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Revista Brasileira de Parasitologia Veterinária

versão impressa ISSN 0103-846Xversão On-line ISSN 1984-2961

Rev. Bras. Parasitol. Vet. vol.24 no.4 Jaboticabal out./dez. 2015  Epub 10-Nov-2015

https://doi.org/10.1590/S1984-29612015073 

Original Article

Serological, parasitological and molecular tests for canine visceral leishmaniosis diagnosis in a longitudinal study

Testes sorológicos, parasitológicos e moleculares para o diagnóstico da leishmaniose visceral canina em estudo longitudinal

Cáris Maroni Nunes1  * 

Valéria Marçal Félix de Lima1 

Guilherme Dias de Melo1 

Henrique Borges de Paula2 

Maria Esther Gonçalves Pereira3 

Cristiana de Melo Trinconi Tronco4 

Roberto Mitsuyoshi Hiramoto5 

Marcia Dalastra Laurenti6 

Marcelo Nascimento Burattini6 

1Faculdade de Medicina Veterinária, Universidade Estadual Paulista – UNESP, Araçatuba, SP, Brasil

2Autonomous Veterinarian, São Paulo, SP, Brasil

3Companhia Integrada de Desenvolvimento Agrícola de Santa Catarina, Florianópolis, SC, Brasil

4Instituto de Ciências Biomédicas, Universidade de São Paulo – USP, São Paulo, SP, Brasil

5Instituto Adolfo Lutz – IAL, São Paulo, SP, Brasil

6Faculdade de Medicina, Universidade de São Paulo – USP, São Paulo, SP, Brasil


Abstract

One of the measures to control visceral leishmaniosis (VL) in Brazil is the identification and culling of the canine reservoir. There is much controversy concerning this strategy, including the proper identification of positive dogs and the fact that the host-parasite relationship changes over time make it more challenging. A dynamic cohort of 62 dogs was followed every three months using serological and parasitological examinations and PCR. Positivity by PCR was higher than by serology and by parasitological examinations and showed a tendency to decrease over time, while serology tended to increase after six months. Concomitant positivity in all tests was observed in 10.4% of the samples, and negativity in 29.1%. Overall sensitivity ranged from 43.6 to 64.1%, and was not uniform over time. The proportion of dogs with or without clinical signs was not different by cytology or PCR but PCR was able to identify a larger number of asymptomatic dogs compared to ELISA and immunochromatography. PCR can be useful for surveillance of areas where cases of canine VL have not yet been detected and in which control strategies can be implemented to limit the spread of the disease. Despite the advance in diagnostic tools CVL diagnosis remains a challenge.

Keywords:  Cohort studies; diagnosis; Leishmania infantum chagasi; parasitological evaluation; PCR; serology

Resumo

Uma das medidas de controle da leishmaniose visceral (LV) no Brasil se baseia na identificação e eliminação do reservatório canino. Existe considerável controvérsia relativa a esta estratégia incluindo a correta identificação dos cães positivos e a variação temporal da relação hospedeiro-parasita, o que torna esta medida ainda mais desafiadora. Uma coorte dinâmica de 62 cães foi acompanhada trimestralmente utilizando-se métodos sorológicos, parasitológicos e a PCR. A taxa de positividade por PCR foi maior em comparação à dos métodos sorológicos e parasitológicos, e mostrou tendência à diminuição com o passar do tempo, enquanto que a positividade sorológica apresentou tendência a aumento, após seis meses. Observou-se positividade concomitante em todos os testes em 10,4% das amostras e, negatividade concomitante, em 29,1%. A sensibilidade geral variou de 43,6% a 64,1%, não sendo uniforme ao longo do estudo. A proporção de cães com e sem sinais clínicos que foram positivos ao exame parasitológico ou à PCR não foi estatisticamente diferente. Contudo, foi possível identificar como positivos um maior número de animais assintomáticos por meio da técnica de PCR, em comparação aos testes ELISA e imunocromatográfico. A PCR pode ser bastante útil para a vigilância epidemiológica de áreas onde casos de LV canina ainda não tenham sido descritos e onde estratégias de controle podem ser implantadas para limitar a disseminação da doença. Não obstante o avanço nas ferramentas diagnósticas, diagnosticar a LVC continua um desafio.

