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Previous Article | Next Article 
Infect Immun, April 1998, p. 1400-1407, Vol. 66, No. 4
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Endotoxin-Neutralizing Protein Protects against
Endotoxin-Induced Endothelial Barrier Dysfunction
Douglas D.
Bannerman,1
Michael J.
Fitzpatrick,1
Dell Y.
Anderson,2
Apurba K.
Bhattacharjee,3
Thomas J.
Novitsky,4
Jeffrey D.
Hasday,2
Alan S.
Cross,2 and
Simeon E.
Goldblum2,*
Departments of
Pathology1 and
Medicine,2 VA Maryland Health Care
System, University of Maryland School of Medicine, Baltimore, Maryland
21201;
Walter Reed Army Institute of Research, Washington, D.C.
203073; and
Associates of Cape Cod,
Falmouth, Massachusetts 025404
Received 7 August 1997/Returned for modification 6 October
1997/Accepted 8 January 1998
 |
ABSTRACT |
Bacterial lipopolysaccharide induces tyrosine phosphorylation of
paxillin, actin reorganization, and opening of the transendothelial paracellular pathway through which macromoles flux. In this study, lipid A was shown to be the bioactive portion of the lipopolysaccharide molecule responsible for changes in endothelial barrier function. We
then studied whether endotoxin-neutralizing protein, a recombinant peptide that is derived from Limulus antilipopolysaccharide
factor and targets lipid A, could block the effects of
lipopolysaccharide on protein tyrosine phosphorylation, actin
organization, and movement of 14C-bovine serum albumin
across bovine pulmonary artery endothelial cell monolayers. In the
presence of serum, a 6-h exposure to lipopolysaccharide (10 ng/ml)
increased transendothelial 14C-albumin flux compared to the
simultaneous media control. Coadministration of endotoxin-neutralizing
protein (
10 ng/ml) with lipopolysaccharide (10 ng/ml) protected
against lipopolysaccharide-induced barrier dysfunction. This protection
was dose dependent, conferring total protection at
endotoxin-neutralizing protein/lipopolysaccharide ratios of 10:1.
Similarly, endotoxin-neutralizing protein was capable of blocking the
lipopolysaccharide-induced endothelial cell responses that are
prerequisite to barrier dysfunction, including tyrosine phosphorylation
of paxillin and actin depolymerization. Finally, endotoxin-neutralizing
protein cross-protected against lipopolysaccharide derived from diverse
gram-negative bacteria. Thus, endotoxin-neutralizing protein offers a
novel therapeutic intervention for the vascular endothelial dysfunction
of gram-negative sepsis and its attendant endotoxemia.
| |
INTRODUCTION |
Gram-negative septic processes can
be complicated by endothelial cell (EC) injury and/or dysfunction that
contributes to systemic vascular collapse, disseminated intravascular
coagulation, and vascular leak syndromes, including the adult
respiratory distress syndrome (ARDS) (5, 26). Endotoxin or
bacterial lipopolysaccharide (LPS) has been implicated as the bacterial
component responsible for much of the EC injury associated with
gram-negative bacterial infections. First, LPS bioactivity has been
detected in the bloodstream of gram-negative septicemic patients, and
in some studies, particularly those focusing on meningococcal sepsis,
levels of circulating LPS predict development of multiple organ
failure, including the adult respiratory distress syndrome
(31). Second, administration of LPS alone to experimental
animals reproduces the EC injury seen after gram-negative bacterial
challenge (13, 26). Lastly, in some animal studies,
interventions that specifically target the LPS molecule appear to
protect against the EC complications associated with gram-negative
sepsis or experimental LPS challenge (1, 33, 34). The
efficacy of most of these interventions has yet to be evaluated in
humans.
Most bactericidal antibiotics that target viable, replicating
gram-negative bacteria do not diminish LPS activity and can actually
liberate free LPS into the circulation (1). One notable exception, polymyxin B (PMB) derived from the bacteria Bacillus polymyxa (6, 23), can bind to the lipid A portion of
LPS and neutralize it. In the past, however, PMB's nephrotoxic
properties have severely limited its therapeutic application. Other
naturally occurring proteins which also bind to and neutralize LPS
include bactericidal/permeability-increasing protein (BPI) and cationic antimicrobial protein 18 found in polymorphonuclear leukocytes (10, 17), high- and low-density lipoproteins (20,
25), and the Limulus anti-LPS factor (LALF) found in
the horseshoe crab, Limulus polyphemus (22). LALF
is a 11.8-kDa protein isolated from the amebocyte, the single blood
cell type found in the horseshoe crab (22). The
amebocyte-derived LALF as well as its recombinant form,
endotoxin-neutralizing protein (ENP), each binds to and neutralizes LPS
(22, 32). The LPS-binding site is 32 to 50 amino acids in
length and forms an amphipathic loop which binds to the lipid A portion
of LPS (18, 24, 32). ENP or LALF neutralizes LPS bioactivity
in the Limulus amebocyte lysate assay (11, 32),
prevents macrophage production of tumor necrosis factor in vitro
(4), and protects against LPS challenge in vivo (11,
33).
