In Vitro and In Vivo Antileishmanial Activity of Thioridazine.

INTRODUCTION: Leishmaniasis is a neglected disease with high prevalence and incidence in tropical and subtropical areas. Existing drugs are limited due to cost, toxicity, declining efficacy and unavailability in endemic places. Drug repurposing has established as an efficient way for the discovery of drugs for a variety of diseases. PURPOSE: The objective of the present work was testing the antileishmanial activity of thioridazine, an antipsychotic agent with demonstrated effect against other intracellular pathogens. METHODS: The cytotoxicity for mouse peritoneal macrophages as well as the activity against Leishmania amazonensis, Leishmania mexicana and Leishmania major promastigotes and intracellular amastigotes, as well as in a mouse model of cutaneous leishmaniasis, were assessed. RESULTS: Thioridazine inhibited the in vitro proliferation of promastigotes (50% inhibitory concentration-IC50-values in the range of 0.73 µM to 3.8 µM against L. amazonensis, L. mexicana and L. major) and intracellular amastigotes (IC50 values of 1.27 µM to 4.4 µM for the same species). In contrast, in mouse peritoneal macrophages, the 50% cytotoxic concentration was 24.0 ± 1.89 µM. Thioridazine inhibited the growth of cutaneous lesions and reduced the number of parasites in the infected tissue of mice. The dose of thioridazine that inhibited lesion development by 50% compared to controls was 23.3 ± 3.1 mg/kg and in terms of parasite load, it was 11.1 ± 0.97 mg/kg. CONCLUSIONS: Thioridazine was effective against the promastigote and intracellular amastigote stages of three Leishmania species and in a mouse model of cutaneous leishmaniasis, supporting the potential repurposing of this drug as an antileishmanial agent.

Antileishmanial activity of 5-nitroindazole derivatives.

Background: Currently, there is no safe and effective vaccine against leishmaniasis and existing therapies are inadequate due to high toxicity, cost and decreased efficacy caused by the emergence of resistant parasite strains. Some indazole derivatives have shown in vitro and in vivo activity against Trichomonas vaginalis and Trypanosoma cruzi. On that basis, 20 indazole derivatives were tested in vitro against Leishmania amazonensis. Objective: To evaluate the in vitro activity of twenty 2-benzyl-5-nitroindazolin-3-one derivatives against L. amazonensis. Design: For the selection of promising compounds, it is necessary to evaluate the indicators for in vitro activity. For this aim, a battery of studies for antileishmanial activity and cytotoxicity were implemented. These results enabled the determination of the substituents in the indazole derivatives responsible for activity and selectivity, through the analysis of the structure-activity relationship (SAR). Methods: In vitro cytotoxicity against mouse peritoneal macrophages and growth inhibitory activity in promastigotes were evaluated for 20 compounds. Compounds that showed adequate selectivity were tested against intracellular amastigotes. The SAR from the results in promastigotes was represented using the SARANEA software. Results: Eight compounds showed selectivity index >10% and 50% inhibitory concentration <1 µM against the promastigote stage. Against intracellular amastigotes, four were as active as Amphotericin B. The best results were obtained for 2-(benzyl-2,3-dihydro-5-nitro-3-oxoindazol-1-yl) ethyl acetate, with 50% inhibitory concentration of 0.46 ± 0.01 µM against amastigotes and a selectivity index of 875. The SAR study showed the positive effect on the selectivity of the hydrophilic fragments substituted in position 1 of 2-benzyl-5- nitroindazolin-3-one, which played a key role in improving the selectivity profile of this series of compounds. Conclusion: 2-bencyl-5-nitroindazolin-3-one derivatives showed selective and potent in vitro activity, supporting further investigations on this family of compounds as potential antileishmanial hits.

Detergent-free parasite transformation and replication assay for drug screening against intracellular Leishmania amastigotes.

