Previous Article | Next Article 
Infection and Immunity, November 2000, p. 6108-6114, Vol. 68, No. 11
Department of
Pathology,1 and Division of Pulmonary and
Critical Care, Department of Internal
Medicine,2 University of Michigan Medical
School, Ann Arbor, Michigan
Received 23 February 2000/Returned for modification 30 May
2000/Accepted 4 August 2000
Previous studies have suggested that the C-C chemokine C10 is
involved in the chronic stages of host defense reactions. The present
study addressed the role of C10 in a murine model of septic peritonitis, induced by cecal ligation and puncture (CLP). Unlike other
C-C chemokines, C10 levels in the peritoneal wash were increased approximately 30-fold above baseline levels at 48 h after CLP surgery. Immunoneutralization of peritoneal C10 levels with polyclonal anti-C10 antiserum during CLP-induced peritonitis negatively impacted mouse survival over 4 days. In contrast, when 500 ng of recombinant murine C10 was administered immediately after CLP surgery, the 4-day
survival rate increased from 20% to over 60%. The C10 therapy appeared to facilitate a rapid and significant enhancement of the
levels of tumor necrosis factor alpha (TNF- Sepsis and sepsis-like
hyperinflammatory states are initiated after a host is exposed to
microbes or microbial products such as lipopolysaccharide (LPS), a
gram-negative bacterial cell wall component. The systemic inflammatory
response, which follows, is mediated by a number of complex,
interacting molecular networks, which include a large array of
mediators such as lipid metabolites, reactive nitrogen and oxygen
metabolites, lipids, nucleotides, and cytokines. Cytokines in
particular appear to function as central soluble initiators and
propagators of the septic inflammatory response. The systemic
production of the early-response, proinflammatory cytokines, tumor
necrosis factor alpha (TNF- Chemokines are distal mediators of the septic inflammatory response and
thus may offer novel avenues for therapy during sepsis. With the
exception of a number of circumstantial observations showing that
several chemokines are produced at higher levels in patients with
sepsis (6), little is known about the specific functions of
chemokines during this inflammatory disorder. However, several
general characteristics of chemokines cast these molecules as
potentially important participants in the septic response. By
definition, chemokines display chemotactic activities for various immune/inflammatory populations. Furthermore, many of the chemokines also appear to activate the cell population(s) for which they are
chemotactic. In this capacity, chemokines are intrinsically proinflammatory. On the other hand, chemokines have more recently been
attributed a variety of regulatory roles in such diverse processes as
fibrinogenesis, angiogenesis, and immune/inflammatory responses
(21). We hypothesized that those chemokines that display unique immunostimulatory properties may be especially relevant during
bacterial sepsis.
C10 chemokine displays amino acid sequence homology to a number of
CCR1-binding chemokines, all of which are structurally large chemokines
due to a genomic structure which contains an unique second exon
(3, 13, 20, 27). Furthermore, the portion of the C10
molecule encoded by this extra exon is necessary for its biological
activity (3). Interestingly, unlike many other chemokines,
C10 is IL-4 inducible but not LPS inducible in macrophages and IL-4
stimulation of these cells results in de novo C10 synthesis
(19). Upon appropriate cytokine stimulation, C10 production
by various cell populations appears to peak between 24 and 48 h
after cytokine stimulation (14, 19). In addition, C10
recruits a diverse array of cell populations including lymphocytes, macrophages, and eosinophils (14, 19). Thus, the present
study explored the possibility that C10 may modulate the host defense response, thereby promoting disease resolution and survival in a
clinically relevant experimental model of bacterial sepsis.
CLP model.
Specific-pathogen-free female CD-1 mice, 6 to l2
weeks old (Charles River Breeding Labs), were caged in groups of five
within the Specific-Pathogen-Free Unit of Laboratory Animal Medicine at
the University of Michigan until the day of each experiment. The cecal
ligation and puncture (CLP) model of acute sepsis was used as
previously described (24). Briefly, mice were anesthetized by an intraperitoneal (i.p.) injection of 3.0 to 3.5 mg of ketamine HCl
(Ketaset; Fort Dodge Laboratories) followed by inhaled methoxyflurane (Metafane; Pitman-Moore Inc.) as required for full anesthesia. A 1- to
2-cm longitudinal incision was made to the lower left quadrant of the
abdomen. The cecum was exposed, and the distal one-third was ligated
with 3-0 silk suture. The ligated cecum was punctured through and
through with a 21-gauge needle. Finally, the cecum was replaced in the
peritoneal cavity and the incision was closed with surgical staples. In
sham controls, the cecum was exposed but not ligated or punctured and
then was returned to the abdominal cavity. All mice were injected with
1 ml of sterile saline subcutaneously as a fluid resuscitation measure
immediately following surgery.