LPS interaction with cells of monocytic lineage has been well
characterized. These cells express membrane-bound CD14, a
glycosylphosphatidylinositol-anchored protein which can recognize
complexes of LPS and LPS-binding protein, resulting in cell activation
(12, 30, 35). In EC, which lack membrane-bound CD14, a
specific EC-binding site(s) or receptor(s), although implied, has not
yet been demonstrated. Circulating LPS, in concert with the accessory
molecules LPS-binding protein and soluble CD14, can be presented to the
non-CD14-bearing EC, evoking EC responses through as yet unidentified
mechanisms (12, 14). One such EC response involves a
sequence of events comprised of protein tyrosine phosphorylation, actin
depolymerization, intercellular gap formation, and loss of EC barrier
function (3). The initial tyrosine phosphorylation events
are clearly a prerequisite to LPS-induced actin changes and disruption
of EC monolayer integrity (3). Further, prior F-actin
stabilization of EC monolayers with phallicidin protects against
LPS-induced increments in transendothelial albumin flux
(15). We therefore studied whether a molecule such as ENP,
which binds to lipid A and has been shown to confer protection against
the deleterious effect of LPS in vivo, could block one or more of the
sequential LPS-induced events leading to increased EC monolayer
permeability. In this work, we have studied whether ENP protects
against LPS-induced protein tyrosine phosphorylation, actin
reorganization, and loss of endothelial barrier function.
| |
MATERIALS AND METHODS |
Reagents.
LPSs phenol extracted from Escherichia
coli serotype O111:B4, E. coli O55:B5, Klebsiella
pneumoniae, Pseudomonas aeruginosa, Salmonella
minnesota, and Serratia marcescens (Sigma Chemical Co.,
St. Louis, Mo.) were suspended in phosphate-buffered saline (PBS) at 5 mg/ml, and these stock solutions were stored at 4°C. Lipid A from
E. coli K-12 (List Biological Laboratories, Campbell, Calif.) was dissolved into chloroform (69%)-methanol (27%)-water (4%) and evaporated under nitrogen, and the dry residue was
resuspended in water. To prepare the O-polysaccharide fraction,
E. coli O111:B4 LPS was hydrolyzed at 100°C for 2 h
with 1% acetic acid, neutralized with 1.0 M NaOH, and centrifuged. The
supernatant containing the O polysaccharide was desalted on a Sephadex
G-25 (Pharmacia Biotech, Piscataway, N.J.) column, using water as the
elutant, and the fractions were tested for O polysaccharide by the
phenol sulfuric acid method of Dubois et al. (9). The
O-polysaccharide-positive fractions were pooled and lyophilized. ENP
was a gift from the Associates of Cape Cod (Woods Hole, Mass.). ENP was
reconstituted at 1 mg/ml in PBS, aliquoted, and stored at 
20°C. PMB
sulfate (Sigma) was reconstituted at 25.8 mg/ml and stored at 4°C.
EC culture.
Bovine pulmonary artery EC (American Type
Culture Collection, Rockville, Md.) were cultured in Dulbecco's
modified Eagle's medium enriched with 20% fetal bovine serum, 4 mM
L-glutamine, nonessential amino acids, and vitamins in the
presence of penicillin (50 U/ml) and streptomycin (50 µg/ml) as
previously described (14, 15). Cell cultures were determined
to be endothelial by uniform cobblestone morphology and quantitative
determination of angiotensin-converting enzyme activity with
commercially available 3H-benzoyl-Phe-Ala-Pro substrate
(Ventex Laboratories, Portland, Maine).
Assay of transendothelial albumin flux.
Transendothelial
14C-bovine serum albumin (14C-BSA) flux was
assayed as we have previously described (3, 14, 15).