Leishmaniasis is an infectious disease caused by protozoan species in the genera Leishmania and Endotrypanum. Current antileishmanial drugs are limited due to adverse effects, variable efficacy, the development of resistant parasites, high cost, parenteral administration and lack of availability in endemic areas. Therefore, active searching for new antileishmanial drugs has been done for years, mainly by academia. Drug screening techniques have been a challenge since the intracellular localization of Leishmania amastigotes implies that the host cell may interfere with the quantification of the parasites and the final estimation of the effect. One of the procedures to avoid host cell interference is based on its detergent-mediated lysis and subsequent transformation of viable amastigotes into promastigotes, their proliferation and eventual quantification as an axenic culture of promastigotes. However, the use of detergent involves additional handling of cultures and variability. In the present work, cultures of intracellular amastigotes were incubated for 72 h at 26 °C after exposure to the test compounds and the transformation and proliferation of parasites took place without need of adding any detergent. The assay demonstrated clear differentiation of negative and positive controls (average Z´ = 0.75) and 50% inhibitory concentrations of compounds tested by this method and by the gold standard enumeration of Giemsa-stained cultures were similar (p = 0.5002) and highly correlated (r = 0.9707). This simplified procedure is less labor intensive, the probability of contamination and the experimental error are reduced, and it is appropriate for the automated high throughput screening of compounds.

Amphotericin B is usually underdosed in the treatment of experimental cutaneous leishmaniasis / La anfotericina B normalmente es subdosificada en el tratamiento de la leishmaniasis cutánea experimental

Introduction: Amphotericin B is an effective drug for the treatment of the different clinical forms of leishmaniasis. However, there are reports of its ineffectiveness in animals experimentally infected withLeishmaniaspp. That is why, the objective of the present work was to evaluate the balance of activity-toxicity at amphotericin B doses over 1 mg/kg, so that its use as a positive control antileishmanial drug were adequate. Method: BALB/c mice were experimentally infected withL. amazonensisand treated with amphotericin B by intraperitoneal route at doses from 5 mg/kg to 12.5 mg/kg, beginning 21 days after infection. The size of the lesions and the body weight of the mice were measured for eleven weeks after the commencement of treatment. The number of parasites was also determined three days after the end of treatment. Results: Amphotericin B at 5 mg/kg retarded lesions growth but neither reduced lesion size nor the parasite load at lesion site. Doses of 7.5 mg/kg to 10 mg/kg, every 48 h for 14 days (7 doses) caused a significant reduction of lesion size and parasite load without evident loss of body weight and without signs of toxicity. Amphotericin B at 12.5 mg/kg was more effective but produced unacceptable toxicity. Conclusions: The results support the use of amphotericin B as a positive control drug in BALB/c mice experimentally infected withL. amazonensisat doses of 7.5 mg/kg to 10 mg/kg to achieve an effect comparable to that observed in clinical practice. (AU)

Introducción: La anfotericina B es un fármaco eficaz para el tratamiento de las distintas formas de leishmaniosis. Sin embargo, existen informes sobre su ineficacia en animales de laboratorio infectados experimentalmente conLeishmaniaspp.Es por ello que el objetivo del presente trabajo fue evaluar el balance de actividad-toxicidad a dosis de Anfotericina B superiores a 1 mg/kg, de modo que su uso como fármaco leishmanicida control positivo sea adecuado. Método: Se infectaron experimentalmente ratones BALB/c conL. amazonensisy se trataron con anfotericina B por vía intraperitoneal a dosis desde 5 mg/kg hasta 12,5 mg/kg, comenzando 21 días después de la infección. Durante once semanas a partir del comienzo del tratamiento se evaluó el tamaño de las lesiones y el peso corporal de los ratones. Tres días después de concluido el tratamiento se determinó el número de parásitos en las lesiones. Resultados: La anfotericina B a 5 mg/kg retrasó el crecimiento de las lesiones, pero no redujo su tamaño ni disminuyó significativamente el número de parásitos en la lesión. Dosis de 7,5 mg/kg a 10 mg/kg, cada 48 h durante 14 días (7 dosis) causaron una reducción significativa del tamaño de la lesión y de la carga parasitaria sin pérdida manifiesta de peso corporal y sin signos de toxicidad. La anfotericina B a 12,5 mg/kg fue más eficaz, pero produjo una toxicidad inaceptable. Conclusiones: Los resultados avalan el uso de la anfotericina B como control positivo en ratones BALB/c infectados experimentalmente conL. amazonensisen dosis de 7,5 mg/kg a 10 mg/kg para lograr un efecto comparable al observado en la práctica clínica. (AU)

Characterization of Actinobacterial Strains as Potential Biocontrol Agents against Macrophomina phaseolina and Rhizoctonia solani, the Main Soil-Borne Pathogens of Phaseolus vulgaris in Cuba.

