|
Xiao-Bing
Fu, Yin-Hui Yang, Tong-Zhu Sun, Wei Chen, Jun-You Li, Zhi-Yong Sheng,
Wound Healing and Cell Biology Laboratory, Burns Institute, 304th
Hospital, Trauma Center of Postgraduate Medical College, Beijing
100037, China
Supported in part by the National Basic Science and Development
Programme (973 Programme, No.G1999054204), Grant for National
Distinguished Young Scientists No. 39525024, Grant for National
Natural Science Foundation of China, No. 39900054, 30170966
Correspondence to: Professor Xiao-Bing Fu, Wound Healing and
Cell Biology Laboratory, 304th Hospital, Burns Institute,
Trauma Center of Postgraduate Medical College, 51 Fu Cheng Road,
Beijing 100037,China. fuxb@cgw.net.cn
Telephone: +86-10-66867396
Fax: +86-10-88416390
Received: 2003-03-04
Accepted: 2003-04-01
Abstract
AIM: Previous studies showed that exogenous basic fibroblast
growth factor (bFGF or FGF-2) could improve physiological
dysfunction after intestinal ischemia/ reperfusion (I/R) injury.
However, the mechanisms of this protective effect of bFGF are still
unclear. The present study was to detect the effect of bFGF on the
activities of mitogen-activated protein kinase (MAPK) signaling
pathway in rat intestine after I/R injury, and to investigate the
protective mechanisms of bFGF on intestinal ischemia injury.
METHODS:
Rat intestinal I/R injury was produced by clamping the superior
mesenteric artery (SMA) for 45 minutes and followed by reperfusion
for 48 hours. Seventy-eight Wistar rats were used and divided
randomly into sham-operated group (A), normal saline control group
(B), bFGF antibody pre-treated group (C), and bFGF treated group
(D). In group A, SMA was separated without occlusion. In groups B, C
and D, SMA was separated and occluded for 45 minutes, then, released
for reperfusion for 48 hours. After the animals were sacrificed,
blood and tissue samples were taken from the intestine 45 minutes
after ischemia in group A and 2, 6, 24, and 48 hours after
reperfusion in the other groups. Phosphorylated forms of p42/p44
MAPK, p38 MAPK and stress activated protein kinase/C-Jun N-terminal
kinase (SAPK/JNK) were measured by immunohistochemistry. Plasma
levels of D-lactate were examined and histological changes were
observed under the light microscope.
RESULTS:
Intestinal I/R injury induced the expression of p42/p44 MAPK, p38
MAPK, and SAPK/JNK pathways and exogenous bFGF stimulated the early
activation of p42/p44 MAPK and p38 MAPK pathways. The expression of
phosphorylated forms of p42/p44 MAPK was primarily localized in the
nuclei of crypt cells and in the cytoplasm and nuclei of villus
cells. The positive expression of p38 MAPK was localized mainly in
the nuclei of crypt cells, very few in villus cells. The activities
of p42/p44 MAPK and p38 MAPK peaked 6 hours after reperfusion in
groups B and C, while SAPK/JNK peaked 24 hours after reperfusion.
The activities of p42/p44 MAPK and p38 MAPK peaked 2 hours after
reperfusion in group D and those of SAPK/JNK were not changed in
group B. D-lactate levels and HE staining showed that the intestinal
barrier was damaged severely 6 hours after reperfusion; however,
histological structures were much improved 48 hours after
reperfusion in group D than in the other groups.
CONCLUSION:
The results indicate that intestinal I/R injury stimulates the
activities of MAPK pathways, and that p42/p44 MAPK and p38MAPK
activities are necessary for the protective effect of exogenous bFGF
on intestinal I/R injury. The protective effect of bFGF on
intestinal dysfunction may be mediated by the early activation of
p42/p44 MAPK and p38 MAPK signaling pathways.
