![[Feedback]](/icons/banner/feedbackACT.gif){kind=icon}
![[For Subscribers]](/icons/banner/subscriberACT.gif){kind=icon}
![[Archive]](/icons/banner/archiveACT.gif){kind=icon}
![[Search]](/icons/banner/searchACT.gif){kind=icon}
![[Contents]](/icons/banner/tocACT.gif){kind=icon}
|
|
|
|
|
||
Vol. 295, Issue 3, 904-911, December 2000
1-Protease Inhibitor on Hepatic
Ischemia-Reperfusion Injury1
Department of Microbiology (N.I., T.A., Y.M., K.H., J.Y., H.M.) and 2nd Department of Surgery (N.I., K.H., M.O.), Kumamoto University School of Medicine, Kumamoto, Japan
 |
Abstract |
|---|
 Top
 Abstract
 Introduction
Experimental Procedures
Results
Discussion
References
|
|---|
S-Nitrosylated compounds (nitrosothiols; RS-NOs)
function as nitric oxide (NO) reservoirs and preserve the antioxidant
activities of NO. We found remarkable cytoprotection by an
S-nitrosylated protease inhibitor from human plasma,
S-nitroso-
1-protease inhibitor (S-NO-1-PI) that possesses a completely
nitrosylated SH group, in hepatic ischemia-reperfusion injuries in
rats. Liver ischemia was induced in rats by occluding both the portal
vein and hepatic artery for 30 min and was followed by reperfusion.
S-NO-1-PI and control compounds such as
native 1-PI, an NO synthase (NOS) inhibitor, and
standard RS-NOs were given via the portal vein just after reperfusion
was initiated. Liver injury was evaluated by measuring the
extracellular release of liver enzymes (aspartate aminotransferase, alanine aminotransferase, and lactate dehydrogenase). Infiltration of neutrophils and induction of apoptosis and heme oxygenase-1 (HO-1) in the liver were also examined. Maximal liver injury occurred at 3 h after reperfusion and then decreased
gradually. Not only did S-NO-1-PI
treatment (0.1 µmol; 5.3 mg/rat) greatly reduce elevation of liver
enzymes in plasma, as well as neutrophil accumulation and apoptotic
change in liver, it also improved the impaired hepatic blood flow as
assessed by laser Doppler flowmetry and potentiated the
induction of HO-1 in the liver. Although native 1-PI
moderately reduced liver injury, low molecular weight RS-NOs such as
S-nitrosoglutathione and
S-nitroso-N-acetyl penicillamine produced
no obvious protective effect. An NOS inhibitor exacerbated the hepatic
ischemia-reperfusion injuries. These results suggest that
S-NO-1-PI exerts a potent cytoprotective
effect on ischemia-reperfusion liver injury by maintaining tissue blood
flow, inducing HO-1, and suppressing neutrophil-induced liver damage
and apoptosis.
| |
Introduction |
|---|
|
Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
|
|---|
Nitric
oxide (NO) produced in biological systems mediates a diverse array of
physiological functions (Ignarro et al., 1988
; Furchgott and Vanhoutte,
1989; Moncada and Higgs, 1993). In the vascular system, NO regulates
organ blood flow, inhibits platelet aggregation, and attenuates
neutrophil adherence (Ignarro et al., 1988; Kubes et al., 1991; Moncada
and Higgs, 1993). A cytoprotective effect of NO has been reported for
ischemia-reperfusion injuries in various organs (Tsao et al., 1990;
Konorev et al., 1995; Liu et al., 1998; Ohmori et al., 1998; Cottart et
al., 1999). Impairment of endothelial NO production may contribute to
the pathogenesis of ischemia-reperfusion injuries, because a decrease
in NO release can trigger neutrophil adherence and exudate into the
ischemic area, which exacerbates reperfusion injury.
