Thereis hardly anyotherdevelopmento

Thereis hardly anyotherdevelopmentofmethods that has reached a varietycornparableto
6thatof enzymeimmunoassays(EIA)basedon thereactionbetweenantigenandantibody.Never-theless, newvariantsare beingsteadilydevelopedwith the aim of (I)increasingsensitivity;(2)increasingspecificity;(3)reducingthedurationof assays;(4)facilitatingtheperformanceof assays.This overview shall provide aninsightintothestateoftheart,outlinetendenciesoffundamen-taltechniquesand behelpfulforthedevelop-ment of EIAs forlaboratoryuse.Basicprinciple ofimmunoassaysImmunoassayscan begenerallydividedintounlabelledand labelIed ones.Mostunlabelledtechniquesare based onsecondaryimmunereac-tions, as, e.g.,precipitationandagglutination.They aremeasuredbylightscatteringorpartidecountingmethods.LabelIedimmunoassaysarebased on the primaryimmunereaction.Therearetwo types,dependingonthereactionprinciple:(l)type I'reagent-observed';(2)type11'analyte-observed'(Ekins, 1981a).Whereasin the type I assaythereis excess ofantibody as binder, it limits thereactionin thetype II assay with excess ofanalyte.Type11assays have got a maximumtheoreticalsensitivityof about 10-14moljl(Ekins, 1981b) and arethereforeone to twoordersofmagnitudelesssensitive than type I assays,Themaximumsensi-tivity of type I assays, which are alsocalled'two-site assay' or'sandwichassay',rangesbetween10-15and10-16moljl(Jacksonet al., 1983).Unliketype II assays, which are used todeter-minebothhaptensandsubstancesof high molec-ular weight, type I assaysrequiresubstancesto beused asanalytewith atleasttwodifferentepi-topesdearlydistinct from eachotherinordertopermitepitope-differentlabelIed andunlabelledantibodiesto bindwithoutsterichindrance.TypeI assaysarethusunsuitableforhaptenquantifica-tion.Thedifferentcharacteristicsof typelandtype11assays are listed inTableI.The decision to useoneor theotherassayprincipleis mainlyinfluencedbythefollowingaspects:TABLEICHARACTERISTICSOFTYPEI'REAGENT-OB·SERVED'ANDTYPEII'ANALYTE·OBSERVED'AS·SAYS(FrornNakamura,R.M., Voller,A.and Bidwell, D.E., 1986)Type I'reagent-observed'(excessantibody)(l)Maximal sensitivity isattainedas amount of antibodyapproachesinfinity,(2)Theoreticalsensitivity of assay is one moleeule ofanalyte,(3)Cross-reactionantigens will beequipotentwith exeessantibody system.(4)Antigen-antibodyreactionis less influenced by substancessuch as salt and urea.(5) Assaytimeis relativelyrapidwith labelIed antibody proce-dures.Type II'analyteobserved'(excessanalyte)(l)Maximal sensitivity isattainedwhen antibodyconcentra-tionapproaeheszero.(2) Thissaturationassay isregulatedbythe equilibrium con-stantof thereactionbetweenanalyteand antibody.(3) Sensitivity of the assay isdependentupon the affinityeonstantoftheantibody.(4)Cross-reactiveantigen willdemonstratea relative poteneydependentupontherateof the equilibriurn eonstants oftheanalyteandcross-reactiveantigen.(5) Assay reactionis slow sinceequilibriummust be reached.- size,availabilityandlabellingcapacity of ana-lytes,-sensitivityandspeedofanalytedetermination.Iftheanalyteis smalI, easy to isolate, synthesizeandlabel,thereare nospecialrequirementsonassaysensitivity,itsdeterminationin a type11assayusinglabelIedantigenwill be obvious. H, ontheotherhand,theanalyteis of highmolecularweight,difficultto purify forlabellingin suffi-cientquantityandrequiresa high sensitivity, thetype I assay usinglabelIedantibodies(MilesandHaies,1968) willbethemethodof choice. Todeterminetheextentoftheimmunereaction,theunboundlabelIedre agenthas to beeithersepa-ra ted fromtheboundone(heterogeneousassay)Oftheactivityof the label has to bechangedtotheextentof theimmunere action in a way tomakeseparationofboundand freereactants(bfseparation)superfluous(homogeneousassay),