Briefly, polycarbonate filters (13-mm diameter; 0.4-µm pore size;
Nucleopore Corp., Pleasanton, Calif.) were impregnated with pig skin
gelatin (Fisher Scientific Co., Pittsburgh, Pa.), mounted in
polystyrene chemotactic chambers (ADAPS Inc., Dedham, Mass.), inserted
into wells of 24-well culture dishes, and sterilized with ethylene oxide. Each upper compartment was seeded with 2 × 105
EC and cultured for 72 h. 14C-BSA (Sigma) with a
specific activity of 1.3 µCi/mg of protein was used as the tracer
molecule. The baseline barrier function of each monolayer was
determined by applying 14C-BSA to each upper compartment
for 1 h, after which the lower compartment was counted in a liquid
scintillation analyzer (Tri-Carb 1500; Packard Instruments Co.). Only
EC monolayers retaining 97% of the 14C-BSA were studied.
EC monolayers were exposed for 6 h to increasing concentrations of
either the lipid A or the O-polysaccharide LPS fraction. In some
experiments, native LPS was coadministered with increasing
concentrations of either PMB or ENP. In other experiments, ENP was
introduced either before or after the LPS challenge. Simultaneous controls with medium alone were performed. Transfer of
14C-BSA across EC monolayers was again assayed immediately
following treatment.
The ability of ENP to cross-protect against endotoxins derived from
diverse gram-negative bacterial strains was also studied. Due to the
differences in the length of the O-specific polysaccharide and lipid A
acyl chains, various endotoxins cannot be compared on a dry
weight/weight basis. However, each LPS molecule, regardless of the
bacterial origin, contains at least one 2-keto-3-deoxyoctonic acid
(KDO) molecule. LPS preparations derived from E. coli
O55:B5, K. pneumoniae, P. aeruginosa, S. minnesota, or S. marcescens each were standardized to
10 ng of LPS per ml derived from E. coli O111:B4 on the
basis of KDO content (19). EC were exposed for 6 h to
either medium alone, ENP (100 ng/ml), equivalent concentrations of LPS
based on KDO content, or each LPS preparation coadministered with ENP.
Immunoblotting for phosphotyrosines.
EC were exposed for
1 h to either medium alone, ENP (1 µg/ml), LPS derived from
E. coli O111:B4 (100 ng/ml), or LPS coadministered with ENP.
EC were then processed for phosphotyrosine immunoblotting as previously
described (3). Briefly, EC were lysed with ice-cold lysis
buffer (50 mM Tris-HCl [pH 8.0], 1% Nonidet P-40, 0.25% sodium
deoxycholate, 150 mM NaCl, 1 mM EGTA, 1 mM phenylmethylsulfonyl fluoride, 1 µg of leupeptin per ml, 1 µg of pepstatin per ml, 1 µg of aprotinin per ml, 1 µg of DNase I per ml, 1 mM sodium orthovanadate, 1 mM NaF, 1 mM disodium pyrophosphate, 1 mM phenylarsine oxide, 500 µM p-nitrophenyl phosphate), scraped,
transferred to a tube, and centrifuged (16,000 × g, 10 min, 4°C). The supernatant from the EC lysate was resolved by sodium
dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE; 25 µg of protein/lane) on an 8 to 16% Tris-glycine gradient gel (Novex
Inc., San Diego, Calif.) and transferred for 3 h to a
polyvinylidene fluoride membrane (PVDF). The blot was blocked with 3%
dry milk, probed with biotinylated antiphosphotyrosine antibody 4G10
(0.7 µg/ml; Upstate Biotechnology Inc. [UBI], Lake Placid, N.Y.),
washed, and incubated with horseradish peroxidase-conjugated
streptavidin (0.5 µg/ml; UBI). The blot was developed with enhanced
chemiluminescence (Amersham Life Sciences, Arlington Heights, Ill.) and
exposed to Du Pont Reflection (NEF-406) film. The films were
subsequently scanned for laser densitometric analysis (Molecular
Dynamics, Sunnyvale, Calif.).
Immunolocalization of phosphotyrosine-containing proteins.
To maintain EC under experimental conditions identical to those of our
permeability assay, we directly stained and visualized EC monolayers
cultured on polycarbonate filters as previously described (3,
15). Briefly, EC cultured to confluence on filters were exposed
for 1 h to medium, LPS (100 ng/ml), ENP (1 µg/ml), or LPS
coadministered with ENP. The monolayers were washed with 1 mM vanadate
in PBS, fixed with 4% paraformaldehyde (30 min) followed by absolute
methanol (8 min, 20°C), and stained with fluorescein isothiocyanate
(FITC)-conjugated antiphosphotyrosine antibody (UBI) (5 µg/ml, 1 h) (3). The filters and their attached monolayers were
mounted cell side up on microscope slides and photographed through a
Zeiss Axioskop 20 microscope equipped for epifluorescence.