It was recently proposed that various redox isoforms of NO have
critical roles in the diverse physiological and pathophysiological events induced by NO. For example, biological S-nitrosation
occurs via one-electron oxidation of NO catalyzed by heavy metal ions, such as copper and iron, and particularly by ceruloplasmin, which is a
major multicopper-containing plasma protein in mammals (Inoue et al.,
1999; Akaike, 2000). Sulfhydryl-containing molecules such as
glutathione are particularly susceptible to nitrosation; a nucleophilic
attack by NO+ results in
S-nitrosothiol adducts (nitrosothiols; RS-NOs) (Stamler et
al., 1992; Akaike, 2000). Nitrosothiols may function as endogenous NO
reservoirs and preserve the antioxidant activities of NO (Ignarro et
al., 1981; Stamler et al., 1992; Gaston et al., 1993; Rauhala et al.,
1998).
We recently found that 1-protease inhibitor
(1-PI) from human plasma is readily
S-nitrosated under physiological conditions and that
its nitrosylation is 10 times more efficient than nitrosylation of
bovine serum albumin and glutathione (Miyamoto et al., 2000a,b). 1-PI, which is the most abundant serine
protease inhibitor in human plasma (30-60 µM), is known to be an
important defense-oriented acute phase protein (Heidtmann and Travis,
1986). 1-PI (mol. wt., 53,000) has no
intramolecular disulfide bridge but does have a single Cys residue at
position 232. In our earlier study, 1-PI was
nitrosylated with isoamylnitrite at this single 
SH, yielding 100%
S-nitrosylated 1-PI
(S-NO-1-PI), which exhibits
discrete homogeneity. More importantly,
S-NO-1-PI has multiple biological functions, including potent antimicrobial activity and inhibition of
cysteine protease (Miyamoto et al., 2000a,b). In the present report, we
describe a clear protective effect of
S-NO-1-PI on hepatic
ischemia-reperfusion injury in rats.
| |
Experimental Procedures |
|---|
|
Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
|
|---|
Materials.
1-PI, provided by
Chemo-Sero-Therapeutic Institute (Kumamoto, Japan), was purified from
human plasma as described previously (Miyamoto et al., 2000a).
S-NO-1-PI was prepared by
S-nitrosation (100%) of a single SH group of
1-PI with isoamylnitrite and was purified to
homogeneity by gel filtration column chromatography (Miyamoto et al.,
2000a,b).
N
-Nitro-L-arginine
methyl ester (L-NAME) was purchased from Sigma Chemical Co. (St. Louis, MO). S-Nitrosoglutathione (GS-NO)
and S-nitroso-N-acetyl penicillamine (SNAP) were
from Dojindo Laboratories (Kumamoto, Japan).
Animals. Male Wistar rats were obtained from a commercial supplier (Kyudo, Inc., Kumamoto, Japan). All animals were maintained under standard conditions and were fed water and rodent chow ad libitum. The animals weighed between 200 and 230 g.
Experimental Protocol.
Guidelines of the Center for Animal
Resource and Development, Kumamoto University, were followed for
anesthesia during the operative procedure and subsequent postoperative
care. The animals were fasted for 9 h before surgery but were
allowed access to water. Rats were anesthetized with ether during the
operation. After the abdomen was shaved and disinfected with 70%
ethanol, a complete midline incision was made. The portal vein and
hepatic artery were exposed and cross-clamped for 30 min with a
noncrushing microvascular clip. Saline or various compounds such as
S-NO-1-PI (6.0, 20, 100, and 200 nmol; 0.3, 1.0, 5.3, 10.6 mg/rat), native 1-PI
(6.0, 20, 100, and 200 nmol; 0.3, 1.0, 5.3, and 10.6 mg/rat), GS-NO
(6.0, 20, and 100 nmol; 2.0, 6.7, and 33.6 µg/rat), SNAP (100 nmol;
22.0 mg/rat), and L-NAME (10 mg/kg) were given
via the portal vein immediately after reperfusion was initiated, and then the abdomen was closed in two layers with 2-0 silk. Rats were kept
under warming lamps until they awakened and became active.