Experimental protocols.
Changes in endogenous C10, monocyte
chemoattractant protein-1 (MCP-1), macrophage inflammatory protein-1
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Chemokine C10 Promotes Disease Resolution and
Survival in an Experimental Model of Bacterial Sepsis
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
) and monocyte chemoattractant protein-1 (MCP-1) and a later increase in
interleukin-13 (IL-13) levels in the peritoneal cavity. In vitro
studies showed that the combination of IL-1
and C10 markedly
augmented TNF- synthesis by peritoneal macrophages and that C10
synthesis was induced in these cells following their exposure to IL-13.
At 24 h after CLP surgery, only 25% of C10-treated mice were
bacteremic versus 85% of the control group that exhibited
dissemination of bacteria into the circulation. The lack of bacteremia
in C10-treated mice appeared to be related, in part, to in vitro
evidence that C10 significantly enhanced the bacterial phagocytic
activity of peritoneal macrophages. In addition, in vivo evidence
suggested that C10 therapy significantly reduced the amount of material that leaked from the damaged gut. Taken together, the results of this
study demonstrate that the C10 chemokine rapidly promotes disease
resolution in the CLP model through its direct effects on the cellular
events critically involved in host defense during septic peritonitis.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
) and interleukin-1 (IL-1)
results in a number of inflammatory events, including widespread
inflammatory-cell recruitment and activation. TNF- and IL-1
instigate inflammation primarily by initiating cascades of downstream
mediators, such as pro- and anti-inflammatory cytokines and
chemokines (4). TNF- and IL-1 presumably play a
central role as proximal mediators of a wide range of vital downstream processes, which explains the failure of clinical therapies targeting these cytokines (1, 2, 8, 11, 12).
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
(MIP-1), and MIP-2 levels in the peritoneum after CLP were initially
examined. At 15 min and 6, 24, and 48 h after CLP surgery, groups
of five mice were killed and peritoneal fluid was obtained from each
mouse by lavaging the peritoneal cavity with 2 ml of sterile saline. Cell-free peritoneal samples were stored at 
20°C prior to
enzyme-linked immunosorbent assay (ELISA) analysis.
20°C prior to ELISA analysis.
Other groups of 10 mice were used to address the effect of recombinant
C10 therapy on the leakage of material from the gut after CLP surgery.
Mice received 5 mg of fluorescein isothiocyanate (FITC)-labeled dextran
(mean molecular mass, 40,000 kDa) per os at 24 and 48 h prior to
CLP surgery. At 24 h after the induction of sepsis by CLP surgery,
the mice were sacrificed and peritoneal lavages were performed with a
total volume of 1 ml of sterile saline. Neat and 1:10 dilutions of the
lavage fluid (100 µl) were added to a Costar flat-bottom, 96-well
microtiter plate (Corning Inc., Corning, N.Y.). The plates were read at
485 nm in a fluorescent plate reader. Standards were 1/2-log-unit
dilutions of FITC-dextran from 1 ng/ml to 1 µg/ml.
Determination of bacteremia. Serum samples were aseptically collected 24 h after CLP surgery. A 10-µl volume of each sample was plated on soy base blood agar plates (Difco). The plates were then incubated at 37°C for 24 h. Colony formation was taken as an indication of bacteremia.
Murine cytokine ELISA.
Cell-free peritoneal lavage samples
were subjected to cytokine ELISA. Murine C10, MCP-1, MIP-1, MIP-2,
TNF-, IL-13, and IL-10 were quantified using a modified
double-ligand assay as previously described (10). Briefly,
flat-bottom 96-well microtiter plates (Nunc Immuno-Plate I 96-F) were
coated at 50 µl/well with rabbit antibody against the various
cytokines (1 µg/ml in 0.6 M NaCl-0.26 M
H3BO4-0.08 M NaOH [pH 9.6]) for 16 h at
4°C and then washed with phosphate-buffered saline (PBS) (pH
7.5)-0.05% Tween 20 (wash buffer). Nonspecific binding sites were
blocked with 2% bovine serum albumin BSA in PBS and incubated for 90 min at 37°C. The plates were rinsed four times with wash buffer.
Diluted (neat and 1:10) cell-free supernatants (50 µl) in duplicate
were added, and the plates were incubated for 1 h at 37°C and
washed four times. Then biotinylated rabbit antibodies against the
specific cytokines (3.5 µg/ml in PBS [pH 7.5]-0.05% Tween 20-2%
fetal calf serum) were added at 50 µl/well. After being incubated at
37°C for 30 min, the plates were washed four times.
