Fig. 1

Purification of recombinant rhodanese protein from Haemonchus contortus (rHCRD) and western blots. a Separation of purified rHCRD by SDS-PAGE using a 12% polyacrylamide gel and Coomassie brilliant blue R250 staining. b Western blots of rHCRD after purification. Antisera obtained from goats experimentally infected with H. contortus was used as the primary antibody to recognize the protein (Lane 1), whereas sera from uninfected goats was used as the control (Lane 2)