Fu
XB, Yang YH, Sun TZ, Chen W, Li JY, Sheng ZY. Rapid mitogen-activated
protein kinase by basic fibroblast growth factor in rat intestine
after ischemia/reperfusion injury. World J Gastroenterol 2003; 9(6): 1312-1317
http://www.wjgnet.com/1007-9327/9/1312.asp
INTRODUCTION
Previous studies have shown that intestinal ischemia/reperfusion
(I/R) injury reduce the expression of endogenous basic fibroblast
growth factor (bFGF) in rats, and the intravenous administration of
exogenous bFGF could induce the expression of endogenous bFGF and
improve the physiological functions of the intestine, lung, kidney,
and other internal organs after I/R injury[1-6]. However,
the protective mechanisms of bFGF on intestinal I/R injury remain
unknown.
Mitogen-activated
protein kinase (MAPK) cascade, a cytoplasmic protein kinase that
requires dual phosphorylation on specific threonine and tyrosine
residues for their activation, can transmit mitogen or
differentiation signals from the cell surface into the nucleus, thus
regulating the gene expression[7-10]. P42/p44 MAPK,
p38MAPK and stress activated protein kinase/C-Jun N-terminal kinase
(SAPK/JNK) are three important members of the MAPK family. The
purpose of the present study was to detect the activities of mitogen-activated
protein kinase (MAPK) signaling pathway in rat intestine after
administration of bFGF, and to investigate the protective mechanisms
of bFGF on intestinal (I/R) injury.
Rat
intestinal I/R injury was produced by clamping the superior
mesenteric artery (SMA) for 45 minutes and by different durations of
reperfusion[11]. The activities of p42/p44 MAPK, p38 MAPK,
and SAPK/JNK were measured after administration of bFGF or bFGF
monoclonal antibody. The results indicate that the early activation
of p42/p44 MAPK and p38 MAPK is necessary for the protective effect
of bFGF on intestinal I/R injury.
MATERIALS
AND METHODS
Animal model
Seventy-eight healthy Wistar rats weighing 220±20 g (Animal Center, Academy of Military
Medical Sciences, Beijing) were used. All animals were housed in the
laboratory and given free access to food and water for 1 week before
being used. The animal was under anesthesia by 3 % sodium
pentobarbital (40 mg/kg), a middle incision was made. The superior
mesenteric artery (SMA) was identified and freed by blunt
dissection. A microvascular clamp was placed at the root of SMA to
cause complete cessation of blood flow for 45 minutes, and
thereafter the clamp was loosened to form reperfusion injury[1,
11].After 2, 6, 24 and 48 hours reperfusion, the animals were
sacrificed and blood samples and intestinal tissue biopsies were
taken. Blood samples were centrifuged and serum was frozen to
measure plasma D-lactate. Tissue biopsies were fixed with 4 %
paraformaldehyde.
In
this study, all operations were performed under aseptic conditions.
The animal experiments were approved by the local animal management
committee.
Experimental
design
The animals were randomly divided into four groups:
sham-operated (A), normal saline control (B), bFGF monoclonal
antibody (Sigma, St. Louis, MO, USA) pre-treated (C) and bFGF
(Sigma, St. Louis, MO, USA) treated groups (D). In group A,
SMA was freed but without occlusion and blood samples and
tissue biopsies were taken 45 minutes after exposure of the SMA. In
groups B and D, 0.15 ml saline or 0.15 ml saline plus bFGF (2 mg/rat) was injected immediately 45 minutes after SMA occlusion
from the tail vein. In group C, 0.15 ml saline plus bFGF monoclonal
antibody (25 mg/rat) was injected right before SMA occlusion from tail vein for
pre-treatment.
Measurement
of phosphorylated forms of p42/p44 MAPK, p38 MAPK and SAPK/JNK
Formalin-fixed, paraffin-embedded small intestinal tissues
were used to measure the expression of phosphorylated forms of
p42/p44 MAPK, p38 MAPK, and SAPK/JNK by immunohistochemistry.
