Your search keyword '"Holland, Christopher J"' showing total 2 results

1. More tricks with tetramers:a practical guide to staining T cells with peptide-MHC multimers

Author

Dolton, Garry, Tungatt, Katie, Lloyd, Angharad, Bianchi, Valentina, Theaker, Sarah M, Trimby, Andrew, Holland, Christopher J, Donia, Marco, Godkin, Andrew J, Cole, David K, Straten, Per Thor, Peakman, Mark, Svane, Inge Marie, Sewell, Andrew K, Dolton, Garry, Tungatt, Katie, Lloyd, Angharad, Bianchi, Valentina, Theaker, Sarah M, Trimby, Andrew, Holland, Christopher J, Donia, Marco, Godkin, Andrew J, Cole, David K, Straten, Per Thor, Peakman, Mark, Svane, Inge Marie, and Sewell, Andrew K

Abstract

Analysis of antigen-specific T-cell populations by flow cytometry with peptide-MHC (pMHC) multimers is now commonplace. These reagents allow the tracking and phenotyping of T cells during infection, autoimmunity and cancer, and can be particularly revealing when used for monitoring therapeutic interventions. In 2009, we reviewed a number of 'tricks' that could be used to improve this powerful technology. More recent advances have demonstrated the potential benefits of using higher order multimers and of 'boosting' staining by inclusion of an antibody against the pMHC multimer. These developments now allow staining of T cells where the interaction between the pMHC and the T-cell receptor is over 20-fold weaker (K(D) > 1 mm) than could previously be achieved. Such improvements are particularly relevant when using pMHC multimers to stain anti-cancer or autoimmune T-cell populations, which tend to bear lower affinity T-cell receptors. Here, we update our previous work to include discussion of newer tricks that can produce substantially brighter staining even when using log-fold lower concentrations of pMHC multimer. We further provide a practical guide to using pMHC multimers that includes a description of several common pitfalls and how to circumvent them.

Published

2015

2. Antibody Stabilization of Peptide–MHC Multimers Reveals Functional T Cells Bearing Extremely Low-Affinity TCRs

Author

Tungatt, Katie, Bianchi, Valentina, Crowther, Michael D, Powell, Wendy E, Schauenburg, Andrea J, Trimby, Andrew, Donia, Marco, Miles, John J, Holland, Christopher J, Cole, David K, Godkin, Andrew J, Peakman, Mark, Straten, Per Thor, Svane, Inge Marie, Sewell, Andrew K, Dolton, Garry, Tungatt, Katie, Bianchi, Valentina, Crowther, Michael D, Powell, Wendy E, Schauenburg, Andrea J, Trimby, Andrew, Donia, Marco, Miles, John J, Holland, Christopher J, Cole, David K, Godkin, Andrew J, Peakman, Mark, Straten, Per Thor, Svane, Inge Marie, Sewell, Andrew K, and Dolton, Garry

Abstract

Fluorochrome-conjugated peptide-MHC (pMHC) multimers are commonly used in combination with flow cytometry for direct ex vivo visualization and characterization of Ag-specific T cells, but these reagents can fail to stain cells when TCR affinity and/or TCR cell-surface density are low. pMHC multimer staining of tumor-specific, autoimmune, or MHC class II-restricted T cells can be particularly challenging, as these T cells tend to express relatively low-affinity TCRs. In this study, we attempted to improve staining using anti-fluorochrome unconjugated primary Abs followed by secondary staining with anti-Ab fluorochrome-conjugated Abs to amplify fluorescence intensity. Unexpectedly, we found that the simple addition of an anti-fluorochrome unconjugated Ab during staining resulted in considerably improved fluorescence intensity with both pMHC tetramers and dextramers and with PE-, allophycocyanin-, or FITC-based reagents. Importantly, when combined with protein kinase inhibitor treatment, Ab stabilization allowed pMHC tetramer staining of T cells even when the cognate TCR-pMHC affinity was extremely low (KD >1 mM) and produced the best results that we have observed to date. We find that this inexpensive addition to pMHC multimer staining protocols also allows improved recovery of cells that have recently been exposed to Ag, improvements in the recovery of self-specific T cells from PBMCs or whole-blood samples, and the use of less reagent during staining. In summary, Ab stabilization of pMHC multimers during T cell staining extends the range of TCR affinities that can be detected, yields considerably enhanced staining intensities, and is compatible with using reduced amounts of these expensive reagents.

Published

2015