Measurement of Liver Enzyme Activity in Plasma. Because blood loss caused by frequent blood sampling might have affected liver functions, animals were sacrificed by taking whole circulating blood via abdominal aorta under anesthesia at various time points after reperfusion was initiated. Plasma alanine aminotransferase (ALT), aspartate aminotransferase (AST), and lactate dehydrogenase (LDH) activities were determined by using a sequential multiple AutoAnalyzer system (Hitachi Ltd., Tokyo, Japan). Activities were expressed in international units per liter.
Hepatic Tissue Blood Flow and Blood Pressure Measurement.
A
laser Doppler flowmeter (Laser Flowmeter, ALF21; Advance Co. Ltd.,
Tokyo, Japan) was used to measure hepatic tissue blood flow before
ischemia and 30 and 60 min after initiating reperfusion. In each
animal, the probe of the flowmeter was inserted at the same site in the
median lobe of the liver. The mean value of the blood flow at
respective time points was calculated and expressed as a percentage of
the preischemic initial blood flow value. For blood pressure
measurement, the femoral artery was cannulated and arterial blood
pressure was continuously recorded by using a pressure transducer as
described previously (Yoshida et al., 1994). These measurements were
performed with the animals under urethane (ethyl carbamate) anesthesia.
Identification of Neutrophil Infiltration and Apoptotic Change in
the Liver.
The liver was removed at various time points after
ischemia-reperfusion and was cut into small tissue blocks (3 × 4 × 5 mm3) with a razor blade. The tissue
blocks were embedded in Tissue-Tek OCT compound (Miles, Elkhart, IN)
and were immediately frozen in dry ice-acetone. Frozen sections, 6 µm
thick, were prepared with a cryostat, and cryosections were air-dried
overnight. After fixation in pure acetone for 10 min at room
temperature, the cryosections were stained with an antileukocyte
monoclonal antibody (Serotec Inc., Raleigh, NC) and were visualized by
use of an indirect immunoperoxidase method, with 3,3'-diaminobenzidine
as a substrate (Doi et al., 1999). Neutrophil infiltration was also
analyzed histochemically with an esterase stain, according to a method
reported earlier (Molony et al., 1960).
) with use of an
apoptosis detection kit (TACS; Trevigen, Inc., Gaithersburg, MD)
according to the manufacturer's instructions. Briefly, after the
sections prepared as just described were fixed with 4% formaldehyde
and endogenous peroxidase activity was inhibited, TdT-mediated biotin
nick labeling was performed, followed by a streptavidin-labeled
peroxidase reaction with TACS Blue Label for blue coloration. In some
experiments, the sections were first immunostained with antileukocyte
antibody, and then apoptotic cells were detected in situ by the TUNEL method.
The sections were examined by light microscopy; photomicrographs were
taken at a magnification of 20×. A total of 100 photomicrographs for
each group were subjected to morphometrical analysis. The number of
infiltrated neutrophils was then counted and expressed per square
millimeter of liver section.
Detection of Heme Oxygenase-1 mRNA Expression in the Liver
after Ischemia-Reperfusion.
Heme oxygenase-1 (HO-1) expression was
analyzed by Northern blotting as described previously (Doi et al.,
1999). Briefly, liver specimens obtained from animals exsanguinated at
various time points after reperfusion were frozen quickly in liquid
nitrogen and were stored at 80°C until RNA extraction. Total RNA
was extracted from the liver after ischemia-reperfusion by using the
guanidine thiocyanate lysis method with Trizol reagent (Life
Technologies, Gaithersburg, MD). Each RNA sample (20 µg) underwent
electrophoresis on agarose gel and was transferred to the
Hybond-N+ nylon membrane, followed by
hybridization of a DNA probe for rat HO-1. The DNA probe was
radiolabeled by the random primer technique using
[-32P]dCTP and the Megaprime labeling system
(Amersham Pharmacia Biotech, Buckinghamshire, UK). An HO-1 cDNA
fragment of 882 base pairs was used for hybridization as reported
previously (Doi et al., 1999), and a cDNA fragment for
glyceraldehyde-3-phosphate dehydrogenase was used as a control for gene
expression. The HO-1 mRNA signals were quantified by densitometric
analysis, after normalization with glyceraldehyde-3-phosphate
dehydrogenase mRNA signals, using a Macintosh computer with an image
scanner (GT6500; Epson Co., Ltd., Tokyo, Japan) and the public domain
IMAGE program (National Institutes of Health).