Immunohistochemical staining was performed according to the
instructions of the PowerVisionTM kit (Santa Cruze, USA). Briefly,
sections (5 mm) were dewaxed and rehydrated in graded alcohols. Endogenous
peroxidase activity was quenched, and antigen retrieval was
performed by heating for 20 minutes at 100 °C in 0.01 mol/L sodium citrate. The primary monoclonal antibodies
for p42/p44 MAPK, p38 MAPK and SAPK/JNK (Cell Signaling Technology,
Inc., USA) were diluted to 1:100 in buffer and incubated for 40
minutes at 37 °C. The sections were then incubated with HRP-conjugated secondary
antibodies (Santa Cruz, USA) for 20 minutes at 37 °C. Positive expression was detected with diaminobenzidine (DAB)
(Sigma, St. Louis, MO, USA). The sections were lightly
counterstained with hematoxylin, dehydrated in graded alcohol, and
mounted. For negative control, the sections were processed similarly
but PBS was used as primary antibodies instead of the MAPKs
monoclonal antibodies.
The result
of positive staining was semi-quantitatively defined as -, +, ++ and
+++. This was observed under microscope with 10 times eyepiece and
40 times objective." -" represents no visible positive
staining," +" less than 10 stained cells and
"++" 10-30 stained cells, while" +++" represents
more than 30 positively stained cells within one high power field.
Measurement
of plasma D-lactate
The levels of plasma D-lactate were measured with modified
Brandt's method[12].
Briefly, heparinized blood was centrifuged at 3 200 rpm for 10 min
and 2 ml of the plasma was deproteinized with 0.2 ml perchloric acid
(PCA) (1/10 vol), mixed and kept in an ice bath for 10 min. The
denatured protein solution was centrifuged at 3 200 rpm for 10 min
and the supernatant solution was removed. To 1.4 ml of supernatant
solution, 0.12 ml KON was added and they were mixed for 20 s.
Precipitant KClO4 was removed by centrifugation at 3 200 rpm for 10
min. The supernatant solution and neutralized-protein-free plasma
were used to measure the absorbency at 340 nm. Plasma D-lactate
concentration was expressed as mmol/L.
Histological
observation
Paraformaldehyde fixed, paraffin embedded small intestine
samples were also cut 5 mm in thickness, deparaffinized in xylene, rehydrated in graded
ethanol, and then stained with haematoxylin-eosin (HE) for
histological observation under light microscope (Olympus, Japan).
Statistical
analysis
Data were expressed as mean ± standard error. Comparisons
between groups of data were analyzed by Student's
t-test. P values <0.05 were
considered statistically significant.
RESULTS
Activities of p42/p44 MAPK and p38 MAPK
Quantitative immunohistochemical results for phosphorylated
forms of p42/p44 MAPK and p38 MAPK were evaluated (Tables 1 and 2).
The expression of activated p42/p44 MAPK was localized in the
cytoplasm and nuclei of villus cells and in the nuclei of crypt
cells, mainly in the epithelium and villus cells (Figure 1).
Activated p38 MAPK was localized primarily in the nuclei of crypt
cells, very few in villus cells (Figure 2). There was a consistent
correlation between positive expression levels and the intensity of
p42/p44 MAPK and p38 MAPK. The positive expression of p42/p44 MAPK
and p38 MAPK was weak in the sham-operated intestinal tissues and
ischemic tissues. However, the number of positive staining cells
increased with high staining intensity after reperfusion injury. In
the normal saline and bFGF antibody pre-treated groups, the number
of positive staining cells of p42/p44 MAPK (Figures 1B and C) and
p38 MAPK (Figures 2B and C) increased 2 hours after reperfusion,
peaked at 6th hours, and decreased from 24 to 48 hours. In the bFGF
treated group, however, the number of positive staining cells and
the intensity of p42/p44 MAPK and p38 MAPK peaked 2 hours after
reperfusion (Figures 1D and 2D) and decreased afterwards, but they
were still higher than those in the sham-operated control at 48
hours. Compared with the normal saline and bFGF treated groups, the
intensity of p42/p44 MAPK and p38 MAPK positive staining in the bFGF
antibody pretreated group was weaker from 2 hours to 48 hours after
reperfusion.
Activities
of SAPK/JNK
Weak staining of SAPK/JNK was observed in small intestine
after I/R injury. Positive staining was localized in the nuclei and
cytoplasm of villus and crypt cells. The staining, however, was weak
without much difference among the groups (Table 3). The positive
staining of SAPK/JNK in bFGF treated group was slightly higher only
at 24 hours after reperfusion. Among all the groups, the positive
staining of SAPK/JNK was weaker than that of p42/p44 MAPK and p38
MAPK.
