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1 Egleston Pediatric
Subspecialists,
Enhancing the clearance of neutrophils by
enhancing apoptotic cell death and macrophage recognition may be
beneficial in acute lung injury. Exogenous nitric oxide gas depresses
neutrophil oxidative functions and accelerates cell death (A. H. Daher,
J. D. Fortenberry, M. L. Owens, and L. A. Brown. Am.
J. Respir. Cell Mol. Biol. 16: 407-412, 1997). We
hypothesized that S-nitrosoglutathione
(GSNO), a physiologically relevant nitric oxide donor, could also
enhance neutrophil DNA fragmentation. Neutrophils were incubated for
2-24 h in the absence and presence of GSNO (dose range 0.1-5
mM) and evaluated for cell death by a fluorescent
viability/cytotoxicity assay. Neutrophil DNA fragmentation was assessed
by cell death detection ELISA and by terminal
deoxynucleotidyltransferase-mediated fluorescence-labeled dUTP nick end
labeling assay. Neutrophil oxidative function was also determined.
Incubation with GSNO increased cell death at 2, 4, and 24 h. GSNO
incubation for 24 h significantly increased DNA fragmentation in a
dose-dependent fashion at 0.5 (median 126% of control value;
P = 0.002) and 5 mM (185% of control value; P = 0.002) by
terminal deoxynucleotidyltransferase-mediated fluorescence-labeled dUTP
nick end labeling and at 0.5 mM by ELISA (164% of control
value; P = 0.03). The
apoptosis-to-total cell death ratio increased with increasing GSNO
concentration (P < 0.05). Effects
were mitigated by coincubation with superoxide dismutase. Five
millimolar GSNO decreased overall superoxide generation and
O2 consumption but not when
adjusted for dead neutrophils. GSNO significantly enhances cell death
and neutrophil DNA fragmentation in a dose-dependent fashion.
nitric oxide; apoptosis; S-nitrosothiol; glutathione
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