Palavras-chave:  Estudo coorte; diagnóstico; Leishmania infantum chagasi; avaliação parasitológica; PCR; sorologia

Introduction

Visceral leishmaniosis (VL) is the most severe form of leishmaniosis, and the domestic dog is the main reservoir for Leishmania infantum (Syn. chagasi), which is transmitted to humans by the sandfly (DESJEUX, 2004). One of the control strategies for VL in Brazil is the serological screening with subsequent culling of seropositive dogs (COSTA & VIEIRA, 2001; PALATNIK-DE-SOUSA et al., 2001; BRASIL, 2006). This approach has been the object of controversy due to the lack of scientific evidence in reducing the incidence of VL, the variability in the diagnostic techniques used and the long delay between a positive diagnosis and the elimination of the infected dog (COURTENAY et al., 2002; REITHINGER et al., 2002; COSTA, 2011; GRIMALDI et al., 2012a; OTRANTO & DANTAS-TORRES, 2013).

The characteristics of the diagnostic methods are important parameters for the detection of an infected and infectious dog when selecting a test for use in the large-scale control of infected dogs (QUINNELL et al., 2013). In general, the parasitological examination presents low sensitivity (ALVAR et al., 2004; OLIVA et al., 2006; REIS et al., 2006; LAURENTI, 2009), while PCR has high sensitivity (SOLANO-GALLEGO et al., 2009). Specifically in Brazil, the immunofluorescent-antibody test (IFAT) and the indirect enzyme-linked immunosorbent assay (ELISA) have been widely used for canine visceral leishmaniosis (CVL) mass-screening surveys (GONTIJO & MELO, 2004; METTLER et al., 2005) until 2012, when a novel immunochromatographic assay (Dual-Path Platform – DPP®) was introduced for mass-screening (GRIMALDI et al., 2012b).

The sensitivity of any diagnostic method seems to vary during the course of the disease, as well as among individuals. At the beginning of the infection, before seroconversion or the onset of clinical signs, parasitological examinations and PCR are more sensitive; however, with disease progression, the variation among individuals and their ability to control the disease leads to higher seroconversion and parasitemia, and the detection of positive dogs tends to be best performed by serological and parasitological examinations (QUINNELL et al., 2001; OLIVA et al., 2006).

Culling is compulsory in Brazil as soon as a positive dog is detected (BRASIL, 2006). However, the controversial performance of the diagnostic tests used in mass screening approach has taken place among researchers, veterinarians and the Brazilian Ministry of Health. Therefore, the aim of this study was to contribute to this discussion by testing the performance of four diagnostic techniques (direct parasitological examination, immunochromatography-DPP® CVL rapid test, PCR and an in-house indirect ELISA) to identify the canine reservoir of VL, considering the evolution of the disease over time in an urban endemic scenario.

Materials and Methods

Study area and study design

This study was conducted in the municipality of Araçatuba, in the state of São Paulo, Brazil (latitude 21° 2' 3” S; longitude 50° 5' 58” W), a town with 179,717 inhabitants in 2005 (IBGE, 2013), when the cohort study was conducted (NUNES et al., 2008). The region has a tropical climate with dry winters and rainy summers. In the cold months the average temperature is 18 °C and in the warmer months is greater than 22 °C (ROLIM et al., 2007).

Since the identification of VL in the municipality of Araçatuba in 1999, dogs are regularly screened by serology by the municipal Zoonosis Control Center. Positive dogs are euthanized with the owners’ permission, in compliance with state law (SÃO PAULO, 2006). As part of VL control measures, vector control based on insecticide spraying was also used in the surround area whenever a human case was confirmed. The dogs included in this dynamic cohort study replaced seropositive dogs that had been previously removed by the Zoonosis Control Center. Once the owners had agreed to take part in the study, visits were scheduled every three months, when data regarding sex, age, breed and the presence of external clinical signs were collected and biological samples were taken (NUNES et al., 2007). Therefore, dogs were included at different times in this study and it was executed during a total of 27 months.

