Diagnosis of arboviruses using indirect sandwich IgG ELISA in horses from the Brazilian Amazon

Casseb, Alexandre do Rosário; Nunes, Márcio Roberto Teixeira; Rodrigues, Sueli Guerreiro; Rosa, Elizabeth Salbé Travassos da; Casseb, Livia Medeiros Neves; Casseb, Samir Manssor Moraes; Silva, Sandro Patroca da; Rodrigues, Érika Dayane Leal; Vasconcelos, Pedro Fernando da Costa

doi:10.1186/1678-9199-20-29

Abstract

Background

The Amazon as a whole is the largest reservoir of arboviruses worldwide, while the Brazilian Amazon hosts the largest variety of arboviruses isolated to date. In this study, the results of an indirect sandwich IgG ELISA, standardized for 19 arbovirustypes circulating among horses in Brazilian Amazon, were compared to results of the hemagglutination inhibition test. A screening test assessed the conditional probability distribution and a Pearson linear correlation test determined the correlation strength among the absorbance values recorded for viruses from the same family.

Findings

Sensitivity varied between 40.85 and 100%; the specificity was low and ranged from 39.71 to 67.0%; and the accuracy varied between 41 and 65.2%. The test developed in this study yielded a large number of serological cross-reactions.

Conclusions

The test can be employed to detect IgG antibodies within one arbovirus family; however, the hemagglutination test or other more specific techniques, such as the serum neutralization test in mice or the plaque-reduction neutralization test, are essential complementary methods for positive cases.

Horses; Arboviruses; ELISA

Findings

The expression ‘arthropod-borne virus’ was introduced in 1942 to describe a group of viruses that were propagated by arthropods and biologically transmitted to vertebrate hosts. Two decades later, the International Committee on the Nomenclature of Viruses officially recommended the term ‘arbovirus’ to denominate the viruses maintained through cycles involving hematophagous arthropod vectors and vertebrate hosts [¹1 . Karabatsos N: International catalogue of arboviruses, including certain other viruses of vertebrates. 3rd edition. San Antonio, USA: ASTMH; 1985:1141.].

Considered as a whole, the Amazon region is the largest reservoir of arboviruses worldwide. To date, 196 out of at least 200 arbovirus types found throughout Brazil were identified in the Brazilian Amazon, where the largest variety have been isolated, while many of the viral strains have not been found in any other location [²2 . Vasconcelos PFC, da Rosa APA T, Pinheiro FP, Shope RE, Degallier N, da Rosa ES T:Arboviruses pathogenic for man in Brazil. InAn overview of arbovirology in Brazil and neighbouring countries. Edited by da Rosa APA T, Vasconcelos PFC, da Rosa JFS T. Belém: Instituto Evandro Chagas; 1998:72-99.

3 . Martins LC, Diniz JA, Silva EV, Barros VL, Monteiro HA, Azevedo RS, Quaresma JA, Vasconcelos PF: Characterization of Minaçu virus (Reoviridae, Orbivirus) and pathological changes in experimentally infected new born mice. Int J ExpPathol 2007, 88(1):63-73.-⁴4 . da Rosa APA T, da Rosa JFS T, Pinheiro FP, Vasconcelos PFC:Arboviroses. In Doenças Infecciosas e parasitárias: enfoque Amazônico. Edited by Leão RNQ. Belém: Cejup: UEPA: Instituto Evandro Chagas; 1997:207-225.].

For more than two decades, the serological study of arboviruses has been restricted to such classical techniques as hemagglutination inhibition (HI), complement fixation (CF) and serum neutralization in mice (SN). Among these, the HI test in microplates is recommended as a routine serological test [²2 . Vasconcelos PFC, da Rosa APA T, Pinheiro FP, Shope RE, Degallier N, da Rosa ES T:Arboviruses pathogenic for man in Brazil. InAn overview of arbovirology in Brazil and neighbouring countries. Edited by da Rosa APA T, Vasconcelos PFC, da Rosa JFS T. Belém: Instituto Evandro Chagas; 1998:72-99.].

The enzyme-linked immunosorbent assay (ELISA) method is widely used for the serological diagnosis of arboviruses because it is not only very sensitive but also easy to perform and standardize; thus, it is able to strengthen the power of some of the classical techniques. The sensitivity and practicality of the ELISA systems are also evident in tests for detecting immunoglobulin G (IgG), which allow many serum samples to be assayed in a single day because the sample amounts can be small and do not require any pretreatment. These facts provided the basis of this study, in which an indirect sandwich IgG ELISA method was standardized to diagnose infections by 19 arboviruses types circulating among horses in the Brazilian Amazon.Blood was collected from the animals throughout 2009 in the state of Pará, Brazil (Figure 1). The animals subjected to bleeding were aged two years old or older, had been born and raised at the sample collection site and had not been vaccinated against arboviruses.