Statistical Analysis. Statistical difference was determined by the two-tailed unpaired t test. Dose-response data were evaluated by two-way ANOVA. A P value of < .05 was considered statistically significant.
| |
Results |
|---|
|
Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
|
|---|
Ischemia-Reperfusion Liver Injury Assessed by Measurement of Liver
Enzymes in Plasma.
Liver injury in this model was evaluated by
measuring the extracellular release of the liver enzymes AST, ALT, and
LDH in the plasma. These enzymes increased to a maximum at 3 h
after reperfusion and then decreased gradually during 24 h (Fig.
1). When
S-NO-1-PI was administered just
after initiating reperfusion, the increased levels of both ALT and AST
were markedly reduced at almost all time points except for 24 h
after reperfusion (Fig. 1A).
S-NO-1-PI treatment also reduced
the elevated LDH levels in the plasma at 3 h after reperfusion
(Fig. 1B). The elevated liver enzyme activities were lowered by
S-NO-1-PI in a dose-dependent manner, as assessed at 3 h after reperfusion (Fig.
2, A and B). Native
1-PI slightly reduced the levels of all these
enzymes (Fig. 2, C and D). However, significant changes in ALT and AST levels were not observed after treatment with the same dose of GS-NO
and SNAP (Fig. 3, A and B).
L-NAME administration tended to exacerbate the
ischemia-reperfusion injury (Fig. 3, A and B). A similar trend of
exacerbation of liver damage as assessed by LDH levels was observed for
groups treated with either GS-NO or SNAP (Fig. 3B).
|
|
|
1-PI is due to enhanced
bioactivity (or bioavailability) of the protein nitrosothiol or whether
it is simply conferred by the additive effect of
1-PI and nitrosothiol, we examined the
dose-responses to GS-NO with or without 1-PI
and S-NO-1-PI over the
dose-response range shown in Fig. 2. In this experiment, we used only
AST values for estimation of the liver injury, because other liver
enzymes showed a tendency to increase by the treatment with GS-NO as
just described. As demonstrated in Fig. 3C, a strong synergy was found in the hepatoprotective effect of
S-NO-1-PI compared with that of
native 1-PI plus GS-NO, as evidenced by
two-way ANOVA of their dose-response curves (P < .01).
These results suggest that NO is beneficial for ischemia-reperfusion
injury in the liver, and S-NO-1-PI
as an NO donor has a remarkable protective effect in the liver. It is
notable that simple NO (NO+) donors such as GS-NO
and SNAP do not necessarily work well; among various nitrosothiols,
S-NO-1-PI appears to be
exceptionally effective in preventing liver damage.
Hepatic Tissue Blood Flow.
Hepatic blood flow before and after
ischemia-reperfusion was measured by using a laser Doppler flowmeter
(Fig. 4). Blood flow decreased
immediately after ischemia and did not change during reperfusion; it
remained significantly lower in the vehicle-treated group at 30 and 60 min after reperfusion was initiated compared with that before ischemia.
In contrast, with S-NO-1-PI, the
impaired hepatic blood flow almost completely recovered after
ischemia-reperfusion: recovery was 95.2% at 30 min and 100.8% at 60 min after reperfusion. GS-NO and SNAP at the same dose did not affect
the reduction of hepatic blood flow induced by ischemia-reperfusion.
