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Revista de la Universidad Industrial de Santander. Salud

Print version ISSN 0121-0807On-line version ISSN 2145-8464

Rev. Univ. Ind. Santander. Salud vol.57  Bucaramanga Jan./Dec. 2025  Epub Sep 24, 2025

https://doi.org/10.18273/saluduis.57.e:25v57r04 

Review Article

Experimental conditions for assessing anti-Trypanosoma cruzi (epimastigotes) activity in vitro: A scoping review

Condiciones experimentales para evaluar la actividad anti- Trypanosoma cruzi (epimastigotes) in vitro: una revisión de alcance

María-Helena Arias1 
http://orcid.org/0000-0002-1011-5157

Jhindy-Tatiana Pérez1 
http://orcid.org/0000-0002-5437-5831

Giovanny Garavito1  * 
http://orcid.org/0000-0002-6055-0501

1 Universidad Nacional de Colombia, Facultad de Ciencias, Departamento de Farmacia, Bogotá, Colombia.

Abstract

Introduction:

Chagas disease, caused by Trypanosoma cruzi, affects 6-8 million people worldwide. Current treatments raise safety concerns. In vitro phenotypic screening variability in parasite strains, life cycle stages, and experimental conditions hinders result comparisons impeding new treatment development.

Objective:

To identify experimental conditions in T cruzi epimastigote model and propose criteria for harmonizing experimental procedures.

Methodology:

Analysis of 63 research articles (106 assays) from indexed journals (2008-2023), on antiparasitic activity against epimastigotes.

Results:

Studies use diverse evolutionary forms, primarily amastigotes and epimastigotes. Despite advancements in culture techniques, establishing uniform conditions remains unfeasible. We propose focusing on specific parasite forms.

Conclusions:

To harmonize experimental conditions, we propose standardizing: strains, culture medium (and enrichment), incubation parameters (temperature and medium replacement frequency). Similarly, the pharmacological test conditions such as infecting inoculum concentration, culture well plate specifications, treatment exposure time, and parasite quantification method-facilitating result comparison and accelerating the development of new treatments.

Key words: Trypanosoma cruzi; Parasitic Sensitivity Tests; Chagas Disease; Scoping Review; Neglected Tropical Diseases; Drug Discovery; In Vitro Techniques

Resumen

Introducción:

La enfermedad de Chagas, causada por Trypanosoma cruzi, afecta entre 6 y 8 millones de personas en todo el mundo. Los tratamientos actuales plantean problemas de seguridad. La variabilidad del tamizaje fenotípico in vitro en cuanto a cepas del parásito, estadios del ciclo vital y condiciones experimentales dificultan la comparación de resultados e impiden el desarrollo de nuevos tratamientos.

Objetivo:

Identificar condiciones experimentales críticas en el modelo de epimastigotes de T. cruzi y proponer criterios para armonizar los procedimientos experimentales.

Metodología:

Análisis de 63 artículos de investigación (106 ensayos) de revistas indexadas (2008-2023), sobre actividad antiparasitaria frente a epimastigotes.

Resultados:

Los estudios utilizan diversas formas evolutivas, principalmente amastigotes y epimastigotes. A pesar de avances en las técnicas de cultivo, establecer condiciones uniformes para todos los estadios sigue siendo inviable. Proponemos focalizar formas parasitarias específicas.

Conclusiones:

Para armonizar condiciones experimentales, proponemos optimizar: cepas, medio de cultivo (y enriquecimiento), parámetros de incubación (temperatura y frecuencia de sustitución del medio). Del mismo modo, las condiciones de prueba farmacológica, como concentración del inóculo infectante, especificaciones de placa de cultivo, tiempo de exposición al tratamiento y método de cuantificación del parásito, facilitan comparación de resultados y aceleran el desarrollo de nuevos tratamientos.

Palabras clave: Trypanosoma cruzi; Pruebas de Sensibilidad Parasitaria; Enfermedad de Chagas; Revisión de Alcance; Enfermedades Desatendidas; Descubrimiento de Fármacos; Técnicas In Vitro

Introduction

The Americas contribute 8.8% of the global burden of neglected infectious diseases (NIDs)1, An estimated 6-8 million people are infected with Trypanosoma cruzi (T. cruzi), the parasitic protozoan that causes Chagas disease (CD) (also known as American Trypanosomiasis), with 65-100 million people at risk worldwide. There are 30,000 new cases annually due to vector transmission and another 8,000 due to congenital transmission, causing approximately 14,000 deaths per year 1-5. The disease is endemic in 21 countries in Latin America and the Caribbean. An upward trend in the number of reported cases has been observed in Canada, Asia, the United States, and Europe, attributed mainly to migration and poverty 1,4,6,7. In 2021 poverty in Latin America affected more than 184 million people (32.3 % of the population) with another 12.9 % living in extreme poverty; these conditions remain higher than before the COVID-19 pandemic. In rural areas poverty and extreme poverty reach 44.1 % and 21.2 %, respectively, mainly affecting children and adolescents up to 17 years of age, women of productive age, people with low education, indigenous people, Afro-descendants and people with disabilities 8. Migration, access to travel, and expansion of international markets, especially to the United States and Europe, combined with poverty, limited access to health systems and deficiencies in housing, water and basic sanitation for migrants, have increased the risk of transmission of infectious diseases in non-endemic countries 1,6,9-11.

The success in the spread of the disease and the difficulties in its control and elimination can be attributed to several factors: the genetic diversity of T. cruzi (classified into seven different discrete typing units or DTUs: Tcl-TcVI and Tcbat 12) and the absence of rapid and specific tests for different genotypes, the parasite's capacity to infect various species of vertebrates and vectors (>100 and >150, respectively), the lack of knowledge about the prevalence and incidence of chronic disease, the low specificity of clinical symptoms, the absence of highly effective vaccines and drugs, the toxicity of existing treatments and poor adherence to them, the high costs that limit access to treatment and the resistance of vectors to insecticides used for their control 3,13-15

Chagas disease progresses through three phases: acute, indeterminate and chronic. The acute phase is characterized by mild, intermittent symptoms and abundant presence of parasitic forms in the bloodstream; followed by an indeterminate and a chronic phases in which the parasites invade nucleated muscle cells potentially leading to coronary (20 - 30 % of cases) or gastrointestinal (10 - 20 % of cases) disease, with the presence of megacolon or megaesophagus. During the acute phase the diagnosis is established mainly by the detection of trypomastigotes in blood, while in the chronic phase, serological tests for the determination of immunoglobulin G (IgG) of specific antibodies that bind to T. cruzi antigens (enzyme-linked immunosorbent assay (ELISA) and immunofluorescence assay (IFA)) are useful.

Nifurtimox and benznidazole, introduced in the l960s, remain the only drugs available for CD treatment. Pharmacological treatment should be initiated in the acute phase of the disease since its effectiveness decreases drastically and is even considered controversial when the chronic phase is reached. In addition, the safety profile of these drugs raises significant concerns due to frequent adverse effects, ranging from digestive disorders and psychic alterations to more severe conditions such as bone marrow depression, peripheral polyneuropathy, lymphadenopathy, thrombocytopenic purpura, and agranulocytosis. Pharmaceutical companies have shown very limited interest in developing new therapies against trypanosomatid parasites, due to the low expected return on investment as the target communities often have little to no purchasing power 3,4,6,16,17.

Recently, a meta-analysis that aimed to establish the in vitro susceptibility of the Y strain to benznidazole showed a wide variability in the IC50 values obtained, without clearly determining the cause of this heterogeneity, leading the authors to conclude that variability could be explained by the lack of uniformity in the experimental procedures for trypanocidal activity tests 18. Two in vitro studies using TcI, TcII and TcV DTUs failed to establish a correlation between benznidazole susceptibility and genetic distances among these DTU strains 19,20, additionally, a systematic review was unable to find statistically significant associations between T. cruzi genotype and clinical outcome 31. These studies employed different sources of parasite stages (e.g., trypomastigotes forms from infected mouse bloodstream or cell culture, amastigotes from different host cell lines, epimastigotes), various culture media, different benznidazole sources (pure active compound or commercial pills), and a variety of methods to determine parasite viability. This variability underscores the critical need for establishing standardized protocols in future research to ensure more consistent and comparable results across studies.

In vitro pharmacological models play a pivotal role as an initial filter in identifying substances with antiparasitic activity against T cruzi, being a fast, simple and inexpensive tool; these models employ a wide variety of cell lines, parasite strains and culture conditions, allowing us to expand our knowledge about the biology, mechanisms of parasitic infection and have been key to the discovery of molecules with antiparasitic activity; however, despite the advantages, the lack of consensus on in vitro screening protocols has emerged as a significant obstacle in the discovery of new drugs to treat Chagas disease.

The absence of well-defined experimental conditions for evaluating promising substances has resulted in poor reproducibility and reliability of results. This inconsistency becomes an obstacle when attempting to compare findings across different studies as a foundation for subsequent stages of the pharmacological research and development (R&D) process. Therefore it is not surprising that despite a large number of compounds with promising activity, in in vitro tests, are frequently reported, only four substances -allopurinol, itraconazole, posaconazole and fluconazole- have advanced to clinical studies 3,22,23; unfortunately, in clinical trials, none of these compounds have demonstrated superior efficacy to benznidazole, particularly when evaluated in patients with chronic CD. The drug R&D processes for Chagas disease are poor leaving an urgent need for new effective treatments, necessary to meet the World Health Organization (WHO)'s roadmap for neglected tropical diseases and to achieve the United Nations Sustainable Development Goals 4,11. The Open Science movement aims to promote research integrity, experimental and analytical reproducibility and full transparency. A major challenge in the research and development of drugs against trypanosomatids remains the lack of defined conditions/standards for the selection and validation of promising compounds. This deficiency often leads to conflicting results between different research teams 3.

Pharmacological models for trypanosome research have recently garnered growing interest, reflected in numerous reviews addressing various aspects such as: advances in Trypanosomatid biology from a drug R&D perspective and the identification of promising molecular targets 7,11, procedural approaches for assessing trypanocidal activity and toxicity in mammalian cells. Additionally, they explore infection characteristics and methodologies 15,22, the evolution of Chagas disease drug discovery techniques and current pharmacological models used in drug R&D cascades 3,24, medicinal chemistry, chemotherapy and therapeutic options in development 4,6,11. To address the challenge posed by Bhattacharya 3 and provide a comprehensive picture of in vitro antitrypanosomal screening conditions used in research and development of new therapeutic alternatives against CD, this scoping review aimed to identify and present available information regarding experimental conditions of epimastigotes models. Additionally, we aimed to propose criteria and conditions for homogenizing experimental protocols (Box 1). Through this approach, we hope to contribute to ensuring consistency and comparability of results across different laboratories.