F-actin quantification.
EC F-actin was fluorimetrically
measured as previously described (3, 15). EC were pretreated
with cycloheximide (50 µg/ml) for 30 min prior to and throughout
treatments with medium, ENP (100 ng/ml), LPS (10 ng/ml), or LPS
coadministered with ENP. EC were washed with 75 mM KCl-1 mM EGTA-3 mM
MgSO4-0.2 mM dithiothreitol-10 mM imidazole-10 µg of
aprotinin per ml-0.1 mM phenylmethylsulfonyl fluoride (pH 7.2), fixed
(3.7% formaldehyde, 15 min), permeabilized (0.2% Triton X-100, 5 min), incubated with NBD-phallicidin (Molecular Probes, Eugene, Oreg.)
(1 U/well, 30 min), and extracted with methanol (overnight, 20°C).
The extracts were assayed in a Perkin-Elmer LS30 luminescence
spectrometer at 465-nm excitation (10-nm slit) and 535-nm emission
(10-nm slit) and F-actin content expressed in arbitrary fluorescence
units per milligram of total EC protein. Since methodologies for
quantifying F- and G-actin pools preclude protein determinations on the
same monolayers, EC were cultured under the same conditions as the
monolayers assayed for F- and G-actin pools, lysed, and assayed for
protein concentration with the standard Bio-Rad DC protein assay
(Bio-Rad Chemical Division, Richmond, Calif.).
DNase I inhibition assay for G-actin.
EC G-actin was
measured by using the DNase I inhibition assay as previously described
(3, 15). This assay utilizes the ability of monomeric
G-actin to inhibit DNase I hydrolysis of type 1 DNA into its component
nucleotides. Briefly, DNase I obtained from bovine pancreas (Sigma) was
mixed with calf thymus DNA type 1 (Sigma) in the cuvette of a
spectrophotometer, and the slope of the linear portion of the
A260 recorded. Purified bovine skeletal muscle actin (Sigma) was used to calibrate the assay. DNase I inhibitory activity within a range of 30 to 70% inhibition is directly
proportional to the concentration of monomeric G-actin. EC monolayers
grown in six-well culture dishes were exposed for 6 h to medium,
LPS (10 ng/ml), ENP (100 ng/ml), or LPS coadministered with ENP. The
monolayers were permeabilized with lysing buffer containing 1% Triton
X-100 for 5 min. The G-actin-containing supernatants were then tested
in the DNase I inhibition assay to generate inhibitory activities that
fell on the linear portion of the standard curve (i.e., 30 to 70%
inhibition). The inhibitory activities were interpolated to G-actin
concentrations, which were used to calculate G-actin expressed in
micrograms per milligram of total EC protein.
Statistical analysis.
One-way analysis of variance was used
to compare the mean responses among experimental and control groups for
all experiments. The Bonferroni post hoc comparison test was used to
determine between which groups significant differences existed. A
P value of 
0.05 was considered significant.
| |
RESULTS |
Structure-function studies of LPS-induced endothelial barrier
dysfunction.
The mean ± standard error (SE) pretreatment
baselines reflecting functional integrity for monolayers to be exposed
to either lipid A or the O-specific polysaccharide fraction were
0.016 ± 0.002 and 0.013 ± 0.002 pmol/h, respectively (Fig.
1A). The mean ± SE
14C-BSA flux across naked filters without endothelial
monolayers was 0.215 ± 0.015 pmol/h. Increasing concentrations of
lipid A caused dose-dependent increases in 14C-BSA flux
across endothelial monolayers, whereas identical concentrations of the
O-specific polysaccharide fraction did not (Fig. 1A). The lowest lipid
A concentration that after a 6-h exposure increased 14C-BSA
flux compared to the simultaneous medium control was 15 ng/ml. Further
dose-dependent increments were evident at concentrations up to 15 µg/ml. The polysaccharide fraction at concentrations up to 15 µg/ml
failed to increase 14C-BSA compared to the simultaneous
medium control.
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FIG. 1.
Effects of LPS fractions on transendothelial
14C-BSA flux. (A) Transendothelial 14C-BSA flux
across monolayers was assayed after exposure for 6 h to increasing
concentrations of either the lipid A fraction or the O-specific
polysaccharide fraction derived from E. coli O111:B4 LPS.