Inhibition of NO production by L-NAME treatment
caused a greater decrease in hepatic blood flow after
ischemia-reperfusion.
|
1-PI (0.1 µmol;
5 mg) into rats with hepatic ischemia-reperfusion injury produced a
transient decline in mean arterial pressure for about 5 min, followed
by recovery to the normal blood pressure (data not shown).
Infiltration of Neutrophils and Apoptotic Change in the Liver after
Ischemia-Reperfusion
Immunostaining with an
antineutrophil antibody revealed a large number of neutrophils in the
exudate in the sinusoidal areas of the liver after
ischemia-reperfusion: 122.1 ± 24.7/mm2 and
114.3 ± 6.9/mm2 in vehicle-treated and
native 1-PI-treated rats, respectively, at
3 h after reperfusion (Fig. 5).
Neutrophil infiltration was also identified by an esterase stain, which
revealed a similar distribution of neutrophils in the liver (data not
shown). The number of neutrophils increased in a time-dependent manner
after reperfusion was initiated, with a peak at 12 h after
reperfusion. S-NO-1-PI treatment
remarkably reduced neutrophil accumulation in the liver: to 53.3 ± 7.8/mm2 at 3 h after reperfusion and
throughout the observation period up to 24 h after
ischemia-reperfusion.
|
1-PI treatment led to
significant reduction in production of apoptotic cells throughout the
course of reperfusion. Native 1-PI, however,
caused moderate improvement of apoptotic change in the liver caused by
ischemia-reperfusion injury (Fig. 6, C and D). As described above,
native 1-PI treatment produced a similar trend
of slight reduction liver injury, as assessed by the release of liver
enzymes into the plasma (Fig. 3).
|
|
HO-1 Induction in the Liver after Ischemia-Reperfusion.
HO-1
mRNA transcript was induced as early as 1 h after perfusion and
peaked sharply at 3 h. It was sustained at a moderately elevated
level for 24 h after reperfusion (Fig.
8A).
S-NO-1-PI administration
significantly potentiated HO-1 mRNA induction obtained at 3 h
after initiating reperfusion, but native 1-PI
had no effect (Fig. 8B). The induction of HO-1 by
S-NO-1-PI was also confirmed by
elevation of enzyme activity determined as described previously (Doi et
al., 1999) (data not shown). In contrast, GS-NO treatment did not
affect HO-1 induction in the liver, at least at the same dose as that
of S-NO-1-PI.
|
| |
Discussion |
|---|
|
Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
|
|---|
The data presented here demonstrate that
S-NO-1-PI exerts potent protective
effects against hepatic ischemia-reperfusion injury as evidenced by
decreased levels of plasma liver enzymes, improvement of impaired of
hepatic blood flow, inhibition of neutrophil infiltration and
apoptosis, and enhanced induction of HO-1 in the liver after
ischemia-reperfusion.
Local excessive formation of NO has pro-inflammatory effects such as
edema formation due to enhanced vascular permeability, inflammatory
cell infiltration, and cytotoxicity (possibly through its conversion to
peroxynitrite and other reactive nitrogen oxides) (Beckman and
Koppenol, 1996; Rubbo et al., 1996; Akaike and Maeda, 2000). However,
NO also has completely opposite physiological functions, i.e.,
anti-inflammatory activities, such as inhibition of platelet
aggregation and of neutrophil adherence to endothelium, anti-apoptotic
effects, and inhibition of lipid peroxidation (Kubes et al., 1991; De
Caterina et al., 1995; Rubbo et al., 1996; Ogura et al., 1997; Mannick
et al., 1999). A number of reports show a beneficial effect of NO on
hepatic microcirculation and liver injury as evidenced by
cytoprotective effects of NO donors and detrimental consequences of NOS
inhibition (Liu et al., 1998; Ohmori et al., 1998; Cottart et al.,
1999). The present experiments support these earlier observations,
because the novel NO donor S-NO-1-PI had a remarkable
ameliorating effect on such injury and the NOS inhibitor
L-NAME exacerbated the injury.