Figure 1
Map of the State of Pará depicting the mesoregions (thick line) and municipalities (solid gray area) where serum from horses were collected.

The ELISA technique was standardized for each of the arbovirus types by adapting the protocols described for the dengue virus (DENV) [⁵5 . Kuno G, Gómez I, Gubler DJ: An ELISA procedure for the diagnosis of dengue infections.J Virol Methods 1991,33(1–2):101-113.]. The test was performed with antigens of 19 different arbovirus types isolated in Brazil (Table 1) from the collection of the Arbovirology and Hemorrhagic Fevers Section of the Evandro Chagas Institute, Ananindeua, Pará, Brazil. The positive-control serum samples exhibited titers ≥ 20 in the HI test, and preferentially presented monotypic reactions [⁶6 . Shope RE: The use of a micro-hemagglutination inhibition test to follow antibody response after arthropod-borne virus infection in a community of forest animals. Ann Microbiol Rio de Janeiro 1963, 11:167-171.,⁷7 . Rodrigues SG, Oliva OP, Araújo FAA, Martins LC, Chiang JO, Henriques DF, Silva EVP, Rodrigues DSG, Prazeres ASC, Tavares-Neto J, Vasconcelos PFC: Epidemiology of Saint Louis encephalitis virus in the Brazilian Amazon region and in the State of Mato Grosso do Sul, Brazil: elevated prevalence of antibodies in horses. Ver Pan-Amaz Saúde 2010,1(1):81-86.]. The negative-control samples exhibited negative results in the HI test (with titers < 20 for all of the 19 viruses under study). The conjugate used was the peroxidase-conjugated affinity pure rabbit anti-equine IgG (Jackson Immunoresearch Laboratories, USA).

Thumbnail

Table 1
Arbovirus antigens comprising 19 arbovirus types isolated in Brazil and belonging to the collection of the arbovirology and hemorrhagic fevers section of the Evandro Chagas Institute, Brazil

After the standardization of the technique, a total of 232 serum samples of the horses for each of the 19 investigated arbovirus types were used. The results of the indirect sandwich ELISA for the IgG detection were compared to the HI test through a conditional probability distribution, using a screening test to establish the sensitivity, specificity and accuracy of each of the tests. A Pearson linear correlation test was used to verify the correlation strength among the absorbance values obtained using the enzyme immunoassay, that is, the possibility of cross-reactions among the antibodies to viruses belonging to the same family; the accepted correlation values (r) varied from -1 ≤ r ≤ 1, as calculated using the software BioEstat 5.0 [⁸8 . Ayres M, Ayres Júnior M, Ayres DL, Santos AS: BioEstat 5.0: aplicações estatísticas nas áreas das ciências biológicas e médicas. 5th edition. Belém: Sociedade Civil Mamirauá, CNPq; 2007:44-45.].

The optimal serum dilution, which varied according to the virus family employed, was 1:100 for the family Togaviridae and 1:200 for the familiesBunyaviridae and Flaviviridae. The conjugated antibodies were used at a dilution of 1:10,000.

The sensitivity varied between 40.85 (ILHV) and 100% (ICOV and BLMV); the specificity was low and ranged from 39.71 (ROCV) to 67.0% (MAYV); and the accuracy varied between 41 (ILHV) and 65.2% (MAYV).

The Pearson correlation coefficient(r) varied for the Flaviviridaefamily from 0.78 between CPCV and VSLE to 0.95 between CPCV and BSQV; for theTogaviridae family, r varied from 0.89 between EEEV and MUCV to 0.96 between EEEV and WEEV. In the Bunyaviridae family, r varied from 0.71 between GROV and UTIV to 0.96 between MAGV and TCMV.

An investigation of anti-arbovirus IgG antibodies has already been performed using ELISA in humans and domestic animals [⁹9 . Calisher CH, Berardi VP, Muth DJ, Buff EE: Specificity of immunoglobulin M and G antibody responses in humans infected with eastern and western equine encephalitis viruses: application to rapid serodiagnosis.J Clin Microbiol 1986,23(2):369-372.

