Use of miltefosine to treat canine visceral leishmaniasis caused by Leishmania infantum in Brazil

dos Santos Nogueira, Fabio; Avino, Valdir Carlos; Galvis-Ovallos, Fredy; Pereira-Chioccola, Vera Lucia; Moreira, Marcio Antonio Batistella; Romariz, Ana Paula Peres Lopes; Molla, Leticia M.; Menz, Ingrid

doi:10.1186/s13071-019-3323-0

Research
Open access
Published: 08 February 2019

Use of miltefosine to treat canine visceral leishmaniasis caused by Leishmania infantum in Brazil

Fabio dos Santos Nogueira¹,
Valdir Carlos Avino²,
Fredy Galvis-Ovallos³,
Vera Lucia Pereira-Chioccola⁴,
Marcio Antonio Batistella Moreira⁵,
Ana Paula Peres Lopes Romariz¹,
Leticia M. Molla² &
…
Ingrid Menz⁶

Parasites & Vectors volume 12, Article number: 79 (2019) Cite this article

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Abstract

Background

Visceral leishmaniasis (VL) is an infectious disease with a variety of clinical signs. The main form of parasite transmission to humans and other mammalian hosts is through the bite of infected arthropod females with Lutzomyia longipalpis serving as the main vector in the Americas. Dogs are the main urban domestic reservoirs of the parasite and the main source of vector infection due to their high prevalence in endemic areas and the large number of parasites in the skin of infected animals. Although miltefosine has been used in Europe since 2002 for treatment of VL infected dogs, in the Americas the treatment of dogs has not been recommended. Therefore, this study aimed to evaluate efficacy of miltefosine observing a reduction of clinical signs in infected dogs and the infectiveness to the vector by Leishmania (L.) infantum.

Methods

To our knowledge, this is the first controlled study using qPCR and xenodiagnosis to evaluate the efficacy of miltefosine (Milteforan®, Virbac) as a single treatment in Brazil. Thirty-five adult dogs with canine visceral leishmaniasis (CVL), confirmed by clinical and laboratory tests, were included in this study. They received miltefosine at a dose of 2 mg/kg every 24 h for 28 days. The dogs were observed over a three-month period, during which clinical evaluations based on a scoring system were conducted at pre-established times. Parasite load was assessed by cytology and real-time polymerase chain reaction (qPCR). Transmissibility to the vector was evaluated by xenodiagnosis.

Results

At the end of the period, the following were observed: (i) the remission of clinical signs with a reduction in clinical scores for 94.2% of the animals; (ii) a statistically significant reduction (98.7%) in parasitic load by qPCR; and (iii) a reduction in infectivity to sand flies. After treatment, 74.2% of the animals remained or had become non-infectious.

Conclusions

Our study indicates that the use of miltefosine administered orally for 4 weeks contributes to a clinical improvement and reduction in infectivity of dogs to L. infantum.

Background

Visceral leishmaniasis (VL) is an infectious, non-contagious, chronic disease with significant clinical and epidemiological control priority in the world. In the last few decades, epidemiological changes in VL, including increases in incidence and lethality rate and its spread to new and even urban areas, have been observed [1,2,3,4,5].

Leishmania (Leishmania) infantum is the aethiological agent of canine visceral leishmaniasis (CVL) distributed in the Old and New World. The main form of transmission of the parasite to humans and other mammalian hosts is through the bite of infected sand flies (Diptera: Psychodidae). In Brazil, the species involved in the transmission are mainly Lu. longipalpis and Lu. cruzi. Unlike in European countries, where there are two well-defined transmission seasons, in Brazil, in the areas with an occurrence of Lutzomyia longipalpis, this vector can be found throughout the entire year. In general, the population density of sand flies increases with high temperature and high relative humidity, resulting in periods of high risk of transmission of the parasite.

Phlebotomine infection occurs when females bite an infected host, thereby ingesting amastigotes. These amastigotes undergo successive divisions and are progressively transformed into infectious metacyclic promastigotes, which are regurgitated in the skin of mammalian hosts during a new blood meal [6,7,8].

CVL diagnosis has been challenging for public health professionals due to the existence of asymptomatic dogs, the high variability of clinical signs and the difficulty of achieving a diagnostic with high sensitivity and specificity. However, new methods based on DNA sequencing are being applied to parasite diagnosis. The use of real-time PCR (qPCR) has expanded over the past decades, since it is possible to detect parasite DNA in infected animals regardless of their clinical status. In addition, qPCR is able to quantify parasitic load and monitor follow-up treatment [9].

