Abstract
In this study, we detected Leishmania spp. infection in R. sanguineus collected from dogs that were naturally infected with L. (L.) infantum. We examined 35 dogs of both sexes and unknown ages. The infected dogs were serologically positive by the immunofluorescence antibody test (IFAT), enzyme-linked immunosorbent assay (ELISA), and Quick Test-DPP (Dual Path Platform), as well as parasitological examination of a positive skin biopsy or sternal bone marrow aspiration. Ten negative dogs were included as controls. The ticks that infested these dogs were collected in pools of 10 adult females per animal. The PCR was performed with specific primers for Leishmania spp., which amplified a 720-bp fragment. Of the 35 analyzed samples, a product was observed in eight samples (8/35; 22.9%). We conclude that the presence of parasite DNA suggests that ticks participate in the zoonotic cycle of canine visceral leishmaniasis, in the city of Teresina, Piauí.
Keywords: Rhipicephalus sanguineus, Canis familiaris, Leishmania spp.
Abstract
Neste estudo foi detectada infecção por Leishmania spp. em Rhipicephalus sanguineus (R. sanguineus) de cães naturalmente infectados por Leishmania (Leishmania) infantum = L. (L.) infantum. Foram utilizados 35 cães de ambos os sexos e idades desconhecidas, sorologicamente positivos pelas técnicas de reação de imunofluorescência indireta (RIFI), enzyme-linked immunosorbent assay (ELISA) e Quick Test-DPP (Dual Path Plataform), e com exame parasitológico positivo em biópsia de pele ou punção de medula óssea esternal e 10 cães domiciliados negativos, como controle. Os carrapatos que infestavam esses cães foram coletados em pool de 10 fêmeas adultas por animal. A Reação em Cadeia pela Polimerase (PCR = Polymerase Chain Reaction) foi realizada com primers para Leishmania spp., que amplificaram 720pb. O resultado das 35 amostras processadas revelou a amplificação de oito amostras (8/35 - 22,9%). Conclui-se que a presença do DNA do parasita sugere que carrapatos podem estar participando do ciclo zoonótico da leishmaniose visceral canina na cidade de Teresina, Piauí.
INTRODUCTION
Canine visceral leishmaniasis (CVL) is a disease of great zoonotic potential5. It is caused by the protozoan L. (L.) infantum in the Americas19. The major means of transmission of the parasite to humans and other vertebrate hosts is through the bite of infected female sand flies25. Currently, Lutzomyia (Lutzomyia) longipalpis is considered the primary transmitter of the species L. (L.) infantum in Brazil. However, Lutzomyia cruzi in the state of Mato Grosso do Sul and Lutzomyia migonei and Lutzomyia firmatoi in Rio de Janeiro are also considered vectors of visceral leishmaniasis (VL)26,29.
The high incidence of CVL in Brazil and the occurrence of autochthonous cases in the absence of phlebotomine vectors suggest the possibility that R. sanguineus participates in the transmission of infection in dogs. The importance of R. sanguineus in the transmission of pathogens to humans and dogs has been substantiated by recent reviews9,10,11,21,22.
R. sanguineus is the most frequent ectoparasite of dogs in Brazil. In a study of dogs in Belo Horizonte and neighboring counties, the rate of infestation by R. sanguineus was found to be 37.9%. In Juiz de Fora, the index was found to be 60.6% in shelter dogs parasitized by this tick species10,16,24.
The likely involvement of R. sanguineus in the transmission of L. (L.) infantum in dogs was demonstrated in the 1930s in France, where the ability of the tick to mechanically transmit the protozoan to rodents was observed4. In Brazil, the presence of morphologically similar forms of Leishmania spp. to “Leptomonas” in ticks collected from dogs with visceral leishmaniasis (VL) has been reported23. Other studies have found ticks to be naturally infected with L. (L.) infantum 7,11. The presence of L. (L.) infantum in the salivary glands of ticks and the presence of Leishmania spp. RNA were recently reported6,11.
The possible participation of R. sanguineus in the transmission of VL, particularly in areas where autochthonous cases of CVL occur without the presence of Lutzomyia (Lutzomyia) longipalpis, should be the focus of further studies8. Similarly, in areas of high endemicity for CVL, where the euthanasia of dogs with VL shows no positive correlation with a decrease in the incidence of the disease14, the possible involvement of other likely vectors should be considered29. In this context, the objective of this study was to detect Leishmania spp. in R. sanguineus fed directly to dogs that were naturally infected by L. (L.) infantum to determine the possible participation of the tick in the cycle of visceral leishmaniasis in the endemic area of Teresina, Piauí.