10 . Paweska JT, Burt FJ, Swanepoel R: Validation of IgG-sandwich and IgM-capture ELISA for the detection of antibody to Rift Valley fever virus in humans. J Virol Methods2005, 124(1–2):173-181.-¹¹11 . Paweska JT, Burt FJ, Anthony F, Smith SJ, Grobbelaar AA, Croft JE, Ksiazek TG, Swanepoel R: IgG-sandwich and IgM-capture enzyme-linked immunosorbent assay for the detection of antibody to Rift Valley fever virus in domestic ruminants.J Virol Methods 2003,113(2):103-112.]. In this study, the serum dilution varied as a function of the arbovirus family and proved to be crucial for standardizing the indirect sandwich IgG ELISA method. An additional crucial factor for standardizing this technique was the dilution of the antibody-enzyme conjugate and the antigen.

When defining an ELISA test cutoff, the most important feature is to select serum samples from animals that are actually infected and from those that have never come into contact with the investigated virus [¹²12 . Jacobson RH: Principles of validation of diagnostic assays for infectious diseases. 4th edition. Paris: Office International des Epizooties; 2000. [Manual of standards for diagnostic tests and vaccines]]. Although the present study took this requirement into account, the degree of cross-reactivity among the investigated arbovirus species was high. To increase the test sensitivity, antigen purification and/or the use of highly specific antibodies may be needed; however, the production of stock and purified viral antigens for ELISA using classical methods is expensive and time-consuming, especially when a viral agent does not reach high multiplication titers in cell cultures [¹³13 . Chu HJ, Zee YC, Ardans AA, Dai K: Enzyme-linked immunosorbent assay for the detection of antibodies to bovine viral diarrhea virus in bovine sera.Vet Microbiol 1985,10(4):325-333. ].

We stress that the HI test detects both IgM and IgG and does not distinguish between them; thus, it is possible that some of the positive results of the HI test were not matched by the indirect sandwich IgG ELISA test used in this study, thus decreasing the calculated sensitivity of ELISA. Another important factor is that all of the investigated animals were aged more than two years, which implies a higher probability for the animals to have contacted a larger number and wider diversity of arboviruses, thus increasing the odds of cross-reactions [¹⁴14 . Guilherme JM, Gonella-Legall C, Legall F, Nakoume E, Vincent J:Seroprevalence of five arboviruses in Zebu cattle in the Central African Republic. Trans R Soc Trop Med Hyg 1996,90(1):31-33.].

The interpretation of serological tests for arboviruses must be performed cautiously because the tests might exhibit cross-reactions among the antigenically most-related arbovirus types in the investigated families, especially in horses with multiple exposures to arthropods and, thus, with a greater risk of contamination by several arboviruses [¹⁵15 . Straatmann A, Santos-Torres S, Vasconcelos PF, da Rosa APA T, Rodrigues SG, Tavares-Neto J: Evidências sorológicas da circulação do arbovírus rocio (Flaviviridae) na Bahia. Rev Soc Bras Med Trop 1997,30(6):511-515.].

The indirect sandwich ELISA test developed in this study for 19 arbovirus types in horses exhibited a large number of serological cross-reactions. Therefore, we conclude that the protocol developed herein can be used to detect IgG within the same arbovirus family, but the method cannot distinguish among the arbovirus species belonging to a given family. Thus, indirect sandwich IgG ELISA must be used together with the HI test or other more specific techniques, such as the SN test or the plaque reduction neutralization test (PRNT).

Acknowledgments

The authors would like to thank CNPq (grant 301641/2010-2), IEC/MoH and The Federal Rural University of the Amazon for their funding of this research.

