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Acta Veterinaria Scandinavica logoLink to Acta Veterinaria Scandinavica
. 2001 Mar 31;42(1):113–121. doi: 10.1186/1751-0147-42-113

Bovine Respiratory Syncytial Virus (BRSV) Pneumonia in Beef Calf Herds Despite Vaccination

LE Larsen 1,, C Tegtmeier 1, E Pedersen 2
PMCID: PMC2202333  PMID: 11455891

Abstract

The present report describes the clinical, pathological, serological and virological findings in calves from 2 larger Danish beef herds experiencing outbreaks of pneumonia. The calves had been vaccinated with an inactivated bovine respiratory syncytial virus (BRSV) vaccine 2 months prior to the outbreak. The clinical signs comprised nasal discharge, pyrexia, cough and increased respiratory rates. A total of 28 calves died in the 2 herds. The laboratory investigations revealed that BRSV was involved and probably initiated both outbreaks. Furthermore, the serological results suggested that the vaccine induced only sparse levels of antibodies probably due to the presence of maternally derived antibodies at the time of vaccination. Necropsy findings in 5 calves revealed changes typical for infectious pneumonia with involvment of BRSV. In conclusion, vaccination of calves against BRSV in 2 Danish beef herds failed to protect the calves against severe or even fatal BRSV mediated respiratory disease 2 months later.

Keywords: Bovine respiratory syncytial virus; BRSV; vaccination; enzootic pneumonia; serology, calves

Introduction

Respiratory disease is one of the most important health problems in young Danish cattle with substantial financial losses for the industry [20,21]. Thus, approximately 20% of the materials from bovines submitted to The Danish Veterinary Laboratory (DVL) for necrosy originate from cattle with a history of respiratory symptoms. Bovine respiratory syncytial virus (BRSV) has been recognised in recent years as the major viral component of the bovine respiratory disease (BRD) complex [15]. This is based on the high prevalence of seropositive individuals [21,22] and the strong correlation between respiratory disease and detection of the virus in diagnostic samples [14]. BRSV has a predilection for the lower respiratory tract and may damage the respiratory tract epithelium directly followed by changes induced by, i.e. inflammatory mediators [9] and/or it may increase the ability of bacteria to invade the lung and cause a secondary bacterial infection [2]. So far it has not been possible to prove a clear link between protection and level of actively produced or passively acquired antibodies in natural BRSV infection. Thus, calves less that 6 months are most frequently infected with BRSV despite the presence of maternally derived antibodies. Furthermore, reinfections occur even in sero-positive calves [23]. Antibodies may be partly protective, however, since the incidence and severity of disease seems to be inversely related to the level of specific maternal antibodies [12]. Several inactivated and modified live BRSV vaccines are commercially available in North-America and Europe, yet none have been registered for use in Denmark (September, 2000). In 1997 approximately 20 Danish beef herds, with confirmed BRSV positive status, received a temporary permission to use an inactivated vaccine against BRSV in calves. The present report describes the clinical, pathological, serological and virological findings in vaccinated calves in 2 Danish beef herds experiencing outbreaks of pneumonia in January 1998.

Materials and methods

Herds and animals

Two beef cattle herds, each producing approximately 1000 calves a year were included. In herd A, new calves, aged 2–4 weeks were purchased from different sources every second month. The calves were reared in groups in 2 different housing systems: An indoor-system where the calves were kept in groups of 45 and an outdoor system where the calves were kept in groups of 15 in calf hutches. In herd B, the calves were purchased and reared as described for herd A. After 5–6 months, however, the calves from this herd were transferred to a separate farm nearby and kept there in a traditionally indoor system and slaughtered at 7–9 months of age. The veterinarian described the management in both farms as "excellent".

Vaccine and vaccination

According to the specifications supplied by the vendor, each 2-ml dose of the betapropiolactone-inactivated vaccine contained at least 0.80 SN.U (1 SN.U is the quantity necessary to obtain 1 log10 sero-neutralising antibodies in the guinea-pig) of inactivated BRSV in aluminium hydroxychloride and saponin adjuvant.

In both herds all calves received 2 subcutaneous vaccinations (2 ml per calf per vaccination), 4 and 7 weeks after arrival, respectively according to the manufacture's guidelines. The vaccination program was finalised December the 1st 1997.