MATERIALS AND METHODS
This study was conducted with 65 dogs of both sexes and mixed breed that were from a Brazilian endemic area (Teresina, state of Piauí) and were infested with ticks. However, only 35 dogs had a positive parasitological result upon skin biopsy or aspiration of sternal bone marrow and a positive serological diagnosis by indirect immunofluorescence techniques (Bio-Manguinhos, Fiocruz), ELISA (Bio-Manguinhos, Fiocruz) and Quick Test-DPP (Dual Path Platform) for the detection of anti-Leishmania antibodies. The serological diagnosis and PCR were performed in the Laboratory of Parasitology of the Center for Health Sciences, Federal University of Piauí. This project was approved by the ethical commission of the Federal University of Piauí as number 007/12.
Collection of ticks: Ten adult female engorged ticks were collected per animal. Ticks were placed in vials with 70% alcohol and taken to the laboratory. The identification of ticks was performed according to the classification key of ARAGÃO & FONSECA (1961)2.
In the laboratory, ticks were washed with distilled water and dried on paper towels. With the aid of a scalpel blade, the ticks were sectioned at the side for the complete extraction of material ingested during its blood meal. The extracted material was placed in an Eppendorf tube and stored in a freezer at -70 °C until the DNA extraction procedure was performed.
PCR: DNA was extracted from samples taken from ticks and the sternal bone marrow of dogs using a commercial kit from Promega (Cat. # A1120, Wizard Genomic DNA Purification Kit), according to the manufacturer's recommendations. The PCR reaction mixture was prepared at a final volume of 25 µL using SuperMix from Invitrogen, which contains 22 mM Tris-HCl (pH 8.4), 55 mM KCl, 1.65 mM MgCl2, 220 mM of each dNTP (deoxynucleotide triphosphate), and 22 U of recombinant Taq DNA polymerase/mL). The primers used were Lin R4 (5 ′- GGG GTA GTT GGT AAA TAG GG - 3′) and Lin 19 (5 ′CAG AAC GCC ACC CCT CG - 3′), which were originally developed by ARANSAY et al. (2000)3 and are specific to the minicircle region of Leishmania spp. The mixture for the PCR reaction included 22 µL of SuperMix, 1 µL of each primer, and 1 µL of the DNA sample. Amplification was performed in a thermocycler (Eppendorf Mastercycler Gradient) for a total of 35 cycles, with an initial cycle of 94 °C for five minutes, followed by 34 cycles of 30 seconds at 95 °C, 30 seconds at 58 °C, and one minute at 72 °C, with a final cycle of seven min at 72 °C. The PCR product was run on a 1.5% agarose gel, stained with ethidium bromide (1.0 µL/10 mL), and viewed in a UV transilluminator (Bioagency). DNA extracts from cultures of Leishmania spp. were used as positive controls. As a negative control, we used a mixture of the reactants used in the PCR reaction without the initial template DNA. Comparative data analyses were performed using Fischer's nonparametric statistical test. The level of significance was set at p < 0.05.
RESULTS
Of the 65 dogs examined, all were parasitized by ticks, but only 35 naturally infected dogs (G1) used in this study were reactive in all serological tests (IFAT, ELISA, and RT - DPP) and parasitological examinations performed on a skin biopsy and/or a sternal bone marrow smear20. The IFAT showed high titers of antibodies to canine IgG in most of the evaluated samples (Tables 1 and 2). Dogs that were uninfected (G2) were all non-reactive in the exams.
Table 1. Examination performed on 35 dogs naturally infected by L. (L.) infantum and pooled ticks collected from these animals. Teresina, Piauí, 2012.
| Tests Dogs | Serology | Parasitological | PCR/Ticks | ||||||
|---|---|---|---|---|---|---|---|---|---|
| P | N | % | P | N | % | P | N | % | |
| Infected | 35 | 0 | 100.0 | 35 | 0 | 100.0 | 08 | 27 | 22.9 |
| Uninfected | 0 | 10 | 100.0 | 0 | 10 | 100.0 | 0 | 10 | 100.0 |
P = positive; N = Negative; PCR = Polymerase chain reaction.