Macrophomina phaseolina and Rhizoctonia solani are considered two major soil-borne pathogens of Phaseolus vulgaris in Cuba. Their management is difficult, not only due to their intrinsic biology as soil-borne pathogens, but also because the lack of active ingredients available against these pathogens. Actinobacteria, a heterogeneous bacterial group traditionally known as actinomycetes have been reported as promising biological control agents (BCAs) in crop protection. Thus, the main objective of this study was to evaluate the effectiveness of 60 actinobacterial strains as BCAs against M. phaseolina and R. solani in vitro by dual culture assays. The most effective strains were characterized according to their cellulolytic, chitinolytic and proteolytic extracellular enzymatic activity, as well as by their morphological and biochemical characters in vitro. Forty and 25 out of the 60 actinobacteria strains inhibited the mycelial growth of M. phaseolina and R. solani, respectively, and 18 of them showed a common effect against both pathogens. Significant differences were observed on their enzymatic and biochemical activity. The morphological and biochemical characters allow us to identify all our strains as species belonging to the genus Streptomyces. Streptomyces strains CBQ-EA-2 and CBQ-B-8 showed the highest effectiveness in vitro. Finally, the effect of seed treatments by both strains was also evaluated against M. phaseolina and R. solani infections in P. vulgaris cv. Quivicán seedlings. Treatments combining the two Streptomyces strains (CBQ-EA-2 + CBQ-B-8) were able to reduce significantly the disease severity for both pathogen infections in comparison with the non-treated and inoculated control. Moreover, they showed similar effect than that observed for Trichoderma harzianum A-34 and with Celest® Top 312 FS (Syngenta®; Basilea, Switzerland) treatments, which were included for comparative purposes.

Actividad anti-leishmanial y citotoxicidad de Jatropha gossypifolia L / Antileishmanial activity and cytotoxicity of Jatropha gossypifolia L

INTRODUCCIÓN: Los extractos acuosos de las hojas de Jatropha gossypifolia L. son utilizados de forma tradicional en el tratamiento de la leishmaniasis. No existen informes concluyentes sobre su efectividad y su citotoxicidad aunque en estudios recientes ha quedado avalada la utilidad de la planta en el tratamiento de la leishmaniasis utilizando otros solventes. MÉTODO: Se determinó la actividad leishmanicida y la citotoxicidad de los extractos acuosos e hidroalcohólicos de las hojas de Jatropha gossypifolia L. utilizando el método de fluorescencia de la resazurina en promastigotes de Leishmania amazonensis y macrófagos peritoneales de ratón Balb/c respectivamente. RESULTADOS: Se obtuvieron unas concentraciones inhibitorias 50 de 0.28 Mig/mL ± 0,15 Mig/mL (n = 3) y 0.59 Mig/mL ± 0,26 Mig/mL (n = 3) para el extracto acuoso e hidroalcohólico respectivamente, aunque no se presentó actividad parasiticida a ninguna de las concentraciones evaluadas. De igual manera las concentraciones citotóxicas 50 obtenidas fueron de 0.91 Mig/mL ± 0,11 Mig/mL (n = 3) y 0.57 Mig/mL ± 0,12 Mig/ml (n = 3).CONCLUSIONES: El extracto acuoso resulta ser más eficaz y menos citotóxico frente a los promastigotes de Leishmania amazonensis. Dichos resultados avalan la utilización tópica de los extractos en su formulación tradicional para el tratamiento de la leishmaniosis cutánea

