Description:

CytokinesaresignalingmoleculesthathavecriticalrolesinmanyBIOLOGicalprocessessuchascellulargrowth,differentiation,geneexpression,migration,immunity,andinflammation.Cytokinesthataresecretedfromcellsbindtocell-surfacereceptors, initiatetheactivationofsignaltransductionpathwaysandmediatecelltocellcommunication.Themalfunctionofcytokinesleadstomanydiseases,includingarthritis,acuteandchronicliverdisease,inflammatoryboweldisease,cardiac-relateddiseases,andcancers.Cytokinesarecommonlyworkingtogether ina biologicalordiseaseprocess.Therefore,thecomprehensiveanalysisoftheexpressionofmultiplecytokinesallowseffectivelyrevealingtheunderneathmechanismofcytokineaction andthealterationleADIngto diseases.TheMouseCytokineELISAPlateArrayisachemiluminescentdetectionthatallowsyoutomonitortheabundanceof24mousecytokinessimultaneously.Thisfastandsensitiveassay canbeusedforquantitativecomparisonof thesecytokinesamongdifferent samples.

ApplicableGrid:

ListofApplicableCytokines

1

2

3

4

5

6

7

8

9

10

11

12

A

TNFa

IL-1a

PDGF-BB

TNFa

IL-1a

PDGF-BB

TNFa

IL-1a

PDGF-BB

TNFa

IL-1a

PDGF-BB

B

IGF-1

IL-1b

b-NGF

IGF-1

IL-1b

b-NGF

IGF-1

IL-1b

b-NGF

IGF-1

IL-1b

b-NGF

C

VEGF

G-CSF

IL-17A

VEGF

G-CSF

IL-17A

VEGF

G-CSF

IL-17A

VEGF

G-CSF

IL-17A

D

IL-6

GM-CSF

IL-2

IL-6

GM-CSF

IL-2

IL-6

GM-CSF

IL-2

IL-6

GM-CSF

IL-2

E

FGFb

MCP-1

IL-4

FGFb

MCP-1

IL-4

FGFb

MCP-1

IL-4

FGFb

MCP-1

IL-4

F

IFNy

MIP-1a

IL-10

IFNy

MIP-1a

IL-10

IFNy

MIP-1a

IL-10

IFNy

MIP-1a

IL-10

G

EGF

SCF

Resistin

EGF

SCF

Resistin

EGF

SCF

Resistin

EGF

SCF

Resistin

H

Leptin

Rantes

IL-12

Leptin

Rantes

IL-12

Leptin

Rantes

IL-12

Leptin

Rantes

IL-12

Principle:

The96-wellwhiteplateisdividedinto3or4sections,andeachsectionhas4or3columnsforonesample.Ineachsection,32(HumanCytokineELISAPlateArrays)or24(MouseCytokineELISAPlateArray)specificcytokinecaptureantibodiesarecoatedon32or24wellsrespectively.Thesample,cellculturesupernatants,celllysates,tissuehomogenates,serum,orplasmasamplesamongothers areincubatedwiththecytokineELISAplate,and thecapturedcytokineproteinsaresubsequentlydetectedwithacocktailofbiotinylateddetectionantibodies.Thetestsampleisallowedtoreactwith apairof antibodies,resultinginthecytokinesbeingsandwichedbetweenthesolidphaseandenzyme-linkedantibodies.Afterincubation,thewellsarewashedtoremoveunbound-labeledantibodies.TheplateisfurtherdetectedwithHRPluminescentsubstrateorHRPsubstrateTMB.Thelevelofexpressionforeachspecificcytokineisdirectlyproportionaltotheluminescentorcolor intensity.

 

Data:

AnalysisofCytokineProteinExpressioninTNFa-TreatedandUntreatedNIH3T3withMouseCytokineELISAPlateArray.NIH/3T3cellswerestarvedfor24hourswithserum-freemedium,subsequentlytreatedthecellswithandwithout20ng/ulTNFfor16hours.Theserum-freeconditionedmediawereincubatedontheplatefor1hour.AfterincubatingwithdetectionantibodymixandHRP,theplatewasdetectedwithchemilumincentsubstratebyaplatereader.

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