References

¹
Karabatsos N: International catalogue of arboviruses, including certain other viruses of vertebrates 3rd edition. San Antonio, USA: ASTMH; 1985:1141.
²
Vasconcelos PFC, da Rosa APA T, Pinheiro FP, Shope RE, Degallier N, da Rosa ES T:Arboviruses pathogenic for man in Brazil. InAn overview of arbovirology in Brazil and neighbouring countries Edited by da Rosa APA T, Vasconcelos PFC, da Rosa JFS T. Belém: Instituto Evandro Chagas; 1998:72-99.
³
Martins LC, Diniz JA, Silva EV, Barros VL, Monteiro HA, Azevedo RS, Quaresma JA, Vasconcelos PF: Characterization of Minaçu virus (Reoviridae, Orbivirus) and pathological changes in experimentally infected new born mice. Int J ExpPathol 2007, 88(1):63-73.
⁴
da Rosa APA T, da Rosa JFS T, Pinheiro FP, Vasconcelos PFC:Arboviroses. In Doenças Infecciosas e parasitárias: enfoque Amazônico Edited by Leão RNQ. Belém: Cejup: UEPA: Instituto Evandro Chagas; 1997:207-225.
⁵
Kuno G, Gómez I, Gubler DJ: An ELISA procedure for the diagnosis of dengue infections.J Virol Methods 1991,33(1–2):101-113.
⁶
Shope RE: The use of a micro-hemagglutination inhibition test to follow antibody response after arthropod-borne virus infection in a community of forest animals. Ann Microbiol Rio de Janeiro 1963, 11:167-171.
⁷
Rodrigues SG, Oliva OP, Araújo FAA, Martins LC, Chiang JO, Henriques DF, Silva EVP, Rodrigues DSG, Prazeres ASC, Tavares-Neto J, Vasconcelos PFC: Epidemiology of Saint Louis encephalitis virus in the Brazilian Amazon region and in the State of Mato Grosso do Sul, Brazil: elevated prevalence of antibodies in horses. Ver Pan-Amaz Saúde 2010,1(1):81-86.
⁸
Ayres M, Ayres Júnior M, Ayres DL, Santos AS: BioEstat 5.0: aplicações estatísticas nas áreas das ciências biológicas e médicas 5th edition. Belém: Sociedade Civil Mamirauá, CNPq; 2007:44-45.
⁹
Calisher CH, Berardi VP, Muth DJ, Buff EE: Specificity of immunoglobulin M and G antibody responses in humans infected with eastern and western equine encephalitis viruses: application to rapid serodiagnosis.J Clin Microbiol 1986,23(2):369-372.
¹⁰
Paweska JT, Burt FJ, Swanepoel R: Validation of IgG-sandwich and IgM-capture ELISA for the detection of antibody to Rift Valley fever virus in humans. J Virol Methods2005, 124(1–2):173-181.
¹¹
Paweska JT, Burt FJ, Anthony F, Smith SJ, Grobbelaar AA, Croft JE, Ksiazek TG, Swanepoel R: IgG-sandwich and IgM-capture enzyme-linked immunosorbent assay for the detection of antibody to Rift Valley fever virus in domestic ruminants.J Virol Methods 2003,113(2):103-112.
¹²
Jacobson RH: Principles of validation of diagnostic assays for infectious diseases 4th edition. Paris: Office International des Epizooties; 2000. [Manual of standards for diagnostic tests and vaccines]
¹³
Chu HJ, Zee YC, Ardans AA, Dai K: Enzyme-linked immunosorbent assay for the detection of antibodies to bovine viral diarrhea virus in bovine sera.Vet Microbiol 1985,10(4):325-333.
¹⁴
Guilherme JM, Gonella-Legall C, Legall F, Nakoume E, Vincent J:Seroprevalence of five arboviruses in Zebu cattle in the Central African Republic. Trans R Soc Trop Med Hyg 1996,90(1):31-33.
¹⁵
Straatmann A, Santos-Torres S, Vasconcelos PF, da Rosa APA T, Rodrigues SG, Tavares-Neto J: Evidências sorológicas da circulação do arbovírus rocio (Flaviviridae) na Bahia. Rev Soc Bras Med Trop 1997,30(6):511-515.

Ethics committee approval

All of the procedures, which involved newborn (2–3 days old) Swiss albino mice and domesticated animals, were performed with utmost strictness to avoid any unnecessary suffering. The present study was submitted to and approved by the Ethics Committee on Animal Research (CEPAN) of the Evandro Chagas Institute (IEC; ruling 054/2009 CEPAN/IEC).

Publication Dates

Publication in this collection
2014

History

Received
16 Oct 2013
Accepted
28 May 2014

This is an Open Access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

[1] ¹
Karabatsos N: International catalogue of arboviruses, including certain other viruses of vertebrates 3rd edition. San Antonio, USA: ASTMH; 1985:1141.

[2] ²
Vasconcelos PFC, da Rosa APA T, Pinheiro FP, Shope RE, Degallier N, da Rosa ES T:Arboviruses pathogenic for man in Brazil. InAn overview of arbovirology in Brazil and neighbouring countries Edited by da Rosa APA T, Vasconcelos PFC, da Rosa JFS T. Belém: Instituto Evandro Chagas; 1998:72-99.

[3] ³
Martins LC, Diniz JA, Silva EV, Barros VL, Monteiro HA, Azevedo RS, Quaresma JA, Vasconcelos PF: Characterization of Minaçu virus (Reoviridae, Orbivirus) and pathological changes in experimentally infected new born mice. Int J ExpPathol 2007, 88(1):63-73.

