Andrade W, Seabrook T J, Johnston M G, Hay J B
Department of Pathology, University of Toronto, Ontario, Canada.
J Immunol Methods. 1996 Aug 14;194(2):181-9. doi: 10.1016/0022-1759(96)00083-x.
In this study we examined the new cell dye CM-DiI for tracking the migration of lymphocytes from blood to lymph. This lipophilic marker intercalates in the plasma membrane like the PKH dyes and older DiI derivatives. The stability and intensity of staining achieved with these dyes is better than most other fluorochromes or radioisotopes, yet they are poorly soluble in aqueous solutions, which can make staining difficult, and they are not fixable in tissue sections. CM-DiI is reported to have increased water solubility and it can be fixed using traditional aldehyde fixatives, making it feasible to detect labeled cells in histological sections. To determine the suitability of CM-DiI as a lymphocyte marker, a labeling protocol was developed. We tested the ability of stained cells to recirculate in vivo. Following the intravenous injection of CM-DiI positive cells, their recovery in lymph over 40 h was comparable to that of cells labeled with other fluorochromes or radioisotopes. The kinetics of recirculation were also very similar, as labeled cells were detectable in lymph within 4 h of injection, and the peak percentage of labeled cells in lymph was generally observed between 20-30 h. We also confirmed that CM-DiI is retained in the lymphocyte membrane following routine paraffin processing. Thus CM-DiI does not appear to alter the process of lymphocyte recirculation, and it should be a useful marker for tracking these cells.
