Open-access Enzootic bovine Leukosis: development of an indirect enzyme linked immunosorbent assay (I-Elisa) in seroepidemiological studies

Leucose Enzoótica Bovina: desenvolvimento de um teste ELISA indireto (ELISA-I) e sua aplicação em estudos epidemiológicos

Abstracts

Bovine Leukemia Virus (BLV) is the etiologic agent of Enzootic Bovine Leukosis, a retrovirus exogenous to the bovine species. Once infected, there is no detectable viraemia but instead there is a strong and persistent immunological response to BLV structural proteins, essentially the gp51 envelope glycoprotein and the mayor core protein p24. We describe the test procedure of an indirect ELISA (I-ELISA) using polyclonal reagents for the detection of antibodies to BLV. For comparison, the sera were simultaneously tested by agar gel immunodiffussion (AGID) test, which is currently used as diagnostic standard for BLV infection. The antigen applied does not require a high degree of purification and the data from the analysis of the negative sera showed that the establishment of a cut-off level corresponding to 3 times the standard deviation (SD) above the mean for the negative control set of sera provided acceptable specificity, reducing the risk of false positives results. A comparison of the results obtained by AGID test and I-ELISA showed that considering a total of 465 serum samples, all of the 234 samples (50%) that were positive by AGID were positive to the I-ELISA. Of 225 serum samples which yielded negative results in the AGID test, 69 (15%) were found to be positive by the I-ELISA and 156 (33%) were negative by both techniques. Few sera (2%) that were non-specific by AGID were defined as negative or positive by I-ELISA.

Bovine Leukaemia; indirect ELISA; seroepidemiology


O Vírus da Leucose Bovina (VLB) é o agente etiológico da Leucose Enzoótica Bovina, um retrovirus exógeno da espécie bovina. Uma vez infectado, não se detecta viremia, mas uma forte e persistente resposta imunológica às proteínas estruturais, sobre tudo para gp51 da coberta e para proteína p24 do core. Neste trabalho se descreve o desenvolvimento de um ELISA indireto (ELISA-I), em que se utiliza o soro policlonal para a detecção de anticorpos para VLB. Os soros foram analisados pela prova de IDGA (imunodifusão dupla em gel de ágar) rotineiramente usada como prova padrão. O antígeno escolhido não necessita de alto grau de purificação e os resultados obtidos com os soros negativos permitiram estabelecer um valor de corte de três desvios padrão (DP) sobre a média do grupo de soros negativos, mostrando aceitável especificidade e reduzindo o risco de falsos positivos. A comparação dos resultados conseguidos por IDGA e ELISA-I demonstrou que em um total de 465 soros, 234 (50%) foram positivas por IDGA e ELISA-I. Dos 225 soros negativos por IDGA, 69 (15%) foram positivos por ELISA-I e 156 (33%) foram negativos pelas duas técnicas utilizadas. Apenas 2% dos soros foram inespecíficos por IDGA e se definiram como positivos ou negativos pelo ELISA-I

Leucose Bovina; ELISA indireto; estudos epidemiológicos


ENZOOTIC BOVINE LEUKOSIS: DEVELOPMENT OF AN INDIRECT ENZYME LINKED IMMUNOSORBENT ASSAY (I-ELISA) IN SEROEPIDEMIOLOGICAL STUDIES

Ester Teresa González1*, Estela Beatriz Bonzo2, María Gabriela Echeverría1,3, María Licursi1, María Elisa Etcheverrigaray1

1Area of Virology, Faculty of Veterinary Sciences, National University of La Plata, La Plata, Argentina. 2Area of Epidemiology, Faculty of Veterinary Sciences, National University of La Plata, La Plata, Argentina. 3Researcher of National Research Council (CONICET)

Submitted: October 15, 1998. Approved: April 06, 1999

ABSTRACT

Bovine Leukemia Virus (BLV) is the etiologic agent of Enzootic Bovine Leukosis, a retrovirus exogenous to the bovine species. Once infected, there is no detectable viraemia but instead there is a strong and persistent immunological response to BLV structural proteins, essentially the gp51 envelope glycoprotein and the mayor core protein p24. We describe the test procedure of an indirect ELISA (I-ELISA) using polyclonal reagents for the detection of antibodies to BLV. For comparison, the sera were simultaneously tested by agar gel immunodiffussion (AGID) test, which is currently used as diagnostic standard for BLV infection. The antigen applied does not require a high degree of purification and the data from the analysis of the negative sera showed that the establishment of a cut-off level corresponding to 3 times the standard deviation (SD) above the mean for the negative control set of sera provided acceptable specificity, reducing the risk of false positives results. A comparison of the results obtained by AGID test and I-ELISA showed that considering a total of 465 serum samples, all of the 234 samples (50%) that were positive by AGID were positive to the I-ELISA. Of 225 serum samples which yielded negative results in the AGID test, 69 (15%) were found to be positive by the I-ELISA and 156 (33%) were negative by both techniques. Few sera (2%) that were non-specific by AGID were defined as negative or positive by I-ELISA.

