Determination of clenbuterol in bovine tissues and urine by enzyme immunoassay

Snnple enzyme unmunoaasays are desclrbed which enable clenbuterol to be determmed m bovme hver homogenate and eye (aqueous humour and chorold/plgmented retmal eptthehum) by drrect anaiysls, and 111 urme followmg sobd-phase extra&on and concentration The sensltnMy, analytxal recovery and lmeanty of r

Procedures are described for optmusmg and vabdatmg an ELISA method for measurmg clenbuterol residues m bovme bver wlthout pnor sample ennchment Optunal assay conddlons are obtamed by premcubatmg bver supematant wllth an unmoblhsed antibody rmed to clenbuterol-ovalbumen After further mcubatlon wrth a

AbStlWt A method for the determmatlon of clenbuterol 111 bovme urme IS described,, which mvolves clean-up and concentration of the sample by nnmunoaffnuty chromatography, followed by nucrofitre plate enzyme unmunoassay of the extract Both the chromatographlc procedure and the assay use ovme antirum

## Abaa-act An enzyme mmmnoassay for sulphametbazme was developed usmg an antiserum rzused m rabtuts by unmumaatlon agamst a sulphamethazme dlazo derwatrve coupled to bovme serum albumm Horseradish perox~dase coupled to sulphametbazme by a carbodurmde method was selected as a tracer The dose of su