Methodology

Search strategy

The review covered PubMed, Scopus and LILACS databases, focused on articles published between the years 2008 and July 2023, a time frame chosen based on preliminary analysis of publication trends. A preliminary search in PubMed for "in vitro antitrypanosomal screening" revelated low and intermittent scientific production (<4 articles / year) between l989 and 2007, which markedly increase from 2008 onwards (>4 articles / year). The search equation included the following terms MeSh (for English) and DeCS (for Spanish and Portuguese) ("Trypanosoma cruzi", "Parasitic Sensitivity Tests" and "Trypanocidal Agents"), in all cases the Boolean operator "AND" was used. To capture relevant articles potentially missed in database searches, reference lists of key sources were examined. Article review and data collection were conducted independently by at least two reviewers. Data were subsequently cross-checked, and discrepancies were resolved through consensus meetings. The study followed current, commonly accepted requirements and guidelines for reporting systematic reviews 25-27.

Study/source of evidence selection

This scoping review used the following inclusion criteria to select articles: English, Spanish or Portuguese language, studies reporting the conduct of in vitro antiparasitic activity against T. cruzi epimastigotes. Articles not specifying strain and parasitic form used and those that correspond to different parasite stages (e.g., trypomastigotes, amastigotes), immunological studies, genetic characterization studies of T. cruzi strains, biological studies, case reports, and non-primary sources were excluded. Article selection involved screening titles, abstracts, and keywords, followed by full-text review when necessary. This scoping review aimed to describe and map the literature to provide a comprehensive picture of in vitro antitrypanosomal screening conditions and to propose risk of bias assessment criteria for such studies.

Data extraction

A comprehensive database was constructed to record information in two main categories: regarding the pharmacological model, T. cruzi strain or isolate, culture media, serum supplementation (type and percentage), culture media enrichment, culture media replacement frequency (in days) and incubation temperature. From the antiparasitic pharmacological test information was extracted regarding infective inoculum (Parasites/mL), treatment exposure time (hours (h)), type of well culture plate and methodology to quantify parasite viability; finally, the active control used (reference drug), concentration tested, treatment duration and antiparasitic activity results were reviewed.

Results

Literature search

The Bibliographic search across all consulted databases, yielded a total of 392 records. After manually removing 189 duplicates and excluding l unavailable article, 202 articles remained for review (Figure 1). The analysis of database overlap revealed a concordance rate of 1.5 % between PubMed-Scopus-LILACS, 47.1 % between PubMed-Scopus, 4.1 % between PubMed-LILACS and 2.9 % between Scopus-LILACS. The remaining 202 articles were reviewed for title, abstract and keywords, of these 139 were discarded due to predetermined exclusion criteria. The remaining articles underwent full-text review by at least two independent readers yielding a final selection of 63 articles, encompassing 105 assays that met all inclusion criteria. The complete article selection process is illustrated in Figure 1.

Figure 1: Article selection process 28

A global analysis of the parasitic forms used in the reports of in vitro trypanocidal activity (data not show). Out of 167 articles reviewed, the most frequently used parasitic forms were: amastigotes (104 reports), epimastigotes (63 reports), blood trypomastigotes (42 reports) and cell culture derived trypomastigotes (49 reports), Figure 2. The use of a single parasitic form was reported in 96 articles (57 %), 52 articles (31 %) reported the use of 2 parasitic forms, and in 19 articles (11 %) 3 parasitic forms were used.

Figure 2:  In vitro trypanocidal activity as a function of the parasitic form used. 

Due to the variability that arises from analyzing different sources of parasite stages simultaneously, such as trypomastigote forms from the bloodstream of infected mice or cell cultures, amastigotes from various host cell lines, and epimastigotes; this scoping review focuses specifically on pharmacological models that assess antitrypanosomal activity in epimastigotes.

Reported conditions in pharmacological model of in vitro culture of T. cruzi epimastigotes

Antiparasitic activity against epimastigote forms was evaluated in 63 reports (106 assays) that informed the use of 28 different strains. Strain Y (Tc II) was the most frequently informed (33 assays), followed by strains CL (Tc VI) (15 assays), Tulahuen (Tc VI) (9 assays) and DM28c (Tc I) (8 assays), four strains were tested in 3-5 assays (SN3(IRHOD/CO/2008/SN3), Silvio X10, RA (Tc VI), Arequipa) and 20 others 1-2 assays (Esmeraldo cl3, Colombiana (Tc I), Maracay, YuYu (Tc I), Berenice 62, VL10, DA (MHOM/CO/01/07), MHOM/ES/2203/BCN590, M6241 cl6, 793, 893, 4166, NR cl3 (Tc V), SO3 cl5 (Tc V), 115, 294, 597, INC-5, NINOA, TH).

The use of liver infusion-tryptose culture medium (LIT) predominated with 58 assays (of which 14 assays correspond to Franco, J., et al.29 and 8 to Zingales, B., et al.30), followed by brain heart infusion (BHI), Roswell Park Memorial Institute (RPMI) 1640 media, Medium Trypanosomes Liquid (MTL) and Biphasic 3N medium (20, 7, 7 and 4 assays each, respectively), and the other media with two or one report (Diamond's monophasic medium, BHT, 3N + MEM, Grace's Insect Medium). Regarding the culture media enrichment with fetal bovine serum (FBS) predominated a concentration of 10% (79 tests of which 14 assays correspond to Franco, J., et al.29 and 8 to Zingales, B., et al.30), followed by FBS (5%) in 14 tests and FBS (20%) in three tests, 10 assays did not inform the FBS concentration used, Figure 3.

The culture media replacement frequency was not frequently reported (79 assays), in the remaining ones, replacement every 7d (9 assays) followed by every 3-4d (8 assays) and every 10d (7 assays) predominated; replacement every 5d and 8d was reported one and two times each respectively. Finally, the most reported incubation temperature, in parasite culture and in pharmacological tests was 28 °C (91 assays) followed by 26 °C (6 assays) and 27 °C (3 assays), 6 assays did not report the temperature used.

Strains with 1-2 assays (each): Esmeraldo cl3, Colombiana (Tc I), Maracay, YuYu (Tc I), Berenice 62, VL10, DA (MHOM/ CO/01/07), MHOM/ES/2203/BCN590, M6241 cl6, 793, 893, 4166, NR cl3 (Tc V), SO3 cl5 (Tc V), 115, 294, 597, INC-5, NINOA, TH. Strains with 3-5 assays (each): SN3(IRHOD/CO/2008/SN3), Silvio X10, RA (Tc VI), Arequipa. Culture media with one report (each): 3N + MEM and Grace's Insect Medium. Culture media with two reports (each): BHT and Diamond's monophasic.

* 14 assays correspond to Franco, J., et al.29. ** 8 assays correspond to Zingales, B., et al.30.

Not reported (NR).

Figure 3: Pharmacological model of epimastigote culture: strain, culture media, enrichment serum percentage and incubation temperature, most frequently used to obtain parasite forms. 

Pharmacological test conditions for T. cruzi epimastigotes

The initial infecting inoculum (parasites/mL) varies across three orders of magnitude, with a minimum value of 1 x 105 parasites/mL and a maximum value of 1 x 107 parasites/mL (100 times higher). This parameter is crucial for harmonizing test conditions, as it directly relates to the challenge faced by the substance being evaluated. A low initial inoculum may incorrectly declare inactive substances as active, while an excessively high infecting inoculum could lead to identify active substances as inactive. The latter scenario is known as a type II error, or false negative. Therefore, careful consideration of the initial inoculum is essential for accurate and reliable test results in parasitology studies.

Two outlier reports, involving 14 and 8 assays each 29,30 significantly distort the overall trend and are highlighted in Figure 4. Excluding these outliers, 97 % of the reports present 3 or fewer tests each. Among these reports, the initial infectious inoculum of 1 x 106 parasites/mL predominates in 27 % of the tests. This is followed by 5 x 105 parasites/mL (10 % of tests) 2 x 106 and 5 x 106 parasites/mL (7 % of tests each), and 1.5 x 106 parasites/mL (6 % of tests). Other infecting inoculum concentrations are reported in 5% or fewer of the cases. Notably, 13% of the tests reported parasite concentration as parasites/well without specifying the volume used in the well, making direct comparisons difficult. Additionally, 7 % of the test did not report units of parasite concentration, and one report failed to provide this important parameter altogether. When the two outlier reports 29,30 are included in the analysis, the proportion of test using I x 107 parasites/mL increase dramatically from 5 % to 25 % of all tests. This shift underscores the significant impact these outliers have on the overall distribution, Figure 4.

The addition of antibiotics in some test is concerning penicillin (5 tests), streptomycin (6 tests), penicillin-streptomycin (9 tests), and gentamicin (4 tests). This practice has been questioned in other pharmacological models, as good laboratory practices should ensure non-contamination of parasite cultures without antibiotic use. Regarding cell counting methods, microscopy with a Neubauer chamber was the predominant method, used in 58 of the reports, only I used microscopy with an Automated cell counter (TC20). Various other techniques were employed to determine parasite viability: colorimetric tests were described in 22 tests (MTT II, CPRG 3, Resazurin 8). Turbidimetry (referred to as absorbance) was informed in 16 tests. Six of the reports mentioned the use of fluorometry (Resazurin 5 and Propidium iodide I). Less frequently, radiometry using [3H]-thymidine was employed (3 reports), Figure 4.

The most frequently reported active control was Benznidazole, used in 70 tests, followed by nifurtimox in 13 tests. Two active controls were used in some tests: Benznidazole + Nifurtimox in 7 tests and Nifurtimox + Miltefosine in I test. However, there are notable omissions in the reporting of controls: 15 reports did not mention the use of any control drug, and 12 reports indicated the use of active control but failed to provide the resulting parasite inhibition data. These omissions are concerning, as the use of active control is essential for demonstrating adecuate experimental design and providing evidence of proper bias control in experimental pharmacology, Figure 4.

* 14 assays correspond to Franco, J., et al.29.

** 8 assays correspond to Zingales, B., et al.30.

***Neubauer (58), Automated cell counter (TC20) (1).

****MTT (II), Resazurin (8), Chlorophenol red-ß-d-galactopyranoside (CPRG) (3).

***** Resazurin (5), Propidium ioide (1).

Not reported (NR).

Figure 4: Epimastigotes screening conditions of in vitro trypanocidal tests: Infective inoculum (Parasites/mL), Active control, Treatment exposure time (Hours (h)) and Methodology to quantify parasite viability. 

