Your search keyword '"Philippa Musoke"' showing total 6 results

1. Analysis of HIV Diversity Using a High-Resolution Melting Assay.

Author

William I. Towler, Maria M. James, Stuart C. Ray, Lei Wang, Deborah Donnell, Anthony Mwatha, Laura Guay, Clemensia Nakabiito, Philippa Musoke, J. Brooks Jackson, and Susan Eshleman

Abstract

AbstractHIV viruses are usually genetically homogeneous shortly after infection, and become more heterogeneous over time. We developed a high-resolution melting (HRM) assay to analyze HIV diversity without sequencing. Plasma samples from the HIVNET 012 trial were obtained from nine Ugandan mother–infant pairs. DNA amplified from the HIV gagregion was analyzed to determine the number of degrees over which the DNA melted (HRM score). HRM gag DNA was also cloned and sequenced (50 clones/mother; 20 clones/infant). The median HRM score for infants (4.3, range 4.2–5.3) was higher than that for control plasmids (3.4, range 3.2–3.8, p< 0.001) and lower than that for mothers (5.7, range 4.4–7.7, p= 0.005, exact Wilcoxon rank sum test). The intraclass correlation coefficient reflecting assay reproducibility was 94% (95% CI: 89–98%). HRM scores were also compared to sequenced-based measures of HIV diversity; higher HRM scores were associated with higher genetic diversity (p< 0.001), complexity (p= 0.009), and Shannon entropy (p= 0.022), but not with length variation (p= 0.111). The HRM assay provides a novel, rapid method for assessing HIV diversity without sequencing. This assay could be applied to any region of the HIV genome or to other genetic systems that exhibit DNA diversity. [ABSTRACT FROM AUTHOR]

Published

2010

2. Analysis of Drug Resistance in Children Receiving Antiretroviral Therapy for Treatment of HIV-1 Infection in Uganda.

Author

William I. Towler, Linda Barlow-Mosha, Jessica D. Church, Danstan Bagenda, Patrick Ajuna, Micheal Mubiru, Philippa Musoke, and Susan H. Eshleman

Abstract

AbstractWe analyzed drug resistance in HIV-infected Ugandan children who received antiretroviral therapy in a prospective, observational study (2004–2006); some children had prior single-dose nevirapine (sdNVP) exposure. Children received stavudine (d4T), lamivudine (3TC), and nevirapine (NVP); treatment was continued if they were clinically and immunologically stable. Samples with >1,000 copies/ml HIV RNA were analyzed by using the ViroSeq HIV Genotyping System (ViroSeq). Subtype A and D pretreatment samples also were analyzed with the LigAmp assay (for K103N, Y181C, and G190A). ViroSeq results were obtained for 74 pretreatment samples (35 from sdNVP-exposed children (median age, 19 months) and 39 from sdNVP-unexposed children (median age, 84 months). This included 39 subtype A, 22 subtype D, 1 subtype C, and 12 inter-subtype recombinant samples. One sample had nonnucleoside reverse transcriptase inhibitor (NNRTI) resistance, one had nucleoside reverse transcriptase inhibitor (NRTI) resistance, and three had protease inhibitor (PI) resistance. Y181C was detected by using LigAmp in five pretreatment samples [four (14.8%) of 37 samples from sdNVP-exposed children, one (4.2%) of 24 samples from children without prior sdNVP exposure; p= 0.35]. Among children who were not virally suppressed at 48 weeks of treatment, all 12 tested had NNRTI resistance, as well as resistance to 3TC and emtricitibine (FTC); three had resistance to other NRTIs. Seven of those children had a ViroSeq result at 96 weeks of treatment; four of the seven acquired resistance to additional NRTIs by 96 weeks. In Uganda, clinically and immunologically stable children receiving nonsuppressive antiretroviral treatment regimens are at risk for development of drug resistance. [ABSTRACT FROM AUTHOR]

Published

2010

3. Comparison of Laboratory Methods for Analysis of Non-nucleoside Reverse Transcriptase Inhibitor Resistance in Ugandan Infants.

Author

Jessica D. Church, Wei Huang, Neil Parkin, Natalia Marlowe, Laura A. Guay, Saad B. Omer, Philippa Musoke, J. Brooks Jackson, and Susan H. Eshleman

