Your search keyword '"M. Fernanda Sábato"' showing total 3 results

1. Comparison of Performance Characteristics of Three Real-Time Reverse Transcription-PCR Test Systems for Detection and Quantification of Hepatitis C Virus

Author

Andrea Ferreira-Gonzalez, Michael R. Langley, M. Fernanda Sábato, Mitchell L. Shiffman, and David S. Wilkinson

Subjects

Microbiology (medical), Reproducibility, genetic structures, Reverse Transcriptase Polymerase Chain Reaction, Hepatitis C virus, Sample processing, Reproducibility of Results, Hepacivirus, Viral Load, Biology, medicine.disease_cause, Hepatitis C, Sensitivity and Specificity, Virology, Reverse transcription polymerase chain reaction, Titer, Linear range, Cobas amplicor, medicine, Humans, RNA, Viral, Reagent Kits, Diagnostic, Viral load

Abstract

We evaluated the performance characteristics of three real-time reverse transcription-PCR test systems for detection and quantification of hepatitis C virus (HCV) and performed a direct comparison of the systems on the same clinical specimens. Commercial HCV panels (genotype 1b) were used to evaluate linear range, sensitivity, and precision. The Roche COBAS TaqMan HCV test for research use only (RUO) with samples processed on the MagNA Pure LC instrument (Roche RUO-MPLC) and Abbott analyte-specific reagents (ASR) with QIAGEN sample processing (Abbott ASR-Q) showed a sensitivity of 1.0 log 10 IU/ml with a linear dynamic range of 1.0 to 7.0 log 10 IU/ml. The Roche ASR in combination with the High Pure system (Roche ASR-HP) showed a sensitivity of 1.4 log 10 IU/ml with a linear dynamic range of 2.0 to 7.0 log 10 IU/ml. All of the systems showed acceptable reproducibility, the Abbott ASR-Q being the most reproducible of the three systems. Seventy-six clinical specimens (50 with detectable levels of HCV RNA and various titers and genotypes) were tested, and results were compared to those of the COBAS Amplicor HCV Monitor v2.0. Good correlation was obtained for the Roche RUO-MPLC and Abbott ASR-Q ( R 2 = 0.84 and R 2 = 0.93, respectively), with better agreement for the Abbott ASR-Q. However, correlation ( R 2 = 0.79) and agreement were poor for Roche ASR-HP, with bias relative to concentration and genotype. Roche ASR-HP underestimated HCV RNA for genotypes 3 and 4 as much as 2.19 log 10 IU/ml. Our study demonstrates that Roche RUO-MPLC and Abbott ASR-Q provided acceptable results and agreed sufficiently with the COBAS Amplicor HCV Monitor v2.0.

Published

2007

2. Laboratory testing of CYP2D6 alleles in relation to tamoxifen therapy

Author

Stuart A. Scott, Julie Gastier Foster, Kristen K. Reynolds, Patrik Vitazka, Victoria M. Pratt, M. Fernanda Sábato, Glenn E. Palomaki, and Elaine Lyon

Subjects

Drug, CYP2D6, Antineoplastic Agents, Hormonal, Genotyping Techniques, media_common.quotation_subject, CYP2D6 Gene, Breast Neoplasms, Bioinformatics, digestive system, Polymorphism, Single Nucleotide, Breast cancer, Gene Frequency, Medicine, Humans, Clinical significance, Tissue Distribution, Allele, skin and connective tissue diseases, Genetics (clinical), Alleles, media_common, Genetics, business.industry, Guideline, Sequence Analysis, DNA, medicine.disease, Tamoxifen, Cytochrome P-450 CYP2D6, Female, business, medicine.drug

Abstract

Tamoxifen, a widely prescribed drug for the treatment and prevention of breast cancer, is metabolized to more potent metabolites by the cytochrome P450 2D6 (CYP2D6) enzyme. Variants in the CYP2D6 gene can cause patients to be either intermediate or poor metabolizers, thereby rendering tamoxifen treatment less effective. Testing for CYP2D6 gene variants is available in Clinical Laboratory Improvement Amendments–certified clinical laboratories; however, the biological complexity of the variants makes result interpretation and phenotype prediction challenging. This article describes the clinical significance of variants as well as important analytical, interpretative, and reporting issues. It is designed to be a guideline for clinical laboratory professionals in performing tests and interpreting results with respect to CYP2D6 genetic variants. Genet Med 2012:14(12):990–1000

Published

2012

3. A simple and rapid genotyping assay for simultaneous detection of two ADRB2 allelic variants using fluorescence resonance energy transfer probes and melting curve analysis

Author

M. Fernanda Sábato, Anne-Marie Irani, David S. Wilkinson, Lawrence B. Schwartz, Bonny L. Bukaveckas, and Andrea Ferreira-Gonzalez

Subjects

Adult, Genotype, Biology, Nucleic Acid Denaturation, Melting curve analysis, Pathology and Forensic Medicine, Gene Frequency, Polymorphism (computer science), Fluorescence Resonance Energy Transfer, Humans, Allele, Child, Genotyping, Allele frequency, Alleles, Genetics, Polymorphism, Genetic, Hybridization probe, Haplotype, Reproducibility of Results, Molecular biology, Asthma, Black or African American, Molecular Medicine, Receptors, Adrenergic, beta-2, DNA Probes, Regular Articles

Abstract

Allelic variants at codons 16 and 27 of the beta(2)-adrenergic receptor gene (ADRB2) have shown clinical and pharmacological implications in asthma, hypertension, ischemic heart failure, diabetes, obesity, and cystic fibrosis. We have developed a simultaneous genotyping assay for the c.46AG and c.79CG allelic variants using hybridization probes and melting curve analysis. The assay was optimized on a panel of 30 DNA samples of known ADRB2 genotype as determined by sequencing with 100% concordance between the two techniques. Melting temperature (Tm) ranges for the different genotypes were obtained using data from three independent experiments. Single peaks for p.Arg16Arg (Tm = 57.76 degrees C +/- 0.10 degrees C) and p.Gly16Gly (Tm = 66.73 degrees C +/- 0.18 degrees C) and two melting peaks for p.Arg16Gly were obtained. Similarly, single peaks for p.Gln27Gln (Tm = 53.98 degrees C +/- 0.19 degrees C) and p.Glu27Glu (Tm = 64.93 degrees C +/- 0.16 degrees C) and two peaks for p.Gln27Glu were detected. Independent operators easily assigned genotypes in a sample set of 385 asthmatic patients. Haplotype and allele frequencies were in concordance with previously published data: Arg allele frequencies in children/adults were 0.34/0.30 in Caucasians and 0.45/0.52 in African Americans, and Gln allele frequencies were 0.58/0.52 in Caucasians and 0.82/0.84 in African Americans. Thus, the ADRB2 genotyping assay represents a highly reliable and rapid technique for routine clinical use in the simultaneous detection of ADRB2 variants.

Published

2008