TY - JOUR
T1 - Intracellular IL-10 detection in T cells by flowcytometry
T2 - The use of protein transport inhibitors revisited
AU - Muris, Anne Hilde
AU - Damoiseaux, Jan
AU - Smolders, Joost
AU - Cohen Tervaert, Jan Willem
AU - Hupperts, Raymond
AU - Thewissen, Mariëlle
N1 - © 2012 Elsevier B.V. All rights reserved
PY - 2012/7/31
Y1 - 2012/7/31
N2 - In the past two decades, interleukin-10 (IL-10) has gained much attention as an important regulatory cytokine involved in self-tolerance. Functional assessment of IL-10 producing immune cells is traditionally done by stimulation and measurement of cytokine production by flowcytometry. Thereby a protein transport inhibitor like monensin is used to accumulate the cytokine of interest intracellularly. In this study we elaborated on the monensin effect on cytokine detection and focused on IL-10 detection in human T cells.Peripheral blood mononuclear cells (PBMC) of 32 study subjects were isolated and stimulated with PMA/ionomycin, in the absence and presence of monensin, and stained intracellularly for IFN-γ, IL-4, IL-10 and IL-17A.Our results re-established that detection of IFN-γ + and IL-4 + T cells benefited from the presence of monensin during stimulation. However, stimulation in the presence of monensin yielded lower proportions of IL-10 + T cells (0.45% (0.28-0.80) versus 0.80% (0.50-1.50) of CD4 + T cells, p<0.01), although monensin addition did result in an increased MFI (2431 (1273-4959) versus 1928 (1147-3760), p<0.01). Detectable fractions of IL-17A + CD4 + T cells were not affected by monensin. A shorter incubation time, but not lower monensin concentrations, was effective in improving the detection of IL-10 + T cells. We found a strong correlation between the fraction of IL-10 + CD4 + T cells in the presence and absence of monensin (R=0.80 p<0.01). Next to this, also the detection of IL-10 + NK-T cells and IL-10 + monocytes, but not IL-10 + B cells, is impaired in the presence of monensin.This study shows that the effect of monensin on cytokine accumulation is time and cytokine dependent. Due to the use of monensin, previous research may have underestimated the number of IL-10 + leukocytes or may even have not been able to detect them at all. It is important to consider this for future research or when interpreting historical IL-10 data.
AB - In the past two decades, interleukin-10 (IL-10) has gained much attention as an important regulatory cytokine involved in self-tolerance. Functional assessment of IL-10 producing immune cells is traditionally done by stimulation and measurement of cytokine production by flowcytometry. Thereby a protein transport inhibitor like monensin is used to accumulate the cytokine of interest intracellularly. In this study we elaborated on the monensin effect on cytokine detection and focused on IL-10 detection in human T cells.Peripheral blood mononuclear cells (PBMC) of 32 study subjects were isolated and stimulated with PMA/ionomycin, in the absence and presence of monensin, and stained intracellularly for IFN-γ, IL-4, IL-10 and IL-17A.Our results re-established that detection of IFN-γ + and IL-4 + T cells benefited from the presence of monensin during stimulation. However, stimulation in the presence of monensin yielded lower proportions of IL-10 + T cells (0.45% (0.28-0.80) versus 0.80% (0.50-1.50) of CD4 + T cells, p<0.01), although monensin addition did result in an increased MFI (2431 (1273-4959) versus 1928 (1147-3760), p<0.01). Detectable fractions of IL-17A + CD4 + T cells were not affected by monensin. A shorter incubation time, but not lower monensin concentrations, was effective in improving the detection of IL-10 + T cells. We found a strong correlation between the fraction of IL-10 + CD4 + T cells in the presence and absence of monensin (R=0.80 p<0.01). Next to this, also the detection of IL-10 + NK-T cells and IL-10 + monocytes, but not IL-10 + B cells, is impaired in the presence of monensin.This study shows that the effect of monensin on cytokine accumulation is time and cytokine dependent. Due to the use of monensin, previous research may have underestimated the number of IL-10 + leukocytes or may even have not been able to detect them at all. It is important to consider this for future research or when interpreting historical IL-10 data.
UR - http://www.scopus.com/inward/record.url?scp=84861572243&partnerID=8YFLogxK
U2 - 10.1016/j.jim.2012.04.011
DO - 10.1016/j.jim.2012.04.011
M3 - Article
C2 - 22565155
AN - SCOPUS:84861572243
SN - 0022-1759
VL - 381
SP - 59
EP - 65
JO - Journal of Immunological Methods
JF - Journal of Immunological Methods
IS - 1-2
ER -