Dogs were resident in the Alvorada neighborhood, which had a CVL prevalence of 10.3%. Most of these dogs’ owners did not use any repellent or topic insecticide to prevent sandflies bites (unpublished data).

Sampling and CVL diagnosis

During each visit, new dogs that had been replaced by the owners were included in this cohort. Thus, to give more consistency to the diagnostic tests performance analysis, we excluded dogs that had less than three samplings in this study. Serum samples were selected using archived material (NUNES et al., 2008) kept at –80 °C. Serological evaluation was performed by indirect ELISA as described by Lima et al. (2005) and by a quick immunochromatographic assay based on Dual-Path Platform technology (DPP®CVL rapid test, Fiocruz/Bio-Manguinhos Unit, Brazil). DNA was extracted from total blood samples using the phenol/chloroform method and PCR was performed using specific Leishmania primers for kDNA amplification (120bp), as previously described (NUNES et al., 2007). Parasitological examination was also performed using popliteal lymph node fine needle aspiration cytology stained with a quick Romanowsky-type stain (Panótico rápido®, Laborclin-Brazil). Indirect ELISA and PCR were performed during the collection period (2002-2005) and the immunochromatographic assay (DPP®CVL rapid test) was performed in 2013.

Statistical analysis

Sensitivity and specificity were calculated using the parasitological evaluation as gold standard and the kappa coefficient (κ) was determined in order to evaluate agreement between the tests (CONRATHS & SCHARES, 2006). Fisher’s exact test was used to compare the proportions of CVL positivity by different diagnostic techniques, and also to assess their relationship with the occurrence of clinical signs.

Ethical issues

This study was approved by our institution’s Ethics and Animal Welfare Committee (CEEA, UNESP; procedural no. 30/04).

Results

Sampling and diagnostic methods validation

The dogs were followed up for 27 months, on a quarterly basis, and 10 samplings were performed, totaling 303 biological samples obtained from 62 dogs. However, one limitation of this study was that, due to the refusal of some owners to permit popliteal lymph node aspiration on every visit, the parasitological examination was performed only on 54 dogs, representing 44.2% (134/303) of the total number of samples.

PCR presented the highest of positivity percentage (46.5%), followed by parasitological examination (29.1%). The serological assays exhibited the lowest percentage of positivity, with 20.5% for indirect ELISA and 14.5% for the immunochromatographic assay.

If the parasitological examination is taken to be the gold standard, this means that only 134 samples could be evaluated. Among these, the sensitivity of PCR (64.1%) was higher than that of ELISA (43.6%) and immunochromatography (46.2%), although its specificity was lower (PCR 61.8%; ELISA 86.3%; immunochromatography 88.2%). The diagnostic sensitivity of the tests was also calculated for each sampling session (Table 1) and higher values were observed within the first year of the follow-up period. Thereafter, many samples were lost. No significant difference was observed between test sensitivities (p > 0.05). Considering the gold standard and the cumulative results of the four diagnostic methods, concomitant positivity in all tests was observed in only 10.4% (14/134) of the samples, and concomitant negativity in 29.1% (39/134).

Table 1 Sensitivity (S) of immunochromatography (DPP), indirect ELISA and PCR for diagnosing visceral leishmaniasis in dogs over time (27 months), taking the parasitological examination as the gold standard. Araçatuba, SP, Brazil. 