Streptavidin-peroxidase conjugate (Bio-Rad Laboratories, Richmond,
Calif.) was added, after which, the plates were again incubated at
37°C for 30 min. The plates were washed four times prior to the
addition of chromogen substrate (Bio-Rad Laboratories) and incubated at
room temperature to the desired extinction, and the reaction was
terminated with 50 µl of 3 M H2SO4 solution
per well. The plates were read at 490 nm in an ELISA reader. Standards
were 1/2-log-unit dilutions of recombinant murine cytokines from 1 pg/ml to 100 ng/ml. ELISA specificity was confirmed for each cytokine
and chemokine measured.
Peritoneal macrophage isolation and phagocytosis assay.
Mice
not subjected to CLP surgery were used for the isolation of peritoneal
macrophages. The peritoneal cavity was exposed, and approximately 10 ml
of sterile saline solution containing 0.05 M EDTA was injected into the
peritoneal cavity. The EDTA-saline solution was withdrawn using a
21-gauge needle. This procedure was repeated approximately three times
per mouse. Upon removal from the peritoneal cavity, the cell-containing
EDTA saline solution was immediately placed on ice. The cells were
pelleted by centrifugation at 1,500 rpm, after which the red blood
cells were lysed using an ammonium chloride red blood cell lysis
buffer. The cells were washed twice in RPMI, after which they were
resuspended in RPMI 1640 containing 10% fetal bovine serum. The
generation of C10 by peritoneal macrophages was evaluated in cultures
of 106 cells exposed for 24 h to either supplemented
RPMI alone or RPMI containing LPS, IL-1, or IL-13. The generation of
TNF- by peritoneal macrophages was determined in cultures of
106 cells exposed for 6 h to IL-1 alone or IL-1
plus C10. Unless otherwise stated, LPS was used at 1 µg/ml and all
cytokines were used at 100 ng/ml. Macrophage phagocytic potential was
evaluated, using a modification of a previously described method
(23). Peritoneal macrophages were incubated for 1 h at
37°C in Hanks' balanced salt solution in eight-well Labteks plates
(Nunc Inc., Naperville, Ill.). Escherichia coli cells
(106) were added to each well, and the plates were
incubated on a shaker at 37°C for 1 h. The supernatants were
removed, and the cells were washed in Hanks' balanced salt solution.
The gasket was removed, and the slides were allowed to air dry, after
which a Diff-Quik (Baxter, McGraw Park, Ill.) staining procedure was performed. Two hundred cells per well were counted to determine the
mean number of intracellular E. coli cells per well.
Statistical analysis. Analysis of variance (ANOVA) followed by Dunnett's test was used in all experiments in which multiple experimental groups were compared to a single control group. A two-tailed Student t test was utilized to assess significance for experiments comparing a single experimental group to a single control. Survival curves were analyzed by the log rank test. All calculations were performed using Prism 2.0 (Graphpad Software, Inc., San Diego, Calif.) or Primer of Biostatistics 3.01 (McGraw-Hill). Significance was assigned for P < 0.05.
| |
RESULTS |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
CLP surgery augments and sustains C10 levels above other C-C
chemokines in the peritoneal cavity.
Previous studies have
documented that chemokine levels are markedly increased during the
course of septic peritonitis after CLP surgery (15, 26). In
the present study, we first examined whether changes in peritoneal
levels of C10 mirrored those of other C-C chemokines such as MCP-1,
MIP-1, and MIP-2 after CLP. To this end, peritoneal levels of all
four chemokines were measured by ELISA. Compared to baseline peritoneal
levels, C10 levels in the peritoneal cavity were markedly elevated at
all times after CLP surgery (Fig. 1). At
48 h after CLP surgery, peritoneal fluids contained 30-fold-higher
levels of C10 than that measured in the peritoneum prior to surgery. In
contrast, MCP-1, MIP-1, and MIP-2 were detected at lower
concentrations in peritoneal fluid before and at all times after CLP.
Furthermore, peak levels of MCP-1 and MIP-1 were measured at 24 h after CLP and the levels of both chemokines were near baseline levels
at 48 h after CLP surgery. The dramatic and sustained increase of
C10 levels after CLP surgery clearly suggested that C10 played a
prominent role during septic peritonitis.
|
Anti-C10 antiserum augments whereas exogenous C10 protein prevents
CLP-induced mortality.
Several studies showing a correlation
between chemokine production and sepsis-associated mortality have
demonstrated that chemokines function as deleterious (MIP-2
[26]) and beneficial (MCP-1 [15])
inflammatory mediators during sepsis. We attempted to determine whether
increased C10 levels in the peritoneal cavity contributed to
sepsis-induced mortality by neutralizing C10 in the context of CLP
surgery. Normal rabbit preimmune serum or anti-C10 antiserum was
administered i.p. 2 h prior to CLP surgery. The administration of
normal rabbit preimmune serum to mice prior to CLP surgery was
protective since more than 60% of these mice were alive on day 4 after
CLP surgery (Fig. 2A), consistent with previous observations in this CLP model (15). The protective effect of normal rabbit serum in the CLP model appears to be a consequence of the macrophage activating factors present within this
biological fluid (A. Matsukawa, unpublished data). In addition, we have
never detected any cytokine or chemokine in rabbit serum that
cross-reacts with murine C10 chemokine. In contrast, when mice received
the same volume of rabbit serum containing polyclonal anti-C10
antibodies, only 35% of these mice were alive on day 4 after CLP (Fig.