Clinical signs and treatments

All calves were inspected daily for signs of disease. On indication, the rectal temperature was measured (data not shown). In the case of clinical signs or increased rectal temperature the veterinarian inspected the calves and eventually initiated treatment with antibiotics.

Sampling

Nasal swabs for virology and plain blood samples for serology were taken from 10 calves with clinical signs of respiratory disease in each of the 2 herds as previously described [21]. A second blood sample was taken 3–4 weeks later from the same calves.

Necropsy and microbiology

Five dead calves in herd B were necropsied on location. The macroscopic findings were recorded and the lungs transported to the DVL where bacteriological and mycoplasma examination, and histological processing was performed as previously described [20]. For virology, material from the necropsied calves and nasal swabs were tested for the presence of BRSV, bovine corona virus (BCV), bovine parainfluenza-3 (PI-3) virus, and bovine viral diarrhoea virus (BVDV) by antigen ELISA as previously described [21,17]. Tests for infectious bovine rhinotracheitis (IBR) virus are not routinely performed since Denmark is considered free from this infection.

Serology

The serum samples were tested for the presence of specific antibodies against BRSV, including IgG1, IgG2, IgM and IgA isotypes and BRSV neutralising serum antibodies (SNT) as described elsewhere [22]. In addition, the paired serum samples were tested for antibodies against BCV and PI-3 as previously described [21].

Results

Clinical signs and treatments

No adverse effects were seen in any of the calves in the 2 herds following vaccination.

In both herds, severe outbreaks of respiratory disease started in January 1998. The clinical signs comprised nasal discharge, pyrexia, coughing, elevated respiratory rates and marked depression. Almost all calves between 4 and 7 months of age were more or less affected and a total of 8/500 and 20/250 calves died during the outbreak in herd A and B, respectively. The outbreak ceased within 2 weeks in both herds, however prolonged treatments (primarily antibiotics) of few severe affected calves were necessary for additional 1–2 weeks.

Laboratory findings

Herd A

The results of the virological and serological analysis are detailed in Table 1a. BRSV antigen was detected in nasal swabs from 2 out of 10 sampled animals of which one died. None of the tested calves had IgM or IgA antibodies against BRSV at the first sampling day, whereas 4 out of 8 calves had moderate levels of IgA one month later. The initial IgG1 titers were low (between 0 and 160) increasing to titers 160–5120 one month later. IgG2 was absent in 8 out of 10 calves at the first sampling and low (titer 40) in the remaining 2 calves, however the titers increased to very high titers at the second sampling (up to 10240). Thus, all surviving calves had significant titer rise in BRSV specific IgG1 and IgG2 antibodies between the 2 samplings. Similarly, the level of neutralising antibodies (SNT) increased from rather low to very high titers (up to 2048) in all but one calf between the 2 samplings. BCV or PI-3 antigen were not detected in any of the calves and only one calf had significant rise in BCV specific antibodies between the 2 samplings. None of the calves showed rise in PI-3 specific antibodies.

Table 1a.

Virological and serological findings in vaccinated calves during acute outbreak of respiratory disease in herd A (a) and herd B (b). Nasal swabs were taken at the acute phase (20/26 Jan) and paired serum samples were taken at the acute phase and one month later (18/19 Feb). The nasal swabs were analysed for the presence of bovine respiratory syncytial virus (BRSV), bovine corona virus (BCV) and parainfluenza-3 virus (PI-3) antigen (Ag) by ELISA. Serum samples were analysed for the presence of antibodies against BRSV (IgM, IgA, IgG1, IgG2 isotypes) and neutralising antibodies (SNT), BCV (Ab) and PI-3 (Ab). Significant change in antibody titers were defined as either sero-conversion (from 0 to any titer) or at least four-fold rises. Dead: The calf died between the two sampling dates. NA: Not applicable. * Insufficient amount of sample for testing.