Changes
of plasma D-lacate levels
Plasma D-lactate levels were measured 2, 6, 24, and 48 hours
after reperfusion in all groups. They were elevated 2 hours after
reperfusion in all groups, peaked at 6th hour, and decreased to
nearly normal 48 hours later (Table 4). The levels at 45 min after
ischemia in the sham-operated group were served as controls.
Figure
1 Immunohistochemical
staining of phosphorylated p42/p44 MAPK in intestinal biopsies in
rats after ischemia/reperfusion injury (SP200). A:
Negative control of p42/p44 MAPK staining. There was no positive
expression signal in this group. B:
The expression of phosphorylated p42/p44 in intestinal biopsies in
the saline control group 2 hours after reperfusion. The activated
p42/p44 MAPK expression was localized in the cytoplasm and nuclei of
villus cells and in the nuclei of crypt cells, mainly in the
epithelium and villus cells. C:
Phosphorylated p42/p44 staining in the bFGF antibody pre-treated
group. The number of positive cells and intensity in this group were
weaker compared with those in the saline control and bFGF treated
groups. D: The
expression of phosphorylated p42/p44 in the bFGF treated group 2
hours after reperfusion. The activated p42/p44 MAPK expression was
localized in the cytoplasm and nuclei of villus cells and in the
nuclei of crypt cells, mainly in the epithelium and villus cells.
The number of positive cells in this group was more than that in the
bFGF antibody pre-treated group. ISH400.
Figure 2 Immunohistochemical
staining of phosphorylated p38 MAPK in intestinal biopsies in rats
after ischemia/reperfusion injury (SP200). A:
Negative control of p38 MAPK staining. There was no positive
expression signal in this group. B:
Phosphorylated p38 MAPK staining in the saline control group 2 hours
after reperfusion. Few p38 MAPK positive expression were localized
in the cytoplasm and nuclei of villus cells and in the nuclei of
crypt cells, mainly in the epithelium and villus cells. C:
P38 MAPK staining in the bFGF antibody pre-treated group. The number
of positive cells and localization of p38 MAPK positive cells were
similar with those in the saline group. D:
Phosphorylated p38 staining in the bFGF treated group 2 hours after
reperfusion. Activated p38 MAPK was localized primarily in the
nuclei of crypt cells, few in villus cells. The number of positive
cells was more than that in the saline control and bFGF antibody
pre-treated groups. In the bFGF treated group, the number of
positive expression cells of p38 MAPK as well as its intensity
peaked 2 hours after reperfusion.ISH×400
Table
1 Semi-quantitative
results of immunohistochemical staining for phosphorylated forms of
p42/p44 MAPK in different groups
| Groups |
Pre-injury |
2
hrs post-injury |
6
hrs post-injury |
24
hrs post-injury |
48 hrs post-injury |
| Group
B |
- |
++ |
++ |
+ |
++ |
| Group
C |
- |
+ |
++ |
+ |
+ |
| Group
D |
- |
+++ |
+++ |
+ |
+ |
"-"
represents no visible positive staining, "+" less than 10
stained cells and "++" 10-30 stained cells, while
"+++" represents more than 30 positively stained cells
within one high power field.
Table
2 Semi-quantitative
results of immunohistochemical staining for phosphorylated forms of
p38 MAPK in different groups
| Groups |
Pre-injury |
2 hrs post-injury |
6
hrs post-injury |
24
hrs post-injury |
48
hrs post-injury |
| Group
B |
- |
++ |
++ |
+ |
++ |
| Group
C |
- |
+ |
++ |
+ |
+ |
| Group
D |
- |
+++ |
++ |
+ |
+ |
"-"
represents no visible positive staining, "+" less than 10
stained cells and "++" 10-30 stained cells, while
"+++" represents more than 30 positively stained cells
within one high power field.