Typical biological actions of NO include vasodilatation (vascular
smooth muscle relaxation) and inhibition of platelet aggregation, which
are mediated partly through elevation of intracellular cGMP produced by
soluble guanylate cyclase activated by NO (Rapoport and Mura, 1983;
Furchgott and Vanhoutte, 1989; Radomski et al., 1990; Moncada and
Higgs, 1993; Ignarro et al., 1988). Some part of the
endothelium-dependent vasodilation and inhibition of platelet aggregation is reported to be cGMP-independent (Bolotina et al., 1994;
Pawloski et al., 1998). In addition, NO has inhibitory effects on
endothelium-neutrophil interaction, partly via NF-
B-mediated down-regulation of the expression of adhesion molecules on both endothelium and neutrophils (Kubes et al., 1991; Gauthier et al., 1994;
De Caterina et al., 1995; Liu et al., 1998) and via suppression of
cytokine production by inflammatory cells (De Caterina et al., 1995).
Also, NO causes hepatic sinusoidal dilatation and improves liver
microcirculation by altering the morphofunctional activity of
fat-storing (Ito) cells (Kawada et al., 1993). In this context, the
potent therapeutic effect of
S-NO-1-PI on hepatic
ischemia-reperfusion injury might be produced by NO supplied to
vascular systems to prevent neutrophil-mediated endothelial damage and
sustain microcirculation in the liver. In fact, only a small amount of
NO, as low as a nanomolar concentration, was produced in our
ischemia-reperfusion model, as identified in an ex vivo perfusion
system of the liver with ischemia-reperfusion injury (data not shown).
However, given the profound effect of
S-NO-1-PI on the microcirculation
in the liver, the reduced neutrophil accumulation may be a consequence of the improved microcirculation and not a direct effect of NO.
It is well documented that the inflammatory response involving
neutrophil infiltration is generally elicited during reperfusion of
various ischemic organs and that neutrophils are the major effector
cells contributing to tissue injury in ischemia-reperfusion (Jordan et
al., 1999; Lentsch et al., 1999). These neutrophils can induce
reperfusion injury of endothelial cells and hepatocytes by releasing a
variety of cytotoxic substances, including proteases such as neutrophil
elastase and matrix metalloproteases, cytokines, leukotrienes, cationic
proteins, and reactive oxygen and nitrogen species, all of which can
cause tissue damage (Beckman and Koppenol, 1996; Rubbo et al., 1996;
Liu et al., 1998; Jordan et al., 1999; Lentsch et al., 1999; Akaike and
Maeda, 2000).
We recently verified that
S-NO-1-PI has potent serine
protease inhibitory activity similar to that of native
1-PI: the inhibitory action of
1-PI against porcine pancreatic trypsin and
pancreatic and neutrophil elastase was not affected by
S-nitrosation (Miyamoto et al., 2000a,b). Although the
protective effect of native 1-PI on
ischemia-reperfusion injury of the rat liver was not as great as that
of S-NO-1-PI, it may be that the
neutrophil elastase inhibitory activity of
S-NO-1-PI contributed in an
additive fashion to its potent cytoprotective effect. It is also of
potential interest that S-NO-1-PI
acquired anti-thiol protease activity after S-nitrosation (Miyamoto et al., 2000a). Of particular importance is the
anti-apoptotic activity of various nitrosothiol compounds through their
inhibition of caspases that are apoptosis-inducing intracellular thiol
proteases (Ogura et al., 1997; Mannick et al., 1999). In fact, our
current study revealed that
S-NO-1-PI significantly suppressed
apoptotic change in the liver induced by ischemia-reperfusion.
Therefore, S-NO-1-PI may function
not only as a simple NO (nitroso) donor but also as a protease
inhibitor with a broad inhibitory spectrum.