Each bar represents mean (± SE) transendothelial 14C-BSA
flux. Pretreatment baseline 14C-BSA flux across monolayers
exposed to either lipid A or O-specific polysaccharide fractions as
well as 14C-BSA flux across naked filters are also shown.
*, significantly increased compared with simultaneous medium control.
n, number of monolayers studied. (B) EC monolayers were assayed for
transendothelial 14C-BSA flux immediately after 6-h
exposures to medium alone, PMB, LPS, or LPS (10 ng/ml) coadministered
with increasing concentrations of PMB. Mean (± SE) pretreatment
baseline 14C-BSA flux is also shown *, significantly
increased compared to medium control; **, significantly decreased
compared to LPS. n, number of monolayers studied.
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PMB binds to and neutralizes the lipid A moiety of LPS (6,
23). To determine whether lipid A was essential for LPS
presentation to the non-CD14-bearing EC, the ability of PMB to block
native LPS-induced barrier dysfunction was also studied (Fig. 1B).
14C-BSA flux was assayed immediately after 6-h exposures to
medium, LPS (10 ng/ml), PMB (10 µg/ml), or LPS coadministered with
increasing concentrations of PMB (10 to 10,000 ng/ml). LPS increased
14C-BSA flux compared to the simultaneous medium control,
whereas PMB alone did not. PMB at a PMB/LPS dry weight-to-weight ratio of 1:1 did not significantly diminish the LPS effect. At PMB
concentrations of 1,000 ng/ml (PMB/LPS dry weight-to-weight ratio of
100:1), PMB completely protected against the LPS effect, returning
barrier function to medium control levels.
Effect of ENP on LPS-induced changes in transendothelial
14C-BSA flux.
ENP protected against LPS-induced
barrier dysfunction (Fig. 2).
14C-BSA flux was assayed immediately after 6-h exposures to
medium, LPS (10 ng/ml), ENP (10 µg/ml), or LPS coadministered with
increasing concentrations of ENP (10 to 10,000 ng/ml). Again, LPS alone
(10 ng/ml) increased 14C-BSA flux compared to the
simultaneous medium control. Protection against LPS-induced increases
in 14C-BSA flux by coadministration of ENP was dose
dependent. ENP at 10 ng/ml significantly decreased LPS-induced
barrier dysfunction. Partial protection was seen at an ENP
concentration of 10 ng/ml (ENP/LPS dry weight-to-weight ratio of 1:1).
Total protection was seen with ENP concentrations of 100 ng/ml
(ENP/LPS ratio of 10:1). When ENP was introduced prior to a 5-min LPS
challenge for either 0.5 or 1.0 h and subsequently removed by
thorough washing, no protection was observed (Table
1). Similarly, if ENP was introduced immediately following the LPS, again no protection could be
demonstrated.
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FIG. 2.
Dose-dependent effects of ENP on LPS-induced barrier
dysfunction. Baseline barrier function was determined for all
monolayers prior to treatment. Transendothelial 14C-BSA
flux across monolayers was assayed after exposure for 6 h to
medium, ENP, LPS, or LPS coadministered with increasing concentrations
of ENP. Each bar represents mean (± SE) transendothelial
14C-BSA flux. *, significantly increased compared to
medium control; **, significantly decreased compared to LPS alone.
n, number of monolayers studied.
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TABLE 1.
ENP treatment either before or after LPS challenge does
not protect against LPS-induced loss of endothelial monolayer
barrier function
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A comparison of the protective effects of PMB (molecular size = 1,450 g/mol) and ENP (molecular size = 12,189 g/mol) suggests that
ENP is more effective at blocking LPS-induced loss of EC barrier
function. Complete protection against LPS (10 ng/ml)-induced transendothelial 14C-albumin flux was observed with either
6.90 × 10
7 M PMB (PMB/LPS dry weight-to-weight
ratio of 100:1) or 8.2 × 109 M ENP (ENP/LPS dry
weight-to-weight ratio of 10:1). Partial protection was observed with
6.90 × 108 M PMB (PMB/LPS dry weight-to-weight
ratio of 10:1) or 8.20 × 1010 M ENP (ENP/LPS dry
weight-to-weight ratio of 1:1).
Effect of ENP on LPS-induced tyrosine phosphorylation of EC
proteins.
Lysates obtained from EC exposed for 1 h to medium
alone, ENP (1.0 µg/ml), LPS (100 ng/ml), or LPS coadministered with
ENP were resolved by SDS-PAGE and transferred to PVDF, and the blot was
probed for phosphotyrosines (Fig. 3).
