlides

Onehumanrenalcarcinomaslides

BlockingBuffer

10XNon-specificblockingbuffer

Diluteat1:10usingdistilledwaterpriortostaining;unusedworkingsolutionmaybestoredat4°Cfor3month.

EquilibriumBuffer

EquilibriumBuffer

Readytousereagent

Rabbitanti-Ki67antibody

Rabbitanti-Ki67antibody

DiluteinAntibodyDiluentsimmediatelybeforeuse(recommenduseat1:100dilution).

AntibodyDiluent

AntibodyDilutent

Readytousereagent

WashBuffer

TrisbufferedsalinewithTween20(pH7.6)

Diluteat1:20usingdistilledwaterpriortostaining;unusedworkingsolutionmaybestoredat4°Cfor3month.

RabbitHRPPolymer

RabbitHRPPolymer

Readytousereagent

DABsubstratebuffer

10XDABsubstratebuffer

HydrogenPeroxide(H2O2)forDABsubstratebuffer

0.3%HydrogenPeroxidesolution

DABChromogen

Diaminobenzedinetetrahydrochloride(DAB)substratesolution(DonotexposeDABcomponentstodirectorbrightlightduringstorageandstainingprocess).

Materialsrequiredbutnotincludedinthekit

Reagents:

Xylene

Ethanol

EndogenousPeroxidaseBlockingSolution(3%HydrogenPeroxide)

Hematoxylin

Mountingmedia

Distilledordeionizedwater

AntigenRetrievalBuffer(10X)0.1MCitrateBuffer(pH6.0)

LabEquipment:

Steamerormicrowaveoven(forantigenretrieval)

PAPpenforrestrainingreagentsonslides

Moistchamberforslidesincubationwithstainingreagents

Generallabequipmentforimmunohistostainingsuchasslideracks,stainingjars,coverslips,timer,Pipettes,etc.Microscopeequipmentandaccessories

StorageandstABIlity

StoreKi67IHCKitsat28°C.Thekitisstableforsixmonthsat4°C.Donotuseafterexpirationdate.

Precautions

Takereasonableprecautionswhenhandlingreagents.UsedisposablegloveswhenhandlingsUSPectedcarcinogensortoxicmaterials(examples:DAB,xyleneandH2O2).Unusedsolutionshouldbedisposedaccordingtoapplicablelocal,stateandfederalregulations.

TheKi67ImmunohistostainingKithasbeendesignedforthestainingoftissuesthathavebeenfixed(usuallyinneutralbufferedformalin)andsubsequentlyembeddedinparaffinbeforesectioning.Thisprotocolisrecommendedasastartingpointandoptimizationbytheindividualend‐usermayberequired.

Note:

·Donotallowspecimenstodryduringthestainingprocedure.Specimendryingmaycauseincreasednonspecificstainingandbackground.

·Sometissuemayneedtobaketoremoveover‐coveredparaffinpriortotheprocedure.Ifneeded,bakeat55‐60°Cfor30minutes.

I.Deparaffinizationandrehydration
Priortostaining,tissuesectionsmustbedeparaffinizedandrehydrated.Incompleteremovalofparaffincancausepoorstainingofthesection.Usepositivecontrolslideprovidedinthekitforqualitycontrolandtrouble-shootingpurpose.
1.Immerseslidesinxyleneandincubatefor5minutes.Repeattwicewithfreshxyleneforanother5minuteseach.
2.Immerseslidesin100%ethanolfor5minutes,andfollowwithimmersionin95%,75%and50%ethanolfor3minuteseach.
3.Rinseslideswithdistilledwaterfor5minutes;keepinwateruntilreadytoperformantigenretrieval.
II.Heatinducedantigenretrieval(HIAR)
Mostformalin‐fixedtissuerequiresanantigenretrievalstepbeforeimmunohistochemicalstainingcanproceed.Heatinducedantigenretrievalcanbeperformedusingasteamer,pressurecooker,oramicrowaveoven.Theretrievaltimewritteninthisprotocolisbasedonusingasteamer.Theheatingtimemayneedtobeadjustedifyouuseadifferentdeviceandmethod.
1.Fillplasticcoplinjar/containerwithAntigenRetrievalBuffer(0.01MCitrateBuffer,pH6.0,notincludedinthekits).
PrepareStockSolution:
A.0.1MSodiumCitrate;
B.0.1MCitricAcid
Tomake250mL1Xantigenretrievalbuffer,mix20.5mLstocksolutionAwith4.5mLstocksolutionBandadddistilledwaterto250mL
2.Placethecoplinjar/containerinsteamerwithlid.
3.Turnonsteamerandpreheatto90‐100°C.Carefullyputslidesintothecoplinjar/containerandsteamfor40min(95‐100°C).
4.Turnoffthesteamer,removethecoplinjar,placeatroomtemperatureandallowslidestocoolfor20min.Keepthejarcoveredallthetime.
5.Rinseslidebyincubationofslideindistilledwaterfor3minutes.Repeatthissteptwiceandbeginstainingprocedure.
III.Stainingprocedure
BlockingofEndogenousPeroxidase