2A). These data suggested that endogenous C10 was required for mouse
survival during CLP-induced sepsis.
|
Recombinant C10 therapy significantly enhances MCP-1, TNF-, and
IL-13 levels in the peritoneum after CLP surgery.
Emerging
evidence suggests that C10 may modulate the production of chemokines
such MCP-1 and cytokines such as IL-13 (14). Furthermore,
TNF- (9) and MCP-1 (15) have major
immune-enhancing and protective effects in CLP models. Recent studies
in this laboratory have shown that endogenous IL-13 is required for
mouse survival following CLP surgery, because of the immunomodulatory
effects of this cytokine (16). These previous findings
provided the impetus to examine the effect of C10 therapy on the
peritoneal chemokine and cytokine profile associated with CLP-induced
sepsis. In C10-treated mice, peritoneal levels of TNF- and MCP-1
were significantly elevated at 15 min after CLP surgery compared with those in CLP controls at this time (Fig.
3). Peritoneal levels of TNF- and
MCP-1 were similar in control and C10-treated mice at 6 h after
CLP surgery (data not shown). Figure 4
depicts the temporal changes in IL-13 levels in peritoneal washes from
control and C10-treated mice before and 6 and 24 h after CLP
surgery and shows that peritoneal IL-13 levels were significantly
elevated in C10-treated mice compared with control mice at 24 h
after CLP surgery. Thus, the exogenous addition of C10 after CLP
surgery rapidly increased levels of two major proinflammatory mediators that promote the clearance of bacteria from the septic peritoneum. In
addition, this therapy promoted the production of IL-13 in the septic
peritoneal cavity, suggesting that immunomodulatory processes were
activated by C10 during sepsis.
|
|
The combination of IL-1 and C10 induces TNF- production by
peritoneal macrophages.
To determine whether C10 induced TNF-
production after CLP surgery, we costimulated peritoneal macrophages in
vitro with septic inflammatory mediators and C10. Neither IL-1 nor
C10 alone induced the release of TNF- by peritoneal macrophages
incubated in vitro for 6 h. However, in the presence of IL-1,
C10 induced TNF- production in a dose-dependent manner, which was
evident after 6 h of culture (Fig.
5A). These data suggested that peritoneal macrophages, in the septic inflammatory setting, probably respond to
C10 therapy by producing TNF-.
|
IL-13 is a potent inducer of C10 production by peritoneal
macrophages.
C10 is a unique C-C chemokine in that it is induced
by IL-4 but not by LPS (19). However, IL-4 is not normally
associated with innate immune responses elicited by septic peritonitis,
and we did not detect it at any time after the CLP-mediated induction of sepsis in the present study. Therefore, we examined whether other
cytokines associated with CLP, namely, IL-1 (18) and IL-13 (16), affected the synthesis of C10 by peritoneal
macrophages. Additional impetus for this study came from the present in
vivo studies showing that IL-13 was constitutively present and induced in the peritoneal cavity after CLP surgery. Compared with cultures exposed to medium alone, LPS, TNF-, or IL-1, the most potent inducer of C10 production by peritoneal macrophages cultured in vitro
was IL-13, as demonstrated by the presence of more than 3 ng of C10 per
ml after 24 h (Fig. 5B).
C10 protein therapy attenuates bacterial infiltration of the
systemic circulation during CLP-induced sepsis: effects on macrophage
phagocytosis and gut leakage.
It is well established in bacterial
sepsis that the development of bacteremia is often a prequel to death
(7). Thus, we examined the incidence of bacteremia after CLP
surgery and in the context of C10 protein therapy. Mice underwent CLP
surgery, and experimental animals received a 500-ng i.p. injection of
C10 immediately after surgery. Bacteremia was assessed 24 h after CLP surgery by incubating serum samples from experimental and control
animals on a nonselective growth medium. C10 protein therapy convincingly attenuated bacterial infiltration of the systemic circulation, as manifested by a significant (P 
0.05)
reduction in the percentage of bacteremic mice from 85% in the control
group (n = 13) to 25% in the C10-treated group
(n = 12).
|
|
| |
DISCUSSION |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
Clinically, the diagnosis of sepsis must satisfy two general requirements (5). The patient must present with symptoms of systemic hyperinflammation, also known as the systemic inflammatory response syndrome. Additionally, the diagnosis of sepsis requires documented evidence of infection. These diagnostic criteria highlight the challenge that the immune system faces during a septic episode. The host must rein in the hyperinflammatory response while simultaneously containing the bacterial infection. Similarly, the design of novel therapeutics must reflect the paradoxical features of sepsis syndrome. Thus, these defining features of clinical sepsis guided our further exploration of the therapeutic mechanism and clinical relevance of C10 therapy in sepsis.
