Development, verification, and validation of an RT-qPCR-based protocol for Yellow Fever diagnosis

Rampazzo, Rita de Cássia Pontello; Zambenedetti, Miriam Ribas; Alexandrino, Fabiana; Jacomasso, Thiago; Tschá, Marcel Kruchelski; Fillipis, Ana Maria Bispo de; Morello, Luis Gustavo; Marchini, Fabrício Klerynton

doi:10.1016/j.ijid.2021.12.361

Cited by 5 publications

(2 citation statements)

References 22 publications

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“…There appears to be limitations in accessible, user-friendly internal controls tailored for MBD screening via RT-qPCR. Many approaches rely on spiking-based internal controls 15 , 16 which, while effective, increases complexity and elevated costs to high-throughput viral screening workflows. Our objective was to devise a dependable internal control that could integrate with multiplexed RT-qPCR assays through the straightforward addition of primers and a probe.…”

Section: Resultsmentioning

confidence: 99%

A cost-effective RNA extraction and RT-qPCR approach to detect California serogroup viruses from pooled mosquito samples

Avramov,

Gallo,

Gross

et al. 2024

Sci Rep

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Mosquito-borne diseases pose ongoing global health concerns, demanding more cost-efficient methods to detect pathogens to support enhanced surveillance efforts. This study introduces an adapted TRIzol-based high-throughput RNA extraction protocol, tailored for the detection of California serogroup viruses in pooled mosquito samples in a rapid and cost-effective manner. This approach provided consistent RNA yields and sensitive viral detection relative to two commercial extraction kits (QIAGEN RNeasy Mini Kit and MACHEREY–NAGEL NucleoSpin RNA Plus Kit). The incorporation of a user-friendly and non-spiking-based RT-qPCR internal control designed for the 18S rRNA gene in mosquitoes minimizes potential false positives/negatives, improving the fidelity of viral detection outcomes. Effective RNA yields, purity, and successful target amplification across 25 mosquito species and varied pool sizes (1–50 mosquitoes per tube) affirm the reliability of our approach. The extraction method is cost-effective, with an incurred cost of $0.58 CAD per sample, in contrast to the $5.25 CAD cost per sample of the two kits, rendering it promising for mosquito-borne disease surveillance initiatives.

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Section: Resultsmentioning

confidence: 99%

A cost-effective RNA extraction and RT-qPCR approach to detect California serogroup viruses from pooled mosquito samples

Avramov,

Gallo,

Gross

et al. 2024

Sci Rep

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show abstract

“…Molecular tests, particularly real-time polymerase chain reaction (qPCR), are sensitive and specific, contributing to the early identification of various pathologies (MADAMET et al, 2022; RAMPAZZO et al, 2022; YU et al, 2021). Although molecular detection tests are available, the diagnosis of leprosy continues to rely primarily on clinical diagnosis (WHO, 2022).…”

Section: Introductionmentioning

confidence: 99%

Validation of the performance of a point of care molecular test for leprosy: from a simplified DNA extraction protocol to a portable qPCR

Bertão-Santos,

Dias,

Ribeiro-Alves

et al. 2024

Preprint

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The study aimed to optimize qPCR reactions using oligonucleotides from the first Brazilian molecular diagnostic kit for leprosy on a portable platform (Q3-Plus). In addition, we sought to develop a simplified protocol for DNA extraction that met point-of-care criteria. During optimization on the Q3-Plus, optical parameters, thresholds, and cutoffs for the16S rRNAand RLEP targets ofM. lepraewere established using synthetic DNA, purified DNA fromM. leprae, and pre-characterized clinical samples. In the simplified extraction step, different lysis solutions were evaluated using chaotropic agents, and purification was carried out by depositing the lysed material on FTA cards. The complete protocol (simplified extraction + qPCR on the portable platform) was evaluated with pre-characterized clinical skin biopsy samples and compared with standard equipment (QuantStudio-5). LOD95%for the optimized reactions was 113.31 genome-equivalents/μL for16S rRNAand 17.70 genome-equivalents/μL for RLEP. Among the lysis solutions, the best-performing was composed of urea (2 M), which provided good dissolution of the skin fragment and a lower Ct value, indicating higher concentrations of DNA. The complete technological solution showed a sensitivity of 52% in reactions. Our results highlight the need for additional optimization to deal with paucibacillary samples, but also demonstrate the applicability of the portable platform in the detection ofM.leprae in low infrastructure settings.

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First DFT-supported point of care and novel electrochemical biosensing: Determination of yellow fever NS1 antibody in human plasma

Liv,

Özerdem

2024

International Journal of Biological Macromolecules

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Development, verification, and validation of an RT-qPCR-based protocol for Yellow Fever diagnosis

Cited by 5 publications

References 22 publications

A cost-effective RNA extraction and RT-qPCR approach to detect California serogroup viruses from pooled mosquito samples

A cost-effective RNA extraction and RT-qPCR approach to detect California serogroup viruses from pooled mosquito samples

Validation of the performance of a point of care molecular test for leprosy: from a simplified DNA extraction protocol to a portable qPCR

First DFT-supported point of care and novel electrochemical biosensing: Determination of yellow fever NS1 antibody in human plasma

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