In addition, the assays were run on frozen PBMC, which

In addition, the assays were run on frozen PBMC, which BI 2536 in vivo were dispatched by express delivery on dry ice. The analyses can therefore be performed at a laboratory that is located far from the site where the samples are taken. Also, cryopreservation of PBMC allows for a large timespan between taking of blood samples and execution of the laboratory measurements. This will enable careful planning and running of the analytical laboratory procedures at an appropriate time-point after completion of serial blood-sampling in clinical trials. Moreover, the reliability of the assays was demonstrated by the fact that the whole validation procedure was done at different laboratories in Europe and the North American

selleckchem continent. Furthermore, the assays allow detection of T cell responses against epitopes present on any influenza protein antigen in one single stimulation in vitro, as the cells are stimulated with whole virus. Since T cell responses have been reported for a wide range of influenza antigens such as internal proteins, structural, non-structural and membrane proteins, including neuraminidase and hemagglutinin, detection of cell-mediated immunity against any of these viral proteins is essential for evaluation of the complete T cell response against influenza. Finally, the inter-laboratory CV values of the granzyme B (CV 29%) and the cytokine

detection assay (CV 49%) make them fairly robust. Specifically, for a clinical trial comparing the efficacy of different vaccination regimens, we determined that to detect a difference of at least 25% (95% CI, power 0.8), 13 individuals per group are needed for analysis of granzyme B responses and 33 subjects per group are needed for analysis of cytokine responses. In comparison, the CV values for humoral assays are considerably higher, i.e. for the hemagglutination inhibition assay geometric coefficients of variation of at least 138% and for the virus neutralisation of at Edoxaban least 256% were reported [40] and [41]. Obviously CV values may be affected, when comparing results obtained with materials from different lots or from different

manufacturers [42]. Taken together, we have standardized and validated two assays based on detection of cellular immune responses against influenza. The validation results indicate that the assays can be evaluated as a correlate of protection or a co-correlate of protection besides other humoral assays [43]. Ultimately, these validated cellular assays may provide an essential and practical tool for evaluating efficacy in clinical studies with influenza vaccines. The authors would like to thank Lonneke Levels (Netherlands Vaccine Institute, Bilthoven, The Netherlands) for her advice in the development of the validation plan, and Yen Lemire (University of Connecticut Health Center, Farmington, CT, USA) for her help in setting up the granzyme B assay. Marina Eichelberger is thanked for critical reading of the manuscript.

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