Monolayers exposed to LPS demonstrated a 2.2-fold increase in tyrosine
phosphorylation of a 66-kDa band compared to medium alone; those
monolayers exposed to LPS in the presence of ENP demonstrated only a
1.3-fold increase in tyrosine phosphorylation of this same 66-kDa
protein. The increased tyrosine phosphorylation of this band in
LPS-exposed EC relative to those exposed to medium alone was inhibited
by 75% when LPS was coadministered with ENP.
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FIG. 3.
Effect of ENP on LPS-induced tyrosine phosphorylation of
a 66-kDa EC protein. For Western blot analysis of protein tyrosine
phosphorylation, EC monolayers were exposed to medium, ENP (1.0 µg/ml), LPS (100 ng/ml), or LPS coadministered with ENP for 1 h.
The EC lysates were resolved by SDS-PAGE, transferred to PVDF, and
probed for phosphotyrosines. Molecular weights (in thousands) are
indicated by arrows on the left. The blot is representative of three
separate experiments.
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EC monolayers exposed for 1 h to medium, to ENP (1.0 µg/ml), to
LPS (100 ng/ml), or to LPS coadministered with ENP were probed with an
FITC-conjugated antiphosphotyrosine antibody, processed for
epifluorescence microscopy, and photographed (Fig.
4). At 1 h, LPS-exposed EC (Fig. 4C)
displayed increased tyrosine phosphorylation of proteins
immunolocalized to the intercellular boundaries compared to both medium
and ENP controls (Fig. 4A and B, respectively). Monolayers treated with
both ENP and LPS (Fig. 4D) could not be distinguished from either the
medium or ENP controls.
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FIG. 4.
Effect of ENP on phosphotyrosine-containing proteins in
LPS-exposed EC. EC monolayers grown on filters were exposed for 1 h to medium (A), ENP (1.0 µg/ml; B), LPS (100 ng/ml; C), or LPS
coadministered with ENP (D). The monolayers were fixed, probed with
FITC-conjugated antiphosphotyrosine antibody, and photographed through
an epifluorescence microscope. Arrows indicate phosphotyrosine signal
at intercellular boundaries. Magnification, ×600.
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Effects of ENP on the LPS-induced changes in the F- and G-actin
pools.
The effect of ENP on the LPS-induced decrement in EC
F-actin, expressed as fluorescence units/milligram of total EC protein, was studied (Fig. 5A). There were no
significant differences in F-actin content between the medium and ENP
controls. A 6-h exposure to LPS (10 ng/ml) decreased F-actin compared
to either simultaneous medium or ENP (100 ng/ml) controls. ENP
coadministered with LPS diminished the LPS-induced F-actin decrement
compared to LPS alone. In fact, F-actin content in EC treated with both
LPS and ENP did not significantly differ from that for the simultaneous
medium control.
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FIG. 5.
Effects of ENP on LPS-induced changes in the F- and
G-actin pools. For G- and F-actin measurements, monolayers were exposed
for 6 h to medium, ENP, LPS, or LPS coadministered with ENP. (A)
For the F-actin studies, monolayers were fixed, permeabilized,
incubated with NBD-phallicidin, and extracted with methanol. The
extracts were spectrofluorimetrically assayed, and F-actin
concentrations were expressed as mean (± SE) fluorescent units per
milligram of total EC protein. *, significantly decreased compared to
medium control; **, significantly increased compared to LPS alone
but not significantly decreased compared to medium alone. (B) For
quantitation of the G-actin pool, EC were permeabilized and the
G-actin-containing supernatants were tested in the DNase I inhibition
assay standardized to pure G-actin. Each bar represents mean (± SE)
G-actin expressed. *, significantly increased compared to medium
control; **, significantly decreased compared to LPS alone but not
significantly increased compared to medium alone. n for each
experimental group is indicated in each bar.
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The effect of ENP on the LPS-induced increment in EC G-actin, expressed
in micrograms/milligram of total EC protein, was also studied (Fig.
5B). A 6-h exposure to LPS (10 ng/ml) increased G-actin compared to
either the simultaneous medium or ENP (100 ng/ml) controls. ENP
coadministered with LPS reduced the LPS-induced G-actin increment
compared to that observed after exposure to LPS alone. This reduction
was complete, reducing G-actin to the basal levels seen in the medium
control. Therefore, LPS provokes reciprocal shifts between the F- and
G-actin pools indicative of EC actin depolymerization, and these
changes are completely blocked by ENP.