Table
3 Semi-quantitative
results of immunohistochemical staining for phosphorylated forms of
SAPK/JNK in different groups
| Groups |
Pre-injury |
2 hrs post-injury |
6
hrs post-injury |
24
hrs post-injury |
48
hrs post-injury |
| Group
B |
- |
+ |
+ |
++ |
+ |
| Group
C |
- |
+ |
+ |
+ |
+ |
| Group
D |
- |
+ |
+ |
++ |
+ |
"-"
represents no visible positive staining, "+" less than 10
stained cells and "++" 10-30 stained cells, while
"+++" represents more than 30 positively stained cells
within one high power field.
Table
4 The changes of
plasma D-lactate levels at different time points in three groups (mmol/L)
(x±s)
| Groups |
Animal
numbers |
Control |
2
hours |
6
hours |
24
hours |
48
hours |
| Group
B |
24 |
0.332±0.132 |
0.372±0.090 |
0.397±0.096 |
0.463±0.147 |
0.511±0.17
9 |
| Group
C |
24 |
0.332±0.132 |
0.309±0.079 |
0.327±0.098 |
0.415±0.177a |
0.425±0.208a |
| Group
D |
24 |
0.332±0.132 |
0.369±0.124 |
0.407±0.089 |
0.475±0.128 |
0.537±0.098 |
aP<0.05
vs compared with control.
Histological
evaluation
Intestinal I/R injury resulted in the damage of intestinal
barrier and the increase of mucosal permeability. HE staining showed
partial loss of the mucosa 2 hours after reperfusion. 6 hours after
reperfusion, however, the damage of intestinal epithelial cells,
hemorrhage and necrosis were observed and accompanied by
inflammatory cell infiltration into the intestinal wall.
Histological structure of the intestinal mucosa was markedly
improved after administration of bFGF.
DISCUSSION
Intestinal I/R injury causes release of bacteria and toxin from the
gut into the host blood circulation and changes of inflammatory
factors, cytokines and growth factors, resulting in damage to the
intestinal barrier and other internal organs[1-3,13-17].
We found that administration of exogenous basic fibroblast growth
factor (bFGF) could reduce the intestinal injury caused by I/R
insult. However, the mechanisms of this protective effect of bFGF
are not elucidated. BFGF is expressed in many normal adult tissues
and has mitogenic activity in a wide variety of cells of mesenchymal,
neuronal, and epithelial origins, and regulates events in normal
embryonic development, angiogenesis, wound repair, and neoplasia[18-20].
Also, it can regulate migration and replication of intestinal
epithelial cells in culture[21]. Recent studies have
shown that L-glutamine, tumor necrosis factor-a
and epidermal growth factor (EGF) stimulate proliferation of
intestinal crypt cells by activating the MAPK pathway, and that
p42/p44 MAPK activities are necessary for both cell cycle
progression and differentiation of the intestinal cells[22-25].
In many other cell types, growth factor controls proliferation and
differentiation via the MAPK pathway. MAPK is a common signal
pathway to transmit the mitogen or the differentiating signals from
the cell surface to the nucleus, and thus ultimately regulates
different gene expression[26-28]. Hence, we hypothesized
that MAPK activation might be involved in the regulation of bFGF
signals in the process of intestinal barrier repair.
To
investigate this hypothesis, we evaluated changes of the activated
MAPK signal pathway after administration of bFGF and bFGF
antibodies. We found that intestinal I/R injury stimulated the
activities of phosphorylated forms of the p42/p44 MAPK and p38MAPK
pathways, and increased the SAPK/JNK activity slightly. p42/p44 MAPK
and p38MAPK activities were increased 2 hours after reperfusion, and
peaked at 6 hours. At the same time, the levels of SAPK/JNK
increased slightly 24 hours after reperfusion compared with those of
the normal control. Phosphorylated forms of p42/p44 MAPK were mainly
localized in the nuclei of crypt cells and in the cytoplasm and
nuclei of villus cells, whereas those of p38MAPK were primarily
localized in the nuclei of crypt cells, few in villus cells. After
administration of bFGF, the expression of both p42/p44 MAPK and
p38MAPK was quickly stimulated, and the activation of both p42/p44
MAPK and p38MAPK peaked 2 hours after reperfusion, declined
gradually to normal at 48 hours. A coherence was noted between the
changes of p42/p44 MAPK and p38MAPK and histological findings. These
results indicate that intestinal I/R injury induces the activities
of the MAPK pathways, and p42/p44 MAPK and p38MAPK activities are
necessary for the protective effects of exogenous bFGF on intestinal
I/R injury. The early stimulation of the p42/p44 MAPK and p38MAPK
signal pathways may mediate the protective effects of bFGF on
intestinal dysfunction.