Key words: Bovine Leukaemia; indirect ELISA; seroepidemiology

INTRODUCTION

Bovine Leukaemia Virus (BLV) is the etiological agent of Enzootic Bovine Leukosis (EBL), a retrovirus exogenous to the bovine species. EBL is highly contagious and cattle become infected by transfer of BLV lymphocytes. The disease can be present without obvious clinical signs as persistent lymphocytosis, a benign proliferation of lymphoid cells, or lymphocarcinoma. Once infected, there is no detectable viraemia but instead there is a strong and persistent response to BLV structural proteins, essentially the gp51 envelope glycoprotein and the mayor core protein p24.

The control and eradication of EBL is based on detection of antibodies against BLV. Our preliminary experience was in applying the Agar Gel Immunodiffussion (AGID) test. The simplicity, reliability and economical advantages of this test performed on individual sera have been extremely important for epidemiological studies and are the only official serological test in Argentina. Since both eradication programmes and surveys determining disease prevalence require testing of a large number of samples, there has been continued interest in methods more suitable than the AGID test for large- scale application.

Considerable effort has been spent evaluating various technical modifications and practical uses of the ELISA test (1, 2, 3, 4, 6, 7, 8, 9, 11, 12, 13, 14, 15, 16, 17, 18, 19, 21, 22). However, not always the results obtained were entirely satisfactory and the routine use in clinical laboratories is therefore restricted. Naif et al. (12) demonstrated false negative readings for some herds even with new generation kits.

In this communication we describe the test procedure of an indirect ELISA (I-ELISA) using polyclonal reagents for the detection of antibodies to BLV and determine the sensitivity, specificity and predictive value of the test. For comparison, the sera were simultaneously tested by AGID test, which is currently used in many countries around the world as a diagnostic standard for BLV infection.

MATERIALS AND METHODS

Antigen: The persistently infected cell line FLK-BLV (kindly supplied by the National Institute of Animal Health, Tsukuba, Japan) was grown in polystyrene tissue culture flasks (Corning) in Dulbecco's modified Eagle's medium (Nissui Pharmaceutical CO. Ltd, Japan) with antibiotics (penicillin 100 IU/ml, dihydroestreptomycin 100 µg/ml) and supplemented with tryptose phosphate broth (TPB) 0.28 %, glutamine 0.03 % and 8% of foetal calf serum. After the complete monolayer was established, the cultures were washed 3 times with sterile Phosphate Buffer Saline (PBS) and medium without foetal calf serum was added. The supernatant fluid of cultures was harvested on 10 occasions; each separated by five days. The final volume was cleared by centrifugation at 12,000 x g for 30 min. Ammonium sulphate was used for the overnight precipitation of viral particles. After centrifugation at 6,000 x g at 4°C, the obtained pellet was dialysed against PBS and concentrated with polyethylene glycol (PEG 6,000) at a concentration 1,000-fold of the initial volume. Disruption of the virus was performed at 0oC with Triton X 100, 1% for 1 h. The preparation was cleared by centrifugation at 10,000 x g for 15 min. at 4oC. This crude antigen was available at a concentration between 33 and 60 mg/ml protein and stored in 0.1 ml aliquots at -20oC until used as the ELISA antigen.

I-ELISA: Polystyrene microtitration plates (Maxisorp F 96 Immuno Plate; Nunc) were used. Hundred microliters per well of the previous selected antigen dilution (using carbonate-bicarbonate buffer 0.05 M pH 9.6) was used. After incubation overnight at 4oC, the plates were washed three times (5 min. each) with PBS containing 0.05% Twin 20 and skimmed milk powder 0.2 % (PBS-T-SMP). To standardise the method each volume of serial two fold dilutions of reference positive and negative control sera starting from a 1:20 dilution were performed in PBS-T-SMP (0.050 ml/well) and incubated overnight at 4oC. The plates were then washed three times, 5 min. each with PBS-T, and 0.050 ml of a 1:1,000 dilution of horseradish peroxidase-labelled rabbit anti-bovine immunoglobulin G (Dakopatts) in PBS-T-SMP was added. After being incubated for 1 h at 37oC, the plates were washed, and substrate solution was added: 2.2'-Azino diethyl-benzothiazoline sulfonic acid (ABTS), Boehringer Mannheim, Germany 10-4 M in citrate phosphate buffer (0.1 M) pH 4.0 and 10-3 M H2O2. After incubation for 35 min. the optical density (OD) at 405 nm was measured in a microplate spectrophotometer (Multiskan, Flow Laboratories). For the ELISA of field sera, the samples were tested at 1:20 dilution and each one was run in duplicate. The test was carefully performed in order to get uniform results. On each microplate, known negative and positive sera were added.