INTRODUCTION: Aqueous extracts of the leaves of Jatropha gossypifolia L. are traditionally used in the treatment of leishmaniasis. These extracts do not have conclusive reports related to their effectiveness and their cytotoxicity although in recent studies the utility of the plant in the treatment of leishmaniasis using other solvents has been supported. METHOD: The antileishmanial activity and the cytotoxicity of the aqueous and hydroalcoholic extracts of the leaves of Jatropha gossypifolia L. were determined using the resazurine fluorescence method. Both, promastigotes of Leishmania amazonensis and peritoneal macrophages of Balb/c mouse were studied. RESULTS: The half-maximal inhibitory concentration for the aqueous and hydroalcoholic extract was 0.28 Mig/mL ± 0.15 Mig/mL (n = 3) and 0.59 Mig/mL ± 0.26 Mig/mL (n = 3) respectively, although they did not show parasiticide activity at any of the evaluated concentrations. Similarly, the mean cytotoxic concentrations obtained were 0.91 Mig/mL ± 0.11 Mig/mL (n = 3) and 0.57 Mig/mL ± 0.12 Mig/ml (n = 3). CONCLUSIONS: The aqueous extract was more effective and less cytotoxic against Leishmania amazonensis promastigotes. The results obtained support the traditional use of the extracts by topical application in the treatment of cutaneous leishmaniasis

Antichagasic, Leishmanicidal, and Trichomonacidal Activity of 2-Benzyl-5-nitroindazole-Derived Amines.

Three different series of new 5-nitroindazole derivatives-1-(ω-aminoalkyl)-2-benzylindazolin-3-ones (series A; ten compounds), 3-(ω-aminoalkoxy)-2-benzylindazoles (series B; four compounds) and 3-alkylamino-2-benzylindazoles (series C; five compounds)-have been synthesized and evaluated against the protozoan parasites Trypanosoma cruzi, Leishmania amazonensis, and Trichomonas vaginalis: etiological agents of Chagas disease, cutaneous leishmaniasis, and trichomoniasis, respectively. Many indazoles of series A, B, and C were efficient against T. cruzi. Some compounds in series A, after successfully passing the preliminary screening for epimastigotes, exhibited activity values against amastigotes of several T. cruzi strains that were better than or similar to those shown by the reference drug benznidazole and displayed low nonspecific toxicity against mammalian cells. On the other hand, preliminary studies against promastigotes of L. amazonensis showed high leishmanicidal activity for some derivatives of series A and C. With regard to activity against T. vaginalis, some indazoles of series B and C were rather efficient against trophozoites of a metronidazole-sensitive isolate and showed low nonspecific toxicities toward Vero cell cultures. Additionally, some of these compounds displayed similar activity against metronidazole-sensitive and resistant isolates, showing the absence of cross-resistance between these derivatives and the reference drug.

The efficacy of 2-nitrovinylfuran derivatives against Leishmania in vitro and in vivo.

Despite recent advances in the treatment of some forms of leishmaniasis, the available drugs are still far from ideal due to inefficacy, parasite resistance, toxicity and cost. The wide-spectrum antimicrobial activity of 2-nitrovinylfuran compounds has been described, as has their activity against Trichomonas vaginalis and other protozoa. Thus, the aim of this study was to test the antileishmanial activities of six 2-nitrovinylfurans in vitro and in a murine model of leishmaniasis. Minimum parasiticide concentration (MPC) and 50% inhibitory concentration (IC50) values for these compounds against the promastigotes of Leishmania amazonensis, Leishmania infantum and Leishmania braziliensis were determined, as were the efficacies of two selected compounds in an experimental model of cutaneous leishmaniasis (CL) caused by L. amazonensis in BALB/c mice. All of the compounds were active against the promastigotes of the three Leishmania species tested. IC50 and MPC values were in the ranges of 0.8-4.7 µM and 1.7-32 µM, respectively. The compounds 2-bromo-5-(2-bromo-2-nitrovinyl)-furan (furvina) and 2-bromo-5-(2-methyl-2-nitrovinyl)-furan (UC245) also reduced lesion growth in vivo at a magnitude comparable to or higher than that achieved by amphotericin B treatment. The results demonstrate the potential of this class of compounds as antileishmanial agents and support the clinical testing of Dermofural(r) (a furvina-containing antifungal ointment) for the treatment of CL.

