1 Dept Sanitat i Anatomia Animals, Fac. Veterinària, Universitat Autònoma de Barcelona, 08193 Bellaterra, Barcelona, Spain
2 Centre de Recerca en Sanitat Animal (CReSA), Universitat Autònoma de Barcelona, 08193 Bellaterra, Barcelona, Spain
3 Fort Dodge Laboratories, Girona, Spain
Correspondence
Enric Mateu
enric.mateu{at}uab.es
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ABSTRACT |
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MAIN TEXT |
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Previous studies on cytokine mRNA expression patterns of PCV2-infected pigs (Darwich et al., 2003) showed an increased level of IL-10 mRNA expression in thymus and decreased levels of IL-4 and IFN-
mRNA in other lymphoid organs. However, the abovementioned report did not test actual cytokine release or determine the effect of PCV2 upon the immune cells. The study presented in this paper determined the cytokine profiles of PMWS-affected and healthy pigs when their peripheral blood mononuclear cells (PBMC) were challenged in vitro with PCV2, with or without co-stimulation with T-cell mitogens or superantigens.
Donor animals were 11 conventional 8-week-old pigs free of porcine reproductive and respiratory syndrome (PRRSV), pseudorabies virus (PRV), porcine parvovirus, swine influenza and Mycoplasma hyopneumoniae as determined by serology. All pigs were obtained from a farm experiencing a PMWS outbreak. Six of them had clinical signs of PMWS (less than 15 days of clinical evolution) and were PCV2-positive as detected by PCR and in situ hybridization. The other five animals were healthy PCV2-negative pigs as detected by both techniques in both blood and lymph nodes. Later, the pigs were sacrificed and the diagnoses were confirmed by histopathological examinations and detection of the PCV2 genome in tissues by in situ hybridization. Blood samples were collected by jugular venipuncture in heparinized tubes and PBMC were separated by density gradient centrifugation using Histopaque-1·077 (Sigma). Washed cells were resuspended in RPMI-1640 supplemented with 10 % foetal calf serum (Invitrogen), 1 mM non-essential amino acids (Invitrogen), 1 mM sodium pyruvate (Invitrogen), 5 mM 2-mercaptoethanol (Sigma), 50 000 IU penicillin 1 l-1 (Invitrogen), 50 mg streptomycin l-1 (Invitrogen) and 50 mg gentamicin l-1 (Sigma) and dispensed in 96-well plates (5x105 cells per well). Differential counts using standard rapid stains for monocytes and lymphocytes were performed to determine the relative proportion of these cell types in the samples.
In the first experiment, cells were stimulated for 24 h (37 °C, 5 % CO2) with a PCV2 strain recovered in swine kidney (SK) cells from experimentally infected pig tissues (Rovira et al., 2002) at an m.o.i. of 0·1, phytohaemagglutinin (PHA) (10 µg ml-1), Aujeszky's disease virus at an m.o.i. of 0·1 (unspecific viral stimulation) or were mock-stimulated with SK cell culture supernatants. Cultures were done in duplicate and supernatants corresponding to the same animal and stimulus were mixed and stored at -80 °C until examined by ELISA.
In the second experiment, PBMC were cultured first in the presence of PCV2 (m.o.i. of 0·1) for 24 or 48 h and then were stimulated with PHA (10 µg ml-1) or staphylococcal enterotoxin B (SEB) (1 µg ml-1). As positive controls, PCV2-uninfected cultures were exposed to PHA or SEB at the same doses as described above. Mock-stimulated cultures (as in the first experiment) were also included. Supernatants were recovered after 24 h of incubation with SEB or PHA and stored at -80 °C until subsequent analysis. Cultures were done in duplicate and supernatants corresponding to the same animal and stimulus were mixed for the analysis.
Supernatants from PBMC cultures were examined by means of capture ELISAs prepared with monoclonal antibodies available commercially (Swine IFN-, IL-10, IL-2, IL-4 CytoSets and Swine IL-1b and IL-8 Immunoassay kits; Biosource Europe, Nivelles, Belgium). The cut-off point of each ELISA was calculated as the average optical density of negative controls plus three standard deviations. Levels of IFN-
, IL-1
, IL-2, IL-4, IL-8 and IL-10 in the examined supernatants were determined using the regression line constructed with the optical densities of the cytokine standards provided by the manufacturer.
All statistics were performed using STATSDIRECT and EPI-INFO V.6.01. One-way analysis of variance with the TukeyKramer multiple comparison method was also used to compare cytokine level production and healthy/PMWS-animal groups. The results with P values 0·05 were considered statistically significant.
Differential counts showed that, in PMWS pigs, the proportion of monocytes in PBMC was below 9·5 % (mean, 5·7 %; standard deviation, 2·1 %; range, 09·5 %). In healthy animals, monocytes accounted for 1·42·8 % of total mononuclear cells (mean, 2·1 %; standard deviation, 0·6 %).
In the first experiment, both PCV2-positive and -negative pigs produced high levels of IL-1 and IL-8 in response to the virus (Fig. 1
). In contrast, stimulation with the virus induced only IFN-
and IL-10 in cells from PMWS pigs (5/6 positive animals for IFN-
; 749 pg ml-1; 3/6 positive animals for IL-10; 3102 pg ml-1). With respect to IL-4, PBMC from diseased pigs failed to release this cytokine when stimulated with PHA or PCV2. All five healthy pigs produced IL-4 upon stimulation with the mitogen but, as expected, did not with PCV2 (Fig. 1
).
