Abstract
T cells from neonates (cord blood) with a tendency to develop allergic diseases express low PKCζ levels. More extensive investigations into PKC isozyme levels in T cell subsets and changes during neonatal T cell maturation are hampered by limitations of Western blot analyses. We have undertaken to validating the specificity of commercially available antibodies marketed for flow cytometry to measure PKCα, βI, βII, δ, ε, η, θ, ζ, ι/λ and μ. Western blot analyses of human peripheral blood mononuclear cell (PBMC) lysates demonstrated that some antibodies were unsuitable for flow cytometry assays. A panel of antibodies with the desirable specificity and reliability in the flow cytometry assay were identified using both PBMC and whole blood assays. The results showed that all PKC isozymes were expressed in CD4+ and CD8+ T cells, monocytes and neutrophils. Murine lymphocytes showed similar patterns of expression. A major finding was that 35.2% and 38.5% of cord blood samples have low PKCζ (≤the 5th percentile of adult levels) in the CD4+ and CD8+ subsets, respectively, consistent with the incidence of allergy development in the population. Furthermore, these low PKCζ levels ‘normalised’ within 24 h after initiation of maturation of these cells in culture, providing a ‘window of opportunity’ for altering PKCζ levels.
Highlights
Cell maturation are hampered by limitations of Western blot analyses
Protein kinase Cs (PKCs) isozyme antibodies for flow cytometry, we examined their specificities against their respective targets by Western blot using lysates from human peripheral blood mononuclear cell (PBMC)
Advancements can be made if levels of the PKC isozymes can be measured by flow cytometry, together with the characterization in T cell subsets and with assessing of cytokine production
Summary
Cell maturation are hampered by limitations of Western blot analyses. We have undertaken to validating the specificity of commercially available antibodies marketed for flow cytometry to measure PKCα, βI, βII, δ, ε, η, θ, ζ, ι/λ and μ. We demonstrate the need to ensure specificity of antibodies designed to be used for flow cytometry assays to measure intracellular levels of PKC isozymes. PKC isozyme antibodies for flow cytometry, we examined their specificities against their respective targets by Western blot using lysates from human PBMC.
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