The inhibition of parasite multiplication achieved by the reference drug is reported in various terms: Inhibitory Concentration 50 (IC50) in 68 % of tests, fifty percent of Parasite Growth Inhibition (PG150) in 4 % of tests, and minorly so as Cytotoxic Concentration 50 (CC50) in 1 % of tests, Percentage of Parasite Death in 1 %, Inhibitory Dose 50 (ID50) in 1 %, fortunately, these last confusing interpretations of terms are rare. However, it is worth noting that 25 % of tests do not report the parasite inhibition generated by the reference drug. Despite the lack of uniformity in the experimental procedures for trypanocidal activity tests,

Table 1 Summarizes the pharmacological activity data reported for the active controls Benznidazole, Nifurtimox and Miltefosine. 

Reference Author, Year T. cruzi strain (DTU) Active control Treatment exposure time (h) Results (μM)
38 Gusmão et al., 201 Y (TcII) Benznidazole 72 30.78
42 Salsi et al., 2019 Y (TcII) Benznidazole 72 15.1
43 Fonseca-Berzal et al., 2018 Y (TcII) Benznidazole 48 28.11
24 218
44 Lima et al., 2018 Y (TcII) Benznidazole 48 61.1
72 16.5
45 Cardoso et al., 2014 Y (TcII) Benznidazole 264 6.6
47 Velásquez et al., 2014 Y (TcII) Benznidazole 72 34
48 Franklim et al., 2013 Y (TcII) Benznidazole 168 2.2
49 Izumi et al., 2013 Y (TcII) Benznidazole 96 6.53
50 Jorge et al., 2013 Y (TcII) Benznidazole 120 22.69
51 Moreira et al., 2013 Y (TcII) Benznidazole 72 34.5
52 Carneiro et al., 2012 Y (TcII) Benznidazole 72 11.5
53 Izumi et al., 2012 Y (TcII) Benznidazole 96 6.5
54 Daliry et al., 2011 Y (TcII) Benznidazole 24 168
56 Veiga-Santos et al., 2010 Y (TcII) Benznidazole 96 7.8
57 Dos Santo Filho et al., 2009 Y (TcII) Benznidazole 264 6.6
58 Batista et al., 2008 Y (TcII) Benznidazole 72 10.3
7 Fonseca-Berzal et al., 2018 CL (TcVI) Benznidazole 72 26.55
29 Franco et al., 2015 CL (TcVI) Benznidazole 72 13.2
30 Zingales et al., 2015 CL (TcVI) Benznidazole 72 13.2
67 Vega et al., 2012 CL (TcVI) Benznidazole 72 27.32
78 Cardoso et al., 2019 DM28c (TcI) Benznidazole 120 6.6
79 Ceole et al., 2018 DM28c (TcI) Benznidazole 24 59
81 Da Silva et al., 2017 DM28c (TcI) Benznidazole 96 48.8
83 Gomes et al., 2016 DM28c (TcI) Benznidazole 264 48.8
84 Espíndola et al., 2015 DM28c (TcI) Benznidazole 120 48.8
72 Paucar et al., 2019 Tulahuen (TcVI) Benznidazole 48 25.3
42 Salsi et al., 2019 Tulahuen (TcVI) Benznidazole 72 17.9
75 Martín-Escolano et al., 2018 Tulahuen (TcVI) Benznidazole 48 19.7
76 Moreno-Viguri et al., 2016 Tulahuen (TcVI) Benznidazole 72 18.7
55 Álvarez et al., 2010 Tulahuen (TcVI) Benznidazole 120 7.4
59 Boiani et al., 2008 Tulahuen (TcVI) Benznidazole 120 4.5
29 Franco et al., 2015 Silvio X10 (TcI) Benznidazole 72 26.1
30 Zingales et al., 2015 Silvio X10 (TcI) Benznidazole 72 26.1
30 Zingales et al., 2015 Esmeraldo cl3 (TcII) Benznidazole 72 26.7
32 Muscia et al., 2020 RA (TcVI) Benznidazole 72 5.8
31 Beer et al., 2016 RA (TcVI) Benznidazole 72 4.99
90 Martín-Montes et al., 2021 SN3(IRHOD/CO/2008/ SN3) (TcI) Benznidazole 72 15.8
72 Paucar et al., 2019 SN3(IRHOD/CO/2008/ SN3) (TcI) Benznidazole 48 15.3
75 Martín-Escolano et al., 2018 SN3(IRHOD/CO/2008/ SN3) (TcI) Benznidazole 48 36.2
76 Moreno-Viguri et al., 2016 SN3(IRHOD/CO/2008/ SN3) (TcI) Benznidazole 72 15.8
85 Ramírez-Macías et al., 2012 SN3(IRHOD/CO/2008/ SN3) (TcI) Benznidazole 72 15.89
29 Franco et al., 2015 Colombiana (TcI) Benznidazole 72 40.5
30 Zingales et al., 2015 Colombiana (TcI) Benznidazole 72 34.1
92 Marín et al., 2011 Maracay (TcVI) Benznidazole 72 15.8
91 Maldonado et al., 2010 Maracay (TcVI) Benznidazole 72 16
86 Hamedt et al., 2014 DA (MHOM/CO/0I/07) (TcI) Benznidazole 72 26.9
87 Di Pietro et al., 2015 MHOM/ES/2203/ BCN590 (TcI) Benznidazole 72 36.2
29 Franco et al., 2015 YuYu (TcI) Benznidazole 72 40.5
30 Zingales et al., 2015 YuYu (TcI) Benznidazole 72 40.5
29 Franco et al., 2015 Berenice 62 (TcII) Benznidazole 72 14.6
30 Zingales et al., 2015 Berenice 62 (TcII) Benznidazole 72 14.6
29 Franco et al., 2015 793 (Tcbat) Benznidazole 72 16.6
29 Franco et al., 2015 893 (TcIII) Benznidazole 72 74.9
29 Franco et al., 2015 SO3 cl5 (TcV) Benznidazole 72 10.6
30 Zingales et al., 2015 115 (TcV) Benznidazole 72 7.6
29 Franco et al., 2015 VL10 (TcII) Benznidazole 72 30.4
30 Zingales et al., 2015 VL10 (TcII) Benznidazole 72 30.4
88 Chacón-Vargas et al., 2017 INC-5 (TcI) Benznidazole 24 42.34
89 Domínguez-Díaz et al., 2021 NINOA (TcI) Benznidazole 48 30.27
89 Domínguez-Díaz et al., 2021 TH (ITRI/MX/2018/TH) (TcI) Benznidazole 48 39.08
72 Paucar et al., 2019 Arequipa (TcV) Benznidazole 48 26.2
76 Moreno-Viguri et al., 2016 Arequipa (TcV) Benznidazole 72 15.8
75 Martín-Escolano et al., 2018 Arequipa (TcV) Benznidazole 48 16.9
41 Espinosa-Bustos et al., 2020 Y (TcII) Nifurtimox 120 7
46 Tapia et al., 2014 Y (TcII) Nifurtimox 120 7
50 Jorge et al., 2013 Y (TcII) Nifurtimox 120 3.78
59 Boiani et al., 2008 Y (TcII) Nifurtimox 120 9.7
62 Scalese et al., 2021 CL (TcVI) Nifurtimox 24 3.68
64 Scalese et al., 2018 CL (TcVI) Nifurtimox 120 2.8
66 Santos et al., 2012 CL (TcVI) Nifurtimox 72 3.16
67 Vega et al., 2012 CL (TcVI) Nifurtimox 72 3.6I
69 Rodríguez et al., 2009 CL (TcVI) Nifurtimox 120 3.4
59 Boiani et al., 2008 CL (TcVI) Nifurtimox 120 4.9
77 López-Lira et al., 2021 DM28c (TcI) Nifurtimox 24 21.05
82 Robledo-O'Ryan et al., 2017 DM28c (TcI) Nifurtimox 24 17.4
84 Espíndola et al., 2015 DM28c (TcI) Nifurtimox 120 5.7
71 Matiadis et al., 2021 Tulahuen (TcVI) Nifurtimox 120 7
73 Aguilera et al., 2019 Tulahuen (TcVI) Nifurtimox 120 7
74 Soares et al., 2019 Tulahuen (TcVI) Nifurtimox 120 5
59 Boiani et al., 2008 Tulahuen (TcVI) Nifurtimox 120 7.7
88 Chacón-Vargas et al., 2017 INC-5 (TcI) Nifurtimox 24 8.74
89 Domínguez-Díaz et al., 2021 NINOA (TcI) Nifurtimox 48 7.09
89 Domínguez-Díaz et al., 2021 TH (ITRI/MX/2018/TH) (TcI) Nifurtimox 48 19.3
73 Aguilera et al., 2019 Tulahuen (TcVI) Miltefosine 120 8

In vitro normalized susceptibility indices (IC50, PGI50, CC50 ID50). DTU: Discrete typing unit, h: Hours.

The treatment exposure time, defined as the period from treatment addition to measurement of phenotypic changes, varies considerably. The minimum value is 24 h, while the maximum is 264 h (II times higher). 72 h predominates in 50 tests, followed by 120 h in 20 tests, 24 h and 48 h (II tests each), 96 h (8 tests) and finally 168 h and 264 h (3 tests each), Figure 4. On T. cruzi Y (TcII), the Benznidazole inhibition of parasite multiplication requires less quantity of drug when increasing exposure time (in the interval 24-72 h), a trend similar to that reported by Vela et al. However, this parameter stabilizes after 72 h, remaining consistent up to exposure times as long as 264 h. This preliminary evidence allows to visualize an optimal treatment exposure time so that this parameter can be harmonized, Table 1.

Treatment exposure time is a crucial parameter in pharmacological tests. It directly impacts the challenge faced by the test substance and can significantly influence the final results. Within timeframes that are realistic from chemical and pharmacokinetic perspectives, different exposure times for the same substance can lead to varying outcomes. This variability in results due to treatment exposure time can have important implications. It may lead to incorrectly rejecting the null hypothesis when it is actually true. These potential errors underscore the importance of harmonize and carefully considering the treatment exposure time in experimental design, Table 1.

A treatment exposure time of 72 h was most common among the reports meeting the selection criteria (even when refining the two references that bring together 22 tests, Figure 4), under these condition, various T. cruzi strains exhibited different susceptibilities to Benznidazole. The strain RA (Tc VI) showed he highest susceptibility, with an IC50 of 5,4 /μM 31,32. In contrast, strain 893 (TcIII) was the most resistant with an IC50 of 74.9 /μM 29 - a value 14 times higher than that of strain RA. This information can guide researchers in selecting appropriate challenge conditions when evaluating test substances. As efforts to harmonize conditions for pharmacological activity tests progress, this data will be further refined, potentially leading to more standardized and comparable results across studies, Figure 5.