[4] ⁴
da Rosa APA T, da Rosa JFS T, Pinheiro FP, Vasconcelos PFC:Arboviroses. In Doenças Infecciosas e parasitárias: enfoque Amazônico Edited by Leão RNQ. Belém: Cejup: UEPA: Instituto Evandro Chagas; 1997:207-225.

[5] ⁵
Kuno G, Gómez I, Gubler DJ: An ELISA procedure for the diagnosis of dengue infections.J Virol Methods 1991,33(1–2):101-113.

[6] ⁶
Shope RE: The use of a micro-hemagglutination inhibition test to follow antibody response after arthropod-borne virus infection in a community of forest animals. Ann Microbiol Rio de Janeiro 1963, 11:167-171.

[7] ⁷
Rodrigues SG, Oliva OP, Araújo FAA, Martins LC, Chiang JO, Henriques DF, Silva EVP, Rodrigues DSG, Prazeres ASC, Tavares-Neto J, Vasconcelos PFC: Epidemiology of Saint Louis encephalitis virus in the Brazilian Amazon region and in the State of Mato Grosso do Sul, Brazil: elevated prevalence of antibodies in horses. Ver Pan-Amaz Saúde 2010,1(1):81-86.

[8] ⁸
Ayres M, Ayres Júnior M, Ayres DL, Santos AS: BioEstat 5.0: aplicações estatísticas nas áreas das ciências biológicas e médicas 5th edition. Belém: Sociedade Civil Mamirauá, CNPq; 2007:44-45.

[9] ⁹
Calisher CH, Berardi VP, Muth DJ, Buff EE: Specificity of immunoglobulin M and G antibody responses in humans infected with eastern and western equine encephalitis viruses: application to rapid serodiagnosis.J Clin Microbiol 1986,23(2):369-372.

[10] ¹⁰
Paweska JT, Burt FJ, Swanepoel R: Validation of IgG-sandwich and IgM-capture ELISA for the detection of antibody to Rift Valley fever virus in humans. J Virol Methods2005, 124(1–2):173-181.

[11] ¹¹
Paweska JT, Burt FJ, Anthony F, Smith SJ, Grobbelaar AA, Croft JE, Ksiazek TG, Swanepoel R: IgG-sandwich and IgM-capture enzyme-linked immunosorbent assay for the detection of antibody to Rift Valley fever virus in domestic ruminants.J Virol Methods 2003,113(2):103-112.

[12] ¹²
Jacobson RH: Principles of validation of diagnostic assays for infectious diseases 4th edition. Paris: Office International des Epizooties; 2000. [Manual of standards for diagnostic tests and vaccines]

[13] ¹³
Chu HJ, Zee YC, Ardans AA, Dai K: Enzyme-linked immunosorbent assay for the detection of antibodies to bovine viral diarrhea virus in bovine sera.Vet Microbiol 1985,10(4):325-333.

[14] ¹⁴
Guilherme JM, Gonella-Legall C, Legall F, Nakoume E, Vincent J:Seroprevalence of five arboviruses in Zebu cattle in the Central African Republic. Trans R Soc Trop Med Hyg 1996,90(1):31-33.

[15] ¹⁵
Straatmann A, Santos-Torres S, Vasconcelos PF, da Rosa APA T, Rodrigues SG, Tavares-Neto J: Evidências sorológicas da circulação do arbovírus rocio (Flaviviridae) na Bahia. Rev Soc Bras Med Trop 1997,30(6):511-515.

Family	Genus	Viral antigens
Togaviridae	Alphavirus	Eastern equine encephalitis virus (EEEV)
		Western equine encephalitis virus (WEEV)
		Mayaro virus (MAYV)
		Mucambo virus (MUCV)
Flaviviridae	Flavivirus	Yellow fever virus (YFV)
		Ilheus virus (ILHV)
		Saint Louis encephalitis virus(SLEV)
		Cacipacore virus (CPCV)
		Bussuquara virus (BSQV)
		Rocio virus (ROCV)
Bunyaviridae	Orthobunyavirus	Guaroa virus (GROV)
		Maguari virus (MAGV)
		Tacaiuma virus (TCMV)
		Utinga virus (UTIV)
		Belem virus (BLMV)
		Caraparu virus (CARV)
		Oropouche virus (OROV)
		Catu virus (CATUV)
	Phlebovirus	Icoaraci virus (ICOV)

Brasil

Brasil

Diagnosis of arboviruses using indirect sandwich IgG ELISA in horses from the Brazilian Amazon

Abstract

Background

Findings

Conclusions

Findings

Acknowledgments

References

Publication Dates

History