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HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY
From the Division of Cardiology, Department of Internal
Medicine, University of Giessen, Germany; and Aventis Behring GmbH,
Research, Marburg, Germany.
The serpin antithrombin III (AT III), the most important natural
inhibitor of thrombin activity, has been shown to exert marked anti-inflammatory properties and proven to be efficacious in
experimental models of sepsis, septic shock, and disseminated
intravascular coagulation. Moreover, clinical observations suggest a
possible therapeutic role for AT III in septic disorders. The molecular mechanism, however, by which AT III attenuates inflammatory events is
not yet entirely understood. We show here that AT III potently blocks
the activation of nuclear factor Antithrombin is one of the most important
endogenous regulators of coagulation, acting as the major inhibitor of
thrombin and interfering with several plasma proteases such as
kallikrein and factors IXa, Xa, XIa, and XIIa.1 Apart from
its role in hemostasis, there is accumulating evidence that
antithrombin III (AT III) exerts anti-inflammatory properties and
improves survival in animal-sepsis models and disseminated
intravascular coagulation (DIC).2-4 There are a number of
compelling reasons why AT III may also be an effective therapeutic
agent in patients with sepsis.5-7 AT III was shown to
reduce leukocyte-endothelial interaction,8 to prevent
microvascular leakage,9 and to ameliorate
ischemia/reperfusion injury.10 These effects, however,
seem to result only in part from interference of AT III with thrombin
activity because inhibition of thrombin generation alone did not prove
similarly effective.11,12 The beneficial effects of AT III
rather appear mainly to result from direct, thrombin-independent
effects on vascular cells. AT III was found to stimulate nitric oxide
synthesis in vascular smooth muscle cells,13 to inhibit
migration and adhesion of neutrophils,14 and to attenuate
cytokine production in monocytes and endothelial cells
(ECs)15 in a thrombin-independent manner. However, despite
the increasing number of reports describing direct effects of AT III on
vascular cells, the molecular mechanisms underlying these effects
remain to be elucidated.
In every inflammatory process, the vast majority of cellular events
require nuclear factor Despite the important role of the NF- Cell culture
Monocytes.
Human peripheral blood mononuclear cells were isolated from buffy coats
obtained from healthy blood donors by Ficoll-Hypaque density gradient
centrifugation (Amersham Pharmacia Biotech AB, Uppsala, Sweden)
and further fractionated as described previously.20 Informed consent was provided according to the Declaration of Helsinki.
The final cultures, suspended at a density of 1 × 106
cells/mL in serum-free culture medium (RPMI 1640; GIBCO BRL), contained
90% to 95% monocytes as evidenced by Pappenheim staining and
fluorescence-activated cell sorter (FACS) analysis, as well as
nonspecific esterase staining of cytocentrifuge preparations.
Endothelial cells.
ECs were isolated from human umbilical veins with trypsin-EDTA solution
according to the method of Jaffe et al.21 All experiments were performed with first-passage cells grown to confluence 2 days
after seeding. All media and buffers were found to contain less than
10.0 pg/mL endotoxin by limulus amoebocyte lysate assay.
Cell viability.
Cell viability in the absence and presence of AT III was determined by
ethidium bromide staining of cell aliquots and subsequent FACS analysis.
Antithrombin III
Preparation of immune-adsorbed AT III.
AT III concentrate (Kybernin P) was obtained from Aventis
Behring (Marburg, Germany). AT III was further purified from Kybernin P
by immune adsorption to a monoclonal antibody (mAb) bound to BrCN-Sepharose (Amersham Pharmacia Biotech AB). In preliminary experiments, the mAb had been demonstrated to bind both isoforms with
identical affinity. Spiking and column-overloading experiments had been
performed to ensure that the isoform proportions of the samples applied
were not altered by the immune-adsorption procedure. AT III
concentrations used in the present study ranged from 0 to 30 IU/mL; by
definition, 1 IU of AT III equals the amount found on average in 1 mL
plasma and is equivalent to 150 µg/mL or 2.6 µM.
Separation of latent AT III and isoforms from AT III concentrate.
AT III isoforms were prepared from AT III concentrate (Kybernin P;
Aventis Behring) by adsorption to Heparin-Fractogel. Twenty thousand units of AT III (Kybernin P) was dissolved in 2.0 L water for
injection and pumped onto the heparin column (500 mL), which had been
equilibrated with 0.015 M Na2H(PO4)-2-hydrate,
0.06 M NaH2(PO4)-2-hydrate, and 0.05 M NaCl, pH
7.2. Latent AT III was obtained by washing the column with
equilibration buffer containing 0.2 M NaCl. The Preparation of Trp49-blocked AT III.