The efficacy of 2-nitrovinylfuran derivatives against Leishmania in vitro and in vivo

Despite recent advances in the treatment of some forms of leishmaniasis, the available drugs are still far from ideal due to inefficacy, parasite resistance, toxicity and cost. The wide-spectrum antimicrobial activity of 2-nitrovinylfuran compounds has been described, as has their activity against Trichomonas vaginalis and other protozoa. Thus, the aim of this study was to test the antileishmanial activities of six 2-nitrovinylfurans in vitro and in a murine model of leishmaniasis. Minimum parasiticide concentration (MPC) and 50% inhibitory concentration (IC50) values for these compounds against the promastigotes of Leishmania amazonensis, Leishmania infantum and Leishmania braziliensis were determined, as were the efficacies of two selected compounds in an experimental model of cutaneous leishmaniasis (CL) caused by L. amazonensis in BALB/c mice. All of the compounds were active against the promastigotes of the three Leishmania species tested. IC50 and MPC values were in the ranges of 0.8-4.7 µM and 1.7-32 µM, respectively. The compounds 2-bromo-5-(2-bromo-2-nitrovinyl)-furan (furvina) and 2-bromo-5-(2-methyl-2-nitrovinyl)-furan (UC245) also reduced lesion growth in vivo at a magnitude comparable to or higher than that achieved by amphotericin B treatment. The results demonstrate the potential of this class of compounds as antileishmanial agents and support the clinical testing of Dermofural(r) (a furvina-containing antifungal ointment) for the treatment of CL.

Toxicological Assessment of the Cochleate Derived from Neisseria meningitidis Proteoliposome in Sprague Dawley Rats.

BACKGROUND: The AFCo1 cochleate is a potential novel adjuvant derived from Neisseria meningitidis B proteoliposome. AIM: The aim was to assessing the safety of AFCo1 by single and repeated doses in Sprague Dawley rats. MATERIALS AND METHODS: Rats were grouped for treatment with AFCo1, placebo formulation or control. The first study was a single intranasal dose of 100 µl and monitoring body weight, water, and food intakes as well as clinical symptoms. Fourteen days later the rats were killed and anatomopathological studies were conducted. In a second study, four similar doses of the test substance were instilled every 5 days. Clinical observations were carried out as for the single dose study and a number of rats from each group were killed 3 and 14 days after the last dose in order to conduct hematological, hemochemical, and anatomopathological studies. RESULTS: No variable showed differences of toxicological relevance; the histological changes found were mild and similarly frequently in the three groups. According to the irritability index calculated form histology of the nasal region, AFCo1 was also classified as nonirritating. CONCLUSION: AFCo1 is potentially safe for human use by nasal route as evidenced by the absence of local and systemic signs of toxicity in Sprague Dawley rats.

A fluorometric method for evaluation of pharmacological activity against intracellular Leishmania amastigotes.

In this work a simple and novel method to evaluate the efficacy of compounds on intracellular Leishmania amastigotes by using a fluorometric assay has been developed. The new method is sensitive, easy to perform and scalable for high throughput and therefore it could be validated for screening of new anti-leishmanial agents.

Repeated dose toxicity study of a live attenuated oral cholera vaccine in Sprague Dawley rats.

BACKGROUND AND AIMS: A live attenuated vaccine candidate against human cholera has been developed from the genetically modified Vibrio cholerae O1, biotype El Tor, serotype Ogawa, 638 strain. Previous single dose toxicity and local tolerance studies have demonstrated that the product is innocuous in Sprague Dawley rats by oral route and single dose. The present paper describes a repeated dose toxicity study using a further dose compared to the proposed clinical schedule. METHODS: Sprague Dawley rats (140-180g) were treated with two doses of the vaccine candidate with a dedicated placebo formulation or were not treated at all (controls). The test products were inoculated at a 21-day interval. Animals were observed daily, body weight was determined weekly and food and water intakes were measured every other day. Three and 14 days after the last inoculation, groups of rats were humanely sacrificed, bled and macroscopically examined. Blood samples were taken for hematology, serum biochemistry and to determine the vibriocide antibody titers. A comprehensive list of tissue and organ samples was taken for microscopic studies. RESULTS: There was no mortality and no animal showed any clinical symptoms. Food and water intake, body weight, and hematological and biochemical variables did not show differences of toxicological and/or statistical relevance among the experimental groups. Macroscopic examination did not demonstrate any alterations and there were no histological findings of toxicological significance. CONCLUSIONS: The vaccine was considered potentially safe for human use as indicated by the results in Sprague Dawley rats.