Follow-up (months) lymph node cytology DPP ELISA PCR
total positive n/total S (%) n/total S (%) n/total S (%)
0 25 3 0/3 0.0 0/3 0.0 0/3 0.0
3 28 12 5/12 41.7 3/12 25.0 8/12 66.7
6 30 9 4/9 44.4 3/9 33.3 6/9 66.7
9 16 5 3/5 60.0 3/5 60.0 2/5 40.0
12 18 5 3/5 60.0 5/5 100.0 4/5 80.0
15 10 2 1/2 50.0 1/2 50.0 2/2 100.0
18 5 2 1/2 50.0 1/2 50.0 2/2 100.0
21 0 0 0/0 0.0 0/0 0.0 0/0 0.0
24 2 1 1/1 100.0 1/1 100.0 1/1 100.0
27 0 0 0/0 0.0 0/0 0.0 0/0 0.0
Cumulative 134 39 18/39 46.2 17/39 43.6 25/39 64.1

CVL diagnosis over time

Only 4.8% of the dogs (numbers 4, 67 and 70) remained negative in all tests up to the end of the follow-up period. Amastigote forms of Leishmania were detected in the popliteal lymph node cytology of 20 dogs, although 40% of them (numbers 40, 41, 42, 43, 47, 65, 77 and 87) did not remain positive in the subsequent sampling session (Figure 1). Among the 23 dogs that presented positive results by the immunochromatographic assay, 26.1% (numbers 8, 16, 30, 42, 47 and 63) presented seroreversion. Moreover, when assessed by means of ELISA, only two out of the 31 dogs (numbers 51 and 76) presented seroreversion, but they seroconverted in the subsequent evaluations, while 9.7% (numbers 8, 49 and 53) seroreverted and seroconverted again by the end of the study (Figure 1).

Figure 1 Individual results from visceral leishmaniasis diagnosis among 62 dogs from which at least three samplings were possible during the 27 months of the experimental period. Diagnosis was performed every three months by means of popliteal lymph node cytological test (CYTO), immunochromatography (DPP), ELISA and PCR. The time at which the onset of clinical signs was observed is shown on the plot. 

PCR presented rather inconsistent results: out of the 53 positive dogs, 35.8% (numbers 8, 9, 16, 17, 20, 29, 30, 31, 34, 38, 42, 43, 50, 52, 60, 65, 76, 92 and 93) presented as seronegative afterwards, and 20.7% (numbers 5, 11, 18, 25, 26, 41, 45, 49, 57, 62 and 74) presented intermittent results, sometimes positive and sometimes negative (Figure 1).

One difficulty inherent to cohort studies is the loss of individuals over time. One hundred and sixteen dogs had initially been selected for this study but, in addition to the expected loss, dogs were included at different time points, thus resulting in an average follow-up of 12 months. Consequently, few samples were taken in the last sampling sessions, which interfered with the percentage positivity.

Agreement among CVL diagnostic methods

The strength of agreement between the parasitological examination and the other tests was considered to be fair, whether for immunochromatography (κ=0.371), ELISA (κ=0.331) or PCR (κ=0.238). The serological tests (immunochromatography and ELISA) showed moderate agreement between each other (κ=0.460). On the other hand, poor agreement was observed between PCR and immunochromatography (κ=0.097) and between PCR and ELISA (κ=0.186).

CVL diagnosis and external clinical signs

The onset of external clinical signs (cutaneous lesions, lymphadenopathy, onychogryphosis and weight loss) was observed in 46.7% (29/62) of the dogs during the follow-up period (see time points highlighted in gray in Figure 1). Considering all the time points combined, during the period of observation of the clinical signs, ten dogs were positive by cytology, 14 by DPP, 19 by ELISA and 22 by PCR. Concomitant positivity was verified in 9.6% of the dogs, whereas concomitant negativity was observed in 6.4% (Figure 2). Moreover, in five dogs (#18, 66, 72, 77 and 104), a positive diagnosis by at least one method was achieved only 3 to 12 months after the onset of clinical signs. Despite the presence of clinical signs, cytology was negative in 58.3% of the dogs over time, whereas DPP was negative in 44.8%; ELISA in 31%, and PCR in 10.3% of the dogs.

Figure 2 Proportion of dogs positive for visceral leishmaniasis in a 27 months follow-up study according to the occurrence of external clinical signs and according to the diagnostic test: popliteal lymph node cytological test (CYTO), immunochromatography (DPP), ELISA and PCR. “Concomitant” indicates simultaneous positivity in all four diagnostic tests, whereas “None” indicates absence of positive results in all tests. Araçatuba, SP, Brazil. 