A single Trp residue in AT III was chemically modified according to the
method of Blackburn et al.22 Labeling of Trp49
was achieved using dimethyl (2-hydroxy-5-nitrobenzyl) sulfonium bromide.
Western blot analysis
Electrophoretic mobility shift assay
RNA isolation and reverse transcriptase-polymerase chain reaction Total cellular RNA was isolated by the acid guanidinum thiocyanate-phenol-chloroform method, as described by Chomczynski and Sacchi.24 Preparation of complementary DNA and subsequent PCR were performed as described previously.20 Sequences of intron spanning TF-specific primers were: sense, 5'-GCCGCCAACTGGTAGACATG-3', and antisense, 5'-TAGCCAGGATGATGACAAGG-3'; and for the housekeeping gene -actin: sense, 5'-AAAGACCTGTACGCC-3',
and antisense, 5'-CGTCATACTCCTGCTTGCTGATCCACATCTG-3'. Negative controls
were performed routinely by running PCR without cDNA to exclude
false-positive amplification products. The specificity of the obtained
TF PCR products was verified by subjecting the related PCR product to
automated DNA sequencing (model 373A; Applied Biosystems,
Überlingen, Germany), essentially as described by the
manufacturer, and comparing the resulting cDNA sequence with the
published human TF cDNA sequence.25
Quantification of IL-6 and TNF-  protein levels from monocyte culture
supernatants were measured quantitatively using a commercially
available, specific enzyme-linked immunosorbent assay (ELISA) (IL-6:
R&D Systems, Minneapolis, MN; TNF-: Hölzel, Köln,
Germany). Serial dilutions of the corresponding recombinant cytokine
provided standard curves for each individual ELISA plate. Absorbance
was measured at 490 nm using an ELISA reader. The quantification was
performed in duplicate.
Statistical methods Data are described as mean ± SEM of at least 3 independent experiments. Statistical significance was estimated with Student t test. Differences were assumed to be statistically significant at P < .05.
AT III inhibits NF-  B was induced by treatment with LPS (monocytes) or TNF-
(ECs), both well-known NF-B-activating agents in these cell types.
This induction was shown by the appearance in nuclear extracts of the DNA-binding activity of NF-B using electrophoretic mobility shift assays (EMSAs) (Figure 1). The
induction of NF-B was prevented when AT III was present in the cell
culture medium. Preincubation with AT III led to a dose-dependent
inhibition of the agonist-induced DNA-binding activity of NF-B in
both monocytes and ECs, whereby 20 U/mL AT III entirely abrogated the
NF-B response to either LPS or TNF- (Figure 1). Moreover, AT III
(20 U/mL) was also found to suppress the low baseline NF-B binding
activity detected in unstimulated cells (Figure 1). The inhibitory
effect was not due to any toxic effect on cells, as evidenced by
ethidium bromide staining (data not shown).
AT III specifically inhibits NF- B, we also
analyzed nuclear extracts from AT III-treated cells for the DNA-binding activity of the transcription factor AP-1 (Figure 2). Treatment of monocytes with LPS or of
ECs with TNF- induced NF-B binding, which was strongly blocked by
20 U/mL AT III. In the same extracts, AT III could not prevent the
induction of AP-1 binding activity.
Inhibition of NF- B induction,
Trp49-modified AT III, which lacks heparin-binding
properties, had no effect (Figure 3). The
hypothesis that the inhibitory effect of AT III on NF-B activation
involves an interaction with heparinlike proteoglycans was supported by
the observation that the AT III -isoform, known to have high
affinity to cell surface proteoglycans, displayed a more effective
suppression of NF-B induction in intact cells than was observed for
the AT III -isoform, which has a lower affinity to heparan sulfate
proteoglycans (Figure 3). Latent AT III displayed only a small effect
on NF-B activity.
AT III interferes with I induce
translocation of NF-B into the nucleus by phosphorylation of its
inhibitory protein IB, which is then ubiquitinated and rapidly
degraded by the 26S proteasome.19 Therefore, to examine
the fate of IB upon stimulation after AT III treatment, we
assayed IB degradation and phosphorylation by immunoblotting.
