Fast and cost-effective protocol to produce Paracoccidioides spp. antigens.

Biomedica

Programa de Pós-Graduação em Ciências, Coordenadoria de Controle de Doenças, Secretaria de Estado da Saúde de São Paulo, São Paulo, Brasil; Laboratório de Imunodiagnóstico das Micoses, Centro de Imunologia, Instituto Adolfo Lutz, São Universidade de São Paulo, São Paulo, Brasil.

Published: August 2023

AI Article Synopsis

  • Existing methods for producing Paracoccidioides spp. antigens face issues like lack of standardization and reproducibility, prompting a need for optimization.
  • The study involved culturing various Paracoccidioides species and testing their antigens for their effectiveness in diagnosing paracoccidioidomycosis.
  • The new protocol developed resulted in stable and reproducible genus-specific antigens that can contribute to earlier diagnosis of the disease in affected regions of Brazil and South America.

Article Abstract

Introduction: The existing methods for Paracoccidioides spp. antigen production are problematic in terms of standardization, specificity, stability, repeatability, and reproducibility.

Objective: To optimize the methodology for Paracoccidioides spp. antigen production and evaluate its applicability in paracoccidioidomycosis immunodiagnosis.

Materials And Methods: The antigens were obtained from Paracoccidioides lutzii isolates (01, 66, and 8334), Paracoccidioides brasiliensis sensu stricto (113), and Paracoccidioides restripiensis (B-339). These fungi were grown at 36 °C ± 1 °C, on modified Fava-Netto agar, according to Freitas et al. (2018). Paracoccidioides lutzii antigens were obtained after , 10, and 20 days of culture, whereas P. brasiliensis and P. restripiensis antigens were obtained after 10 days. Antigens were evaluated in natura, 10 and 20 times concentrated. Antigenic capacity was evaluated using a double immunodiffusion assay against serum samples from patients with paracoccidioidomycosis, histoplasmosis, and aspergillosis, and random blood donors.

Results: Cross-reactivity between Paracoccidioides spp. antigens was observed when P. brasiliensis, P. restrepiensis antigens, and P. lutzii antigens were evaluated with the polyclonal antibodies against P. lutzii and P. brasiliensis, respectively. No cross-reactivity was obtained for polyclonal antibodies against Histoplasma capsulatum, Aspergillus fumigatus, and random blood donors. The proposed protocol allowed stable, repeatable, and reproducible genus-specific antigen production at a low cost and in a short cultivation time.

Conclusion: The proposed protocol allowed us to obtain genus-specific antigens that can be developed and reproduced in all laboratories in Brazil and South America, where paracoccidioidomycosis is a neglected disease, contributing to an early diagnosis, especially in endemic regions, regardless of the species.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10594581PMC
http://dx.doi.org/10.7705/biomedica.6874DOI Listing

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