(28). All procedures were approved and carried out in accordance with the Animal Care Committee of Virginia Tech. Equal numbers of female and castrated male lambs were represented in each breed. Lambs were born in January, weaned at approximately 70 days of age and maintained on native pastures until the start of the study in June. Mean body weights in June averaged 19·9 and 27·5 kg for hair and wool lambs respectively. These pastures were known to be contaminated with H. contortus and provided prior
exposure to the parasite. Measurements taken in this study therefore reflect acquired rather than innate immune responses. Levels of parasitaemia were not quantified before the start of the study, but signs of Trichostatin A molecular weight CFTR modulator clinical haemonchosis were not observed. In addition, lambs were infected with 3000 H. contortus infective third stage larvae (L3) weekly for four consecutive weeks prior to the start of the experiment to further standardize previous exposure to the parasite. One week after receiving the last dose of infective larvae (i.e. at day −11 relative to experimental parasite challenge), lambs were moved to drylot
and treated with levamisole (8 mg/kg body weight) and fenbendazole (10 mg/kg body weight) on days −11 and −8 to remove existing worms. No eggs were detected in lamb faecal samples taken immediately prior to experimental infection. Small numbers of coccidial oocysts were seen throughout the study, but symptoms
of coccidiosis were not apparent. Twelve lambs of each breed were randomly assigned to receive experimental parasite infection and were moved to raised indoor pens on day −4, de-wormed again at day −3 to remove any remaining worms and orally infected with 10 000 H. contortus L3 larvae on day 0. These lambs remained in these pens until the end of the study. For reasons of space limitations, the 14 control lambs of each breed remained in drylot for an additional 2 weeks. Control lambs were moved to indoor pens on day 7 relative to infected animals and de-wormed on day 8 to approximate treatment of infected animals. However, control lambs were accidentally infected on day 11 and therefore required additional de-worming on days 12 and 14 to prevent establishment of Sorafenib mouse infection. At all time points assessed, no parasitic nematode eggs were present in the faeces of control animals, but this accidental transient exposure to L3 larvae changes interpretations of responses in control lambs in ways that will be discussed below. Infected animals of each breed (n = 6) were euthanized at 3 or 27 days post-infection (p.i.). These days were selected to represent responses to larvae (day 3) and adult worms (day 27). Control animals of each breed were sacrificed on days 17 (n = 4), 27 (n = 6) and 38 (n = 4), relative to day 0 of infected animals, corresponding to days 6, 16 and 27 following exposure to the parasite and subsequent immediate de-worming.