Am. J. Respir. Cell Mol. Biol., Vol 11, No. 3, Sep 1994, 344-350.
Dendritic cells and their precursors isolated from human bronchoalveolar lavage: immunocytologic and functional properties
JM van Haarst, HC Hoogsteden, HJ de Wit, GT Verhoeven, CE Havenith and HA Drexhage
Department of Immunology, Erasmus University, Rotterdam, The Netherlands.
Human bronchoalveolar lavage (BAL) has been described to contain, besides a
large number of alveolar macrophages (AM) (approximately 95%), small
numbers of monocyte-like cells (approximately 2%) and dendritic cells (DC)
(approximately 0.4%). To separate AM (high autofluorescence) from DC, we
used a fluorescence activated cell sorter (FACS) to separate BAL cells into
a low autofluorescent (LAF) fraction and a high autofluorescent (HAF)
fraction. Immunocytologic and functional properties of these fractions were
investigated. The LAF fraction was composed of acid phosphatase (APh)- and
RFD9-negative cells, which were strongly positive for HLA-DR, L25, RFD1,
and CD68. A portion of these cells expressed CD1a (22%) and My4 (60%). The
marker pattern of these cells is reminiscent to that of intraepithelial
bronchial DC and to that of blood DC. The majority of the LAF cells had a
monocyte-like morphology, but after overnight culture the percentage of LAF
cells with long cytoplasmic extensions (DC morphology) was strongly
augmented (from 18 to 51%). The HAF fraction contained 100% AM, strongly
positive for APh, HLA-DR, CD68, RFD7, and RFD9. In culture, the LAF cells
formed clusters with T cells and vigorously stimulated the proliferation of
allogeneic T cells and naive (CD45RO- negative) T cells. BAL and LAF cells
produced higher responses in nonsmokers than in smokers. In contrast, HAF
cells did not form clusters with T cells and did not stimulate allogeneic T
cell proliferation. HAF cells even suppressed mitogen-driven T cell
proliferation.(ABSTRACT TRUNCATED AT 250 WORDS)
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Copyright © 1994 American Thoracic Society.
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