The results represent the mean ± SD of in vitro normalized susceptibility indices (IC50, PG150, CC50 ID50). *2 Independent tests, ** 3 Independent tests, *** 4 Independent tests, **** 7 Independent tests, the other strains I report.

Figure 5: Benznidazole as an active control: T cruzi multiplication inhibition at 72h treatment exposure. 

The use of 96-well plates was most common (30 %, 32 tests), closely followed by 24-well plates (29 %, 31 tests). Notably, over a quarter of the test did not report the plate type used (28 tests). 15 reports used tubes or culture boxes (7 and 8 respectively). Regarding the number of parasite strains, the vast majority of reports (84 %) used a single strain. A small number of studies used two or three strains (5 % and 8 % respectively). Extreme values of eight and fourteen strains per article are reported on one occasion each.

Discussion

During its life cycle, T. cruzi alternates among different morphological and functional forms and involves both mammalian and triatomine bug hosts. The various parasitic stages of T. cruzi can be cultured in vitro using either axenic cultures or mammalian cells. Different forms of the parasite can be obtained or induced in laboratory conditions: epimastigote forms can transform into trypomastigote forms through nutrient or culture media suppression, epimastigote forms can be obtained from blood trypomastigotes, intracellular amastigotes or culture-derived trypomastigotes (by infecting mammalian cell cultures with trypomastigote forms) and axenic amastigotes can also be cultured 33,34. However, despite advances in maintaining these different evolutionary forms in the laboratory, it remains unfeasible to establish uniform culture conditions valid for all stages. This challenge arises from their distinct biological developmental contexts: trypomastigote and amastigote are found in the vertebrate host, and epimastigote and metacyclic trypomastigotes are found in the invertebrate host.

Furthermore, the morphogenetic and cell cycle modifications that occur during the progression of these three parasitic forms in their complex life cycle 13,34.

The determination of T. cruzi susceptibility in pharmacological activity tests is complex due to two main aspects: the first, mentioned above (related to the diversity of parasite evolutionary forms) confers wide variability in terms of morphology, cell tropism, infectivity, virulence, antigenic composition, metabolic activity, adaptation to the culture medium, drug susceptibility and natural resistance of the different known strains; and the second aspect is directly related to the experimental conditions under which the pharmacological activity tests is performed, which include the strain, the culture medium (and supplementation), the Infective inoculum and the interaction time between the parasite and the test substances, among others 18. Given these complexities, a systematic approach focusing on parasite forms is necessary. This approach aims to identify the most representative variables of both the biological model and the pharmacological test. The goal is to propose initial conditions for harmonization, enabling different research teams to develop equivalent and comparable tests.

The use of in vitro pharmacological models for screening trypanocidal activity offer several advantages related to costs and biosafety. These benefits include: In vitro T. cruzi cultivation allows for a significant reduction in the number of animals used in experimental infection models. This contributes to the ethical aspects of animal reducing and replacement in research (3 Rs principle). In vitro models generally require less laboratory infrastructure compared to in vivo methods. These models allow for reduced experiment duration compared to in vivo methods, potentially accelerating the research process. In vitro cultivation procedures present a lower risk of human infection during culture procedures, improving overall laboratory safety. Finally the combination of reduced animal use, lower infrastructure needs, and shorter experiment times can lead to significant cost savings in research 34.

In general, the Y strain of T. cruzi is the most frequently used in susceptibility testing, both in vitro and in vivo. This strain is characterized by high virulence and mortality in animal models, giving it clinical relevance and making it an appropriate biological model for pharmacological testing 35,36. However, it is crucial to recognize the biological diversity of T. cruzi. Whenever possible, it is essential to include several strains in anti-trypanosomal activity assays, this is particularly important for strains belonging to the DTU's: TcI, TcII, TcV and TcVI which are associated with human infection 7. This approach enhances the translational potential of preclinical studies, potentially leading to more effective treatments for Chagas disease.

Our global analysis found that amastigotes were the most commonly used parasitic form in in vitro pharmacological tests to determine T. cruzi susceptibility, followed by trypomastigotes and epimastigotes (Figure 2). Vela et al.18, reported epimastigotes as the most commonly used parasitic form, in pharmacological tests to determine sensitivity of different parasitic forms to benznidazole (47 %), followed by amastigotes (29 %) and trypomastigotes (24 %). The preference of amastigotes (104 tests) in drug sensitivity testing is highly relevant. This parasitic form is replicative in the human host and predominates in the late phase of the disease, when different organs may be affected, including cardiac complications leading to death. Moreover evidence about the effectiveness of benznidazole in this disease phase remains contradictory, driving research focus towards determining compounds efficacy against amastigotes 5,7.

Epimastigotes possess distinct metabolic, proteomic, and ultrastructural organization compared to trypomastigotes and amastigotes, suggesting that drug targets likely differ substantially between these parasite forms. While researchers currently discourage using extracellular epimastigote forms as primary pharmacological model for human and mammalian infections, these forms remain valuable for complementary screening, particularly as experimental evidence indicates potential oral transmission routes 96,97. Moreover, these forms allow for high parasite multiplication rates in a short time and at a low cost compared to intracellular forms, which require prior mammalian cell culture. However, it is important to note that test molecule activity may appear more promising in extracellular forms due to direct parasite-molecule interaction. This interaction may be reduced or absent when the substance must cross cell membranes to contact parasite. Therefore, a multistage testing is crucial: initial in vitro screening with intracellular amastigotes, complementary screening with extracellular forms, and then scaling up to in vivo models testing. This stepwise approach ensures a comprehensive evaluation of potential trypanocidal compounds 5,7.

Pharmacological model of in vitro culture of T. cruzi epimastigotes

For susceptibility testing of epimastigote forms, strain Y (TcII) is the most frequently used 33,37-60. Other commonly used DTUs include TcVI (strains CL, Tulahuen) 29,30,42,43,55,59,61-76 and TcI (strain DM28c) 77-84, Figure 3. These strains are associated with human infection, as recommended by Fonseca-Berzal et al.7. Our analysis of pharmacological tests using benznidazole as an active control against epimastigote forms revealed the use of 23 strains distributed across DTUs as follows: TcI 43.5 % 29,30,72,75,76,78,79,81,83-90, TcII 17,4 % 29,30,38,42-45,47-54,56-58, TcIII 4.3 % 29, TcV 13 % 29,30,72,75,76, TcVI 17.4 % 29-32,42,43,55,59,67,72,75,76,91,92 and Tcbat 4.3 % 28 -TcIV strains were not reported-. This information is summarized from 55 articles including 65 assays. Table 2. Vela et al.18, reported different frequencies in their analysis: TcI 69 %, TcII 12 %, TcIII 4 %, TcV 8 % and TcVI 6 % -TcIV strains were not reported-. The choice of strain for a pharmacological model should prioritize human infection-related DTUs (TcI, TcII, TcY and TcVI). This focus ensures that the testing is most relevant to clinical applications and potential drug development for human Chagas disease.

Table 2 Assays of epimastigote susceptibility to benznidazole across T. cruzi Discrete Typing Units (DTUs). 

T. cruzi DTU No. articles No. assays No. strains
TcI 16 21 10
TcII 18 23 4
TcIII 1 1 I
TcV 5 5 3
TcVI 14 14 4
Tcbat 1 1 1
Total 55 65 23

The most frequently used culture media for T. cruzi are LIT, BHI, RPMI 1640, and MTL. These media are typically enriched with FBS at various concentrations, with 10 % being the most common, followed by 5 % and 20 %. The FBS enrichment may vary depending on the state of the parasite culture. However, for consistent and comparable results, test conditions should be reported and harmonized when possible. A commonly recommended standard is the use of LIT medium enriched with 10% FBS.

Pharmacological test conditions for T. cruzi epimastigotes

In in vitro antitrypanosomal test for epimastigotes forms, a standardized and consistent parasite population is crucial for reliable and reproducible results. The infecting inoculum (parasites/mL) directly relates to the challenge faced by the substance to be evaluated. Therefore, this parameter should be homogenized to achieve reproducibility across different laboratories. Growth kinetic studies of various parasite strains, under standardized conditions, are necessary to identify the optimal density. This density should allow robust parasite growth without overcrowding the culture while enabling the detection of drug-induced effects. This review indicates that an initial infection inoculum of approximately 1 x 106 parasites/mL can serve as a basis for optimization and harmonization processes 37,41,44,46,49,52,56,57,59,64,69,71,73,74,89,93. It's important to note that two reports involving 14 and 8 assays each 29,30 significantly deviate this trend (Figure 4). Therefore, our refined analysis considered only the reports presenting three or less assays each, which represent 97% of the total reports. In the assessment of experimental anti-infectious pharmacology studies, the inoculum concentration should be part of a critical evaluation of methodological quality (assessment of risk of bias) of the evidence sources.

The size of the culture plate well influences the appropriate parasite density. Larger wells may require higher parasite densities to effectively cover the surface, and a consistent ratio of parasites per unit volume is required when using different types of plates. This review found the following distribution of culture plate types: 96-well plates predominated in 32 assays 31,37,43-45,51,61,62,64-67,72,75,78,79,83,84,86-89,94, while 24-well plates were used in 31 assays (though 22 of these derived from only two reports) 29,30,48,49,53,55,56,68,90. Additionally, 28 assays did not report this condition. The duration of the test (treatment exposure time) is another crucial factor in determining optimal parasite density. For extended pharmacological tests, researchers must consider parasite replication and growth over time. Among the studies reviewed, a treatment exposure time of 72 hours was the most commonly reported duration for antitrypanosomal test on epimastigotes.

The final parasite density levels must be compatible with the limits of the chosen quantification method. For example, if microscopy is involved, the final parasite density must be sufficient to allow easy visualization and quantification. The traditional method for parasite quantification is counting parasitic forms using a Neubauer chamber. Our review found this method to be the most used due its simplicity and low cost. However, its usefulness is compromised when evaluating a large number of samples, as it is time-consuming and may be subject to counting errors 95,99,100. Other methodologies that have gained popularity measure metabolic activity through colorimetric and fluorescence methods. These are efficient for high-throughput screening as they improve productivity in the number of compounds tested. However, in developing countries, few laboratories have the economic and technical capacity to implement these new methods 7,24,95. Turbidimetry (referred to as absorbance 600nm) has gained prominence as a quantification method. While turbidity-based quantification doesn't require the addition of any stain, it's essential to establish a standard curve relating turbidity to parasite density using a reference method (such as direct cell counting with a Neubauer chamber or flow cytometry) 99,100. This allows for accurate estimation of parasite concentration based on turbidity measurements. Additionally, factors such as culture conditions and the presence of debris in the culture medium can affect turbidity readings and should be taken into account during quantification. The choice of method should be based on the specific research needs, available resources, and the scale of the screening process.