Although the production of various chemokines from both the C-C and CxC
superfamilies has been correlated with the pathologic changes
associated with septic peritonitis (25, 26), the C-C chemokine C10 has not previously been examined in the context of an
acute inflammatory response like sepsis. Unlike many other chemokines,
C10 is IL-1, IL-4, and IL-13 but not LPS inducible (19).
Thus, we were interested in determining whether an acute inflammatory
response to bacterial pathogens would result in upregulated C10
production. Interestingly, mice that had undergone CLP surgery clearly
produced more C10 than other C-C chemokines at each time point examined
(6, 24, and 48 h after CLP surgery). In addition, although other
C-C chemokines were at or near baseline levels at 48 h after CLP
surgery, the C10 levels remained 30-fold higher than the baseline
levels. These findings are consistent with those of Wu et al.
(28), who recently showed that C10 accumulation was
sustained for 10 days after the intraperitoneal introduction of
thioglycolate. In this sterile peritonitis model, the pattern of
expression of C10 was unique since MIP-1 expression occurred early
and was transient (28). Thus, there is a growing consensus that C10 is involved in the later stages of the inflammatory process, although its precise role is still under investigation.
The observed pattern of C10 production following CLP surgery suggested two divergent possibilities. (i) Because CLP-induced C10 production at 48 h after CLP surgery greatly exceeded production at earlier time points, septic mice might have suffered from an acute deficiency in C10. (ii) Because C10 production during CLP-induced sepsis correlated with sepsis-induced death, C10 might have functioned as a deleterious mediator of sepsis. The former possibility was addressed by the immunoneutralization of C10 during CLP-induced sepsis, which resulted in a substantial increase in sepsis-related mortality. In contrast, the administration of recombinant C10 protein to mice immediately after CLP surgery yielded an impressive therapeutic effect, improving survival from 20 to 60%. Thus, these data suggest that C10 production during CLP-induced sepsis constitutes a necessary host response. Subsequent experimentation was aimed at determining the therapeutic mechanism and potential clinical significance of C10 therapy for sepsis.
We analyzed the temporal production of a number of inflammatory
mediators by mice that had undergone CLP surgery and treatment with C10
protein, in order to evaluate the effect of C10 therapy on the septic
inflammatory state. The administration of C10 significantly increased
peritoneal TNF- and MCP-1 levels at 15 min after CLP surgery.
TNF- has been previously shown to exert a major protective effect
during CLP-induced septic peritonitis (9), whereas MCP-1 stimulates local immunity by augmenting macrophage microbicidal and
phagocytic function and by facilitating neutrophil and macrophage recruitment (17). To further dissect the ability of C10 to
stimulate TNF- synthesis, peritoneal macrophages were stimulated
with C10 concomitant with other proinflammatory cytokines commonly
produced during a septic response. In the presence of IL-1, C10
induced TNF- production by peritoneal macrophages in a
dose-dependent manner. While C10 therapy appeared to rapidly enhance
the peritoneal production of proinflammatory mediators such as TNF-
and MCP-1, by 24 h after CLP surgery the predominant cytokine in
peritoneal washes from C10-treated mice was IL-13. Although IL-13 is an
established Th2-type anti-inflammatory cytokine, our laboratory has
also demonstrated a beneficial role for IL-13 in the setting of
CLP-induced sepsis (16), and results of the present study
suggested that it was a potent stimulus of C10 production by isolated
peritoneal macrophages. Taken together, these findings suggested that
C10 rapidly induced immune events in the peritoneal cavity that
involved the production of cytokines relevant to a beneficial outcome
after CLP surgery.