Xenodiagnosis is a useful method for the identification and isolation of parasites in their natural arthropod vectors, or for identification of the infectiveness of the infected host [10, 11]. This method has been used to evaluate the infectivity of Lu. longipalpis females which fed on naturally or experimentally infected dogs and the association between this infectivity and host symptoms [12,13,14,15].

Different treatment protocols have shown that parasitic forms in the skin and lymphoid organs of dogs are significantly reduced after treatment. Since most of these treated animals continue to be reservoirs, and consequently a source of infection, their monitoring is of extreme importance [3, 16,17,18].

Miltefosine (hexadecilfosfocoline) was originally studied and classified as an anti-tumor drug [19] and its leishmanicide potential was identified in the 1980s. Its compound is the first oral anti-Leishmania drug, which was studied in partnership with the World Health Organization (WHO) and registered as efficient for treatment of infections caused by L. (L.) donovani in humans [20, 21]. Miltefosine inhibits the biosynthesis of the glycosyl phosphatidyl inositol (GPI) receptor, the key molecule for Leishmania intracellular survival. It also interferes with the synthesis of phospholipase and protein kinase C, which are Leishmania-specific. The metabolic action of this compound can affect the biosynthesis of glycolipids and membrane glycoproteins of the parasite, causing apoptosis. Other studies suggest that this drug has immunomodulatory properties [22,23,24,25].

In 2007, Virbac Laboratories launched miltefosine on the European veterinary market as Milteforan for the purpose of treating dogs with CVL. According to Gradoni et al. [26], treatment of asymptomatic and oligosymptomatic dogs results in high rates of recovery and avoidance of the development of clinical disease. According to the WHO [27], the reduction of cutaneous parasitism and clinical signs, and the recovery of cellular immune response, could reduce the capacity to infect sand flies, consequently reducing the prevalence of the disease in canines and humans in endemic areas [11, 26, 28, 29]. Based on these data, the present study aimed to evaluate the efficacy of miltefosine in reducing clinical signs in naturally infected dogs and the infectivity to sand flies.

Methods

Dog housing conditions

This study was conducted in Andradina, located in the northwestern region of the state of São Paulo, Brazil, an area endemic for VL with canine and human transmission [27]. Dogs were maintained in a 45 m² kennel with an antechamber. The kennels were completely protected with a 1 mm mesh tissue screen to prevent sand fly access. As a vector surveillance measure, a CDC light trap was installed and turned on daily between 17:00 and 06:00 h. Video cameras were used to monitor the kennels for the occurrence of dog fights and accidents.

Dogs

For this study 35 adult dogs (18 males and 17 females), weighing between 4–24 kg and of different breeds (2 Dachshunds, 2 Poodles, 3 Brazilian Terriers, 1 Cocker Spaniel and 27 mixed breeds), were selected. All dogs had previously been naturally infected by L. (L.) infantum. CVL was determined by clinical, serological and molecular diagnoses. All dogs were neutered, spayed, and fed with a balanced commercial dog food ad libitum. They were kept inside a screened kennel and were microchipped with Virbac Backhome® microchips and then photographed with their microchip numbers.

Inclusion, exclusion and efficacy criteria

Dogs showing clinical signs characteristic of CVL and with infection status proven by serological, parasitological and/or molecular diagnosis were selected to start the therapy. Serology was performed using the ELISA method and the immunochromatographic DPP test at Instituto Adolfo Lutz in São Paulo, Brazil. All dogs were positive for L. (L.) infantum (ELISA cut-off = 0.174).

Dogs with significant alterations in renal and/or hepatic function or with other infectious diseases were excluded.

Efficacy criteria were determined by reduction in clinical scores [18, 30, 31], in decreasing of parasite DNA and infectiveness to sand flies. The score was defined according to the severity of each clinical sign and the final value was obtained from the sum of all the values. Quantitative parasite load was estimated through qPCR and the transmissibility of parasites to sand flies was evaluated through xenodiagnosis.

Sample size

The sample size was determined by using a confidence interval of 95%, aiming for results similar to those found in a study conducted by Virbac in France [Study code: F-107.010000-60003], which showed a treatment success rate of 82.7% and a variability of 70–96%. Thus, the minimum number of dogs was 32. Thirty-five animals were initially selected, taking into account possible losses by mortality or fights. The number of dogs requested for this study was obtained according to the following equation (Lwanga & Lemeshow [32]):

$$ n=\frac{\left\{{\left[z(alpha)\right]}^2\times p\times \left(1-p\right)\right\}}{d^2} $$

where n is the sample size; z(alpha) is the value obtained through the normal distribution to obtain a confidence interval of 95%: z(alpha) = 1.96%; p is the expected ratio; and d is the accuracy of estimate (d = range size/2).