ENP cross-protects against LPS derived from diverse gram-negative
bacterial strains.
ENP offered protection against loss of barrier
function in response to a variety of endotoxins normalized on the basis
of KDO content to 10 ng of LPS per ml derived from E. coli
O111:B4 (Fig. 6). Monolayers were assayed
for 14C-BSA flux immediately after 6-h exposures to the
following: medium, LPS derived from E. coli O111:B4,
E. coli O55:B5, K. pneumoniae, P. aeruginosa, S. minnesota, or S. marcescens
or an equivalent concentration of each LPS preparation coadministered
with ENP (100 ng/ml). All LPS preparations except that derived from
S. marcescens induced comparable increments in
14C-BSA flux. ENP completely protected against LPS-induced
increments in 14C-BSA transendothelial flux for all
endotoxins tested.
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FIG. 6.
ENP cross-protects against a wide variety of endotoxins.
Transendothelial 14C-BSA flux was assayed immediately
following 6-h exposures to medium (open bar), equivalent concentrations
based on KDO content of LPS derived from E. coli O111:B4 (10 ng/ml), E. coli 055:B5, P. aeruginosa, K. pneumoniae, S. marcescens, or S. minnesota
(cross-hatched bars), or these same LPS preparations coadministered
with ENP (100 ng/ml) (gray bars). Each bar represents mean (± SE)
transendothelial 14C-BSA flux. Baseline barrier function
for all monolayers studied is also indicated. *, significantly
decreased compared to LPS alone at P < 0.05 but not
significantly increased compared to medium control.
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DISCUSSION |
In this report, we first confirmed that lipid A was the portion of
the LPS molecule presented to the non-CD14-bearing EC. Neither the LPS
polysaccharide fraction nor native LPS coadministered with either PMB
or ENP simulated the LPS-induced loss of endothelial barrier function.
Lipid A has previously been shown to be the active LPS fraction that
stimulates CD14-bearing cells (27). Because EC do not
express CD14, it was unclear whether EC barrier dysfunction was due to
the lipid A portion of LPS. The lipid A fraction in concentrations up
to 15 µg/ml induced dose-dependent increases in 14C-BSA
flux, whereas the O-polysaccharide fraction did not. This lipid
A-induced dose-dependent increase in EC monolayer permeability was
similar to the native LPS effect previously described (14). PMB binds with 1:1 stoichiometry to the lipid A portion of LPS and has
been shown to neutralize LPS in a number of in vitro and in vivo models
(6, 23). Coadministration of LPS with PMB blocked
LPS-induced EC barrier dysfunction, demonstrating that in native
endotoxin, lipid A is the portion responsible for inducing increments
in permeability.
On the basis of these structure-function studies, we tested ENP, which
directly targets the lipid A portion of LPS. ENP at concentrations of
100 ng/ml totally blocked LPS (10 ng/ml)-induced increases in
transendothelial albumin flux. These studies were performed in the
presence of serum at concentrations which support the LPS effect. This
finding suggests that ENP successfully operates in the presence of
serum proteins known to bind to the lipid A portion of LPS, notably LBP
and soluble CD14 (14). BPI is a protein found in the
azurophilic granules of human neutrophils that is homologous to LBP
(4, 10, 28). However, the differences between the two
molecules are sufficient that LBP facilitates and enhances LPS
bioactivity (28) whereas BPI is inhibitory (10).
This homology between LBP and BPI promotes competition between the two
proteins for binding to LPS (7, 16). In the circulation, BPI
is present in lower concentrations than LBP. In addition, LBP is an
acute-phase protein that can increase from basal levels of 2 to 6 µg/ml to 50 µg/ml within 24 h after induction of the
acute-phase response (28). Therefore, any effective clinical intervention for endotoxemia must be capable of performing in the
presence of LBP as ENP apparently has in these experiments.
ENP and PMB have each been previously reported to bind to lipid A with
a 1:1 stoichiometry (6, 23, 32). The LPS-neutralizing activities of these two proteins were compared in the barrier function
assay in the presence of serum (Fig. 1B and 2). On a molar basis, ENP
(molecular size = 12,189 g/mol) was ~80-fold more effective at
blocking LPS-induced loss of endothelial barrier function than was PMB
(molecular size = 1,450 g/mol).
