Literature DB >> 32414606

Tracking immunodynamics by identification of S-G2/M-phase T cells in human peripheral blood.

Miguel Muñoz-Ruiz1, Irma Pujol-Autonell2, Hefin Rhys3, Heather M Long4, Maria Greco5, Mark Peakman2, Tim Tree2, Adrian C Hayday6, Francesca Di Rosa7.   

Abstract

The ready availability of human blood makes it the first choice for immuno-monitoring. However, this has been largely confined to static metrics, particularly resting T cell phenotypes. Conversely, dynamic assessments have mostly relied on cell stimulation in vitro which is subject to multiple variables. Here, immunodynamic insights from the peripheral blood are shown to be obtainable by applying a revised approach to cell-cycle analysis. Specifically, refined flow cytometric protocols were employed, assuring the reliable quantification of T cells in the S-G2/M phases of the cell-cycle (collectively termed "T Double S" for T cells in S-phase in Sanguine: in short "TDS" cells). Without protocol refinement, TDS could be either missed, as most of them layed out of the conventional lymphocyte gates, or confused with cell doublets artefactually displaying high DNA-content. To illustrate the nature of TDS cells, and their relationship to different immunodynamic scenarios, we examined them in healthy donors (HD); infectious mononucleosis (IM) patients versus asymptomatic EBV+ carriers; and recently-diagnosed T1D patients. TDS were reproducibly more abundant among CD8+ T cells and a defined subset of T-regulatory CD4+ T cells, and were substantially increased in IM and a subset of T1D patients. Of note, islet antigen-reactive TDS cell frequencies were associated with an aggressive T cell effector phenotype, suggesting that peripheral blood can reflect immune events within tissues in T1D, and possibly in other organ-specific autoimmune diseases. Our results suggest that tracking TDS cells may provide a widely applicable means of gaining insight into ongoing immune response dynamics in a variety of settings, including tissue immunopathologies where the peripheral blood has often not been considered insightful.
Copyright © 2020. Published by Elsevier Ltd.

Entities:  

Keywords:  CD8 T cells; Immuno-monitoring; Type 1 diabetes

Year:  2020        PMID: 32414606      PMCID: PMC7527781          DOI: 10.1016/j.jaut.2020.102466

Source DB:  PubMed          Journal:  J Autoimmun        ISSN: 0896-8411            Impact factor:   7.094


  32 in total

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4.  Distribution and compartmentalization of human circulating and tissue-resident memory T cell subsets.

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Review 5.  CD8 T Cell Exhaustion in Chronic Infection and Cancer: Opportunities for Interventions.

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6.  Human memory T cells from the bone marrow are resting and maintain long-lasting systemic memory.

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7.  Primary Epstein-Barr virus infection does not erode preexisting CD8⁺ T cell memory in humans.

Authors:  Oludare A Odumade; Jennifer A Knight; David O Schmeling; David Masopust; Henry H Balfour; Kristin A Hogquist
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8.  Antibody stabilization of peptide-MHC multimers reveals functional T cells bearing extremely low-affinity TCRs.

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Journal:  J Immunol       Date:  2014-12-01       Impact factor: 5.422

9.  Resting T cells are hypersensitive to DNA damage due to defective DNA repair pathway.

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Authors:  Fan Zhao; Michael J Sikora; Naresha Saligrama; William S Serratelli; Ricardo A Fernandes; David M Louis; Winnie Yao; Xuhuai Ji; Juliana Idoyaga; Vinit B Mahajan; Lars M Steinmetz; Yueh-Hsiu Chien; Stephen L Hauser; Jorge R Oksenberg; K Christopher Garcia; Mark M Davis
Journal:  Nature       Date:  2019-08-07       Impact factor: 49.962

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2.  OMIP-079: Cell cycle of CD4+ and CD8+ naïve/memory T cell subsets, and of Treg cells from mouse spleen.

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