Experimental design

The dogs were treated orally with miltefosine (Milteforan®, Virbac) 2 mg/kg body weight, for four weeks (W0-W3). After each administration, the dogs were observed for 1 h to monitor for vomiting and/or regurgitation to ensure complete absorption of the drug. Animal weight, infection status (serological, cytological and parasite load-qPCR) and infectivity to sand flies (xenodiagnosis) were evaluated before treatment at week 0 (W0). Dog weight and clinical status were evaluated every two weeks from the beginning of treatment, through W12. Serological, cytological and parasite load-qPCR were evaluated at W6 and W12. Infectivity to sand flies was evaluated again at W12.

Clinical evaluation

The dogs were weighed and given routine physical examinations immediately before beginning therapy and at 14-day intervals. The same researcher conducted all clinical evaluations in a minimum observation time of 20 min per dog to maintain consistency.

Clinical scores [30] were classified according to the severity of clinical signs as shown in Table 1.

Table 1 Clinical scores used to evaluate variables before and after treatment

Full size table

Skin qPCR

Skin fragments obtained from the ear pinna, collected at the same site immediately after xenodiagnosis, were analysed for quantification of parasitic load. Prior to DNA extraction, the skin samples were digested in a lysis buffer (10 mM Tris-HCl, pH 8.0; 10 mM EDTA, 0.5% SDS; 0.01% N-laurilsarcozil and 100 g/ml proteinase K) and then incubated in a water bath at 56 °C for 2–18 h until complete tissue lysis had occurred [33]. The DNA molecules were extracted using a QIAamp DNA Mini Kit (Qiagen, Venlo, Netherland) according to the manufacturer’s instructions and in equipment specifically used for DNA purification (a QIAcube robotic workstation, Qiagen). The concentrations and purity of DNA molecules were determined by the optical density (OD) ratio at 260/280 nm in a NanoDrop ND1000 (Thermo Scientific, Waltham, USA). qPCR had been previously standardized at the Instituto Adolfo Lutz (São Paulo) using serial dilutions of DNA extracted from reference strain cultures of L. (L.) infantum (MHOM/BR/1972/LD) [34]. The set of molecular markers used in the qPCR was LinJ31, sense and reverse (5'-CCG CGT GCC TGT CG-3' and 5'-CCC ACA CAA GCG GGA ACT-3'), and a TaqMan probe MGB (5'-CCT CCT TGG ACT TTG C-3'), marked with FAM (region 5') and with NFQ (region 3') [35]. The quality of the extracted DNA was confirmed by amplification of the canine gene glyceraldehyde-3-phosphate dehydrogenase, spermatogenicto (GAPDHS; GenBank: XM_533693.2) (Applied Biosystems, Waltham, USA), which was used as an internal control gene. The reactions were conducted with a final volume of 20 μl. The canine samples (3 μl of 100 ng/μl) or DNA control (50 ng) were added to a mixture of 10 μl of 2× TaqMan Universal PCR Master Mix and 1 μl of the molecular marker mix (18 μM of sense and reverse molecular markers and 5 μM of TaqMan probe). The amplifications were conducted using an Applied Biosystems 7500 Real-time PCR, using a thermal cycle including 2 min at 50 °C and 10 min at 95 °C, followed by 40 cycles of 95 °C for 15 s and 60 °C for 1 min. Each DNA extraction set also included a negative tissue sample for Leishmania spp. together with the unknown sample in order to monitor cross-contamination during extraction. In each PCR run, a blank control consisting of DNA-free water plus PCR mix was used as blank control. Separate rooms were used for (i) DNA extraction; (ii) PCR mix and primer preparation; and (iii) addition of DNA from clinical samples (in duplicate) and positive control [34].

The results were based on a standard curve where known concentrations of parasites were used to perform the qPCR [34]. The curve had been constructed using seven different DNA concentrations (in triplicate) extracted from L. (L.) infantum (1 × 10⁷ to 1 × 10^-1 promastigotes). The cycle threshold (C_t) values were plotted on a graph (average of triplicates) versus the concentrations of DNA to determine the limit of detection of molecular marker LinJ31.

Parasite concentrations (number of amplified copies/3 μl DNA sample) were calculated using the linear regression equation [36]

$$ y= ax+b $$

where y is C_t); a is the slope of the curve; x is the number of parasites; and b is the detection limit, where the curve crosses the y-axis (y-intercept). The detection limit of LinJ31 for L. (L.) infantum was at C_t of 37.75 with R2 of 0.9957. Then the number of amplified copies/3 μl DNA sample was log₁₀-transformed.