We further examined the therapeutic potential of C10 by assessing whether the controlled enhancement of local inflammation positively affected clinically relevant parameters of bacterial containment. Bacteria play a central yet paradoxical role in the pathogenesis of sepsis, since bacterial components initiate the overwhelming inflammatory response that characterizes sepsis. Yet, an impotent host inflammatory response can result in uncontrolled bacterial growth, leading to bacterial infiltration of the systemic circulation. Clearly, the development of bacteremia is a common prequel to death in many septic cases (7). The administration of recombinant C10 chemokine to mice significantly reduced the incidence of bacteremia at 24 h after CLP surgery. This impressive maintenance of circulatory sterility after C10 therapy probably resulted from some enhancement in bacterial containment within the peritoneum. This hypothesis was supported by in vitro experiments showing that the stimulation of peritoneal macrophages with C10 enhanced their phagocytic capacity. During clinical and experimental sepsis, the bowel wall represents an important barrier to the overwhelming infiltration of intestinal microbes into the peritoneal cavity and subsequently into the systemic circulation (24). However, once pathogenic agents have subverted the intestinal barrier function, the resident peritoneal macrophage represents the first and perhaps most important line of defense. Likewise, the administration of C10 to animals that had undergone CLP surgery significantly attenuated the leakage of FITC-labeled dextran from the bowel into the intestine. While the effect of C10 on the host defense response requires further investigation, these data suggest that C10 enhances bacterial containment in septic mice by enabling the peritoneal macrophage to better control the bacteria that do subvert the intestinal barrier and by attenuating the leakage of intestinal microbes into the peritoneal cavity.
In conclusion, C10 displayed a therapeutically potent yet focused enhancement of inflammatory parameters, which enabled septic mice to contain microbial invaders of the peritoneum while preventing the exacerbation of systemic inflammation. Due to the ever-increasing incidence of antibiotic-resistant bacteria, it is becoming increasingly important to develop methods of safely enhancing the host immune function during a bacterial or septic insult. The unique resolution-promoting properties of the chemokine C10 during murine bacterial sepsis validate an additional examination of the therapeutic potential of human C10 homologues for the treatment of human sepsis.
| |
ACKNOWLEDGMENTS |
|---|
This work was supported by National Institutes of Health grants IP50HL56402, HL35276, HL31963, AI36302, IP50HL60289, and CA66180.
| |
FOOTNOTES |
|---|
* Corresponding author. Mailing address: Department of Pathology, University of Michigan Medical School, 1301 Catherine Rd., Ann Arbor, MI 48109-0602. Phone: (734) 936-1020. Fax: (734) 764-2397. E-mail: slkunkel{at}umich.edu.
Editor: R. N. Moore
| |
REFERENCES |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
| 1. | Abraham, E., A. Anzueto, G. Gutierrez, S. Tessler, G. San Pedro, R. Wunderink, A. Dal Nogare, S. Nasraway, S. Berman, R. Cooney, H. Levy, R. Baughman, M. Rumbak, R. B. Light, L. Poole, R. Allred, J. Constant, J. Pennington, and S. Porter. 1998. Double blind randomized controlled trial of monoclonal antibody to human tumor necrosis factor in treatment of septic shock. NORASEPT II Study Group. Lancet 351:929-933[Medline]. |
| 2. |
Abraham, E.,
R. Wunderink,
H. Silverman,
T. M. Perl,
S. Nasraway,
H. Levy,
R. Bone,
R. P. Wenzel,
R. Balk,
R. Allred, et al.
1995.
Efficacy and safety of monoclonal antibody to human tumor necrosis factor alpha in patients with sepsis syndrome. A randomized, controlled, double-blind, multicenter clinical trial. TNF-alpha MAb Sepsis Study Group.
JAMA
273:934-941 |
| 3. | Berger, M. S., D. D. Taub, A. Orlofsky, T. R. Kleyman, B. Coupaye-Gerard, D. Eisner, and S. A. Cohen. 1996. The chemokine C10: immunological and functional analysis of the sequence encoded by the novel second exon. Cytokine 8:439-447[CrossRef][Medline]. |
| 4. |
Blackwell, T., and J. Christman.
1996.
Sepsis and cytokines: current status.
Br. J. Anaesth.
77:110-117 |
| 5. |
Bone, R. C.,
R. A. Balk,
F. B. Cerra,
R. P. Dellinger,
A. M. Fein,
W. A. Knaus,
R. M. H. Schein, and W. J. Sibbald.
1992.
Definitions for sepsis and organ failure and guidelines for the use of innovative therapies in sepsis. The ACCP/SCCM Consensus Conference Committee American College of Chest Physicians Society of Critical Care Medicine.
Chest
101:1644-1655 |
| 6. |
Bossink, A. W.,
L. Paemen,
P. M. Jansen,
C. E. Hack,
L. G. Thijs, and J. Van Damme.
1995.
Plasma levels of the chemokines monocyte chemotactic proteins-1 and -2 are elevated in human sepsis.
Blood
86:3841-3847 |
| 7. |
Brun-Buisson, C.,
F. Doyon,
J. Carlet,
P. Dellamonica,
F. Gouin,
A. Leptoutre,
J. C. Mercier,
G. Offenstadt, and B. Regnier.
1995.
Incidence, risk factors and outcome of severe sepsis and septic shock in adults. A multicenter prospective study in intensive care units.
