Murine CXCR3+CD27bright NK cells resemble the human CD56bright NK‐cell population

N Marquardt, E Wilk, C Pokoyski… - European journal of …, 2010 - Wiley Online Library
N Marquardt, E Wilk, C Pokoyski, RE Schmidt, R Jacobs
European journal of immunology, 2010Wiley Online Library
Human NK cells can be subdivided into CD56dim and CD56bright NK cells, which exhibit
different phenotypical and functional characteristics. As murine NK cells lack CD56 or a
distinct correlate, direct comparative studies of NK cells in mice and humans are limited.
Although CD27 is currently proposed as a feasible subset marker in mice, we assume that
the usage of this marker alone is insufficient. We rather investigated the expression of the
chemokine receptor CXCR3 for its suitability for distinguishing murine NK‐cell subsets with …
Abstract
Human NK cells can be subdivided into CD56dim and CD56bright NK cells, which exhibit different phenotypical and functional characteristics. As murine NK cells lack CD56 or a distinct correlate, direct comparative studies of NK cells in mice and humans are limited. Although CD27 is currently proposed as a feasible subset marker in mice, we assume that the usage of this marker alone is insufficient. We rather investigated the expression of the chemokine receptor CXCR3 for its suitability for distinguishing murine NK‐cell subsets with simultaneous consideration of CD27. Compared with CXCR3 NK cells, exerting stronger cytotoxic capability, CXCR3+ NK cells displayed an activated phenotype with a lower expression of Ly49 receptors, corresponding to human CD56bright NK cells. Also in common with human CD56bright NK cells, murine CXCR3+ NK cells exhibit prolific expansion as well as robust IFN‐γ, TNF‐α and MIP‐1α production. We additionally demonstrated changes in both CXCR3 and CD27 expression upon NK‐cell activation. In summary, CXCR3 serves as an additional applicable marker for improved discrimination of functionally distinct murine NK‐cell subsets that comply with those in humans.
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