Stive qualities and, consequently, incubation time, temperature, and concentration of enzymes have to be optimized with respect to cell viability, cell yield, and preservation of antigens that could be investigated by FCM. In the case of quite sensitive antigens, that are destroyed during tissue digestion, IL-25/IL-17E Proteins Purity & Documentation isolated cells might be cultured over night to permit re-expression of affected cell surface proteins. Principally, cells TRAIL Proteins Source obtained right after enzymatically tissue digestion are considerably more stressed than suspension cells and consequently, call for the identification of dead cells and their exclusion from the evaluation as described in Chapter III, Section 4: Dead cell exclusion, cell viability, and sample freezing. As described there, dead cells will raise background signals due toAuthor Manuscript Author Manuscript Author Manuscript Author ManuscriptEur J Immunol. Author manuscript; obtainable in PMC 2020 July 10.Cossarizza et al.Pagea general improve in autofluorescence or due to the improved unspecific binding of staining reagents. An incredibly detailed protocol to isolate thymic epithelial cells is given by Jain and Gray [304] and for human skin mast cells by Gr zkau et al. [305]. Furthermore, The tissue dissociation guide from Worthington summarizes all aspects of tissue dissociation inside a pretty extensive way (Worthington Biochemical Corporation Tissue Dissociation Guide [306]). Though flow cytometric analyses must ideally be performed with fresh samples, there are several possibilities to stabilize cells or blood samples before preparation for FCM (see also Chapter III, Section three: Preparation of single-cell suspensions; Section four: Dead cell exclusion, cell viability, and sample freezing; and Section five: Cell fixation and permeabilization for flow cytometry). Short-term preservation of blood for up to 24 h by Ficoll 70 kDa is mainly aiming at inhibiting blood settling-induced stress that is caused by RBC aggregation [307]. For long-term storage, the cryopreservation of PBMCs is a further solution. But it must to become kept in thoughts that some surface molecules, like CD62L or chemokine receptors in general, can be negatively affected by this process. Furthermore, some cell forms could possibly be far more sensitive to this type of remedy, which has to be determined individually for each cell population of interest. Also, there are many commercial reagents available, that can be made use of for long-term storage of blood samples, which include TransFix (CYTOMARK, Caltag Medsystems, Buckingham, UK), Cyto-Chex BCT (Streck, Omaha, US) and Intelligent Tube (Wise Tube, San Carlos, CA) [308]. The latter one particular even enables analyzing frozen blood samples immediately after suitable remedy without losing granulocytes.Author Manuscript Author Manuscript Author Manuscript Author ManuscriptBut for all these stabilizing protocols, it really is strongly recommended that they have completely been validated for the surface markers of interest. Live cells might be sensitive to prolonged in vitro handling procedures or may well actively internalize surface molecules or shed them from the surface, e.g., soon after labeling with Abs. This could be avoided by gentle therapy, e.g., cautious pipetting, short handling time, low temperature (on ice), or addition of sodium azide to the staining buffers, which blocks active shedding/internalization. Soon after staining, cells must be promptly analyzed or strictly be kept on ice and in the dark to prevent photobleaching. For the detection and analysis of cell subsets which might be det.
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