Quality assessment of in vitro antitrypanosomal screening studies should include a comprehensive risk of bias evaluation. This assessment should consider several key design criteria: Presence of infection monitor groups and active control groups. Duration of follow-up (treatment exposure time). Experimental design bias (consistent time-period between treatment exposure and outcome for samples and controls). Performance of experiments in replicates necessary for adequate estimation of IC50. Measures to monitor assay performance (e.g. inter-plate and intra-plate variability). Adequate reporting (including detailed descriptions of methods, results, and statistical analyses). Criteria such as randomized assignment of treatments (plate positions) or blinding of the evaluators of the results are not commonly employed in this type of experimental pharmacology study. This structured approach to quality assessment ensures a thorough evaluation of the methodological rigor in in vitro antitrypanosomal screening studies. By considering these criteria, researchers can improve the reliability and reproducibility of their results, ultimately contributing to more effective drug discovery efforts against Trypanosoma cruzi.

Drug discovery pipelines for Chagas disease are sparse, and there remains an urgent need for new therapeutic options 10. Pharmacological models of in vitro phenotypic screening are essential tools in the search for substances with potential trypanocidal activity. These models have played a protagonist role in the recent development of anti-trypanosomatid drugs for human African Trypanosomiasis and Visceral Leishmaniasis. Drug discovery against T. cruzi is hampered by the small number of well-established targets. This limitation has led to the widespread adoption of phenotypic approaches, which have become the mainstay of Chagas disease R&D. The use of these phenotypic screening models is particularly crucial in the context of CD, where the complex lifecycle of the parasite and limited understanding of druggable targets make target-based approaches challenging.

The research and development of new drugs for CD have improved in the last years, thanks to the work of some organizations and institutions 98. However, the situation remains challenging, and new effective therapeutic alternatives for CD are lacking 4. Several promising approaches are being explored to address this need: Ethnopharmacology-derived natural products continue to be an important scaffold for affordable phytotherapeutic products. The discovery of new biologically active compounds offers potential for novel drug development. Drug repositioning presents a promising strategy to re-introduce known drugs with a history of use in humans. Considering the high attrition rate in the discovery and development of new drugs and the increasing cost of research, the harmonization of experimental conditions in pharmacological research models is a compelling need. By addressing these challenges and capitalizing on these promising approaches, the field of CD drug discovery can continue to progress towards the goal of developing effective, affordable, and accessible treatments for this neglected tropical disease.

Conclusions

Pharmacological models of in vitro phenotypic screening are an essential tool in the search for substances with potential trypanocidal activity, however harmonizing testing conditions is crucial for ensuring consistency comparability and confidence of results across different laboratories and research settings.

Scientific articles reporting the evaluation of antiparasitic activity against T. cruzi reveal a wide variety of parasite forms, parasite strains (and cell lines) and culture conditions, which makes it difficult to the effective selection of promising substances for advanced research stages. An initial approach focusing on specific parasitic forms is necessary to advance in the optimization of test conditions.

To ensure the viability and reproducibility of epimastigotes in in vitro culture models, several conditions need to be homogenized. These include strains, culture medium (and enrichment), and incubation parameters (temperature and culture medium replacement frequency). Similarly, pharmacological test conditions like infecting inoculum concentration, culture well plates specifications, duration of exposure to treatment, and method of parasite quantification must also be homogenous.

Quality assessment of in vitro antitrypanosomal screening studies involves experimental design bias (active and infection controls), duration of follow-up, measures to monitor assay performance, replicates necessary for adequate estimation of IC50, and adequate reporting. Harmonizing these conditions is crucial for improving the reliability and comparability of results across different studies, facilitating the reliable identification of potential drug candidates and supporting their further development. Moreover, it promotes the sharing of knowledge and data across the scientific community, fostering collaboration and accelerating drug discovery efforts.

Box 1 Recommended starting points for harmonizing experimental conditions in in vitro pharmacological models for assessing activity against t. cruzi epimastigotes 

Model of in vitro culture of epimastigote forms

Strains: Strain Y (TcII) is the most frequently used. Whenever possible include several strains, especially those belonging to the DTUs: TcI, TcII, TcV and TcVI, which are associated with human infection. Different T. cruzi strains show different susceptibility.

Culture medium: Liver infusion-tryptose culture medium (LIT) predominates.

Enrichment of Culture medium: Fetal bovine serum (FBS) at a concentration of 10 % is most common. FBS concentration may vary depending on the stage of the culture.

Incubation parameters:

• Culture medium replacement frequency: Around every 7 d (range 3-10 d).

• Incubation temperature at 28 °C.

Pharmacological test conditions

Infecting inoculum: Around I x 106 parasites/mL.

Culture well plates: 96-well plates are predominantly used.

Treatment exposure time: 72 h is most reported. On Benznidazole IC50 values generally decrease as incubation time increases but, stabilizing after 72 h.

Method of parasite quantification: Microscopy through the Neubauer chamber is the method traditionally used for this purpose, however, limited usefulness for large sample numbers. Alternative methods correspond to colorimetric, turbidimetric (referred to as absorbance) and fluorescence-based. In turbidity measurements it's essential to establish a standard curve relating turbidity to parasite density using a reference method, culture conditions and the presence of debris can affect readings and should be considered during quantification.

•Active control: The most frequently reported is Benznidazole 5.5 times more than nifurtimox. On Y (TcII) strain, at 72 h, Benznidazole shows IC50 of 21.8 +/-10.8 μM *

DTU: Discrete typing unit, h: Hours. * The results represent the mean ± SD of in vitro IC50, 7 Independent reports.

References

1. Pan American Health Organization. Neglected infectious diseases in the Americas: Success stories and innovation to reach the neediest; 2016. [Internet] [Consultado 11 de octubre de 2024] Available from: Available from: https://iris.paho.org/handle/10665.2/31250Links ]

2. Pan American Health Organization. Decálogo para la toma de decisiones sobre la prevención, el control y la atención de la enfermedad de chagas; 2022. [Internet] [Consultado 13 de marzo de 2025] Available from: Available from: https://www.paho.org/es/documentos/decalogo-para-toma-decisiones-sobre-prevencion-control-atencion-enferme-dad-chagasLinks ]

3. Bhattacharya A, Corbeil A, do Monte-Neto RL, Fernandez-Prada C. Of Drugs and Trypanosomatids: New Tools and Knowledge to Reduce Bottlenecks in Drug Discovery. Genes. 2020; 11(7): 722. doi: https://doi.org/10.3390/genes11070722Links ]

4. Santos SS, de Araújo RV Giarolla J, Seoud OE, Ferreira EI. Searching for drugs for Chagas disease, leishmaniasis and schistosomiasis: a review. Int J Antimicrob Agents. 2020; 55(4): 105906. doi: https://doi.org/10.1016/j.ijanti-micag.2020.105906Links ]

5. Lidani KCF, Andrade FA, Bavia L, Damasceno FS, Beltrame MH, Messias-Reason IJ, et al. Chagas Disease: From Discovery to a Worldwide Health Problem. Front Public Health. 2019; 7: 166. doi: https://doi.org/10.3389/fpubh.2019.00166Links ]

6. Scarim CB, Jornada DH, Chelucci RC, de Almeida L, dos Santos JL, Chung MC. Current advances in drug discovery for Chagas disease. Eur J Med Chem. 2018; 155: 824-38. doi: https://doi.org/10.1016/j.ejmech.2018.06.040Links ]

7. Fonseca-Berzal C, Arán VJ, Escario JA, Gómez-Barrio A. Experimental models in Chagas disease: a review of the methodologies applied for screening compounds against Trypanosoma cruzi. Parasitol Res. 2018; 117(11): 336780. doi: https://doi.org/10.1007/s00436-018-6084-3Links ]

8. Comisión Económica para América Latina y el Caribe (CEPAL). Panorama Social de América Latina y el Caribe; 2022. [Internet]. [Consultado 5 de junio de 2025] Available from: Available from: https://repositorio.cepal.org/bitstream/hand-le/11362/48518/1/S2200947_es.pdfLinks ]

9. Conners EE, Vinetz JM, Weeks JR, Brouwer KC. A global systematic review of Chagas disease prevalence among migrants. Acta Trop. 2016; 156: 68-78. doi: https://doi.org/10.1016/j.actatropica.2016.01.002Links ]

10. Belaunzarán ML. Enfermedad de Chagas: globalización y nuevas esperanzas para su cura. Rev Argent Microbiol. 2015; 47(2): 85-7. doi: https://doi.org/10.1016/j.ram.2015.04.001Links ]

11. De Rycker M, Wyllie S, Horn D, Read KD, Gilbert IH. Anti-trypanosomatid drug discovery: progress and challenges. Nat Rev Microbiol. 2023; 21(1): 35-50. doi: https://doi.org/10.1038/s41579-022-00777-yLinks ]

12. Zingales B, Miles MA, Campbell DA, Tibayrenc M, Macedo AM, Teixeira MMG, et al. The revised Trypanosoma cruzi subspecific nomenclature: Rationale, epidemiological relevance and research applications. Infect Genet Evol. 2012; 12(2): 240-53. doi: https://doi.org/10.1016/j.meegid.2011.12.009Links ]

13. Chatelain E. Chagas disease research and development: Is there light at the end of the tunnel? Comput Struct Biotechnol J. 2017; 15: 98-103. doi: https://doi.org/10.1016/j.csbj.2016.12.002Links ]

14. Tarleton RL. Chagas Disease: A Solvable Problem, Ignored. Trends Mol Med. 2016; 22(10): 835-8. doi: https://doi.org/10.1016/j.molmed.2016.07.008Links ]

15. Duran-Rehbein GA, Vargas-Zambrano JC, Cuéllar A, Puerta CJ, Gonzalez JM. Mammalian cellular culture models of Trypanosoma cruzi infection: a review of the published literature. Parasite. 2014; 21: 38. doi: https://doi.org/10.1051/parasite/2014040Links ]

16. Bern C. Chagas' Disease. Longo DL, editor. N Engl J Med. 2015; 373(5): 456-66. doi: https://doi.org/10.1056/NEJMra1410150Links ]

17. Steverding D. The history of Chagas disease. Parasit Vectors. 2014; 7(1): 317. doi: https://doi.org/10.1186/1756-3305-7-317Links ]

18. Vela A, Coral-Almeida M, Sereno D, Costales JA, Barnabé C, Brenière SF. In vitro susceptibility of Trypanosoma cruzi discrete typing units (DTUs) to benznidazole: A systematic review and meta-analysis. Gürtler RE, editor. PLoS Negl Trop Dis. 2021; 15(3): e0009269. doi: https://doi.org/10.1371/journal.pntd.0009269Links ]

