Publications by authors named "B Sundararaman"

Article Synopsis
  • α/β T cells are essential for adaptive immunity, with their specificity determined by the unique sequences of their T cell receptor (TCR) chains.
  • Traditional bulk TCR sequencing is cost-effective but lacks paired chain data, while single-cell methods provide this data but are expensive and low-throughput.
  • The new method, TIRTL-seq, efficiently generates paired TCR libraries from live cells in under 7 hours, enabling extensive profiling of T cell responses with high scalability and reduced costs.
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Pathogenic bacteria, viruses, fungi, and protozoa can cause food and waterborne diseases. Surveillance methods must therefore screen for these pathogens at various stages of water distribution and of food from production to consumption. Detection using nucleic acid amplification methods offer rapid identification, but such methods have limited utility for characterizing populations, variant types or virulence traits of pathogens.

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Emerging infectious diseases require continuous pathogen monitoring. Rapid clinical diagnosis by nucleic acid amplification is limited to a small number of targets and may miss target detection due to new mutations in clinical isolates. Whole-genome sequencing (WGS) identifies genome-wide variations that may be used to determine a pathogen's drug resistance patterns and phylogenetically characterize isolates to track disease origin and transmission.

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Hybridization capture approaches allow targeted high-throughput sequencing analysis at reduced costs compared to shotgun sequencing. Hybridization capture is particularly useful in analyses of genomic data from ancient, environmental, and forensic samples, where target content is low, DNA is fragmented and multiplex PCR or other targeted approaches often fail. Here, we describe a DNA bait synthesis approach for hybridization capture that we call Circular Nucleic acid Enrichment Reagent, or CNER (pronounced 'snare').

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