BRSV Ag BRSV-IgM BRSV-IgA BRSV-IgG1 BRSV-IgG2 BRSV-SNT






Calf # 20 Jan 20 Jan 19 Feb 20 Jan 19 Feb 20 Jan 19 Feb Rise 20 Jan 19 Feb Rise 20 Jan 19 Feb Rise
332 + 0 Dead 0 Dead 0 Dead NA 0 Dead NA 64 Dead NA
338R 0 0 0 0 40 80 2560 YES 0 2560 YES 16 2048 YES
325 + 0 * 0 0 40 160 YES 0 * NA 16 1024 YES
340 0 0 0 0 20 160 1280 YES 40 2560 YES 64 256 YES
244N 0 0 Dead 0 Dead 40 Dead NA 0 Dead NA 8 Dead NA
416 0 0 0 0 20 20 2560 YES 0 640 YES 4 128 YES
421H 0 0 0 0 160 20 160 YES 0 10240 YES 16 2048 YES
426H 0 0 0 0 0 40 160 YES 40 160 YES 256 32 NO
407H 0 0 0 0 0 0 320 YES 0 1280 YES 2 1024 YES
436H 0 0 0 0 0 40 5120 YES 0 40 YES 8 2048 YES

BCV Ag BCV Ab PI-3 Ag PI-3 Ab




Calf # 20 jan 20 Jan 19 Feb Rise 20 Jan 20 Jan 19 Feb Rise

332 0 800 Dead NA 0 0 Dead NA
338R 0 12800 12800 NO 0 0 0 NO
325 0 1600 3200 NO 0 8 8 NO
340 0 3200 1600 NO 0 8 8 NO
244N 0 3200 Dead NA 0 8 Dead NA
416 0 1600 1600 NO 0 0 0 NO
421H 0 3200 3200 NO 0 0 0 NO
426H 0 800 6400 YES 0 0 0 NO
407H 0 1600 1600 NO 0 0 0 NO
436H 0 3200 6400 NO 0 0 0 NO

Herd B

The results of the virological and serological analysis are detailed in table 1b. No virus specific antigen was detected in nasal swabs from any of the 10 sampled animals. As 5 of the 10 calves died between the 2 sampling days, paired serum samples were available from only 5 calves. Four of the 10 tested calves had IgM and/or IgA antibodies against BRSV at the first sampling day. In addition, 3 out of 5 calves had low levels of IgA one month later including the 2 calves that were IgA negative at the first sampling. The initial IgG1 titers were high (between 320 and 5120) and only one calf out of 5 had significant rise in IgG1 titers between the 2 samplings. IgG2 was present in low levels in only 4 out of 10 calves at the first sampling and increased to moderate to high titers at the second sampling in all calves tested. The level of neutralising antibodies (SNT) varied between titer 8 and 2048 at the first sampling and increased in only two calves, which had initial low titers. There was no clear correlation between level of BRSV specific antibodies in the initial sample and the fate of the calf, i.e. calves with low as well as high SNT titers died between the 2 sampling days. Three out of 5 calves had significant rise in BCV specific antibodies between the 2 samplings. One of the calves seroconverted to PI-3 virus (titer 0 → 8). At necropsy, acute bronchopneumonia characterized by red consolidated tissue, interstitial edema and marked interstitial emphysema was observed in all 5 cases. The results of the histo-pathological and microbiological findings are summarized in Table 2. Mannheimia (Pasteurella) haemolytica (M. haemolytica), Mycoplasma dispar (M. dispar), Mycoplasma bovirhinis (M. bovirhinis), Mycoplasma bovis (M. bovis) and Ureaplasma diversum (U. diversum) was isolated either alone or concomitantly from one or more of the 5 cases. Histological examinations revealed a fibrinous-necrotizing pneumonia in 2 cases whereas the remaining three cases were diagnosed as suppurative bronchopneumonias. In all cases, variable numbers of syncytial cells were seen.

Table 1b.

Virological and serological findings in vaccinated calves during acute outbreak of respiratory disease in herd A (a) and herd B (b). Nasal swabs were taken at the acute phase (20/26 Jan) and paired serum samples were taken at the acute phase and one month later (18/19 Feb). The nasal swabs were analysed for the presence of bovine respiratory syncytial virus (BRSV), bovine corona virus (BCV) and parainfluenza-3 virus (PI-3) antigen (Ag) by ELISA. Serum samples were analysed for the presence of antibodies against BRSV (IgM, IgA, IgG1, IgG2 isotypes) and neutralising antibodies (SNT), BCV (Ab) and PI-3 (Ab). Significant change in antibody titers were defined as either sero-conversion (from 0 to any titer) or at least four-fold rises. Dead: The calf died between the two sampling dates. NA: NOt applicable. * Insufficient amount of sample for testing.