19. Villarreal D, Barnabé C, Sereno D, Tibayrenc M. Lack of correlation between in vitro susceptibility to Benznidazole and phylogenetic diversity of Trypanosoma cruzi, the agent of Chagas disease. Exp Parasitol. 2004; 108(1-2): 24-31. doi: https://doi.org/10.1016/j.exppara.2004.07.001Links ]

20. Revollo S, Oury B, Vela A, Tibayrenc M, Sereno D. In Vitro Benznidazole and Nifurtimox Susceptibility Profile of Trypanosoma cruzi Strains Belonging to Discrete Typing Units TcI, TcII, and TcV Pathogens. 2019; 8(4): 197. doi: https://doi.org/10.3390/pathogens8040197Links ]

21. Messenger LA, Miles MA, Bern C. Between a bug and a hard place: Trypanosoma cruzi genetic diversity and the clinical outcomes of Chagas disease. Expert Rev Anti Infect Ther. 2015; 13(8): 995-1029. doi: https://doi.org/10.1586/14787210.2015.1056158Links ]

22. Romanha AJ, Castro SL de, Soeiro M de NC, Lannes-Vieira J, Ribeiro I, Talvani A, et al. In vitro and in vivo experimental models for drug screening and development for Chagas disease. Mem Inst Oswaldo Cruz. 2010; 105(2): 233-8. doi: https://doi.org/10.1590/S0074-02762010000200022Links ]

23. Molina I, Gómez I Prat J, Salvador F, Treviño B, Sulleiro E, Serre N, et al. Randomized Trial of Posaconazole and Benznidazole for Chronic Chagas' Disease. N Engl J Med. 2014; 370(20): 1899-908. doi: https://doi.org/10.1056/NEJMoa1313122Links ]

24. Bustamante JM, Tarleton RL. Methodological advances in drug discovery for Chagas disease. Expert Opin Drug Discov. 2011; 6(6): 653-61. doi: https://doi.org/10.1517/17460441.2011.573782Links ]

25. Page MJ, McKenzie JE, Bossuyt PM, Boutron I, Hoffmann TC, Mulrow CD, et al. The PRISMA 2020 statement: An updated guideline for reporting systematic reviews. PLOS Med. 2021; 18(3): e1003583. doi: https://doi.org/10.1371/journal.pmed.1003583Links ]

26. Siddaway AFP Wood AM, Hedges LV How to Do a Systematic Review: A Best Practice Guide for Conducting and Reporting Narrative Reviews, Meta-Analyses, and Meta-Syntheses. Annu Rev Psychol. 2019; 70(1): 747-70. doi: https://doi.org/10.1146/annurev-psych-010418-102803Links ]

27. Peters MDJ, Godfrey C, McInerney P Khalil H, Larsen P Marnie C, et al. Best practice guidance and reporting items for the development of scoping review protocols. JBI Evid Synth. 2022; 20(4): 953-68. doi: https://doi.org/10.11124/JBIES-21-00242Links ]

28. Haddaway NR, Page MJ, Pritchard CC, McGuinness LA. PRISMA 2020: An R package and Shiny app for producing PRISMA 2020-compliant flow diagrams, with interactivity for optimised digital transparency and Open Synthesis. Campbell Syst Rev. 2022; 18(2). doi: https://doi.org/10.1002/cl2.1230Links ]

29. Franco J, Ferreira RC, Ienne S, Zingales B. ABCG-like transporter of Trypanosoma cruzi involved in benznidazo-le resistance: Gene polymorphisms disclose inter-strain intragenic recombination in hybrid isolates. Infect Genet Evol. 2015; 31: 198-208. doi: https://doi.org/10.1016/j.meegid.2015.01.030Links ]

30. Zingales B, Araujo RGA, Moreno M, Franco J, Aguiar PHN, Nunes SL, et al. A novel ABCG-like transporter of Trypanosoma cruzi is involved in natural resistance to benznidazole. Mem Inst Oswaldo Cruz. 2015; 110(3): 43344. doi: https://doi.org/10.1590/0074-02760140407Links ]

31. Beer MF, Frank FM, Germán Elso O, Ernesto Bivona A, Cerny N, Giberti G, et al. Trypanocidal and leishmanici-dal activities of flavonoids isolated from Stevia satureiifolia var. satureiifolia. Pharm Biol. 2016; 54(10): 2188-95. doi: https://doi.org/10.3109/13880209.2016.1150304Links ]

32. Muscia GC, Roldán Pacheco FJ, Asís SE, Buldain GY, Frank FM. Hit-to-lead optimization of novel 2-alkyla-minomethylquinoline derivatives as anti-chagas agents. Eur J Med Chem. 2020; 186: 111877. doi: https://doi.org/10.1016/j.ejmech.2019.111877Links ]

33. Lourenço AM, Faccini CC, Costa CA de J, Mendes GB, Fragata Filho AA. Evaluation of in vitro anti-Trypanosoma cruzi activity of medications benznidazole, amiodarone hydrochloride, and their combination. Rev Soc Bras Med Trop. 2018;51(1):52-6. doi: https://doi.org/10.1590/0037-8682-0285-2017Links ]

34. Jassica Gonçalves Moreno C, Wysllas De Freitas Oliveira J, Castelo Branco J, Araújo L, Maria Queiroz A, Tavares Donato S, et al. Cell Culture and Maintenance of the Evolutionary Forms of Trypanosoma cruzi for Studies of Parasitic Biology. En: De Souza W, editor. Biology of Trypanosoma cruzi. IntechOpen; 2019 doi: https://doi.org/10.5772/intechopen.84733Links ]

35. Amato Neto V Origin of the «Y strain» of Trypanosoma cruzi. Rev Inst Med Trop São Paulo. 2010; 52(3): 171-171. doi: https://doi.org/10.1590/S0036-46652010000300012Links ]

36. Cortez C, Martins RM, Alves RM, Silva RC, Bilches LC, Macedo S, et al. Differential Infectivity by the Oral Route of Trypanosoma cruzi Lineages Derived from Y Strain. Traub-Csekö YM, editor. PLoS Negl Trop Dis. 2012; 6(10): e1804. doi: https://doi.org/10.1371/journal.pntd.0001804Links ]

37. Da Silva MJV, Jacomini AP, Gonçalves DS, Pianoski KE, Poletto J, Lazarin-Bidóia D, et al. Discovery of I,3,4,5-te-trasubstituted pyrazoles as anti-trypanosomatid agents: Identification of alterations in flagellar structure of L. amazonensis. Bioorganic Chem. 2021; 114: 105082. doi: https://doi.org/10.1016/j.bioorg.2021.105082Links ]

38. Gusmão AS, Abreu LS, Tavares JF, De Freitas HF, Silva Da Rocha Pita S, Dos Santos EG, et al. Computer-Guided Trypanocidal Activity of Natural Lactones Produced by Endophytic Fungus of Euphorbia umbellata. Chem Biodivers. 2021; 18(10): e2100493. doi: https://doi.org/10.1002/cbdv.202100493Links ]

39. Moreira FF, Portes JDA, Barros Azeredo NF, Fernandes C, Horn A, Santiago CP, et al. Development of new dinuclear Fe( iii ) coordination compounds with in vitro nanomolar antitrypanosomal activity. Dalton Trans. 2021; 50(35): 12242-64. doi: https://doi.org/10.1039/dIdt01048dLinks ]

40. Llanos MA, Sbaraglini ML, Villalba ML, Ruiz MD, Carrillo C, Alba Soto C, et al. A structure-based approach towards the identification of novel antichagasic compounds: Trypanosoma cruzi carbonic anhydrase inhibitors. J Enzyme Inhib Med Chem. 2020; 35(1): 21-30. doi: https://doi.org/10.1080/14756366.2019.1677638Links ]

41. Espinosa-Bustos C, Vázquez K, Varela J, Cerecetto H, Paulino M, Segura R, et al. New aryloxy-quinone derivatives with promising activity on Trypanosoma cruzi. Arch Pharm (Weinheim). 2020; 353(1): 1900213. doi: https://doi.org/10.1002/ardp.201900213Links ]

42. Salsi F, Bulhões Portapilla G, Simon S, Roca Jungfer M, Hagenbach A, De Albuquerque S, et al. Effect of Fluo-rination on the Structure and Anti- Trypanosoma cruzy Activity of Oxorhenium(V) Complexes with S, N, S-Tridentate Thiosemicarbazones and Benzoylthioureas. Synthesis and Structures of Technetium(V) Analogues. Inorg Chem. 2019; 58(15): 10129-38. doi: https://doi.org/10.1021/acs.inorgchem.9b01260Links ]

43. Fonseca-Berzal C, Ibáñez-Escribano A, Vela N, Cumella J, Nogal-Ruiz JJ, Escario JA, et al. Antichagasic, Leish-manicidal, and Trichomonacidal Activity of 2-Benzyl-5-nitroindazole-Derived Amines. ChemMedChem. 2018; 13(12): 1246-59. doi: https://doi.org/10.1002/cmdc.201800084Links ]

44. Lima DB, Mello CP Bandeira ICJ, Pessoa Bezerra De Menezes RRP Sampaio TL, Falcão CB, et al. The dinopone-ratoxin peptides from the giant ant Dinoponera quadriceps display in vitro antitrypanosomal activity. Biol Chem. 2018; 399(2): 187-96. doi: https://doi.org/10.1515/hsz-2017-0198Links ]

45. Cardoso MVDO, Siqueira LRPD, Silva EBD, Costa LB, Hernandes MZ, Rabello MM, et al. 2-Pyridyl thiazoles as novel anti-Trypanosoma cruzi agents: Structural design, synthesis and pharmacological evaluation. Eur J Med Chem. 2014; 86: 48-59. doi: https://doi.org/10.1016/j.ejmech.2014.08.012Links ]

46. Tapia RA, Salas CO, Vázquez K, Espinosa-Bustos C, Soto-Delgado J, Varela J, et al. Synthesis and biological characterization of new aryloxyindole-4,9-diones as potent trypanosomicidal agents. Bioorg Med Chem Lett. 2014; 24(16): 3919-22. doi: https://doi.org/10.1016/j.bmcl.2014.06.044Links ]

47. Velásquez AMA, Francisco AI, Kohatsu AAN, Silva FADJ, Rodrigues DF, Teixeira RGDS, et al. Synthesis and tri-panocidal activity of ferrocenyl and benzyl diamines against Trypanosoma brucei and Trypanosoma cruzi. Bioorg Med Chem Lett. 2014; 24(7): 1707-10. doi: https://doi.org/10.1016/j.bmcl.2014.02.046Links ]

