2) Lymphocytes from immunised pigs in experiment 1 were collecte

2). Lymphocytes from immunised pigs in experiment 1 were collected at various times post-immunisation and IFN-γ ELISPOT and proliferation assays were performed with OURT88/3 or Benin 97/1 as antigen. In all 3 pigs, the numbers of ASFV specific IFN-γ producing cells was rapidly increased after the OURT88/3 inoculation and further increased after the OURT88/1 boost. Both OURT88/3 and Benin 97/1 isolates stimulated lymphocytes from immunised pigs to an approximately equal amount (Fig. 4A–C). Low levels of proliferation were detected in all pigs

at 1 or 2 weeks post-OURT88/3 inoculation, but the amount of proliferation was dramatically increased after the OURT88/1 boost (Fig. 4D–F). In two of the pigs (Fig. 4D and E) levels of T cell proliferative responses dropped following Panobinostat order challenge with Benin 97/1 isolate and in the other pig levels continued to rise (Fig. 4F). At the termination of the experiment, lymphocytes from these pigs were Libraries tested for cross-reactivity Selleckchem Venetoclax stimulated with various ASFV isolates by IFN-γ ELISPOT assays (Fig. 5A). Immune lymphocytes from all 3 pigs responded similarly to OURT88/3, OURT88/1 and Benin 97/1. Lymphocytes from two pigs (VR89, VR90) also responded well to genotype 1 isolate Malta 78 and genotype X isolate Uganda 1965 and lymphocytes from pig VR90 also responded well to genotype I isolate Lisbon 57. Lymphocytes from pig VR92 responded less well to Malta 78, Uganda 1965 and Lisbon 57 and those

from pig VR89 also showed a reduced response to Lisbon 57. No cross-reactivity was observed Cytidine deaminase to genotype VIII isolate Malawi Lil 20/1. In the second experiment (Fig. 5B), lymphocytes were collected from pigs just prior to challenge. Lymphocytes from 2 of the immunised pigs (1829, 1837) showed a much stronger response in IFN-γ ELISPOT assays against OURT88/1 and

Benin 97/1 than the other 3 immunised pigs (1809, 1811, 1844). Interestingly, 2 of the pigs from which lymphocytes responded least (1811, 1844) in IFN-γ ELISPOT assays (Fig. 5B) were those which were not protected against Benin 97/1 challenge (Fig. 3C and D). No response was observed in IFN-γ ELISPOT assays when lymphocytes from non-immune pigs 1806, 1816, 1825 (Fig. 5B) were stimulated with ASFV, confirming the specificity of the assay. In the third experiment IFN-γ ELISPOT assay was carried out using lymphocytes collected prior to challenge and the results were too high to be read accurately by the ELISPOT reader (data not shown). This indicates that strong T cell immunity was induced in all pigs before the challenge. A competitive ELISA based on the p72 major capsid protein was used to measure development of anti-ASFV specific antibodies. The results from analysis of sera collected in experiment 2 and 3 are shown in Fig. 6. An antibody response developed in all pigs immunised with OURT88/3 followed by OURT88/1 boost, except pig 76 from experiment 3 in which antibody against p72 was not detected prior to boost (Fig. 6C).

Leave a Reply

Your email address will not be published. Required fields are marked *

*

You may use these HTML tags and attributes: <a href="" title=""> <abbr title=""> <acronym title=""> <b> <blockquote cite=""> <cite> <code> <del datetime=""> <em> <i> <q cite=""> <strike> <strong>