MAPK
family is composed of "extracellular
signal regulated" p42/p44 MAPK, "stress-regulated"
MAPK (SR-MAPKs), stress-activated protein kinases (SAPKs)/c-Jun
N-terminal kinases (JNKs) and p38-MAPKs. On stimulation, MAPKs are
translated into the nucleus where they may phosphorylate nuclear
transcription factors and thus regulate gene expression. The four
principal differentiated cell lineages of intestinal epithelium are
derived from common multipotent stem cells located near the base of
each crypt. These crypt stem cells divide to produce daughter stem
cells as well as more rapidly replicating transit cells, which in
turn undergo 4-6 rapid cell divisions in the proliferative zone
located in the lower half of each crypt[29,30].
Factors determining whether cells continue to proliferate,
cease dividing, and begin to differentiate, appear to operate during
the first gap phase (G1) of the cell cycle. P42/p44 is activated
during G0 to G1 transition, and the activity remains elevated up to
S phase entry, implicating this family of protein quinces in the
control of G1 progression[31,32]. Activation of p42/p44
MAPK is also necessary for growth factor-dependent proliferation of
some cell lines.
We propose
the possible mechanisms of the protective effects of bFGF on
intestinal I/R injury be involved in the activation of MAPK pathway.
First, to protect the survival of intestinal stem cells within crypt
and mediate the proliferation and differentiation of these cells.
Intestinal epithelium is maintained by continuous and rapid
replacement of differentiated epithelial cells by replication of
undifferentiated epithelial cells. Exogenous bFGF markedly enhances
the survival of crypt stem cells before and after irradiation injury[33].
Microvascular endothelial apoptosis is the primary lesion leading to
stem cell dysfunction, while endothelial apoptosis could be
inhibited by intravenous bFGF[34]. Second, to regulate
the inflammation reactions after I/R injury. The TNF translation by
IL-10 is inhibited mainly by inhibiting the activation of the p38
MAPK pathway[35]. This is necessary for maintenance of
immune homeostasis in the gut.
In
the perfused heart, ischemia/reperfusion activates stress-regulated
MAPKs, direct pharmacological activation of p38 triggers delayed
preconditioning of the heart, and there is minimal activation of the
p42/p44 MAPK subfamily by heart I/R injury[35-37]. Yet
phosphorylation of p42/p44 MAPK occurs consistently in the grey
matter penumbra of brain tissue after ischemic stroke, and may be
associated with neuronal survival and/or angiogenic activity in the
recovering brain tissue[38]. The results indicate that
the MAPK pathways respond differently to ischemic injury in
different sites.
The
changes of serum D (-)-lactate were used as a predictor of
intestinal I/R injury in this study. D (-)-lactate is the
stereoisomer of mammalian L (+)-lactate. Mammalian tissue does not
produce D (-)-lactate and only slowly metabolizes it. It is a strict
product of bacterial fermentation. Since mammals do not possess the
enzyme systems to rapidly metabolize D (-)-lactate[11, 39,40],
the released D (-)-lactate will pass through the gut barrier and
liver in an unchanged form and appear in the peripheral blood. As
intestinal ischemia injury causes mucosal injury and subsequent
bacterial proliferation, D (-)-lactate is released from gut into the
circulation. In this study, the serum D (-)-lactate level was
increased after injury, but in the bFGF treated group, it was not
significantly increased as in the control group, indicating that
bFGF exerts a positive protective effect on the mucosal barrier and
decreases the intestinal permeability.
In
summary, intestinal I/R injury induces the activities of the MAPK
pathways, and p42/p44 MAPK and p38MAPK activities are necessary for
the protective effect of exogenous bFGF on intestinal I/R injury.
The protective effect of bFGF on intestinal dysfunction may be
mediated by the early stimulation of the p42/p44 MAPK and p38 MAPK
signaling pathways.
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