Reacción en cadena de la polimerasa en tiempo real para la cuantificación del ADN del virus de la hepatitis B

Rodríguez Lay, Licel de los Ángeles; Montalvo Villalba, María Caridad; Sariego Frómeta, Susel; Bello Corredor, Marité; Mora Laguna, Elin; Kourí Cardellá, Vivian; Martínez Rodríguez, Pedro Ariel; Sánchez Wong, Meilin; Marrero, Bárbara

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Revista Cubana de Medicina Tropical

versión impresa ISSN 0375-0760

Resumen

RODRIGUEZ LAY, Licel de los Ángeles et al. Real-time polymerase chain reaction assay for Hepatitis B virus DNA quantification. Rev Cubana Med Trop [online]. 2012, vol.64, n.3, pp. 290-303. ISSN 0375-0760.

Introduction: viral DNA levels in serum samples are a useful marker to monitor the disease progression and the treatment response in patients with chronic hepatitis B. Commercial kits for this purpose are available, but they are considerably expensive. Objectives: to evaluate the analytical performance of a real-time polymerase chain reaction (RT-PCR) assay for Hepatitis B virus DNA quantification. Methods: specific primers to the gene C and TaqMan chemistry in a LightCycler 1.5 equipment was used. A standard curve was made and evaluated. Two hundred and seventy-two serum samples were used to assess the clinical and analytical specificity, the genotypic accuracy and specificity, the intra-assay and interassay coefficients of variation and the comparison with a commercial assay and with the qualitative PCR. Results: the standard curve showed a strong linear correlation (r= -1) and low error values in the tested target DNA concentration. Analytical and clinical specificities were 100 %. Genotype accuracy and specificity showed that the differences between the results obtained by RT-PCR assay and those of the reference assay were less than 0.5 Log₁₀. The 95% HBV DNA detection end-point assessed by Probit analysis was 16.41 IU/µL with a dynamic range of quantification of 10⁸IU/mL. Intra-assay and interassay coefficients of variation ranged from 0.16 to 1.45 % and 0.9 to 2.62 % respectively. The RT-PCR assay correlated well with those from a commercial assay (r= 0.964 and r²= 0.929) and with the HBV qualitative PCR, thus confirming its better sensitivity and advantages. Conclusions: the RT-PCR assay is well suited to monitoring HBV DNA levels showing to be sensitive, specific and reproducible. Its application in the clinical practice ensures a better diagnosis and management of patients with chronic hepatitis B in Cuba.

Palabras clave : real-time polymerase chain reaction; hepatitis B; hepatitis B virus DNA quantification; standardization of diagnostic reagents.

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