Xenodiagnosis

To avoid repelling or killing the sand flies, no topical and/or oral treatment against ectoparasites were applied before or during the study. After clinical evaluation, the dogs were sedated intramuscularly with acepromazine 1% (Acepram, Vetnil), 0.22 mg/kg and anesthetized intravenously with tiletamine and zolazepam (Zoletil®50, Virbac), 0.12 ml/kg and transferred to the xenodiagnosis room. The sand fly feeding was conducted in the right internal ear of each dog, and a skin fragment from the same ear was collected for qPCR. This procedure was carried out using a 4 mm diameter “punch” (Dermatological Sterile Disposable Punch, Kolplast, Paulinia, Brazil), sterile surgical anatomical tweezers, a scalpel blade, a needle holder and mononylon thread. The fragments were immediately placed in 1.5 ml tubes (Eppendorf PCR Tubes, Eppendorf®, São Paulo, Brazil) with saline solution 0.9% for the qPCR procedure.

Lutzomyia longipalpis females used for the xenodiagnosis were from a closed colony kept in the Departamento de Parasitologia of the Universidade Federal de Minas Gerais (UFMG). For transport to the isolated kennel, the insects were maintained in a container designed by da Costa-Val et al. [14] consisting of a transparent box 10 cm high by 8.7 cm in diameter, covered with a nylon screen lid, 10 cm in diameter, 80 rows per cm², fastened to the outer edges of the box with silicon glue (Fig. 1a). Cotton moistened with water and sucrose 10% was placed on top of the screen lid to feed the insects during transport. The “phlebocontainers”, each with 60 to 75 sand flies of which 70% were females, were carefully placed in styrofoam boxes with moistened paper to preserve humidity at 70–80% and transported to the location of the experiment. Due to the aggregated feeding behavior of this species, male insects (30%) were included to stimulate the females during their feeding on the dogs. After transport, the “phlebocontainers” were evaluated for viability of the insects and taken to the xenodiagnosis room to be maintained at an ideal temperature (between 25–28 °C) and humidity levels for 24 h. A container was then placed over one of each dog’s ears, covered with a black cloth, and left in place for 60 min to expose the ear to the sand flies. After exposure the insects were released into individual cages (30 × 30 cm) of the same 1 mm mesh tissue screen, coded with the animal’s microchip number, for stabilization of the peritrophic membrane and maintenance until dissection of the females. A cotton wad soaked with sucrose 10% solution was placed on each cage for 6 days. After this period, the sand flies were anesthetized with ether, transferred to small flasks, and taken to the clinical laboratory for dissection. Parasite count was undertaken as described by Diniz et al. [37]. The number of infected and uninfected females was determined from the total number of dissected females per dog. Information was obtained on the different sites in the gut where the parasites were found. After defecation, the females were dissected and evaluated to detect L. infantum promastigotes under an optical microscope at 400× (Zeiss® Cx40, Jena, Germany). The dogs were considered infective if at least one parasite was found in the sand fly. Details about the stages of xenodiagnosis are presented in Fig. 1b-j.

Data analysis

The non-parametric Wilcoxon test [38] was used for comparison of averages taken at two evaluation time points.

Repeated measures analysis of variance [39] was used to compare weight, clinical score, parasite load by qPCR and infectivity to sand flies. When the assumption of normality of data was rejected, Friedman’s non-parametric test [38] was used. The significance level used for the tests was 5%. SPSS 17.0 software for Windows was used for the calculations.

Results

Variation in dog weights

During the 12-week period of observation (W0 to W12), the dogs showed a weight gain. Using analysis of variance, a significant change in dog weight throughout the period of evaluation (Repeated measures ANOVA F_(6,204) = 7.88, P < 0.001) was found. There was a significant difference in weight loss between W0 and W2 (Repeated measures ANOVA: F_(1,34) = 7.85, P = 0.008) as well as W0 and W4 (Repeated measures ANOVA contrast W0-W4: F_(1,34) = 5.52, P = 0.025). Significantly lower values were obtained for W4 than for W6 (Repeated measures ANOVA contrast W4-W6: F_(1,34) = 6.20, P = 0.018), W8 (Repeated measures ANOVA contrast W4-W8: F_(1,34) = 11.93, P = 0.002), W10 (Repeated measures ANOVA contrast W4-W10: F_(1,34) = 14.04, P < 0.001) and W12 (Repeated measures ANOVA contrast W4-W12: F_(1,34) = 17.08, P < 0.001) (Fig. 2).