JAMA
274:968-974 |
| 8. | Cohen, J., and J. Carlet. 1996. INTERSEPT: An international, multicenter, placebo-controlled trial of monoclonal antibody to human tumor necrosis factor-alpha in patients with sepsis. Crit. Care Med. 24:1431-1440[CrossRef][Medline]. |
| 9. | Echtenacher, B., D. N. Mannel, and L. Hultner. 1996. Critical protective role of mast cells in a model of acute septic peritonitis. Nature 381:75-77[CrossRef][Medline]. |
| 10. | Evanoff, H., M. Burdick, S. Moore, S. Kunkel, and R. Strieter. 1992. A sensitive ELISA for the detection of human monocyte chemoattractant protein-1 (MCP-1). Immunol. Investig. 21:39-45[Medline]. |
| 11. |
Fisher, C. J., Jr.,
J. M. Agosti,
S. M. Opal,
S. F. Lowry,
R. A. Balk,
J. C. Sadoff,
E. Abraham,
R. M. Schein, and E. Benjamin.
1996.
Treatment of septic shock with the tumor necrosis factor receptor:Fc fusion protein. The Soluble TNF Receptor Sepsis Study Group.
N. Engl. J. Med.
334:1697-1702 |
| 12. |
Fisher, C. J., Jr.,
J. F. Dhainaut,
S. M. Opal,
J. P. Pribble,
R. A. Balk,
G. J. Slotman,
T. J. Iberti,
E. C. Rackow,
M. J. Shapiro,
R. L. Greenman, et al.
1994.
Recombinant human interleukin 1 receptor antagonist in the treatment of patients with sepsis syndrome. Results from a randomized, double-blind, placebo-controlled trial. Phase III rhIL-1ra Sepsis Syndrome Study Group.
JAMA
271:1836-1843 |
| 13. | Hara, T., K. B. Bacon, L. C. Cho, A. Yoshimura, Y. Morikawa, N. G. Copeland, D. J. Gilbert, N. A. Jenkins, T. J. Schall, and A. Miyajima. 1995. Molecular cloning and functional characterization of a novel member of the C-C chemokine family. J. Immunol. 155:5352-5358[Abstract]. |
| 14. |
Hogaboam, C. M.,
C. S. Gallinat,
D. D. Taub,
R. M. Strieter,
S. L. Kunkel, and N. W. Lukacs.
1999.
Immunomodulatory role of C10 chemokine in a murine model of allergic bronchopulmonary aspergillosis.
J. Immunol.
162:6071-6079 |
| 15. |
Matsukawa, A.,
C. M. Hogaboam,
N. W. Lukacs,
P. M. Lincoln,
R. M. Strieter, and S. L. Kunkel.
1999.
Endogenous monocyte chemoattractant protein-1 (MCP-1) protects mice in a model of acute septic peritonitis: cross-talk between MCP-1 and leukotriene B4.
J. Immunol.
163:6148-6154 |
| 16. |
Matsukawa, A.,
C. M. Hogaboam,
N. W. Lukacs,
P. M. Lincoln,
H. L. Evanoff,
R. M. Strieter, and S. L. Kunkel.
2000.
Expression and contribution of endogenous IL-13 in an experimental model of sepsis.
J. Immunol.
164:2738-2744 |
| 17. |
Nakano, Y.,
T. Kasahara,
N. Mukaida,
Y. C. Ko,
M. Nakano, and K. Matsushima.
1994.
Protection against lethal bacterial infection in mice by monocyte-chemotactic and -activating factor.
Infect. Immun.
62:377-383 |
| 18. | O'Reilly, M., G. M. Silver, J. H. Davis, R. L. Gamelli, and J. C. Hebert. 1992. Interleukin 1 beta improves survival following cecal ligation and puncture. J. Surg. Res. 52:518-522[CrossRef][Medline]. |
| 19. | Orlofsky, A., E. Y. Lin, and M. B. Prystowsky. 1994. Selective induction of the beta chemokine C10 by IL-4 in mouse macrophages. J. Immunol. 152:5084-5091[Abstract]. |
| 20. |
Pardigol, A.,
U. Forssmann,
H. D. Zucht,
P. Loetscher,
P. Schulz-Knappe,
M. Baggiolini,
W. G. Forssmann, and H. J. Magert.
1998.
HCC-2, a human chemokine: gene structure, expression pattern, and biological activity.
Proc. Natl. Acad. Sci. USA
95:6308-6313 |
| 21. |
Rollins, B. J.
1997.
Chemokines.
Blood
90:909-928 |
| 22. | Sartor, R. B. 1995. Current concepts of the etiology and pathogenesis of ulcerative colitis and Crohn's disease. Gastroenterol. Clin. North Am. 24:475-507[Medline]. |
| 23. |
Steinhauser, M. L.,
C. M. Hogaboam,
S. L. Kunkel,
N. W. Lukacs,
R. M. Strieter, and T. J. Standiford.
1999.