The results were expressed as following: (Xs - Xn) / (Xp - Xn)

Were Xs: Average of two serum sample readings

Xn: Average of two negative control serum readings

Xp: Average of two positive control serum readings

The negative and positive control samples (giving a negative and positive reaction in the AGID test, respectively) were obtained from cattle from geographic regions in which BLV infection was nonendemic (patagonic region) and endemic respectively (central region).

Sera: The following groups of sera were used in this experiment:

1) Sera collected from 99 cattle (between 2 to 3 years old) belonging to three herds which had been proved to be free from BLV infection during 3 consecutive investigations applying AGID test with 3 months interval.

2) Four reference sera: A local positive bovine anti-BLV, a European reference positive serum (E4, Council Directive 64, EEC, July 1988, Annex G), a negative bovine anti-BLV and a positive bovine anti-BVDV (kindly supplied by NIAH, Tsukuba, Japan and the Virology Institute, INTA, Castelar, Argentina).

3) 465 serum samples (between 1 to 8 years old) obtained from different geographical regions of Argentina. These bovine serum samples were previously tested by the AGID test.

AGID test: This test (10) was performed on all the samples with a commercial kit produced in our laboratory (approved by SENASA, National Service for Animal Health, Argentina). Agar plates were placed in humidified trays and incubated at 37oC for 1-3 days. The AGID test detects undiluted positive reference sera and E4 diluted 1:10 in negative serum (Council Directive 64, EEC, July 1988, Annex G) as weak positive.

RESULTS

The choice of the optimal concentration of antigen used for the coating onto the wells was based on obtaining maximal absorbance readings for BLV- positive control samples and minimal background values for BLV-negative control samples (Fig. 1). The coated plates were usually used immediately but could be stored at 4oC for up to 3 months without a decrease in reactivity. As shown in Fig. 1, for all concentrations of the antigen tested, there was no increase in the background values from BLV-negative control samples. An optimal level of discrimination between positive and negative control samples was obtained with protein concentrations ranging between 77 to 192 mg/ml (equivalent to a dilution 1:500 to 1:1,000. of the original antigen preparation). An antigen working concentration of a 1.9 10-2 mg of total protein by well (dilution: 1:1,000) was selected and used for coating onto the wells throughout this study.

Figure 1:
Titration curves of the I-ELISA antigen using AGID positive and AGID negative sera

The more convenient dilution of the serum samples should provide a quantitative answer derived from the average of two readings at a determined dilution. We choose a working dilution of samples 1:20 at which both, the positive and negative control samples gave reliable results.

For determination of a reliable cut-off, a total of 99 serum samples from BLV-free herds were used to determine the normal range of variability applying the I-ELISA test. The I-ELISA values of these sera showed a normal distribution as shown in Fig. 2. Therefore, assuming a 1% probability of misclassification (mean value plus 3 standard deviation, X + 3 SD), the upper limit of an ELISA value for the negative population was determinated as 0.18. On the basis of these results, cattle with ELISA values of more than 0.18 were regarded as positive reactors.

Figure 2:
a) Distribution of I-ELISA values of sera collected from BLV free herds. b) Normal distribution of calculated values of negative serum samples applying I-ELISA. All sera showing I-ELISA values more than 0.18 (mean value plus 3 standard deviation, X + 3 SD) were considered positives.

Specificity of I-ELISA: Since some sublines of FLK-BLV are known to be contaminated with BVDV, anti-BVDV reference sera were tested against our I-ELISA system. Sera having antibodies to BVDV, but not to BLV, showed no reaction in the ELISA, although sera having antibodies to BLV, but not to BVDV, showed a positive reaction. As was expected, reference European positive serum E4 (originally diluted 1:10 in negative serum) gave a positive result.

A comparison of the results obtained by the AGID test and ELISA is shown in Table 1. A total of 465 serum samples previously tested by the AGID technique were subjected to the I-ELISA. All of the 234 samples that were positive by AGID were positive by ELISA (50%). Of 225 serum samples which yielded negative results in the AGID test, 69 sera (15 %) were found to be positive by the I-ELISA. From 6 sera (2%) non-specific by AGID, 3 were negative and 3 were positive by I-ELISA. None sera negative by I-ELISA was positive by AGID.

DISCUSSION

This article reports the evaluation of an I-ELISA developed in our laboratory and its comparison with the AGID technique, which is currently used as a diagnostic standard for BLV infection. However, the interpretation of AGID results is sometimes subjective and reliability depending on a great extent on the training and experience of the laboratory personnel.

