Differential effects of iron deficiency on the expression of CD80 and CD86 co‐stimulatory receptors in mitogen‐treated and untreated murine spleen cells

The interaction of CD28 and its ligands (CD80, CD86) on antigen presenting cells and that of TCR/CD3‐MHC are required for T lymphocyte activation. To determine whether impaired lymphocyte proliferation associated with iron deficiency is due to reduced expression of these ligands, spleen cells obtained from eight to nine C57BL/6 mice/group of iron deficient (ID), iron replete (R), control (C), pair‐fed (PF), and high iron (HI) mice were labeled with anti‐CD80‐fluorescein isothiocyante (FITC) and anti‐CD86‐FITC. Diets differed only in iron concentration: 5, 50, and 125 mg/kg for the ID, C, and HI, respectively. Mean levels of hemoglobin and liver iron stores of ID and R mice were less than 50% those of C mice ( P  < 0.005). In non‐activated and concanavalin A‐treated cultures, significant differences were observed among groups in the percentage of CD80 + cells: ID>R > C = PF = HI ( P  < 0.05). The same trend was observed for CD86 + cells ( P  > 0.05). Fluorescence intensity (FI) of either marker did not significantly change by iron status. In vitro iron chelation by deferoxamine (20, 200 μg/ml) for 1, 2, and 24 h increased FI of both markers on unactivated B and T cells ( P  < 0.05). However, it had no effect on FI of either marker of mitogen‐treated cells presumably because the maximum levels are achieved by the mitogen. Lymphocyte proliferative responses to mitogens positively and significantly correlated with CD80 and CD86 FI (r = 0.41−0.59) but negatively correlated with the percentages of CD80 + cells (r = −0.48) ( P  < 0.05). Data suggest that impaired lymphocyte proliferation associated with iron deficiency is not due to reduced CD80 and CD86 expression. J. Cell. Biochem. 86: 571–582, 2002. © 2002 Wiley‐Liss, Inc.