Inhibition of bovine T lymphocyte responses by extracts of the stomach worm Ostertagia ostertagi

Authors

M.T. Gómez-Muñoz, Universidad Cardenal Herrera-CEUFollow
A. Canals-Caballero, CISA-INIA, Valdeolmos
S. Almeria, Veterinaria, Universidad Autónoma de Barcelona
P. Pasquali, Dipartimento di Sanità Alimentaire ed Animale, Instituto Superiore di Sanita
D.S. Zarlenga, USDA, ARS, ANRI, Immunology and Disease Resistance Laboratory
L.C. Gasbarre, USDA, ARS, ANRI, Immunology and Disease Resistance Laboratory

Date of this Version

1-14-2004

Citation

2004 Elsevier B.V. All rights reserved.

Comments

M.T.Gomez-Muñozetal./VeterinaryParasitology120(2004)199–214

Abstract

Lowered immune responses during bovine ostertagiosis have been reported in both in vivo and in vitro assay systems. In the present study we have employed three different life cycle stages of the ne- matode Ostertagia ostertagi to determine if products of this economically important parasite inhibit in vitro proliferation of Con A-stimulated cells from uninfected animals. We have demonstrated an inhibitory effect upon the growth of Con A-stimulated lymphocytes after addition of fourth stage larval (L4) soluble extract (L4SE) to the cultures. In contrast, extracts from the third stage larvae (L3) had little or no inhibitory activity. The suppressive products were also shown to be secreted by the late L4. The suppressive activity is reversible if the L4 products are removed from culture. There is no immediate effect on proliferating cells and the L4SE must be in culture for 24–48 h before suppression is observable. The L4SE caused slight but not statistically significant decreases in the percentage of T cells and increases in B cell percentages in cultures when compared with cultures stimulated with Con A alone. No changes were seen in percentage of cells positive for markers for CD4, CD8, 􏰃􏰄 T cells, or monocytes/macrophages as a consequence of the addition of L4SE. In contrast, there was a strong and significant reduction in the expression of the IL-2 receptors in cells cultured in the presence of the worm extract. There was no evidence of either necrosis or apoptosis resulting from the presence of L4 products in culture. The expression of messenger RNA for interleukin-2, -4, -13, tumor necrosis factor-alpha (TNF-􏰅), and gamma-interferon (􏰃-IFN) was decreased when L4SE was included in cultures of Con A-stimulated cells compared to cul- tures stimulated with Con A only. In contrast, messenger RNA expression of transforming growth factor-beta (TGF-􏰆) and interleukin-10 (IL-10) was increased in cells growing in the presence of L4 products. The potential role of these cytokines during ostertagiosis is discussed.