Although the pro-oxidant activity of NO is now well recognized,
particularly in view of cytotoxic actions of NO-related reactive nitrogen species such as peroxynitrite (Beckman and Koppenol, 1996;
Rubbo et al., 1996; Akaike and Maeda, 2000), an apparently contradictory but important function of NO is its antioxidant potential, observed, for example, in lipid peroxidation (Rubbo et al.,
1996) and iron-overload-induced neurotoxicity (Rauhala et al., 1998).
Nitrosothiol formation may be critically involved in such antioxidant
and cytoprotective actions of NO (Konorev et al., 1995; Rauhala et al.,
1998; Akaike, 2000): NO is protected from reaction with superoxide
after thiol-adduct formation of NO, and thus production of the potent
cytotoxic peroxynitrite is attenuated. It is thought that
S-NO-1-PI could act as a nitroso donor rather than a pure NO donor after in vivo administration. The
cytoprotective effect of S-NO-1-PI
obtained in the present study, therefore, might also be attributable to
antioxidant activity of nitrosothiols introduced by
S-NO-1-PI.
Another important finding is that administration of
S-NO-1-PI potentiated induction of
HO-1 in the liver after ischemia-reperfusion; its effect was greater
that that of vehicle and native 1-PI. Lancaster's group reported that pretreatment of rat hepatocytes with a
low dose of NO donor conferred resistance to oxidative damage of the
cell, possibly through induction of HO-1 (Kim et al., 1995). We
confirmed a similar cytoprotective function of HO-1 in our recent in
vivo study using a solid tumor model (rat hepatoma cells, AH136B) (Doi
et al., 1999). HO-1, which catalyzes the conversion of heme to
biliverdin and CO, has been shown to be constitutively expressed in the
liver and spleen (Maines, 1997). Furthermore, HO-1 is readily induced
by heme compounds, heavy metals, UV irradiation, and various oxidative
stresses (Kim et al., 1995; Maines, 1997). One possible mechanism of
the protective effect of HO-1 induction is thought to be the
antioxidant action of bilirubin (Doré et al., 1999), which is
generated by reduction of biliverdin, a product of the enzymatic
reaction of HO-1 using heme as a substrate. In addition, ferritin,
whose expression was triggered by iron release during heme breakdown
catalyzed by HO-1, has been proposed to protect against oxidative
stress by sequestering iron (Kim et al., 1995). On the basis of these
findings, the beneficial effect of
S-NO-1-PI on ischemia-reperfusion
injury of the liver seems to result from its direct antioxidant
activity and indirectly induced antioxidant levels produced by HO-1 in
the liver after ischemia-reperfusion injury.
In conclusion, the present results suggest that
S-NO-1-PI has a potent
cytoprotective effect on hepatic ischemia-reperfusion injury, possibly
by maintaining tissue blood flow, suppressing neutrophil-induced liver
damage, and inducing HO-1. The beneficial effect of
S-NO-1-PI was found to be far
superior to that of other nitrosothiols such as GS-NO, SNAP, and
S-NO-albumin (data not shown), and thus the multiple
biological activities of S-NO-1-PI (protease inhibitory and nitrosothiol-mediated actions) may contribute to its potent cytoprotective activity. Another advantage of using S-NO-1-PI as an NO donor is that
S-NO-1-PI can be readily formed from the endogenous 1-PI that exists at a high
level in human plasma, so that clinical application of this compound
should be more feasible than that of other synthetic NO donors.
| |
Acknowledgment |
|---|
We thank Judith Gandy for editing the manuscript.
| |
Footnotes |
|---|
Accepted for publication August 18, 2000.
Received for publication May 17, 2000.
1 This work was supported by grants-in-aid from the Ministry of Education, Science, Sports and Culture of Japan (to Y.M. and T.A.), and grants from the Ministry of Health and Welfare of Japan (to T.A.).