Table 2. The results of PCR performed on 35 pooled samples of R. sanguineus collected from dogs naturally infected with L. (L.) infantum. Teresina, Piauí, 2012.
| Clinical status | PCR | |||||
|---|---|---|---|---|---|---|
| P | % | N | % | T | % | |
| Infected | 08 | 22.9 | 27 | 77.1 | 35 | 100.0 |
| Uninfected | 0 | 0.0 | 10 | 100.0 | 10 | 100.0 |
In the 35 naturally infected dogs (G1), the most frequent clinical manifestations were increased superficial lymph node size, weight loss, onychogryphosis, skin lesions, conjunctivitis, ulceration of the skin, alopecia, coryza, desquamation of the skin, keratitis, depigmentation of the nose, pale mucous, apathy, hyperkeratosis and edema as found in other study1.
Most uninfected dogs (Group 2) showed no clinical signs of CVL, with the exception of four dogs that had only one clinical sign, either alopecia, weight loss, onychogryphosis, or hyperkeratosis.
The PCR results of pooled samples of R. sanguineus collected from eight dogs were positive (8/35-22.9%). In the group of uninfected dogs, no DNA amplification was observed in the collected R. sanguineus or bone marrow samples.
DISCUSSION
In this study, PCR performed on material extracted from pools of ten engorged adult female ticks from each of the dogs that were naturally infected with L. (L.) infantum revealed that 22.9% of the ticks were infected. It is important to note that we used only adult female ticks that were engorged by spending time feeding on the host. COUTINHO et al. (2005)7 analyzed ticks collected in various life cycle stages from 21 dogs with symptoms of CVL from the endemic area of Minas Gerais and identified DNA from Leishmania spp. in six ticks (15.4%). Another study of 128 ticks collected from dogs from an endemic area of VL in Italy found DNA from Leishmania spp. in 13 ticks (10.1%)28. The results of the present study, conducted in the endemic area of Teresina, present a higher percentage of ticks infected by L. (L.) infantum, which is significant and alongside other epidemiological factors may be related to participation of ticks in the infectious cycle of the disease, as has been previously suggested7,11,15. However, amastigote forms of the parasite were not detected in ticks in this study. Nonetheless, transmission has been demonstrated experimentally, and flagellated forms, such as the infective form of the parasite, have been observed in material extracted from ticks7,23,27.
The involvement of ticks in the epidemiology of CVL requires further study. However, many studies have detected DNA and RNA from Leishmania spp. in ticks, with an infection rate that is higher than the natural rate of infection in Lutzomyia longipalpis 7,11,18. Notably, RNA from Leishmania spp. has been detected in R. sanguineus maintained after blood feeding in a greenhouse under appropriate temperature and humidity conditions for ten days. Additional factors support the participation of the tick in the life cycle of CVL, including its extremely common contact with dogs, its longevity, its ability to adapt to the environment, the process and durability of blood feeding and the locomotion capacity of males seeking a new host6,9,10,28.
In addition to these considerations, one very important fact is that DNA found in adult females has also been detected under experimental conditions in eggs and in the subsequent life stages of the tick13. When feeding on the host, R. sanguineus excretes a substantial amount of potentially contaminated saliva. A study reported the presence of L. (L.) infantum DNA in the salivary glands of ticks11.
Although it has not been proven that ticks can transmit infections to dogs, dogs can transmit infections to ticks. One study demonstrated this by placing healthy ticks maintained in a laboratory on dogs with VL. After a few days, Leishmania spp. DNA was detected in the respective ticks, and this infection was present in subsequent stages of tick development 23.
In the slides examined in our study, which were created with material extracted from ticks, no evolutionary form of Leishmania spp. or any similarly flagellated forms were observed. However, specimens of R. sanguineus infected with shapes similar to promastigotes of L. (L.) infantum have been reported, but this result should be viewed with some caution because some monogenetic trypanosomatids found in R. sanguineus can be easily confused with promastigotes of Leishmania spp.17,23,27.
The possibility of transmission of L. (L.) infantum by R. sanguineus implies that new measures are necessary for the control of VL due to the difficulty of controlling this ectoparasite, which is widespread in Brazil10. New experimental studies for adapting a proper method of xenodiagnostic testing using ticks and demonstrating the transmission of infection from an infected tick to a dog will be needed to definitively prove the role of R. sanguineus in the transmission of L. (L.) infantum to dogs.
Based on the results presented herein, we conclude that the presence of Leishmania spp. in ticks collected from parasitologically positive dogs from areas in which CVL is endemic demonstrates that this arthropod is infected and may have epidemiological importance, particularly given the large number of positive dogs and the low incidence of natural infection in sandflies (less than 1.0%)18. This possibility should be corroborated with various autochthonous VL cases in which the presence of Lutzomyia longipalpis is not detected.
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