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Neutrophil differentiated HL‐60 cells model Mac‐1 (CD11b/CD18)‐independent neutrophil transepithelial migration
Author(s) -
Carrigan Svetlana O.,
Weppler Amy L.,
Issekutz Andrew C.,
Stadnyk Andrew W.
Publication year - 2005
Publication title -
immunology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.297
H-Index - 133
eISSN - 1365-2567
pISSN - 0019-2805
DOI - 10.1111/j.1365-2567.2005.02131.x
Subject(s) - integrin alpha m , cd18 , n formylmethionine leucyl phenylalanine , chemotaxis , monoclonal antibody , microbiology and biotechnology , biology , cell culture , cell migration , chemistry , cell , immunology , receptor , antibody , flow cytometry , biochemistry , genetics
Summary During active intestinal inflammation granulocytes accumulate in the lumen of the gut where they damage the epithelium through the release of various products such as reactive oxygen species and proteolytic enzymes. Previously, using function blocking monoclonal antibodies, we showed that neutrophil migration across intestinal epithelial monolayers in response to various chemoattractants was partially β 2 integrin Mac‐1 (CD11b/CD18)‐independent. Here, we show that treating neutrophils with intact monoclonal antibody (mAb) to CD18 activates the cells to express more CD11b. Thus our goal now was to determine whether neutrophil Mac‐1‐independent transepithelial migration proceeds independently of prior cell activation through Mac‐1. We took two approaches, one using blocking Fab′ fragments of mAb to CD18 and the second was to develop a neutrophil differentiated HL‐60 cell line which is Mac‐1 deficient to further study neutrophil/epithelial cell interaction. Anti‐CD18 Fab′ minimally activated neutrophils but inhibited approximately 75% of transepithelial migration to fMLP while having a minimal effect (≤25% inhibition) on the migration to C5a. Upon incubation with dimethylsulphoxide, HL‐60 cells differentiated and up‐regulated CD11b expression and migrated to C5a and n ‐formyl methionyl leucyl phenylalanine in a similar manner to peripheral blood neutrophils. In contrast, CD11b expression was minimal on HL‐60 cells differentiated with dibutytyl cAMP to a neutrophil‐like phenotype. These cells, however, readily migrated across both intestinal and lung epithelial monolayers in response to C5a. We conclude that Mac‐1‐independent transepithelial migration does not require prior activation of cells via Mac‐1 ligation because HL‐60 cells lacking Mac‐1 (CD11b/CD18) expression migrate effectively. HL‐60 cells differentiated with dbcAMP should greatly assist in the search for the Mac‐1‐independent ligands for neutrophil migration across epithelium.