The signal transduction pathway for LPS-induced EC barrier dysfunction
is still poorly understood. Protein tyrosine phosphorylation has been
shown to be operative in the activation of CD14-bearing monocytes and
macrophages (29, 35). More recently, the response of the
non-CD14-bearing EC to LPS has been shown to also involve protein
tyrosine phosphorylation (2, 3). LPS stimulates tyrosine
phosphorylation of several mitogen-activated protein kinases, and
protein tyrosine kinase inhibition blocks LPS-induced interleukin-6
biosynthesis and lactic dehydrogenase release. Recently, we have
demonstrated that protein tyrosine kinase inhibition protects against
LPS-induced barrier dysfunction (3). In addition, we have
shown that LPS induces tyrosine phosphorylation of EC proteins localized to the intercellular boundaries as well as of paxillin, a
66-kDa protein which links the actin cytoskeleton to areas of the
plasma membrane involved in cell-matrix adhesion (3).
On the basis of the ability of ENP to neutralize LPS bioactivity in the
permeability assay, we attempted to show whether ENP blocks the
previously described EC responses that are prerequisites to LPS-induced
barrier dysfunction. ENP prevented LPS-induced tyrosine phosphorylation
of paxillin and EC proteins localized to the intercellular boundaries
as well as the G-actin increase and the reciprocal F-actin decrease
that is indicative of F-actin depolymerization. Thus, inhibition of
LPS-induced protein tyrosine phosphorylation by ENP at 1 h prevents
the subsequent actin reorganization and loss of barrier function seen
at 2 h, suggesting that ENP acts at an early step in the pathway
proximal to tyrosine phosphorylation.
To our knowledge, only one previous report has studied the ability of a
Limulus-derived factor to neutralize LPS bioactivity in an
EC system (8). That work, however, differed in several aspects. First, the authors used EC derived from a different species and anatomical source. Second, they used anti-LPS factor derived from
Tachypleus tridentatus, the Japanese horseshoe crab. We used a recombinant form of anti-LPS factor, ENP, which was derived from
anti-LPS factor isolated from the American horseshoe crab. ENP differs
from anti-LPS factor in its mannose content (11). Further,
the LPS-induced EC response they attempted to block was EC adhesiveness
for neutrophils. Unlike LPS-induced increments in transendothelial
albumin flux (15), the EC response they report requires de
novo protein synthesis. Finally, these and other investigators who have
studied the ability of anti-LPS factor or ENP to neutralize endotoxins
derived from various gram-negative bacteria have standardized their LPS
preparations on a dry weight/weight basis (8, 32). The
variability in the length of the lipid A acyl and O-specific
polysaccharide chains precludes such comparison. We, therefore,
standardized the endotoxins studied to 10 ng of E. coli O111:B4 per ml
on the basis of KDO content (19).
In this study, ENP was able to protect against a wide variety of
endotoxins. Clinical intervention for gram-negative septic shock and
its complications must offer protection against the enormous diversity
of endotoxins found in nature. ENP has been previously shown to protect
against LPS-induced tissue injury indirectly mediated through
host-derived factors (4, 11, 34). In animal models, ENP
protects against LPS-induced pulmonary hypertension, systemic
hypotension, metabolic acidosis, neutropenia, and pyrogenicity (1,
34). ENP also reduces circulating levels of free LPS and tumor
necrosis factor (1). Pretreatment, coadministration, or even
administration of ENP following the LPS challenge results in increased
survival rates in sheep, mice, and rats (1, 34). In addition
to the ability of LPS to indirectly cause injury through the hosts'
mediator systems, LPS is able to directly provoke increases in vascular
permeability (3, 14, 15, 21). In this study, we have
demonstrated that ENP is capable of preventing the direct effects of
LPS on the endothelial barrier. The ability of ENP to protect against
the effects of LPS on the host mediator systems and against the direct
effects of LPS on the endothelium, offers a potential therapeutic
intervention to protect against gram-negative sepsis and its vascular
complications.
| |
ACKNOWLEDGMENTS |
This work was supported in part by the Office of Research and
Development, Department of Veterans Affairs and the U.S. Army Medical
Research and Development Command (grant DAMD17-94-J-4117). Douglas D. Bannerman and Michael J. Fitzpatrick are each a recipient of a
Department of Defense Augmentation Award for Science and Engineering
Research Training.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Medical Service
(111) Rm5D-139, Department of Veterans Affairs Medical Center, 10 North Greene St., Baltimore, MD 21201. Phone: (410) 605-7182. Fax: (410) 605-7914.
Editor: J. R. McGhee
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Abstract
Introduction