BRSV Ag BRSV-IgM BRSV-IgA BRSV-IgG1 BRSV-IgG2 BRSV-SNT






Calf # 26 Jan 26 Jan 18 Feb 26 Jan 18 Feb 26 Jan 18 Feb Rise 26 Jan 18 Feb Rise 26 Jan 18 Feb Rise
1064/5 0 0 0 * 40 * ≥ 1280 10240 NA * 5120 NA 64 2048 YES
2535/5 0 0 Dead 80 Dead 2560 Dead NA 80 Dead NA 2048 Dead NA
2537/5 0 0 0 0 0 320 320 NO 0 320 YES 128 256 NO
642/5 0 0 Dead 0 Dead 1280 Dead NA 0 Dead NA 64 Dead NA
829/5 0 640 0 80 20 640 160 NO 20 160 YES 64 32 NO
1057 0 0 0 0 0 1280 2560 NO 0 640 YES 256 128 NO
821 0 0 Dead 80 Dead 1280 Dead NA 20 Dead NA 2048 Dead NA
799 0 0 Dead 0 Dead 320 Dead NA 0 Dead NA 64 Dead NA
795 0 320 Dead 80 Dead 5120 Dead NA 0 Dead NA 1024 Dead NA
1317 0 0 0 0 20 640 2560 YES 20 160 YES 8 148 YES

BCV Ag BCV Ab PI-3 Ag PI-3 Ab




Calf # 26 jan 26 Jan 18 Feb Rise 26 Jan 26 Jan 18 Feb Rise

1064/5 0 * ≥ 25600 NA 0 * 0 NA
2535/5 0 6400 Dead NA 0 0 Dead NA
2537/5 0 3200 12800 YES 0 0 0 NO
642/5 0 800 Dead NA 0 0 Dead NA
829/5 0 800 ≥ 25600 YES 0 0 8 YES
1057 0 1600 ≥ 25600 YES 0 0 0 NO
821 0 6400 Dead NA 0 16 Dead NA
799 0 3200 Dead NA 0 0 Dead NA
795 0 3200 Dead NA 0 8 Dead NA
1317 0 12800 12800 NO 0 8 0 NO
Table 2.

Results of post mortem diagnostic examinations of lungs from five calves that died during the outbreak in herd B. The lungs were examined macroscopic and microscopic and samples were tested for the presence of bacteria, mycoplams and virus.

Animal ID Virus Bacteria Mycoplasm Histopathology
1408 Negative M. haemolytica U. diversum
M. dispar
Fibrino-necrotizing bronchopneumonia
2131 Negative M. haemolytica U. diversum
M. bovirhinis
Fibrino-necrotizing bronchopneumonia
1083 BRSV NO bacterial pathogens isolated U. diversum Suppurative bronchopneumonia
0782 BRSV NO bacterial pathogens isolated U. diversum
M. bovis
Suppurative bronchopneumonia
1004 Negative NO bacterial pathogens isolated U. diversum Suppurative bronchopneumonia

M. haemolytica: Mannheimia haemolytica; M. dispar: Mycoplasms dispar, M. bovis: Mycoplasms bovis, M. bovirhinis: Mycoplasms bovirhinis, U. diversum: Ureaplasma diversum.

Discussion

The detection of BRSV antigen in 2 calves, and the serological responses in the majority of calves strongly indicated that BRSV was involved in the outbreak in herd A. Similarly, the presence of BRSV antigen in 2 of the necropsied calves, and the serological responses suggested that this was also true for the outbreak in herd B.

Previous studies on the pathogenesis of BRSV infection have shown that BRSV antigen may be detected in nasal swabs material from days 2–3 until days 8–10 post infection [14,25]. Studies on the kinetics of BRSV specific antibody isotypes in serum have revealed that IgM and IgA may be present from day 8–10 until days 14–25 [12]. IgG1 being detectable from days 10–17, peaking on days 24–38 and remaining detectable for up to 8 months (half-life 21–32 days) [19,12]. The IgG2 isotype did not appear in serum until days 25–86, peaking on days 38–90 and lasting for at least 9 months. Thus, the detection of antigen in the nasal cavity and the lack of IgM and IgA at the first sampling in herd A indicated these samples were taken shortly after infection, i.e. prior to day 8–10.

