Flow cytometric lymphocyte subset enumeration: 10 years of external quality assessment in the Benelux countries

Levering, Wilfried H.B.M.; Wieringen, Wessel N. van; Kraan, Jaco; Beers, Wil A.M. van; Sintnicolaas, K.; Rhenen, D.J. van; Gratama, Jan W.

doi:10.1002/cyto.b.20370

Cited by 28 publications

(32 citation statements)

References 49 publications

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“…Data collected in the present study indicate that CVs of the improved flow cytometry procedure fall well within the range of CV values observed in large international quality assay exercises for the enumeration of other rare circulating cell populations such as CD34 + hematopoietic progenitors or some lymphocyte subsets (21,22). Although CEC/CEP enumeration in fresh samples has the advantage of allowing an absolute cell count (in frozen samples, after mononuclear cell purification, the absolute cell count is calculated based on a complete blood cell count obtained at the same time of blood collection; see ref.…”

Section: Discussionsupporting

confidence: 75%

Validation of a Standardized Method for Enumerating Circulating Endothelial Cells and Progenitors: Flow Cytometry and Molecular and Ultrastructural Analyses

Mancuso

Antoniotti

Quarna

et al. 2008

Clinical Cancer Research

150

140

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Purpose: Antigenic overlap among circulating endothelial cells (CEC) and progenitors (CEP), platelets, and other blood cells led to the need to develop a reliable standardized method for CEC and CEP quantification. These cells are emerging as promising preclinical/clinical tools to define optimal biological doses of antiangiogenic therapies and to help stratify patients in clinical trials. Experimental Design: We report the experimental validation of a novel flow cytometry method that precisely dissects CEC/CEP from platelets and other cell populations and provides information about CEC/CEP viability.+ CECs, investigated by electron microscopy, were found to be bona fide endothelial cells by the presence of Weibel-Palade bodies. More than 75% of the circulating mRNAs of the endothelial-specific gene,VE-cadherin, found in the blood were present in the sorted population. CECs were 140 F 171/mL in healthy subjects (n = 37) and 951 F1,876/mL in cancer patients (n = 78; P < 0.0001). The fraction of apoptotic/necrotic CECs was 77 F 14% in healthy subjects and 43 F 23% in cancer patients (P < 0.0001). CEPs were 181 F 167/mL in healthy donors and 429 F 507/mL in patients (P = 0.00019). Coefficients of variation were 4 F 4% (intrareader), 17 F 4% (interreader), and 17 F 7% (variability over 0-72 h), respectively. Parallel samples were frozen by a standardized protocol. After thawing, coefficients of variation were 12 F 8% (intrareader), 16 F 10% (interreader), and 26 F 16% (variability over 0-14 days of frozen storage), respectively. Conclusions: This procedure enumerates a truly endothelial cell population with limited intrareader and interreader variability. It appears possible to freeze samples for large-scale CEC enumeration during clinical trials.This approach could be enlarged to investigate other angiogenic cell populations as well.

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Section: Discussionsupporting

confidence: 75%

Validation of a Standardized Method for Enumerating Circulating Endothelial Cells and Progenitors: Flow Cytometry and Molecular and Ultrastructural Analyses

Mancuso

Antoniotti

Quarna

et al. 2008

Clinical Cancer Research

150

140

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“…In the case of small populations, which are given similar weight in standardized lymphocyte fractions, small variations in staining intensity can lead to large VARIABILITY AND CLUSTERING OF LYMPHOCYTE SUBSETS relative changes. Others have also found that variability was proportionally greater for measurements of numerically smaller subsets of lymphocytes (5,6,10,12). In the case of absolute cell counts, additional sources of variation including analytical (e.g., the complete blood count (13), and the use of a dual platform method, as discussed above) and biological [e.g., diurnal shifts (14)], contribute to increased inter-and intraindividual variability.…”

Section: Discussionmentioning

confidence: 99%

Circulating lymphocyte subsets in normal adults are variable and can be clustered into subgroups

Sekiguchi

Smith

Sutter

et al. 2011

Cytometry Part B Clinical

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Background: Flow cytometry is used to monitor lymphocyte subsets in both the clinical and research settings. An understanding of the degree of inter-and intrasubject variability of these populations is critical for data interpretation.Methods: Peripheral blood lymphocytes of 18 healthy adults were analyzed on two separate occasions using a multicolor flow cytometric panel with B, T, and NK cell markers. Variability was calculated using the coefficient of variation and compared between and within individuals using agglomerative clustering.Results: Each subject appears to have B and T cell subset profiles that are stable over the two time points, but differ from the profiles of other subjects. Thus, the range of measurements for a particular B or T cell subset is larger between subjects and narrower for an individual. In addition, the level of variability correlates inversely with the size of the lymphocyte subset. When lymphocyte profiles are analyzed by agglomerative clustering, replicate samples from the same individual tend to cluster. When single samples from different individuals are analyzed, individuals appear to cluster into different subgroups.Conclusions: Variability of lymphocyte subsets is usually greater between individuals than within a single individual and each person appears to have a characteristic profile of lymphocyte subsets. These results underscore the importance of obtaining a baseline value for each subject when investigating the impact of a treatment on lymphocyte subsets over time. These results also highlight the potential utility of cluster analysis as a tool for immune subset profiling and biomarker discovery.

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“…In a study of lymphocyte subset enumeration, the results indicated no significant difference between "lyse no wash" and a few observations using "no lyse no wash" methods from those obtained using "lyse and wash" methods (38). Some consider, no lyse-no wash methods better suited for absolute counting, for example enumeration of CD341 cells or CD41 T-cells (39,40).…”

Section: Surface and Intracellular Staining: Lysis And Permeabilizatimentioning

confidence: 97%

“…Simple serial dilution antibody titrations against both positive and negative cellular targets are invaluable for antibody concentration optimization. It is preferable to perform antibody titrations against multiple sample sources that cover the expected range of population percentages and antigen expression as will be observed in the sample population (38). Use of cell lines is only acceptable for the evaluation of antibodies not expressed in healthy samples and to evaluate antibody performance at extreme limits of expected ranges.…”

Section: Antibody and Fluorochrome Conjugate Optimizationmentioning

confidence: 99%

Validation of cell‐based fluorescence assays: Practice guidelines from the ICSH and ICCS – part III – analytical issues

Davis¹,

Dasgupta

Kussick

et al. 2013

Cytometry Part B Clinical

112

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Flow cytometric lymphocyte subset enumeration: 10 years of external quality assessment in the Benelux countries

Cited by 28 publications

References 49 publications

Validation of a Standardized Method for Enumerating Circulating Endothelial Cells and Progenitors: Flow Cytometry and Molecular and Ultrastructural Analyses

Validation of a Standardized Method for Enumerating Circulating Endothelial Cells and Progenitors: Flow Cytometry and Molecular and Ultrastructural Analyses

Circulating lymphocyte subsets in normal adults are variable and can be clustered into subgroups

Validation of cell‐based fluorescence assays: Practice guidelines from the ICSH and ICCS – part III – analytical issues

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