48. Franklim T, Freire-de-Lima L, De Nazareth Sá Diniz J, Previato J, Castro R, Mendonça-Previato L, et al. Design, Synthesis and Trypanocidal Evaluation of Novel I,2,4-Triazoles-3-thiones Derived from Natural Piperine. Molecules. 2013; 18(6): 6366-82. doi: https://doi.org/10.3390/molecules18066366Links ]

49. Izumi E, Ueda-Nakamura T, Veiga-Júnior V, Nakamura C. Toxicity of Oleoresins from the Genus Co-paifera in Trypanosoma cruzi: A Comparative Study. Planta Med. 2013; 79(11): 952-8. doi: https://doi.org/10.1055/s-0032-1328712Links ]

50. Jorge SD, Palace-Berl F, Mesquita Pasqualoto KF, Ishii M, Ferreira AK, Berra CM, et al. Ligand-based design, synthesis, and experimental evaluation of novel benzofuroxan derivatives as anti-Trypanosoma cruzi agents. Eur J Med Chem. 2013; 64: 200-14. doi: https://doi.org/10.1016/j.ejmech.2013.03.053Links ]

51. Moreira RRD, Martins GZ, Magalhaes NO, Almeida AE, Pietro RCLR, Silva FAJ, et al. In vitro trypanocidal activity of solamargine and extracts from Solanum palinacanthum and Solanum lycocarpum of brazilian cerrado. An Acad Bras Ciênc. 2013; 85(3): 903-7. doi: https://doi.org/10.1590/S0001-37652013000300006Links ]

52. Carneiro PF, Do Nascimento SB, Pinto AVI Pinto MDCFR, Lechuga GC, Santos DO, et al. New oxirane derivatives of I,4-naphthoquinones and their evaluation against T. cruzi epimastigote forms. Bioorg Med Chem. 2012; 20(16): 4995-5000. doi: https://doi.org/10.1016/j.bmc.2012.06.027Links ]

53. Izumi E, Ueda-Nakamura T, Veiga VF, Pinto AC, Nakamura CV Terpenes from Copaifera Demonstrated in Vitro Antiparasitic and Synergic Activity. J Med Chem. 2012; 55(7): 2994-3001. doi: https://doi.org/10.1021/jm201451hLinks ]

54. Daliry A, Pires MQ, Silva CF, Pacheco RS, Munde M, Stephens CE, et al. The Trypanocidal Activity of Amidine Compounds Does Not Correlate with Their Binding Affinity to Trypanosoma cruzi Kinetoplast DNA. Antimicrob Agents Chemother. 2011; 55(10): 4765-73. doi: https://doi.org/10.1128/aac.00229-11Links ]

55. Alvarez G, Aguirre-López B, Varela J, Cabrera M, Merlino A, López GV et al. Massive screening yields novel and selective Trypanosoma cruzi triosephosphate isomerase dimer-interface-irreversible inhibitors with anti-trypa-nosomal activity. Eur J Med Chem. 2010; 45(12): 5767-72. doi: https://doi.org/10.1016/j.ejmech.2010.09.034Links ]

56. Veiga-Santos P, Pelizzaro-Rocha KJ, Santos AO, Ueda-Nakamura T, Filho BPD, Silva SO, et al. In vitro anti-trypanosomal activity of elatol isolated from red seaweed Laurencia dendroidea. Parasitology. 2010; 137(11): 1661-70. doi: https://doi.org/10.1017/S003118201000034XLinks ]

57. Dos Santos Filho JM, Leite ACL, Oliveira BGD, Moreira DRM, Lima MS, Soares MBP et al. Design, synthesis and cruzain docking of 3-(4-substituted-aryl)-I,2,4-oxadiazole-N-acylhydrazones as anti-Trypanosoma cruzi agents. Bioorg Med Chem. 2009; 17(18): 6682-91. doi: https://doi.org/10.1016/j.bmc.2009.07.068Links ]

58. Batista Jr. JM, Lopes AA, Ambrósio DL, Regasini LO, Kato MJ, Bolzani VDS, et al. Natural Chromenes and Chro-mene Derivatives as Potential Anti-trypanosomal Agents. Biol Pharm Bull. 2008; 31(3): 538-40. doi: https://doi.org/10.1248/bpb.31.538Links ]

59. Boiani L, Aguirre G, González M, Cerecetto H, Chidichimo A, Cazzulo JJ, et al. Furoxan-, alkylnitrate-derivatives and related compounds as anti-trypanosomatid agents: Mechanism of action studies. Bioorg Med Chem. 2008; 16(17): 7900-7. doi: https://doi.org/10.1016/j.bmc.2008.07.077Links ]

60. Freire-de-Lima L, Ribeiro TS, Rocha GM, Brandão BA, Romeiro A, Mendonça-Previato L, et al. The toxic effects of piperine against Trypanosoma cruzi: ultrastructural alterations and reversible blockage of cytokinesis in epi-mastigote forms. Parasitol Res. 2008; 102(5): 1059-67. doi: https://doi.org/10.1007/s00436-008-0876-9Links ]

61. Cockram PE, Turner CA, Slawin AMZ, Smith TK. Convenient Synthesis of Alternatively Bridged Tryptophan Keto-piperazines and Their Activities against Trypanosomatid Parasites. ChemMedChem. 2022; 17(4): e202100664. doi: https://doi.org/10.1002/cmdc.202100664Links ]

62. Scalese G, Machado I, Salinas G, Pérez-Díaz L, Gambino D. Heteroleptic Oxidovanadium(V) Complexes with Activity against Infective and Non-Infective Stages of Trypanosoma cruzi. Molecules. 2021; 26(17): 5375. doi: https://doi.org/10.3390/molecules26175375Links ]

63. Mosquillo MF, Bilbao L, Hernández F, Machado I, Gambino D, Garat B, et al. Effect of a new anti-T. cruzi metallic compound based on palladium. BioMetals. 2018; 31(6): 961-74. doi: https://doi.org/10.1007/s10534-018-0140-4Links ]

64. Scalese G, Machado I, Fontana C, Risi G, Salinas G, Pérez-Díaz L, et al. New heteroleptic oxidovanadium(V) complexes: synthesis, characterization and biological evaluation as potential agents against Trypanosoma cruzi. JBIC J Biol Inorg Chem. 2018; 23(8): 1265-81. doi: https://doi.org/10.1007/s00775-018-1613-1Links ]

65. Ghashghaei O, Kielland N, Revés M, Taylor M, Kelly J, Di Pietro O, et al. Tetrasubstituted Imidazolium Salts as Potent Antiparasitic Agents against African and American Trypanosomiases. Molecules. 2018; 23(1): 177. doi: https://doi.org/10.3390/molecules23010177Links ]

66. Santos KKA, Matias EFF, Sobral-Souza CE, Tintino SR, Morais-Braga MFB, Guedes GMM, et al. Trypanocide, cytotoxic, and antifungal activities of Momordica charantia. Pharm Biol. 2012; 50(2): 162-6. doi: https://doi.org/10.3109/13880209.2011.581672Links ]

67. Vega MC, Rolón M, Montero-Torres A, Fonseca-Berzal C, Escario JA, Gómez-Barrio A, et al. Synthesis, biological evaluation and chemometric analysis of indazole derivatives. I,2-Disubstituted 5-nitroindazolinones, new prototypes of antichagasic drug. Eur J Med Chem. 2012; 58: 214-27. doi: https://doi.org/10.1016/j.ejmech.2012.10.009Links ]

68. Fytas C, Zoidis G, Tzoutzas N, Taylor MC, Fytas G, Kelly JM. Novel Lipophilic Acetohydroxamic Acid Derivatives Based on Conformationally Constrained Spiro Carbocyclic 2,6-Diketopiperazine Scaffolds with Potent Trypanocidal Activity. J Med Chem. 2011; 54(14): 5250-4. doi: https://doi.org/10.1021/jm200217mLinks ]

69. Rodríguez J, Arán VJ, Boiani L, Olea-Azar C, Lavaggi ML, González M, et al. New potent 5-nitroindazole derivatives as inhibitors of Trypanosoma cruzi growth: Synthesis, biological evaluation, and mechanism of action studies. Bioorg Med Chem. 2009; 17(24): 8186-96. doi: https://doi.org/10.1016/j.bmc.2009.10.030Links ]

70. Cavazzuti A, Paglietti G, Hunter WN, Gamarro F, Piras S, Loriga M, et al. Discovery of potent pteridine reductase inhibitors to guide antiparasite drug development. Proc Natl Acad Sci. 2008; 105(5): 1448-53. doi: https://doi.org/10.1073/pnas.0704384105Links ]

71. Matiadis D, Saporiti T, Aguilera E, Robert X, Guillon C, Cabrera N, et al. Pyrazol(in)e Derivatives of Curcu-min Analogs As a New Class of Anti- Trypanosoma Cruzi Agents. Future Med Chem. 2021; 13(8): 701-14. doi: https://doi.org/10.4155/fmc-2020-0349Links ]

72. Paucar R, Martín-Escolano R, Moreno-Viguri E, Azqueta A, Cirauqui N, Marín C, et al. Rational modification of Mannich base-type derivatives as novel antichagasic compounds: Synthesis, in vitro and in vivo evaluation. Bioorg Med Chem. 2019; 27(17): 3902-17. doi: https://doi.org/10.1016/j.bmc.2019.07.029Links ]

73. Aguilera E, Perdomo C, Espindola A, Corvo I, Faral-Tello P Robello C, et al. A Nature-Inspired Design Yields a New Class of Steroids Against Trypanosomatids. Molecules. 2019; 24(20): 3800. doi: https://doi.org/10.3390/molecules24203800Links ]

74. Soares FGN, Göethel G, Kagami LP, Das Neves GM, Sauer E, Birriel E, et al. Novel coumarins active against Trypanosoma cruzi and toxicity assessment using the animal model Caenorhabditis elegans. BMC Pharmacol Toxicol. 2019; 20(SI): 76. doi: https://doi.org/10.1186/s40360-019-0357-zLinks ]

75. Martín-Escolano R, Moreno-Viguri E, Santivañez-Veliz M, Martin-Montes A, Medina-Carmona E, Paucar R, et al. Second Generation of Mannich Base-Type Derivatives with in Vivo Activity against Trypanosoma cruzi. J Med Chem. 2018; 61(13): 5643-63. doi: https://doi.org/10.1021/acs.jmedchem.8b00468Links ]

76. Moreno-Viguri E, Jiménez-Montes C, Martín-Escolano R, Santivañez-Veliz M, Martin-Montes A, Azqueta A, et al. In Vitro and in Vivo Anti- Trypanosoma cruzi Activity of New Arylamine Mannich Base-Type Derivatives. J Med Chem. 2016; 59(24): 10929-45. doi: https://doi.org/10.1021/acs.jmedchem.6b00784Links ]