Contrary to the situation in herd A, the lack of antigen in nasal swabs and the presence of IgM and IgA in herd B indicated that the first samples were taken later than 8–12 days after infection. At this time detectable amounts of IgG1 and SNT antibodies may have been produced in response to the active infection, especially in vaccinated calves (see below). The relatively high titers of IgG1 and SNT encountered in herd B at the first sampling do not necessarily represent antibodies induced by the vaccine. Similarly, the low IgG1 and SNT titers at the first sampling in herd A may represent either residues of maternal derived antibodies or antibodies induced by the vaccine.

Whatsoever, the low titers indicated either that the vaccine induced only low levels of antibodies or that these had vanished by the time of sampling (approximately 2 months after last vaccination). The failure of the vaccine to induce higher titers of antibodies may be due to either poor immunigenicity or the presence of moderate or high levels of maternally derived antibodies at the time of vaccination. Thus, presence of maternally or naturally acquired antibodies have been shown to suppress both the local and systemic antibody responses following experimental BRSV infection [3,10]. Interestingly, these studies also revealed that a memory response might be mounted even in the absence of a detectable primary response in seropositive calves. Therefore, vaccinated calves may display a stronger and more rapid systemic antibody response at challenge. Indeed, the high IgG1, IgG2 and SNT titers in the second sample in both herds were in surplus of the titers normally seen in naturally infected calves [22].

Published field trials, with live or inactivated BRSV vaccines, revealed different levels of protection [4,13,7,24,18] while others found that vaccination enhanced disease in calves [5,8]. Kimman and co-workers investigated the effect of routes of administration and maternal antibodies on the protective effect of modified live and inactivated vaccines [11]. Intramuscular administration, especially in calves that possessed maternal antibodies, proved least effective in inducing protection and intranasal inoculation of live virus in colostrum deprived calves proved most effective.

Multiple infectious agents: M. haemolytica, M. dispar, M. bovirhinis, M. bovis and U. diversum were isolated from one or more of the 5 lungs, in addition to the BRSV antigen detected in 2 cases. These findings were in accordance with previous microbiological studies on pneumonic calf lung tissue, where multiple pathogens frequently were isolated [20]. The presence of one or more of the isolated microorganisms may likely have contributed to the development and severity of pneumonia. However, viral agents, such as BRSV, are usually considered the primary pulmonary pathogen, capable of destroying the respiratory epithelial lining to a degree allowing other agents to colonize [2]. In a former study [20], performed on pneumonic lung tissue submitted to the DVL for diagnostic purposes, BRSV antigen was often detected in cases of suppurative bronchopneumonias, in which syncytial cells and interstitial emphysema could be observed. Syncytial cells and interstitial emphysema were features present in all 5 cases necropsied in the present study, thereby indicating that BRSV was, or had been, present in the examined lungs.

The significant rise in BCV specific antibodies in 3 out of 5 calves in herd B and the presence of high titers of BCV antibodies in most of the other sampled calves in both herds confirm previous findings, that BCV is common in Danish cattle [14]. However, the association between the presence of BCV and BCV antibodies and outbreak of respiratory disease is still controversial [16]. Experimental infections with BCV failed to induce fulminate respiratory disease [6], but the detection of BCV in nasal swabs and specific rise in BCV titers were strongly correlated to outbreaks of respiratory disease in a large survey recently performed in 20 Danish dairy herds [1].

Thus, presently BCV may be considered involved in the BRD complex, but the virus is probably not capable of inducing fulminate respiratory disease without the presence of other contributing factors. Interpretation of BCV serological and virological data is further complicated by the fact that the diagnostic assays employed did not distinguish between BCV strains involved in BRD and strains involved in enteric infections.

In conclusion, the data obtained in the present investigation strongly indicated that BRSV was involved, and probably initiated, both outbreaks of BRD despite prior vaccination with an inactivated BRSV vaccine. The company withdrew the vaccine from the European marked in the early spring of 1998.

Acknowledgments

Acknowledgements

The excellent technical assistance of Ivan Larsen, Jannie Pedersen, Flemming D. Jacobsen are highly acknowledged. The study was supported in parts by grants from the Danish Ministry of Food, Agriculture and Fisheries (SVIV 96-4) and the Danish Research Centre for the Management of Animal Production and Health (CEPROS). (CEP 97-6).

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