For Laboratory Or Hospital High Accuracy HBsAg Elisa Test Kit

INTENDED USE

  HBsAgELISAisanenzyme-linkedimmunosorbentassay(ELISA) forqualitativedetectionofHBsAginhumanserum orplasma. It isintendedforscreeningofblooddonorsandfordiagnosingofpatientsrelatedtoinfectionwithhepatitis Bvirus.

PROCEDURE

Reagentspreparation:

Allowthereagentstoreachroomtemperature(18-30°C).ChecktheWashbufferconcentrate for thepresenceofsaltcrystals. Ifcrystalshaveformed, resolubilizebywarmingat37°Cuntilcrystalsdissolve.Dilute theWashbuffer (20X)as indicated in the instructions forwashing.Usedistilledordeionizedwaterandonlyclean vesselstodilutethebuffer.AllotherreagentsareREADYTOUSEASSUPPLIED.

Step1 Preparation:MarkthreewellsasNegativecontrol (e.g.B1,C1,D1), twowellsasPositivecontrol (e.g. E1,F1)andoneBlank(e.g.A1,neithersamplesnorHRP-Conjugateshouldbeadded intotheBlank well). If theresultswillbedeterminedbyusingdualwavelengthplatereader, therequirement foruseof Blankwellcouldbeomitted.Useonlynumberofstripsrequiredforthetest.

Step2 AddingSample:Add50μlofPositivecontrol,Negativecontrol,andSpecimenintotheirrespectivewells except theBlank.Note:Useaseparatedisposalpipettetipforeachspecimen,NegativeControl, PositiveControltoavoidcross-contamination.Mixbytappingtheplategently.

Step3 AddingHRP-Conjugate:Add50μl of HRP-Conjugate intoeachwell except theBlank, andmixby tappingtheplategently.

Step4 Incubating:Covertheplatewiththeplatecoverandincubatefor60minutesat37°C.

Step5 Washing:At theendof theincubation,removeanddiscardtheplatecover.Washeachwell5timeswith dilutedWashingbuffer.Eachtimeallowthemicrowellstosoakfor30-60seconds.Afterthefinalwashing cycle,turndowntheplateontoblottingpaperorcleantowelandtapittoremoveanyremainders.

Step6 Coloring:Add50μlofChromogenAand50μlChromogenBsolutionsintoeachwell includingtheBlank. Incubate the plate at 37°C for 15minutes avoiding light. The enzymatic reaction between the ChromogensolutionsandtheHRP-ConjugateproducesbluecolorinPositivecontrolandHBsAgpositive samplewells.

Step7 StoppingReaction:Usingamultichannelpipetteormanually,add50μlofStopSolutionintoeachwell andmixgently.IntensiveyellowcolordevelopsinPositivecontrolandHBsAgpositivesamplewells.

Step8 MeasuringtheAbsorbance:CalibratetheplatereaderwiththeBlankwellandreadtheabsorbanceat 450nm. Ifadual filter instrument isused, set thereferencewavelengthat630nm.CalculatetheCut-off valueand evaluate the results. (Note: read the absorbancewithin 10minutes after stopping the reaction).