IL-10 is a major mediator of sepsis-induced impairment in lung antibacterial host defense.
J. Immunol.
162:392-399 |
| 24. |
Steinhauser, M. L.,
C. M. Hogaboam,
N. W. Lukacs,
R. M. Strieter, and S. L. Kunkel.
1999.
Multiple roles for IL-12 in a model of acute septic peritonitis.
J. Immunol.
162:5437-5443 |
| 25. | Walley, K., N. Lukacs, T. Standiford, R. Strieter, and S. Kunkel. 1997. Elevated levels of macrophage inflammatory protein 2 in severe murine peritonitis increase neutrophil recruitment and mortality. Infect Immun. 65:3847-3851[Abstract]. |
| 26. | Walley, K. R., N. W. Lukacs, T. J. Standiford, R. M. Strieter, and S. L. Kunkel. 1996. Balance of inflammatory cytokines related to severity and mortality of murine sepsis. Infect. Immun. 64:4733-4738[Abstract]. |
| 27. | Wang, W., K. B. Bacon, E. R. Oldham, and T. J. Schall. 1998. Molecular cloning and functional characterization of human MIP-1 delta, a new C-C chemokine related to mouse CCF-18 and C10. J. Clin. Immunol. 18:214-222[CrossRef][Medline]. |
| 28. | Wu, Y., M. B. Prystowsky, and A. Orlofsky. 1999. Sustained high-level production of murine chemokine C10 during chronic inflammation. Cytokine 11:523-530[CrossRef][Medline]. |
Infection and Immunity, November 2000, p. 6108-6114, Vol. 68, No. 11
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
This article has been cited by other articles:
-
Coelho, A. L., Schaller, M. A., Benjamim, C. F., Orlofsky, A. Z., Hogaboam, C. M., Kunkel, S. L.
(2007). The Chemokine CCL6 Promotes Innate Immunity via Immune Cell Activation and Recruitment. J. Immunol.
179: 5474-5482
[Abstract] [Full Text] -
Noda, S., Aguirre, S. A., Bitmansour, A., Brown, J. M., Sparer, T. E., Huang, J., Mocarski, E. S.
(2006). Cytomegalovirus MCK-2 controls mobilization and recruitment of myeloid progenitor cells to facilitate dissemination. Blood
107: 30-38
[Abstract] [Full Text] -
Berahovich, R. D., Miao, Z., Wang, Y., Premack, B., Howard, M. C., Schall, T. J.
(2005). Proteolytic Activation of Alternative CCR1 Ligands in Inflammation. J. Immunol.
174: 7341-7351
[Abstract] [Full Text] -
Ness, T. L., Carpenter, K. J., Ewing, J. L., Gerard, C. J., Hogaboam, C. M., Kunkel, S. L.
(2004). CCR1 and CC Chemokine Ligand 5 Interactions Exacerbate Innate Immune Responses during Sepsis. J. Immunol.
173: 6938-6948
[Abstract] [Full Text] -
Ma, B., Zhu, Z., Homer, R. J., Gerard, C., Strieter, R., Elias, J. A.
(2004). The C10/CCL6 Chemokine and CCR1 Play Critical Roles in the Pathogenesis of IL-13-Induced Inflammation and Remodeling. J. Immunol.
172: 1872-1881
[Abstract] [Full Text] -
Benjamim, C. F., Hogaboam, C. M., Lukacs, N. W., Kunkel, S. L.
(2003). Septic Mice Are Susceptible to Pulmonary Aspergillosis. Am. J. Pathol.
163: 2605-2617
[Abstract] [Full Text] -
Ness, T. L., Hogaboam, C. M., Strieter, R. M., Kunkel, S. L.
(2003). Immunomodulatory Role of CXCR2 During Experimental Septic Peritonitis. J. Immunol.
171: 3775-3784
[Abstract] [Full Text] -
Oliveira, S. H. P., Taub, D. D., Nagel, J., Smith, R., Hogaboam, C. M., Berlin, A., Lukacs, N. W.
(2002). Stem cell factor induces eosinophil activation and degranulation: mediator release and gene array analysis. Blood
100: 4291-4297
[Abstract] [Full Text] -
Matsukawa, A., Kaplan, M. H., Hogaboam, C. M., Lukacs, N. W., Kunkel, S. L.
(2001). Pivotal Role of Signal Transducer and Activator of Transcription (Stat)4 and Stat6 in the Innate Immune Response during Sepsis. JEM
193: 679-688
[Abstract] [Full Text]
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
Copyright © 2009 by the American Society for Microbiology. For an alternate route to Journals.ASM.org, visit: http://intl-journals.asm.org | More Info»