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Blood, Vol. 93 No. 5 (March 1), 1999:
pp. 1738-1748
Cell-Specific Peptide Binding by Human Neutrophils
Luca Mazzucchelli,
James B. Burritt,
Algirdas J. Jesaitis,
Asma Nusrat,
Tony W. Liang,
Andrew T. Gewirtz,
Frederick J. Schnell, and
Charles A. Parkos
From the Department of Pathology, Brigham and Women's
Hospital and Harvard Medical School, Boston, MA; the Department of
Pathology and Laboratory Medicine, Emory University, Atlanta, GA; and
the Department of Microbiology, Montana State University, Bozeman, MT.
Analysis of peptide binding to human neutrophils (PMN) using phage
display techniques has revealed cell-specific motifs reactive with the
PMN surface. Phage libraries displaying either linear 9-mer or cyclic
10-mer and 6-mer peptides were incubated with normal human neutrophils
followed by elution of bound phage with low pH (pH 2.2) and non-ionic
detergent. Three rounds of selection generated several related peptide
sequences that bound with high avidity to PMN. Using the linear 9-mer
library, PMN-binding phage expressed peptides with the motif
(G/A)PNLTGRW. The binding of phage bearing this motif was highly
specific since no binding was observed on lymphocytes, fibroblasts,
epithelial, or endothelial cells. Functional assays revealed that phage
bearing the sequence FGPNLTGRW induced a pertussis toxin-sensitive
increase in PMN cytosolic calcium analogous to that observed with
G i coupled receptors. Other prominent motifs identified
included phage bearing the consensus DLXTSK(M/L)X(V/I/L), where X
represents a non-conserved position. Phage with this motif bound
exclusively to a sub population of human PMN that comprised
approximately 50% of the total and did not elicit a calcium response.
The binding of such phage to PMN was prevented by co-incubation with
competing peptides displaying identical or similar sequences
(IC50 range from 0.6 µmol/L to 50 µmol/L for DLXTSK and
GPNLTG, respectively). We speculate that these techniques will be
useful in identifying functional cell-specific binding motifs and
contribute to the development of new therapeutic and diagnostic
strategies in human disease.

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