Publications by authors named "Casey J A Anttila"

Article Synopsis
  • Interleukin-22 (IL-22) production by intestinal group 3 innate lymphoid cells (ILC3) is crucial for gut health, but both low and high levels can cause issues like barrier defects or tumors.
  • Researchers used single-cell RNA sequencing to discover key genes linked to increased IL-22 production, with a focus on programmed cell death 1 (PD-1), which is vital for ILC3's ability to generate IL-22 efficiently.
  • The study found that PD-1 expression on ILC3 is influenced by factors like microbiota and inflammation, and its absence can lead to diminished IL-22 production, compromised gut barrier integrity, and increased vulnerability to colitis in mice.
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Single-cell RNA sequencing (scRNA-Seq) has emerged as a powerful tool for understanding cellular heterogeneity and function. However the choice of sample multiplexing reagents can impact data quality and experimental outcomes. In this study, we compared various multiplexing reagents, including MULTI-Seq, Hashtag antibody, and CellPlex, across diverse sample types such as human peripheral blood mononuclear cells (PBMCs), mouse embryonic brain and patient-derived xenografts (PDXs).

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Inheritance of a BRCA2 pathogenic variant conveys a substantial life-time risk of breast cancer. Identification of the cell(s)-of-origin of BRCA2-mutant breast cancer and targetable perturbations that contribute to transformation remains an unmet need for these individuals who frequently undergo prophylactic mastectomy. Using preneoplastic specimens from age-matched, premenopausal females, here we show broad dysregulation across the luminal compartment in BRCA2 tissue, including expansion of aberrant ERBB3 luminal progenitor and mature cells, and the presence of atypical oestrogen receptor (ER)-positive lesions.

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A modified Chromium 10x droplet-based protocol that subsamples cells for both short-read and long-read (nanopore) sequencing together with a new computational pipeline (FLAMES) is developed to enable isoform discovery, splicing analysis, and mutation detection in single cells. We identify thousands of unannotated isoforms and find conserved functional modules that are enriched for alternative transcript usage in different cell types and species, including ribosome biogenesis and mRNA splicing. Analysis at the transcript level allows data integration with scATAC-seq on individual promoters, improved correlation with protein expression data, and linked mutations known to confer drug resistance to transcriptome heterogeneity.

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