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The evaluation of IL-1 levels showed that uninfected cultures from PMWS pigs had an extremely reduced ability to produce this cytokine upon stimulation with PHA or SEB, in comparison to healthy animals (Fig. 3
). In PCV2-infected cultures, no differences were seen between groups at 48 h upon PHA or SEB challenge. However, at 72 h of incubation, cell culture supernatants from healthy animals had higher levels of IL-1
after the addition of the different stimuli, whereas in samples from PMWS pigs the level of IL-1
remained as low as at 48 h (Fig. 3
). Finally in the case of IL-8, PHA and PCV2 induced the production of high amounts of this cytokine in both groups. Notwithstanding, PMWS pigs whose cells were stimulated with SEB were poor IL-8 producers compared to the controls (Fig. 3
).
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Different hypotheses can be formulated from these observations. One theory could be that the infection acts upon regulatory or suppressor mechanisms of the immune system. It is known that persistent antigenic stimulation in vivo, for example as happens in a systemic infection with the lymphocytic choriomeningitis virus in mice, can induce the generation of anergic CD4+ or CD8+ T-cells (Mueller et al., 1989; Zajac et al., 1998
). These anergic or unresponsive cells are unable to proliferate upon antigen stimulation and fail to develop cytolytic effector functions. However, they have the capacity to produce high levels of IL-10 (Buer et al., 1998
). It has been suggested that T-cells rendered anergic in vivo could act as regulatory cells, influencing neighbouring immune responses through the release of IL-10 (Buer et al., 1998
). We recently reported the presence of high IL-10 mRNA levels in the thymus in PMWS-affected pigs (Darwich et al., 2003
), associated with a massive destruction of the organ structure and an evident thymocyte depletion. In this report, we showed that most cultures from PMWS pigs produced IL-10 after stimulation with recall viral antigen. This fact and the inability to produce IL-2 or IL-4 could be signs of the activity of regulatory or suppressing cells.
A different explanation for the specific changes observed in our PMWS pigs is based on the kinetics of depletion for the different mononuclear cell subsets during the course of PCV2 infection. As is already known, PMWS is accompanied by intense lymphopenia (Darwich et al., 2002; Segalés et al., 2001
; Shibahara et al., 2000
). Interestingly, Nielsen et al. (2003)
recently reported that depletion affects all lymphocyte subsets and also natural killer (NK) cells. The collapse of CD3 T-cells occurs around 14 days p.i. but remnants of CD8+ and
cells persist until 21 days p.i.. NK cells virtually disappear at this later time. Blood samples were taken from our PMWS pigs at approximately 14 days p.i., and thus the inability of PBMC to produce IL-2 or IL-4 in response to recall viral antigens may well reflect that memory/effector cells (corresponding to the CD4/CD8 double-positive subset) had virtually disappeared. On the other hand, since some levels of IFN-
and IL-10 were released in response to the virus, it is tempting to think of NK and
subsets as responsible for this.
With respect to the IL-1 and IL-8 results, it is evident that the virus acts by stimulating the inflammatory response. This fact could explain the typical granulomatous lesions observed in PCV2-infected pigs. This mechanism can contribute to the attraction of macrophages to the infection sites, thus enhancing the chances of the virus finding new target cells. However, Kim and Chae (2003)
reported that IL-8 mRNA was not detected in macrophages from injured tissues from pigs with PMWS. This discrepancy can be explained by the nature of IL-8 expression as an early inflammatory phenomenon. As we have shown previously, IL-8 mRNA expression is high when the amount of PCV2 is low and lesions are slight (early phases of infection) but is low in more advanced cases that have more severe lesions (Darwich et al., 2003
).
On the other hand, the data for IL-1 revealed an interesting fact in cultures from PMWS pigs. While stimulation of cell cultures with PCV2, PHA or SEB for 24 h did not show differences between both groups with respect to IL-1
, when cultures were first infected with PCV2 and then, after 24 or 48 h of infection, stimulated with PHA or SEB, cells from PMWS pigs produced considerably lower amounts of this cytokine compared to healthy animals. This fact became clearer as the period of infection increased. With the present data, it is difficult to interpret this; however, we consider that it might reflect a regulatory response.
Taking all these observations together, it seems clear that the capabilities of PBMC from PMWS pigs to respond to recall viral antigens, mitogens or superantigens are clearly altered, or even non-existent, compared to a normal profile. Considering that extensive lymphocyte depletion is the main feature of this syndrome, we opine that the study of the immune response to PCV2 in asymptomatic and diseased pigs will be one of the keys to understanding PMWS. However, the fact that remains a paradox is, if PCV2 is able to alter the immune responses of PBMC in all the examined pigs, why do only some of them develop the disease. In our opinion, this could be the result of individual factors, such as the genetic background of the immune response that counteracts PCV2, the need for some coadjuvant phenomenon or even of the timing and amount of virus received.
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ACKNOWLEDGEMENTS |
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Received 9 May 2003;
accepted 20 August 2003.