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(Received for publication, February 8, 1996, and in revised form, August 16, 1996)
From the Bristol-Myers Squibb Pharmaceutical Research Institute,
Seattle, Washington 98121
The monoclonal antibody (mAb) J393 induces
apoptosis in Jurkat T-cells. NH2-terminal amino acid
sequence analysis identified the 140-kDa surface antigen for mAb J393
as CD43/leukosialin, the major sialoglycoprotein of leukocytes. While
Jurkat cells co-expressed two discrete cell-surface isoforms of CD43,
recognized by mAb J393 and mAb G10-2, respectively, only J393/CD43
signaled apoptosis. J393/CD43 was found to be hyposialylated, bearing
predominantly O-linked monosaccharide glycans, whereas
G10-2/CD43 bore complex sialylated tetra- and hexasaccharide chains.
Treatment with soluble, bivalent mAb J393 killed 25-50% of the cell
population, while concomitant engagement of either the CD3·TcR
complex or the integrins CD18 and CD29 significantly potentiated this
effect. Treatment of Jurkat cells with mAb J393 induced tyrosine
phosphorylation of specific protein substrates that underwent
hyperphosphorylation upon antigen receptor costimulation. Tyrosine
kinase inhibition by herbimycin A diminished J393/CD43-mediated
apoptosis, whereas inhibition of phosphotyrosine phosphatase
activity by bis(maltolato)oxovanadium-IV enhanced cell death.
Signal transduction through tyrosine kinase activation may lead to
altered gene expression, as J393/CD43 ligation prompted decreases in
the nuclear localization of the transcriptional regulatory protein
NF-
Volume 271, Number 44,
Issue of November 1, 1996
pp. 27686-27695
©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
B and proteins binding the interferon-inducible regulatory
element. Since peripheral blood T-lymphocytes express cryptic epitopes
for mAb J393, these findings demonstrate the existence of a tightly
regulated CD43-mediated pathway for inducing apoptosis in human T-cell
lineages.
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