Note:PeroxidaseBlockingisoptional.Ifnonon-specificstainingisobserved,skipthesestepsandgotostep3.
1.Tapoffexcesswater.DrawacirclearoundthespecimenontheslidewithPAPpen(notincludedinthekit.Alternatively,foldedKimwipescouldbeusedtobrieflyblotthewateraroundthespecimen.Repeatthisblotstepeachtimebeforeaddreagentonslide).Apply200μlormoreofPeroxidaseBlockingSolution(notincludedinthekit)sufficienttocoverspecimen,andincubatefor5minutes.
2.Rinseslidebyincubationofslideindistilledwaterfor3minutes.Repeatthissteptwice.
3.RinseslidebyincubationslideinPBSfor3minutes.
BlockingofNon-specificbinding

4.TapoffexcessPBS.(IfthePeroxidaseBlockingstepisskipped,drawacirclearoundthespecimenontheslidewithPAPpenorusingtheedgeoffoldedKimwipestoquicklyblotthewateraroundthespecimen).Apply200μl1XBlockingBufferimmediatelytocoverspecimenandincubateinamoistchamberfornomorethan10minutes
Note:10Xblockingbuffermayformprecipitatesat4°C.Completelydissolvetheprecipitatesbeforemakingworkingsolution
5.RinseslidebyincubationslideinPBSfor3minutes.

PrimaryAntibody
6.TapoffexcessPBS.Apply200μlEquilibriumBufferimmediatelytocoverspecimenandincubateinamoistchamberfor30minutes
7.TapoffexcessEquilibriumBuffer.Apply200μlanti‐Ki67antibody(recommend1:100dilutioninAntibodyDiluent)tocoverspecimenimmediatelyandincubateinamoistchamberovernightat4°C.
8.Rinseslidebyincubationin0.5-2mLWashBufferfor3minutes.Repeatthissteptwicewithfreshbuffer.
9.RinseslidebyincubationofslideinPBSfor3minutes.
Secondary/HRPConjugates

10.TapoffexcessPBS.Apply200μlRabbitHRPPolymerimmediatelytocoverspecimenandincubateinamoistchamberfor60minutes.
11.Rinseslidebyincubationin0.5-2mLWashBufferfor3minutes.Repeatthissteptwicewithfreshbuffer.
12.RinseslidebyincubationinwithPBSfor3minutes.
DABChromogen
13.TapoffexcessPBS.ApplyenoughDABSubstrateSolutiontocoverspecimenimmediatly.Checkdarkbrowncolordevelopmentundermicroscopeandincubateuntildesiredstainintensitydevelops.
Tomake1mLDABSubstrateSolution,mixthefollowingreagents:
DistilledWater860μL
10XDABsubstratebuffer100μL
0.3%HydrogenPeroxidesolution15μL
DABChromogen25μL
14.Rinseslideintapwaterfor3minutes.
Counterstaining
15.Ifdesired,completecounterstain(Seeinstructionforhematoxylincounterstaining).Rinseintapwatertoclear.
Mounting
16.Immerseslidesin70%,80%,95%Ethanolfor2minuteseach,and100%Ethanolfor10minutestwicefollowedbyXylenefor5minutestwice.
17.Dryandmountslides.
IV.InstructionforHematoxylincounterstaining
1.Immerseslidesinhematoxylinsolution.Incubatefor30secondsto5minutes,dependingonthestrengthofhematoxylinused.
2.RinsetoclearwithtapwaterandcontinuedehydrationfromStep16.