77. López-Lira C, Tapia RA, Herrera A, Lapier M, Maya JD, Soto-Delgado J, et al. New benzimidazolequinones as trypanosomicidal agents. Bioorganic Chem. 2021; 111: 104823. doi: https://doi.org/10.1016/j.bioorg.2021.104823Links ]

78. Cardoso MVDO, Oliveira Filho GBD, Siqueira LRPD, Espíndola JWP Silva EBD, Mendes APDO, et al. 2-(phen-ylthio)ethylidene derivatives as anti-Trypanosoma cruzi compounds: Structural design, synthesis and antiparasitic activity. Eur J Med Chem. 2019; 180: 191-203. doi: https://doi.org/10.1016/j.ejmech.2019.07.018Links ]

79. Ceole LF, Gandhi H, Villamizar LH, Soares MJ, O'Sullivan TP. Synthesis of Novel Quinine Analogs and Evaluation of Their Effects on Trypanosoma Cruzi. Future Med Chem. 2018; 10(4): 391-408. doi: https://doi.org/10.4155/fmc-2017-0184Links ]

80. Moncada-Basualto M, Lapier M, Maya JD, Matsuhiro B, Olea-Azar C, Delogu GL, et al. Evaluation of Trypano-cidal and Antioxidant Activities of a Selected Series of 3-amidocoumarins. Med Chem. 2018; 14(6): 573-84. doi: https://doi.org/10.2174/1573406414666180419113437Links ]

81. Da Silva EB, Oliveira E Silva DA, Oliveira AR, Da Silva Mendes CH, Dos Santos TAR, Da Silva AC, et al. Desing and synthesis of potent anti-Trypanosoma cruzi agents new thiazoles derivatives which induce apoptotic parasite death. Eur J Med Chem. 2017; 130: 39-50. doi: https://doi.org/10.1016/j.ejmech.2017.02.026Links ]

82. Robledo-O'Ryan N, Matos MJ, Vazquez-Rodriguez S, Santana L, Uriarte E, Moncada-Basualto M, et al. Synthesis, antioxidant and antichagasic properties of a selected series of hydroxy-3-arylcoumarins. Bioorg Med Chem. 2017; 25(2): 621-32. doi: https://doi.org/10.1016/j.bmc.2016.11.033Links ]

83. Gomes PATDM, Oliveira AR, Cardoso MVDO, Santiago EDF, Barbosa MDO, De Siqueira LRP et al. Phthalimi-do-thiazoles as building blocks and their effects on the growth and morphology of Trypanosoma cruzi. Eur J Med Chem. 2016; 111: 46-57. doi: https://doi.org/10.1016/j.ejmech.2016.01.010Links ]

84. Espíndola JWP Cardoso MVDO, Filho GBDO, Oliveira E Silva DA, Moreira DRM, Bastos TM, et al. Synthesis and structure-activity relationship study of a new series of antiparasitic aryloxyl thiosemicarbazones inhibiting Trypanosoma cruzi cruzain. Eur J Med Chem. 2015; 101: 818-35. doi: https://doi.org/10.1016/j.ejmech.2015.06.048Links ]

85. Ramírez-Macías I, Marín C, Chahboun R, Messouri I, Olmo F, Rosales MJ, Gutierrez-Sánchez R, Alvarez-Man-zaneda E, Sánchez-Moreno M. In Vitro and In Vivo Studies of the Trypanocidal Activity of Four Terpenoid Derivatives against Trypanosoma cruzi. Am J Trop Med Hyg. 2012; 87(3): 481-8. doi: https://doi.org/10.4269/ajt-mh.2012.11-0471Links ]

86. Hamedt AL, Ortiz IC, García-Huertas PA, Sáenz J, Araujo ACD, De Mattos JCP, et al. Cytotoxic, mutagenic and genotoxic evaluation of crude extracts and fractions from Piper jericoense with trypanocidal action. Acta Trop. 2014; 131: 92-7. doi: https://doi.org/10.1016/j.actatropica.2013.12.008Links ]

87. Di Pietro O, Vicente-García E, Taylor MC, Berenguer D, Viayna E, Lanzoni A, et al. Multicomponent reaction-based synthesis and biological evaluation of tricyclic heterofused quinolines with multi-trypanosomatid activity. Eur J Med Chem. 2015; 105: 120-37. doi: https://doi.org/10.1016/j.ejmech.2015.10.007Links ]

88. Chacón-Vargas K, Nogueda-Torres B, Sánchez-Torres L, Suarez-Contreras E, Villalobos-Rocha J, Torres-Martinez Y, et al. Trypanocidal Activity of Quinoxaline I,4 Di-N-oxide Derivatives as Trypanothione Reductase Inhibitors. Molecules. 2017; 22(2): 220. doi: https://doi.org/10.3390/molecules22020220Links ]

89. Domínguez-Díaz LR, Eugenia Ochoa Ma, Soto-Castro D, Farfán N, Morales-Chamorro M, Yépez-Mulia L, et al. In vitro, ex vivo and in vivo short-term screening of DHEA nitrate derivatives activity over Trypanosoma cruzi Ninoa and TH strains from Oaxaca State, México. Bioorg Med Chem. 2021; 48: 116417. doi: https://doi.org/10.1016/j.bmc.2021.116417Links ]

90. Martín-Montes A, Kolodová K, Marín C, Rosales-Lombardo MJ, Sánchez-Moreno M, De Andrés-Gordo L, et al. In vitro Leishmanicidal and Trypanosomicidal Properties of Imidazole-Containing Azine and Benzoazine Derivatives. ChemMedChem. 2021; 16(23): 3600-14. doi: https://doi.org/10.1002/cmdc.202100413Links ]

91. Maldonado CR, Marín C, Olmo F, Huertas O, Quirós M, Sánchez-Moreno M, et al. In Vitro and in Vivo Trypa-nocidal Evaluation of Nickel Complexes with an Azapurine Derivative against Trypanosoma cruzi. J Med Chem. 2010; 53(19): 6964-72. doi: https://doi.org/10.1021/jm100581zLinks ]

92. Marín C, Ramírez-Macías I, López-Céspedes A, Olmo F, Villegas N, Díaz JG, et al. In Vitro and in Vivo Trypanoci-dal Activity of Flavonoids from Delphinium staphisagria against Chagas Disease. J Nat Prod. 2011; 74(4): 744-50. doi: https://doi.org/10.1021/np1008043Links ]

93. Jobe M, Anwuzia-Iwegbu C, Banful A, Bosier E, Iqbal M, Jones K, et al. Differential in vitro activity of the DNA topoisomerase inhibitor idarubicin against Trypanosoma rangeli and Trypanosoma cruzi. Mem Inst Oswaldo Cruz. 2012; 107(7): 946-50. doi: https://doi.org/10.1590/S0074-02762012000700018Links ]

94. Sülsen VP, Frank FM, Cazorla SI, Anesini CA, Malchiodi EL, Freixa B, et al. Trypanocidal and Leishmanicidal Activities of Sesquiterpene Lactones from Ambrosia tenuifolia Sprengel (Asteraceae). Antimicrob Agents Chemother. 2008; 52(7): 2415-9. doi: https://doi.org/10.1128/aac.01630-07Links ]

95. Suganuma K, Yamasaki S, Molefe NI, Musinguzi PS, Davaasuren B, Mossaad E, et al. The establishment of in vitro culture and drug screening systems for a newly isolated strain of Trypanosoma equiperdum. Int J Parasitol Drugs Drug Resist. 2017; 7(2): 200-5. doi: https://doi.org/10.1016/j.ijpddr.2017.04.002Links ]

96. Dias JCP Ramos AN, Gontijo ED, Luquetti A, Shikanai-Yasuda MA, Coura JR, et al. [Brazilian Consensus on Chagas Disease, 2015]. Epidemiol E Serv Saude Rev Sist Unico Saude Bras. 2016; 25(spe): 7-86. doi: https://doi.org/10.5123/S1679-49742016000500002Links ]

97. De Souza W, Barrias ES. May the epimastigote form of Trypanosoma cruzi be infective? Acta Trop. 2020; 212: 105688. doi: https://doi.org/10.1016/j.actatropica.2020.105688Links ]

98. Chatelain E, Ioset JR. Drug discovery and development for neglected diseases: the DNDi model. Drug Design, Development and Therapy. 2011; 5: 175-181. doi: https://doi.org/10.2147/DDDT.S16381Links ]

99. Arias MA, Rodríguez YV, Garavito G. Adaptación y optimización de un método de lectura por fluorometría en el modelo farmacológico in vitro de cultivo de Plasmodium falciparum. Rev Colomb Cienc Quím Farm. 2016; 45(1): 127-146. doi: https://doi.org/10.15446/rcciquifa.v45n1.58024Links ]

100. Arias MH, Deharo E, Valentin A, Garavito G. Adaptation and optimization of a fluorescence-based assay for in vivo antimalarial drug screening. Parasitol Res. 2017; 116: 1955-62. doi: https://doi.org/10.1007/s00436-017-5477-zLinks ]

Suggested citation: Arias MH, Pérez JT, Garavito G. Experimental conditions for assessing anti-Trypanosoma cruzi (epimastigotes) activity in vitro: A scoping review. Salud UIS. 2025; 57: e25v57r04. doi: https://doi.org/10.18273/saluduis.57.e:25v57r04

Contributions of Authors MHA: Data curation, Formal analysis, Validation, Writing-review & editing. JTP: Data curation, Writing-original draft. GG: Writing-review & editing, Validation, Supervision, Project administration, Conceptualization.

Ethical considerations This work is classified as non-risk research, as it uses techniques and methods of documentary research on reports of in vitro experimental pharmacology. The study followed standard guidelines for systematic review reporting to ensure result integrity and validity, avoid selection and extraction bias, and maintain transparency in data presentation. Potential limitations are discussed in this report.

Funding MH Arias gratefully acknowledges the Departamento Administrativo de Ciencia, Tecnología e Innovación (Colciencias) for providing a PhD scholarship (Convocatoria 647, Doctorados Nacionales 2014). This work was funded by the Universidad Nacional de Colombia through the Call for support for the development of doctoral theses of the School of Sciences at the Bogotá Campus 2020.

AI technology support The authors report they did not use AI, language modeling, machine learning or similar technologies to create or assist with the creation or editing of any of the contents of this document.

Received: May 16, 2025; Accepted: August 20, 2025

* pggaravitoc@unal.edu.co

Declaration of Conflicts of Interest

The authors report there are no competing interests to declare.

Creative Commons License This is an open-access article distributed under the terms of the Creative Commons Attribution License

 
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