Aldehyde Fixation of Thiol-reactive Fluorescent Cytoplasmic Probes for Tracking Cell Migration

Journal of Histochemistry and Cytochemistry

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ARTICLE

Aldehyde Fixation of Thiol-reactive Fluorescent Cytoplasmic Probes for Tracking Cell Migration

Charles A. West^a, Chufa He^a, Mei Su^a, Scott J. Swanson^a, and Steven J. Mentzer^a
^a Laboratory of Immunophysiology, the Dana-Farber Cancer Institute, Brigham and Women's Hospital, and Harvard Medical School, Boston, Massachusetts

Correspondence to: Steven J. Mentzer, PBB Lobby, Brigham & Women's Hospital, 75 Francis Street, Boston MA 02115.

Tracking of cell migration plays an important role in the studyof morphogenesis, inflammation, and metastasis. The recent developmentof probes that exist as intracellular peptide-fluorescence dyeadducts has offered the possibility of aldehyde fixation ofthese dyes for detailed anatomic studies of lymphocyte trafficking.To define the conditions for fixation of these cytoplasmic fluorescentprobes, we compared fixation conditions containing formaldehyde,glutaraldehyde, paraformaldehyde, zinc formaldehyde, and glyoxylate,as well as fixation by quick-freezing in liquid nitrogen-cooledmethylbutane. The efficacy of aldehyde fixation of the cellfluorescence was assessed by quantitative tissue cytometry andflow cytometry. We studied cytoplasmic fluorescent dyes withdiscrete emissions in the green [5-chloromethylfluorescein diacetate(CMFDA); 492 ex, 516 em] and orange [5-(and-6)-(4-chloromethyl(benzoyl)amino)tetramethylrhodamine (CMTMR); 540 ex, 566 em] spectra. The resultsdemonstrated that aldehyde fixation preserved cell fluorescencefor more than 6 months. The primary difference between the aldehydefixatives was variability in the difference between the yieldof the cell fluorescence and the relevant background fluorescence.Formaldehyde and paraformaldehyde were superior to the otherfixatives in preserving cell fluorescence while limiting backgroundfluorescence. With these fixatives, both the CMFDA and CMTMRfluorescent dyes permitted sufficient anatomic resolution forreliable localization in long-term cell tracking studies.

(J Histochem Cytochem 49:511–517, 2001)

Key Words: fluorescent dyes, cell migration, aldehydes, histocytochemistry,fluorescence cytometry

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