Problems
PossIBLeCauses
Solutions
Overstaining
1.Toolongincubationtimeofprimaryantibody,ortoohightemperaturewhendoingstaining

2.ToolongincubationtimeofDABsubstrate.
3.Slidedriedduringstainingprocess
Dependingontissuesections,theincubationtimeofprimaryantibodycanbereducedto2hours;Checktheroomtemperaturerangeisat20-250Cwhendoingstaining.
ReduceincubationtimeofDABsubstrate
Avoidsectionstodryduringstainingprocess.
Weakornostaining
1.Incompleteremovalofparaffin

2.Tissuesoverfixation

3.Notefficientantigenretrieval

4.Reagentsnotusedinproperorderoromittedsteps

5.Expiredantibodyorreagents
Deparaffinizesectionslongerorchangetofreshxylene;sometissuearraymayneedtobaketo
removeovercoveredparaffin.
Increasingtheconcentrationofprimaryantibodyto1:40;ifthisdoesnotwork,reducedurationof
postfixation.
Adjustantigenretrievaltimebasedonthesettingforsectionfixationandretrievaldeviceused.
Reviewnotesandprocedureused.

Checkkitexpirationdatesandkitstorageconditions
Highbackground
1Sectionsdriedduringstainingprocess

2Slidenotrinsedthoroughly

3Antigenoverretrieval
Donotallowsectionstodryduringstainingprocess;usehumidcontainerduringincubation
withprimaryantibody.
Usefreshsolutioninbufferjars;rinseatleastthreetimesbetweensteps.
Optimizeantigenretrievaltimeifyouusedmicrowaveorpressurecookerforretrieval.

Everest Biotech的山羊多克隆抗体以Everest Elite Grade或Aspiring Grade产品的形式发布,这取决于它们的测试性能和对靶蛋白的了解程度。Everest Biotech提供了圣克鲁斯多克隆产品系列的高质量替代品 精英级抗体保证按数据表上的规定工作,或退款。肽ELISA数据显示它们可以识别免疫肽。Western印迹数据显示生理相关组织或细胞系上的正确大小带。IHC / IF数据和特定出版物(如果有)。100%满意保证也可批量提供给化验开发人员 有抱负的抗体快速将市场上几乎没有或没有商业抗体可用且在文献中几乎没有表达数据的靶标引入市场。由肽ELISA数据支持。背景低但带大小错误或在可用于测试的常见细胞系和组织范围内没有信号。以大幅降低的价格出售,但我们不确定他们会在任何应用中识别天然蛋白质。100%满意保证奖励分享显示抗体成功发挥作用的数据-将您的数据提交到support@everestbiotech.com可获得您选择的免费抗体。免疫肽产生抗体的肽可用于封闭实验以100µg冻干肽的形式出售

  • 资质认证

    获得国家资质,权威认证!

  • 全国联保

    全国联保,官方无忧售后

  • 正规发票

    正规发票,放心购买

  • 签订合同

    签订合同,保障您的权益

购物指南
购物流程
注册登录
账户管理
订单查看
常见问题
FAQS
蚁豆兑换
物流说明
评论规则
发票说明
价格说明
支付说明
服务协议
版权声明
诚信保障
免责申明
销售协议
隐私条款
法律申明
售后服务
退换货政策
工作时间
退款说明
售后支持
售后申请表模板列表
关于我们
公司简介
联系我们
资质证书
人才招聘
商务合作
万众创业
网址导航
蚂蚁淘商城
科研狗
苏州蚂蚁淘
生物信息网
现货促销

微信公众号

copyright©2005-2021 蚂蚁淘在线版权所有 苏州蚂蚁淘生物科技有限公司 www.assay-online.com ICP号:苏ICP备17049038号-16

/**/