8 research outputs found

    An investigation of spatial strategy in observational drawing

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    Vertical T cell immunodominance and epitope entropy determine HIV-1 escape.

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    HIV-1 accumulates mutations in and around reactive epitopes to escape recognition and killing by CD8+ T cells. Measurements of HIV-1 time to escape should therefore provide information on which parameters are most important for T cell–mediated in vivo control of HIV-1. Primary HIV-1–specific T cell responses were fully mapped in 17 individuals, and the time to virus escape, which ranged from days to years, was measured for each epitope. While higher magnitude of an individual T cell response was associated with more rapid escape, the most significant T cell measure was its relative immunodominance measured in acute infection. This identified subject-level or “vertical” immunodominance as the primary determinant of in vivo CD8+ T cell pressure in HIV-1 infection. Conversely, escape was slowed significantly by lower population variability, or entropy, of the epitope targeted. Immunodominance and epitope entropy combined to explain half of all the variability in time to escape. These data explain how CD8+ T cells can exert significant and sustained HIV-1 pressure even when escape is very slow and that within an individual, the impacts of other T cell factors on HIV-1 escape should be considered in the context of immunodominance

    International Interlaboratory Digital PCR Study Demonstrating High Reproducibility for the Measurement of a Rare Sequence Variant

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    This study tested the claim that digital PCR (dPCR) can offer highly reproducible quantitative measurements in disparate laboratories. Twenty-one laboratories measured four blinded samples containing different quantities of a <i>KRAS</i> fragment encoding G12D, an important genetic marker for guiding therapy of certain cancers. This marker is challenging to quantify reproducibly using quantitative PCR (qPCR) or next generation sequencing (NGS) due to the presence of competing wild type sequences and the need for calibration. Using dPCR, 18 laboratories were able to quantify the G12D marker within 12% of each other in all samples. Three laboratories appeared to measure consistently outlying results; however, proper application of a follow-up analysis recommendation rectified their data. Our findings show that dPCR has demonstrable reproducibility across a large number of laboratories without calibration. This could enable the reproducible application of molecular stratification to guide therapy and, potentially, for molecular diagnostics

    Twentieth- and Twenty-First-Century Keats Criticism

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    This essay offers a survey of major twentieth- and twenty-first-century interpretations of Keats's life and work. Mapping lines of influence between distinctive formal, theoretical and historical approaches to Keats's oeuvre, I highlight significant critical trends and areas of recurrent formal and thematic interest in Keats studies. When appropriate, current confluences between these theoretical and historical methodologies are noted. Given the wide scope of material available, prominence has been given to those projects (where possible, emphasis is given to critical books) which both represent particular twentieth-century critical perspectives or thematic concerns and are important studies in themselves. This survey closes by indicating potential areas for future research and observes that many twentieth-century critical viewpoints and issues remain vital to Keats studies at the start of the twenty-first century

    Subretinal Hyperreflective Material in the Comparison of Age-Related Macular Degeneration Treatments Trials

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