Your search keyword '"Dilernia D"' showing total 2 results

1. Centrifugation improves the detection of HIV-1 p24 antigen in plasma from children born to mothers infected with HIV-1.

Author

dos Ramos Farías MS, Garcia MN, Dilernia D, Rabinovich RD, and Avila MM

Subjects

Adult, Female, Humans, Infant, Infant, Newborn, Mothers, Sensitivity and Specificity, Young Adult, Centrifugation, HIV Core Protein p24 blood, HIV Infections diagnosis, HIV-1 isolation & purification, Infant, Newborn, Diseases virology, Plasma virology

Abstract

Detection of HIV proteins and/or nucleic acids is necessary for the diagnosis of perinatal HIV infection. Despite its low sensitivity, detection of p24 antigen in plasma is a simple and economic method for the diagnosis of HIV in exposed children. The aim of this study was to improve the sensitivity of detection of p24 using centrifugation of plasma. Forty-seven selected stored samples from 37 children (23 infected, 14 uninfected, median age of 137 days) were examined. Plasma samples (volume 0.3-1.5 ml) were defrosted, centrifuged at 23,500 x g at 4 degrees C for 60 min and determination of p24 was carried out in the resuspended pellet (0.12 ml). In 32 plasma samples from infected children, p24 was found originally in 6 (18.7%) and resulted positive in 24 (75%) pellets. When only one sample per child was considered, sensitivity was significantly higher in pellets, 3/23 uncentrifuged plasma samples and 15/23 pellets (McNemar Test, p<0.001). Specificity was 100%. The absorbance/cut-off ratio was always higher in the pellets from positive children (p=0.028). Plasma samples with volumes of 1 ml or more achieved a higher sensitivity (91.7% vs. 36.4%, p=0.009). Centrifugation of plasma samples prior to determination of p24 in pediatric patients resulted in a significant increase in sensitivity.

Published

2009

2. Examination of real-time PCR for HIV-1 RNA and DNA quantitation in patients infected with HIV-1 BF intersubtype recombinant variants.

Author

Schvachsa N, Turk G, Burgard M, Dilernia D, Carobene M, Pippo M, Gómez-Carrillo M, Rouzioux C, and Salomon H

Subjects

DNA, Viral analysis, Genetic Variation, HIV Infections virology, HIV Long Terminal Repeat genetics, HIV-1 classification, HIV-1 genetics, Humans, Nucleic Acid Amplification Techniques, Viral Load, HIV Infections diagnosis, HIV-1 isolation & purification, Polymerase Chain Reaction methods, RNA, Viral analysis, Recombination, Genetic

Abstract

The impact of HIV-1 genetic diversity on the performance of laboratory testing is an issue that has to be monitored continuously. An "in-house" real-time PCR assay was developed by the Agence Nationale de Recherche sur le SIDA (ANRS) in France for viral load (VL) quantitation based on the amplification of the HIV-1 long terminal repeat (LTR) region. This technology has not been used in Argentina yet and considering the HIV-1 diversity in the country, a comparative analysis of this assay was undertaken versus the Versant HIV-1 RNA 3.0 Assay (b-DNA). The performance was assessed on 30 drug-naïve HIV-1 infected patients who were characterized previously by phylogenetic analysis of the pol and vpu gene. The results showed that there is a significant linear correlation between values of transformed viral load logarithms measured by both, bDNA and real-time PCR assay and that this assay can be used to quantify viral load in samples from BF-infected patients with the same accuracy and reliability as for B subtype samples. The use of "in-house" real-time PCR to measure DNA in PBMCs correlated strongly with the HIV-1 RNA levels in all specimens.

Published

2007