Among the remaining 33 dogs with no clinical signs, eight were positive by cytology, seven by DPP, 12 by ELISA, and 27 were positive by PCR (Figure 2). No difference was determined between the proportions of dogs with or without clinical signs that were positive by cytology (p=0.1806) or by PCR (p=0.4826). However, the proportions of positivity by ELISA (p=0.0126) and by DPP (p=0.0084) were higher in dogs with clinical signs.

Discussion

Sixty-two dogs from an urban area that is endemic for VL were followed up, thus allowing us to observe variations in the CVL diagnosis according to the diagnostic method and disease progression over time. This is an essential difference to similar reports, in which the diagnostic comparison is usually made by cross-sectional studies, evaluating samples taken at only one time point (ASHFORD et al., 1995; SOLANO-GALLEGO et al., 2001; REITHINGER et al., 2002; MOREIRA et al., 2007; FALQUETO et al., 2009; GRIMALDI et al., 2012b; SILVA et al., 2013).

A limited number of longitudinal studies have been conducted in Brazil on cases of naturally infected dogs. These studies involved different designs with different diagnostic techniques (QUINNELL et al., 2001, 2003, 2013; FRANÇA-SILVA et al., 2005; OLIVA et al., 2006; CARSON et al., 2009; GRIMALDI et al., 2012a; COURA-VITAL et al., 2013), and this makes comparisons with the data presented here more difficult.

Overall, we detected low sensitivity ranging from 43.6 to 64.1%. This result may have been an underestimate, because of the low number of samples that we were able to include in this study, the low sensitivity of the parasitological test that was used as the gold standard (MAIA & CAMPINO, 2008; LAURENTI, 2009), and the complex relationship between Leishmania and the canine host, thus leading to changes to test sensitivity over the clinical course of the disease.

The evolution of CVL is diverse in the population and depends on the host-specific immune response and the parasite’s pathogenicity (GRIMALDI et al., 2012a), thus making its diagnosis even more challenging. The sensitivity of a diagnostic technique is very important with regard to detecting the canine VL reservoir (QUINNELL et al., 2013). In our study, PCR on blood samples was seen to have greater sensitivity than the DPP or ELISA tests within the first six months of the follow-up period (Table 1). This was possibly because the dogs may have only recently been infected, since the owners had replaced them within the last four months (NUNES et al., 2008), but it is more likely to have been influenced by the sample size. Although blood samples might not be the best biological sample for detecting DNA by PCR, blood collection is less invasive and it can be a useful approach when dogs have just been introduced into an area, resulting in early detection of the canine reservoir. Nevertheless, although PCR techniques are fast, expertise and equipment are required for them to be performed, thus restricting their mass use in developing countries.

After six months of follow-up, the serological tests (DPP or ELISA) obtained higher sensitivity values in our study. Furthermore, among dogs with a positive VL diagnosis, only 16.1% presented reversion of positivity according to ELISA and 26.1% as seen on immunochromatography. On the other hand, PCR showed that positivity was reverted in 35.8%, thus suggesting that despite its high sensitivity, positive results are more consistent when using serological evaluation than when using PCR performed on blood samples. Oliva et al. (2006) also observed several cases of dogs found to be positive by nested-PCR that were negative by other tests, but most of the dogs remained negative until the end of the study (32 months). Another follow-up study conducted in Italy also detected high variability among the diagnostic techniques over time among naturally infected dogs (PARADIES et al., 2010). Grimaldi et al. (2012a) observed similar sensitivity for the DPP test (47%), but their reversion rate was also higher (50%), either because they used a different sample (whole blood instead of serum) or because the dogs surveyed could be more resistant to infection.

Rapid tests like DPP are practical and can be performed at the owners’ home when using whole blood, thus giving the owners the chance to actually see the results. However, the Brazilian Ministry of Health currently recommends its use with serum samples. Thus, DPP is performed in a laboratory and positivity is confirmed by means of an ELISA test (EIE-Bio-Manguinhos®) in order to ensure greater sensitivity and specificity (ARRUDA et al., 2013). Silva et al. (2013) observed greater sensitivity for DPP (93%) than was seen from the data presented herein. However, their data were derived from only one time point, while ours were based on a longitudinal study, in which positivity was influenced by the course of the disease.

