Objectives. To develop an immunization protocol in order to produce avian Igy immunoglobulins against Bothrops atrox Peruvian snake venom and to evaluate its neutralizing capacity. Materials and methods. Six Hy Line Brown hens were immunized each two weeks using 500μg/doses of B. atrox venom in a period of two months. Each week, eggs were collected for Igy isolation from yolk using two consecutive steps with caprilic acid and ammonium sulfate. Detection of Igy anti-B. atrox were performed by double immunodiffusion, whereas title and cross-reactivity were analyzed using ELISA and Western Blot technics, respectively. furthermore, letal dose (DL50) and Medium Effective Dose (DE50) were obtained by Probit analysis. Results. As a result of this protocol, chicken Igy's were obtained in a concentration of 8,5 ± 1,35 mg/yolk mL DE50 from avian antivenom was 575 μL/venom mg. Cross-reactivity studies showed Bothrops atrox venom share more commom epitopes with Bothrops brazili (47%) than others Bothrops venoms showing Lachesis muta (19%) and Crotalus durissus (12%) venoms a low crossing reactivity, instead. Conclusions. Using this procedure, we could purify chicken Igy with a neutralizant capacity of B. atrox venom which is comparable to the antivenom of equine origin and demonstrate its capacity as a immunoanalitical tool to evaluate the cross reactivity with others peruvian snakes.
|Translated title of the contribution||Experimental efficacy of igy antibodies produced in eggs against the venom of the peruvian snake: Bothrops atrox|
|Number of pages||7|
|Journal||Revista Peruana de Medicina de Experimental y Salud Publica|
|State||Published - Mar 2012|
Copyright 2020 Elsevier B.V., All rights reserved.