The Impact of ATRA on Shaping Human Myeloid Cell Responses to Epithelial Cell-Derived Stimuli and on T-Lymphocyte Polarization

<table class="table-group" id="tab2"><tr><td><table class="table"><tr><td class="thead-hr" colspan="4"><hr/></td></tr><tr class="thead"><td align="left"> </td><td align="center">CD1a</td><td align="center">DC SIGN</td><td align="center">CD14</td></tr><tr><td class="thead-hr" colspan="4"><hr/></td></tr><tr><td align="left">GMCSF+IL-4</td><td align="center">200.88</td><td align="center">32.6</td><td align="center">75.63</td></tr><tr><td align="left">GMCSF</td><td align="center">66.31</td><td align="center">10.5</td><td align="center">183.29</td></tr><tr><td align="left">MCSF</td><td align="center">6.01</td><td align="center">4.3</td><td align="center">369.47</td></tr><tr class="table-tr"><td colspan="4"><hr class="tbody-hr"/></td></tr></table></td></tr></table>

Expression of CD1a, DC-SIGN, and CD14 cell surface molecules on monocyte-derived cells generated in the presence of the colony stimulating factors GM-CSF+IL-4, GM-CSF, or M-CSF. Peripheral blood-derived monocytes were differentiated in the presence of GM-CSF+IL-4, GM-CSF, or M-CSF in RPMI + 10% FCS for 3 days and the expression of the cell surface markers CD1a, DC-SIGN/CD209, and CD14 was monitored by flow cytometry using fluorescent labeled specific antibodies. The expression levels of CD1a, DC-SIGN, and CD14 are indicated as mean fluorescence intensity (MFI).

Mediators of Inflammation

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Table 2

Table 2: The Impact of ATRA on Shaping Human Myeloid Cell Responses to Epithelial Cell-Derived Stimuli and on T-Lymphocyte Polarization 