Send reprint requests to: Hiroshi Maeda, Department of Microbiology, Kumamoto University School of Medicine, 2-2-1 Honjo, Kumamoto 860-0811, Japan. E-mail: msmaedah{at}gpo.kumamoto-u.ac.jp
| |
Abbreviations |
|---|
NO, nitric oxide;
RS-NO, nitrosothiol;
S-NO-1-PI, S-nitroso-1-protease inhibitor;
TUNEL, terminal deoxynucleotide transferase (TdT)-mediated dUTP-biotin
nick end-labeling;
NOS, NO synthase;
HO-1, heme oxygenase-1;
L-NAME, N-nitro-L-arginine
methyl ester;
GS-NO, S-nitrosoglutathione;
SNAP, S-nitroso-N-acetyl penicillamine;
ALT, alanine
aminotransferase;
AST, aspartate aminotransferase;
LDH, lactate
dehydrogenase.
| |
References |
|---|
|
Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
|
|---|
1-proteinase inhibitor, in
Proteinase Inhibitors (Barrett AJ andSalvesen G eds) pp 441-456,
Elsevier Scientific Publishers BV, Amsterdam.1-protease inhibitor on hepatic ischemia-reperfusion injury, in
The Biology of Nitric Oxide Part 7 (Moncada S,
Gustafsson L andHiggs EA eds)
Portland Press, London, in press.1-protease inhibitor after S-nitrosylation: Inhibition of cysteine protease and antibacterial activity.
Biochem Biophys Res Commun
267:
918-923[Medline].1-protease inhibitor
Biochim Biophys Acta
1477:
90-97[Medline].This article has been cited by other articles:
|
|
 |
|
  Y. Ishima, T. Akaike, U. Kragh-Hansen, S. Hiroyama, T. Sawa, A. Suenaga, T. Maruyama, T. Kai, and M. Otagiri S-Nitrosylated Human Serum Albumin-mediated Cytoprotective Activity Is Enhanced by Fatty Acid Binding J. Biol. Chem., December 12, 2008; 283(50): 34966 - 34975. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 Y. Ishima, T. Sawa, U. Kragh-Hansen, Y. Miyamoto, S. Matsushita, T. Akaike, and M. Otagiri S-Nitrosylation of Human Variant Albumin Liprizzi (R410C) Confers Potent Antibacterial and Cytoprotective Properties J. Pharmacol. Exp. Ther., March 1, 2007; 320(3): 969 - 977. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 R. M. Tuder, T. Yoshida, I. Fijalkowka, S. Biswal, and I. Petrache Role of Lung Maintenance Program in the Heterogeneity of Lung Destruction in Emphysema Proceedings of the ATS, November 1, 2006; 3(8): 673 - 679. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 I. Petrache, I. Fijalkowska, T. R. Medler, J. Skirball, P. Cruz, L. Zhen, H. I. Petrache, T. R. Flotte, and R. M. Tuder {alpha}-1 Antitrypsin Inhibits Caspase-3 Activity, Preventing Lung Endothelial Cell Apoptosis Am. J. Pathol., October 1, 2006; 169(4): 1155 - 1166. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 I. Petrache, I. Fijalkowska, L. Zhen, T. R. Medler, E. Brown, P. Cruz, K.-H. Choe, L. Taraseviciene-Stewart, R. Scerbavicius, L. Shapiro, et al. A Novel Antiapoptotic Role for {alpha}1-Antitrypsin in the Prevention of Pulmonary Emphysema Am. J. Respir. Crit. Care Med., June 1, 2006; 173(11): 1222 - 1228. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 T. D. Blydt-Hansen, M. Katori, C. Lassman, B. Ke, A. J. Coito, S. Iyer, R. Buelow, R. Ettenger, R. W. Busuttil, and J. W. Kupiec-Weglinski Gene Transfer-Induced Local Heme Oxygenase-1 Overexpression Protects Rat Kidney Transplants From Ischemia/Reperfusion Injury J. Am. Soc. Nephrol., March 1, 2003; 14(3): 745 - 754. [Abstract] [Full Text] [PDF]
|
|
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
 |
 |
 |
|
 |
 |
 |
