Parasite Detection in Visceral Leishmaniasis Samples by Dye-Based qPCR Using New Gene Targets of Leishmania infantum and Crithidia

Nayore Tamie Takamiya; Luana Aparecida Rogerio; Caroline Torres; João Augusto Franco Leonel; Geovanna Vioti; Tricia Maria Ferreira de Sousa Oliveira; Karoline Camila Valeriano; Gabriane Nascimento Porcino; Isabel Kinney Ferreira de Miranda Santos; Carlos H N Costa; Dorcas Lamounier Costa; Tauana Sousa Ferreira; Rodrigo Gurgel-Gonçalves; João Santana da Silva; Felipe Roberti Teixeira; Roque Pacheco De Almeida; José M C Ribeiro; Sandra Regina Maruyama

doi:10.3390/tropicalmed8080405

Parasite Detection in Visceral Leishmaniasis Samples by Dye-Based qPCR Using New Gene Targets of Leishmania infantum and Crithidia

Trop Med Infect Dis. 2023 Aug 8;8(8):405. doi: 10.3390/tropicalmed8080405.

Authors

Nayore Tamie Takamiya¹, Luana Aparecida Rogerio¹, Caroline Torres¹, João Augusto Franco Leonel², Geovanna Vioti², Tricia Maria Ferreira de Sousa Oliveira^{2

3}, Karoline Camila Valeriano⁴, Gabriane Nascimento Porcino⁴, Isabel Kinney Ferreira de Miranda Santos⁴, Carlos H N Costa⁵, Dorcas Lamounier Costa⁵, Tauana Sousa Ferreira⁶, Rodrigo Gurgel-Gonçalves⁶, João Santana da Silva⁷, Felipe Roberti Teixeira¹, Roque Pacheco De Almeida⁸, José M C Ribeiro⁹, Sandra Regina Maruyama¹

Affiliations

¹ Department of Genetics and Evolution, Center for Biological Sciences and Health, Federal University of São Carlos (UFSCar), São Carlos 13565-905, SP, Brazil.
² Post-Graduate Program in Experimental Epidemiology Applied to Zoonoses at the Faculty of Veterinary Medicine and Animal Science, University of São Paulo, São Paulo 05508-270, SP, Brazil.
³ Department of Veterinary Medicine, Faculty of Animal Science and Food Engineering, University of São Paulo, Pirassununga 13635-900, SP, Brazil.
⁴ Ribeirão Preto Medical School, University of São Paulo, FMRP-USP, Ribeirão Preto 14049-900, SP, Brazil.
⁵ Natan Portela Institute of Tropical Diseases, Teresina 64002-510, PI, Brazil.
⁶ Laboratory of Medical Parasitology and Vector Biology, Faculty of Medicine, University of Brasília, Brasília 70910-900, DF, Brazil.
⁷ Fiocruz-Bi-Institutional Translational Medicine Project, Oswaldo Cruz Foundation, Ribeirão Preto 14040-900, SP, Brazil.
⁸ Department of Medicine, Center for Biology and Health Sciences, Federal University of Sergipe (UFS), Aracaju 49060-108, SE, Brazil.
⁹ National Institute of Allergy and Infectious Diseases, National Institutes of Health, NIH/NIAID, Rockville, MD 20892, USA.

Abstract

Visceral leishmaniasis (VL) is a neglected disease considered a serious public health problem, especially in endemic countries. Several studies have discovered monoxenous trypanosomatids (Leptomonas and Crithidia) in patients with VL. In different situations of leishmaniasis, investigations have examined cases of co-infection between Leishmania spp. and Crithidia spp. These coinfections have been observed in a wide range of vertebrate hosts, indicating that they are not rare. Diagnostic techniques require improvements and more robust tools to accurately detect the causative agent of VL. This study aimed to develop a real-time quantitative dye-based PCR (qPCR) assay capable of distinguishing Leishmania infantum from Crithidia-related species and to estimate the parasite load in samples of VL from humans and animals. The primer LinJ31_2420 targets an exclusive phosphatase of L. infantum; the primer Catalase_LVH60-12060_1F targets the catalase gene of Crithidia. Therefore, primers were designed to detect L. infantum and Crithidia sp. LVH60A (a novel trypanosomatid isolated from VL patients in Brazil), in samples related to VL. These primers were considered species-specific, based on sequence analysis using genome data retrieved from the TriTryp database and the genome assembling of Crithidia sp. LVH60A strain, in addition to experimental and clinical data presented herein. This novel qPCR assay was highly accurate in identifying and quantifying L. infantum and Crithidia sp. LVH60A in samples obtained experimentally (in vitro and in vivo) or collected from hosts (humans, dogs, cats, and vectors). Importantly, the screening of 62 cultured isolates from VL patients using these primers surprisingly revealed that 51 parasite cultures were PCR+ for Crithidia sp. In addition, qPCR assays identified the co-infection of L. infantum with Crithidia sp. LVH60A in two new VL cases in Brazil, confirming the suspicion of co-infection in a previously reported case of fatal VL. We believe that the species-specific genes targeted in this study can be helpful for the molecular diagnosis of VL, as well as for elucidating suspected co-infections with monoxenous-like trypanosomatids, which is a neglected fact of a neglected disease.

Keywords: Crithidia sp. LVH60A; Leishmania infantum; molecular diagnosis; quantitative PCR (qPCR); trypanosomatid co-infection; visceral leishmaniasis.

Grants and funding

Z01 AI000810/ImNIH/Intramural NIH HHS/United States