The sensitivity of both tests strongly depends on the quality of the BLV antigen used. Impurities cause relatively high background values or non-specific reactions. In general, the use of highly purified antigen significantly increases the cost of the test. In this I-ELISA test the antigen applied does not require a high degree of purification. In consequence, purification by sucrose-gradient followed by pelleting was not necessary.

Since pre-coated plates can be prepared in advance and stored at 4oC for at least 4 month, this I-ELISA reduces by less than 2 days the time required for BLV serological detection.

For any given serological test, sensitivity and specificity are determinated by the cut-off value. There are considerable benefits associated with standardised diagnostic tests, particularly in relationship to export testing, animal health regulations, and disease control (20). Arbitrary methods include the recommendation of a subjective cut-off value or use of a statistical parameter (such as 3 SD above the mean for the negative control set of sera). Our main effort was to focus on overcoming the inherent problem of significant background associated with the indirect technique. The data from the analysis of the negative sera showed that the establishment of a cut-off level corresponding to 3 times the SD above the mean for the negative control set of sera, provided high specificity, reducing the risk of false positives results. We established a reliable cut-off working with high number of negative sera -99- from animals of different ages and from three different areas. Our current cut-off value (0.11: 2 SD) or another somewhat lower value is appropriate for pre-export testing by exporters to ensure that very few false-negative diagnoses are made. This value is in accord with Ridge et al. (20) who pointed out that the two extreme cut-off values, 0.05 and 0.25 represent the points that provide nearly perfect sensitivity and perfect specificity, respectively. Depending on analytical variation, it is possible, within certain limits, to select a lower cut-off level, in order to increase sensitivity with only a slight reduction in specificity (4). The cut-off value could be changed to a higher value (in our case 0.18 3 SD) for almost all routine diagnostic testing and for herds for which a planned eradication program is undertaken.

As with many infections, the initial appearance of the antibodies at detectable levels and their continuing detection during long periods even using a very sensitive test, may depend upon differences in the immune system of individual cattle, as well as upon other factors such as persistent infection with bovine viral diarrhoea virus (BVDV) which has been shown to depress antibody responses to BLV.

Comparing our results from the I-ELISA and AGID tests, they were found to agree in the vast majority of cases but ELISA sensitivity was found to be higher than the AGID test. The epidemiological significance of I-ELISA positive but AGID negative cattle is that they might be a source of BLV infection.

Both tests are used routinely in the laboratory because ELISA may complement the AGID test in a number of cases. The AGID test run in optimal conditions is the most practical, cheapest and easiest technique with high sensitivity. Besides, the crucial point is that the ELISA test system includes a number of steps and must be correctly carried out with trained operators.

ACKNOWLEDGMENTS

The authors are grateful to Dr. A. Valera, CEDIVE, Fac. Vet. Sci. UNLP, Argentine and Dr. G. Freneau, Escola de Veterinaria, Univ. Fed. Goiás, Goiânia, GO, Brazil.

RESUMO

Leucose Enzoótica Bovina: desenvolvimento de um teste ELISA indireto (ELISA-I) e sua aplicação em estudos epidemiológicos

O Vírus da Leucose Bovina (VLB) é o agente etiológico da Leucose Enzoótica Bovina, um retrovirus exógeno da espécie bovina. Uma vez infectado, não se detecta viremia, mas uma forte e persistente resposta imunológica às proteínas estruturais, sobre tudo para gp51 da coberta e para proteína p24 do core. Neste trabalho se descreve o desenvolvimento de um ELISA indireto (ELISA-I), em que se utiliza o soro policlonal para a detecção de anticorpos para VLB. Os soros foram analisados pela prova de IDGA (imunodifusão dupla em gel de ágar) rotineiramente usada como prova padrão. O antígeno escolhido não necessita de alto grau de purificação e os resultados obtidos com os soros negativos permitiram estabelecer um valor de corte de três desvios padrão (DP) sobre a média do grupo de soros negativos, mostrando aceitável especificidade e reduzindo o risco de falsos positivos. A comparação dos resultados conseguidos por IDGA e ELISA-I demonstrou que em um total de 465 soros, 234 (50%) foram positivas por IDGA e ELISA-I. Dos 225 soros negativos por IDGA, 69 (15%) foram positivos por ELISA-I e 156 (33%) foram negativos pelas duas técnicas utilizadas. Apenas 2% dos soros foram inespecíficos por IDGA e se definiram como positivos ou negativos pelo ELISA-I

Palavras-chave: Leucose Bovina; ELISA indireto; estudos epidemiológicos.

References

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  • *
    Corresponding author. Mailing address: Area of Virology, Faculty of Veterinary Sciences, National University of La Plata, 60 y 118, La Plata (1900), Argentina. Fax (+5554) 221-4253276. E-mail:
  • Publication Dates

    • Publication in this collection
      17 Sept 1999
    • Date of issue
      1999

    History

    • Received
      15 Oct 1998
    • Accepted
      06 Apr 1999
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