After biotinylation, tetramers are formed by mixing the biotinyla

After biotinylation, tetramers are formed by mixing the biotinylated peptide–HLA complex with fluorophore-labelled avidin [22,46]. The traditional avidin-based tetramers have been superseded by complexes of five HLA/peptides, known as pentamers. HLA class II tetramers have been more

difficult to produce because the peptide complexes are less stable than HLA class I and interactions with the TCR are weaker than HLA class I/ CD8+ T cell interactions [46]. None the less, recombinant class II molecules that incorporate ‘leucine zipper’ motifs can be produced in stably transfected Drosophila cells and purified by affinity chromatography [50]. Because of the very low frequencies of CD4+ T cells specific for self-antigens, this assay often utilizes an in vitro amplification step BGJ398 concentration to increase the threshold of detection [51]. Loading tetramers with modified agonist peptides can increase the tetramer’s binding affinity and allow low-avidity T cell populations to be detected [52,53]. Parallel sorting of tetramer-positive cells, followed by RNA transcription profiling, enables extensive determination of NVP-BEZ235 their functional phenotypes [54]. The recently developed fluorescent quantum dots have been used to label HLA class I tetramers. Quantum dots have narrow emission spectra, making

them ideal for multiplexed tetramer staining [55]. Quantum dots may also prove useful for labelling HLA class II reagents. Advantages. Tetramers and pentamers are unique reagents

because they can identify antigen-specific T cells directly. This property makes them very useful for validating epitopes identified by other means. Ex-vivo tetramer staining (class I and class II) enables direct estimation of the frequency of antigen-specific T cells [56]. Disadvantages.  Class II tetramers are not suitable for use in routine clinical monitoring to detect biomarkers of disease. In vitro expansion of the antigen-specific T cells is required to increase their frequency to detectable levels and may lead to over- or under-estimation of the cell populations depending upon their capacity to proliferate in vitro. Furthermore, large pheromone volumes (∼50 ml) of blood are required to isolate the required numbers of PBMC. One possible limitation of both class I and class II tetramer assays is that low-affinity TCR-bearing cells may not be detected. Therefore, tetramer staining combined with proliferation and/or cytokine secretion assay may yield more information than either assay alone [57]. HLA-A*0201 pentamers (ProImmune, Oxford, UK) loaded with the autoantigenic epitopes of choice, positive control viral epitope(s) and negative control epitope. Cell sample, e.g. blood sample (RBC-depleted), PBMCs or T cell line. Pro5® recombinant MHC pentamer conjugated to the fluorescent label of choice (note: ensure that the stock pentamer is stored consistently at 4°C in the dark, with the lid tightly closed).

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