Abstract

AbstractDetailed comparisons of HIV drug resistance assays are needed to identify the most useful assays for research studies, and to facilitate comparison of results from studies that use different methods. We analyzed nonnucleoside reverse transcriptase inhibitor (NNRTI) resistance in 40 HIV-infected Ugandan infants who had received nevirapine (NVP)-based prophylaxis using the following assays: an FDA-cleared HIV genotyping assay (the ViroSeq HIV-1 Genotyping System v2.0), a commercially available HIV genotyping assay (GeneSeq HIV), a commercially available HIV phenotyping assay (PhenoSense HIV), and a sensitive point mutation assay (LigAmp). ViroSeq and GeneSeq HIV results (NVP resistance yes/no) were similar for 38 (95%) of 40 samples. In 6 (15%) of 40 samples, GeneSeq HIV detected mutations in minor subpopulations that were not detected by ViroSeq, which identified two additional infants with NVP resistance. LigAmp detected low-level mutations in 12 samples that were not detected by ViroSeq; however, LigAmp testing identified only one additional infant with NVP resistance. GeneSeq HIV and PhenoSense HIV determinations of susceptibility differed for specific NNRTIs in 12 (31%) of the 39 samples containing mixtures at relevant mutation positions. PhenoSense HIV did not detect any infants with NVP resistance who were not identified with GeneSeq HIV testing. In this setting, population sequencing-based methods (ViroSeq and GeneSeq HIV) were the most informative and had concordant results for 95% of the samples. LigAmp was useful for the detection and quantification of minority variants. PhenoSense HIV provided a direct and quantitative measure of NNRTI susceptibility. [ABSTRACT FROM AUTHOR]

Published

2009

4. In UteroHIV Infection Is Associated with an Increased Risk of Nevirapine Resistance in Ugandan Infants Who Were Exposed to Perinatal Single Dose Nevirapine.

Author

Jessica D. Church, Anthony Mwatha, Danstan Bagenda, Saad B. Omer, Deborah Donnell, Philippa Musoke, Clemensia Nakabiito, Chineta Eure, Paul Bakaki, Flavia Matovu, Michael C. Thigpen, Laura A. Guay, Michelle McConnell, Mary Glenn Fowler, J. Brooks Jackson, and Susan H. Eshleman

Abstract

AbstractUse of single dose nevirapine (sdNVP) to prevent HIV mother-to-child transmission is associated with the emergence of NVP resistance in many infants who are HIV infected despite prophylaxis. We combined results from four clinical trials to analyze predictors of NVP resistance in sdNVP-exposed Ugandan infants. Samples were tested with the ViroSeq HIV Genotyping System and a sensitive point mutation assay (LigAmp, for detection of K103N, Y181C, and G190A). NVP resistance was detected at 6–8 weeks in 36 (45.0%) of 80 infants using ViroSeq and 33 (45.8%) of 72 infants using LigAmp. NVP resistance was more frequent among infants who were infected in uterothan among infants who were diagnosed with HIV infection after birth by 6–8 weeks of age. Detection of NVP resistance at 6–8 weeks was not associated with HIV subtype (A vs. D), pre-NVP maternal viral load or CD4 cell count, infant viral load at 6–8 weeks, or infant sex. NVP resistance was still detected in some infants 6–12 months after sdNVP exposure. In this study, in uteroHIV infection was the only factor associated with detection of NVP resistance in infants 6–8 weeks after sdNVP exposure. [ABSTRACT FROM AUTHOR]

Published

2009

5. Short CommunicationHIV Type 1 Variants with Nevirapine Resistance Mutations Are Rarely Detected in Antiretroviral Drug-Naive African Women with Subtypes A, C, and D.

Author

Jessica D. Church, Sarah E. Hudelson, Laura A. Guay, Shu Chen, Donald R. Hoover, Neil Parkin, Susan A. Fiscus, Francis Mmiro, Philippa Musoke, Newton Kumwenda, J. Brooks Jackson, Taha E. Taha, and Susan H. Eshleman

Abstract

K103N is frequently detected in HIV-infected women after single dose (SD) nevirapine (NVP). K103N-containing variants were detected more frequently by the ViroSeq HIV-1 Genotyping System in women with subtype C (69.2) than subtypes A (19.4, p< 0.0001) or D (36.1, p< 0.0001). K103N-containing variants were also detected more frequently and at higher levels in women with subtype C by the LigAmp assay. In this report, we analyzed samples collected prior to or within hours after SD NVP administration from antiretroviral drug-naive African women with subtypes A, C, and D. Only 1254 samples had an NVP resistance mutation detected with the ViroSeq system, and only 4236 samples had K103N detected at < 0.5 with the LigAmp assay [2110 (1.8) with subtype A, 146 (2.2) with subtype C, and 180 (1.3) with subtype D] (p 0.92). We did not detect significant differences in the pre-NVP frequency of NVP resistance mutations or the pre-NVP levels of K103N-containing variants in women with subtypes A, C, and D that explain the dramatic subtype-based differences in emergence of HIV-1 variants with these mutations after SD NVP exposure. [ABSTRACT FROM AUTHOR]

Published

2007

6. Genetic Linkage of Nevirapine Resistance Mutations in HIV Type 1 Seven Days after Single-Dose Nevirapine.

Author

Dana Jones, Neil Parkin, Sarah E. Hudelson, Laura A. Guay, Philippa Musoke, Francis Mmiro, J. Brooks Jackson, and Susan H. Eshleman

Published

2005