Estudio de tolerancia local de la vacuna vax-TyVi® en ratas Sprague Dawley / Local tolerance study of vax-TyVi® vaccine in Sprague Dawley rats

La vacuna antitifoídica vax-TyVi® consiste en una preparación de polisacárido capsular Vi deSalmonella typhi, el cual es diluido en una solución buffer isotónica solución amortiguador, a la que se le añade fenol como preservo. Cada dosis de 0,5 mL contiene 25 µg de polisacárido como sustancia activa. En nuestro país el esquema de vacunación contra la fiebre tifoidea con vax- TyVi® se aplica a los alumnos de 9-10 años (5to grado), una 2da dosis a la edad de 12-13 años (8vo grado) y una 3ra dosis a la edad de 16-17 años (11no grado). Además, es vacunado el personal de riesgo de Salud Pública y el personal que manipula alimentos. En el presente trabajo se describe el ensayo de tolerancia local llevado a cabo con la vacuna vax-TyVi® durante su fase de estudios preclínicos, actualmente utilizada en la vacunación contra la fiebre tifoidea en Cuba. Se empleó un total de 170 ratas que fueron tratadas con la vacuna, su placebo (todos los componentes, excepto la materia prima activa), o que no recibieron tratamiento alguno(controles). Se realizaron observaciones clínicas diarias durante todo el ensayo, se determinó el consumo de agua y alimentos y se realizaron investigaciones anatomopatológicas a animales sacrificados 3, 7, 14, 21, 28, 35 y 42 días después de la inoculación. No se observaron muerte ni síntomas de toxicidad; no se encontraron diferencias estadísticamente significativas entre los pesos vivos, el consumo de agua ni el de alimentos entre los grupos del ensayo. Tampoco seobservaron lesiones anatomopatológicas que indicaran toxicidad por parte del producto inoculado. Los resultados permitieron concluir que la potencialidad de la vacuna vax-TyVi® para producir efectos adversos locales es baja(AU)

Prueba toxicológica de dosis única para la vacuna antileptospirósica vax-SPIRAL en ratones / Single-dose toxicological test for leptospirosis vaccine vax-SPIRAL in rats

Se realizó la prueba toxicológica de dosis única para la vacuna antileptospirósica vax-SPIRAL en ratones. No se encontraron síntomas clínicos de toxicidad y las diferencias entre las variables evaluadas no fueron importantes desde el punto de vista biológico

Prueba toxicológica de dosis única para la vacuna antileptospirósica vax-SPIRAL en ratones / Single-dose toxicological test for leptospirosis vaccine vax-SPIRAL in rats

Se realizó la prueba toxicológica de dosis única para la vacuna antileptospirósica vax-SPIRAL en ratones. No se encontraron síntomas clínicos de toxicidad y las diferencias entre las variables evaluadas no fueron importantes desde el punto de vista biológico(AU)

Aplicación de un método alternativo al conteo en cámara de Neubauer para determinar la concentración de Trichomonas vaginalis / Application of an alternative method to the count in camera of Neubauer to determine the concentration of Trichomonas vaginalis

Se demostró que existe relación entre la concentración celular y la lectura de los parásitos en un lector de ELISA. Se determinó que la absorbancia tiene valores significativos en las longitudes de onda del rango visible y se escogió la longitud de onda mínima posible (450 nm) para garantizar un máximo de sensibilidad. Pudo comprobarse que ocurre un aumento significativo de la absorbancia (p<0,001) después de llenada la placa, que se estabiliza en el intervalo de 40 min hasta 4 h. Al aplicar 100, 150, 200 ó 300 µL por pozo de las diferentes concentraciones de células se demostró que el volumen óptimo era de 150 µL, se obtuvo un r2 = 0,9986, y resultaron altamente significativos el coeficiente de correlación (p<0,001) y la pendiente (p<0,001). En el intervalo de 5 x 104 a 1,5 x 107 células/mL se obtuvo un coeficiente de variación medio de 1,75 por ciento (0,25-3,17 por ciento). En estas condiciones el límite de cuantificación fue de 5,14 x 104 células/mL. Por último se demostró que hubo significación de la correlación entre el conteo en cámara de Neubauer y la densidad óptica(AU)