The ELISA and DPP tests more readily detected symptomatic positive dogs than asymptomatic ones. It is widely agreed that immunity against VL depends on how the host responds to the infection, either by a Th1 or Th2 immune response. Symptomatic dogs tend to mount a Th2 response, leading to a B-cell polyclonal activity and then to hypergammaglobulinemia (BARBIÉRI, 2006; REIS et al., 2009). Since these serological assays detect IgG, it is more likely that they will detect symptomatic than asymptomatic dogs, in contrast to PCR or cytological tests, which detect the parasite itself.

Forty percent of the parasitologically positive dogs turned out to be negative in the following evaluations. This could be due to the parasite distribution within the host, thereby leading to low diagnostic sensitivity, or it could be due to the recovering from infection. In fact, two of the parasitologically positive dogs (numbers 42 and 47) showed seroconversion according to DPP and two (numbers 42 and 43) turned out to be PCR-negative over time (Figure 1). Detection of the canine reservoir by PCR also showed a proportion of dogs (35.8%) that later on presented as seronegative and, although technical flaws may have influenced this result, a considerable number of dogs may have cleared the infection, as previously postulated by Dye (1996). However, when PCR presents greater positivity than the gold standard test, a decrease in specificity may occur, and vice versa (CONRATHS & SCHARES, 2006), as observed in our study.

Regarding the ELISA test, the lower sensitivity (43.6%) and specificity (86.3%) observed in our study, in comparison with others (QUINNELL et al., 1997, 2001; REITHINGER et al., 2002; ALMEIDA et al., 2005; ROSÁRIO et al., 2005), may have been because we included all the samples collected over the entire period and not just single samplings. Methodological differences, such as the antigen and reagents used, are likely to have contributed to this difference as well. Similarly, immunochromatography presented lower sensitivity in dogs with or without clinical signs, in comparison to the data reported by Grimaldi et al. (2012b).

The relationship between infection and serological data changes during the course of the disease (QUINNELL et al., 1997) resulting in variation in the percentage of positivity, as well as the sensitivity of each diagnostic technique. At the beginning, parasitological examinations and PCR are more sensitive; with the evolution of the infection, symptomatic dogs present an increase in serum antibody levels and parasite load (QUINNELL et al., 2001, 2003). In our study, despite the effect of the sample size, this effect was observed, with greater positivity according to parasitological examinations and PCR in the first nine months, which subsequently decreased. In contrast, ELISA and immunochromatography showed low positivity at the beginning, with a gradual increase until a maximum peak of positivity at 12 months, which later decreased. Furthermore, PCR was able to identify a larger number of asymptomatic dogs, in comparison to immunochromatography and ELISA. It may provide a useful diagnostic test when considering surveillance in areas where cases of CVL have not yet been detected and in which control strategies can be implemented, thus limiting the spread of the disease.

One of the limitations of our study is that although the total follow-up period was considerable (27 months), the period that each individual dog was followed up was variable and occasionally was less than six months. Despite this, we were able to confirm that positivity for CVL varied depending on the diagnostic technique and on the evolution of the disease. In general, the serological evaluation by means of immunochromatography and ELISA showed greater potential for mass-screening identification of infected dogs in endemic areas, although more than one test should be performed in order to ensure proper identification of the canine reservoir. Despite the advance in diagnostic tools, diagnosing canine VL remains a challenge.

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Received: May 05, 2015; Accepted: September 14, 2015

*Corresponding author: Cáris Maroni Nunes. Departamento de Apoio, Produção e Saúde Animal, Faculdade de Medicina Veterinária, Universidade Estadual Paulista “Júlio de Mesquita Filho” – UNESP, Rua Clóvis Pestana, 793, CEP 16050-680, Araçatuba, SP, Brasil. e-mail: caris@fmva.unesp.br.

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