Figure 4 shows that preincubation with AT
III prevented agonist-induced IB degradation in a dose-dependent manner in both cell types. The loss of cytoplasmic IB was
consistent with the occurrence of phosphorylated IB 15 minutes
after stimulation, as monitored by immunoblot analysis using
antibodies specific for the Ser32-phosphorylated form of IB.
However, when stimulation was performed in the presence of AT III,
reduced phosphorylated IB was detected in both monocytes and ECs.
Again, not only did AT III block IB phosphorylation in stimulated
cells, but it also suppressed the basal phosphorylation rate of
IB in unstimulated cells. In conclusion, AT III seems to be a
useful agent allowing interference with the mobilization of NF-B by
suppressing IB degradation in vascular cell types.
AT III affects NF- B binding activity led us
to investigate whether AT III affects the induction
of NF-B-controlled genes in monocytes and ECs. For this purpose,
the transcription of the TF gene and the secretion of IL-6 and TNF-
were analyzed in both cell types and were assayed by reverse
transcriptase-polymerase chain reaction (RT-PCR) and ELISA,
respectively, upon stimulation of cells in the presence or absence of
AT III. As shown in Figure 5, stimulation
of cells resulted in strong induction of TF mRNA expression, which was
suppressed by AT III in a dose-dependent manner to nearly baseline
levels. Additionally, monocytes showing negligible basal IL-6 and
TNF- secretion exhibited a several-fold increase in cytokine
secretion after LPS stimulation (Figure
6). Pretreatment of cells with AT III
reduced LPS-induced IL-6 and TNF- production in a dose-dependent
manner to a very low level. This indicates that the proinflammatory
activation of cells is abolished if AT III is present in the culture
medium in sufficient concentrations.
In this study, we demonstrate that AT III is a potent endogenous
regulator allowing for interference with the mobilization of NF- Simultaneous activation of the coagulation system is an almost
invariable consequence of local or systemic inflammation. This interaction of coagulation and inflammation, which may have developed from evolutionary forces favoring survival of individuals able to
localize and to contain the source of injury or infection, involves
several mechanisms in which, on the one hand, inflammatory processes
can activate coagulation, and, conversely, coagulation influences
inflammation (for review, see Opal26). The interaction of
coagulation and inflammation is evident from observations that several components of the coagulation system can, for example, stimulate inflammatory cytokines such as IL-1, IL-6, IL-8, and TNF- The results of the present study suggest a decrease in the rate of
transcription of NF- In this study, we investigated whether AT III affects agonist-induced
induction of NF- Blockade of NF- Because cell-cell contact and cross-talk between monocytes and
endothelium are believed to play central roles in the interaction of
coagulation and inflammation during septic disorders and DIC, we tested
whether AT III is able to suppress the induction of NF- Next we analyzed in more detail the molecular basis of the inhibitory
action of AT III. In resting cells, NF- In this regard, an important observation might be that the
Further studies are required to investigate, on the one hand, whether a
distinct receptor for AT III exists among cell surface molecules
related to the family of heparan sulfate glycosaminoglycans, and, on
the other hand, whether the
We would like to thank B. Parviz for excellent technical assistance.
Submitted August 7, 2001; accepted January 31, 2002.
Supported by the Deutsche Forschungsgemeinschaft (DFG), Sonderforschungsbereich 547, and by the Gesellschaft für Thrombose- und Hämostaseforschung (GTH). C.O. is a scholar of the DFG-Graduiertenkolleg 534.
J.R. and H.S. are employed by Aventis whose product was studied in the present work.
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Hans Hölschermann, Division of Cardiology, Department of Internal Medicine, University of Giessen, Klinikstrasse 36, D-35392 Giessen, Germany; e-mail: hans.f.hoelschermann{at}innere.med.uni-giessen.de.
1. Bauer KA, Rosenberg RD. Role of antithrombin III as a regulator of in vivo coagulation. Semin Hematol. 1991;28:10-18[Medline] [Order article via Infotrieve]. 2. Emerson TE Jr, Fournel MA, Redens TB, Taylor FB Jr. Efficacy of antithrombin III supplementation in animal models of fulminant Escherichia coli endotoxemia or bacteremia. Am J Med. 1989;87(suppl B3):27S-33S[CrossRef][Medline] [Order article via Infotrieve].
3.
Dickneite G, Leithäuser B.
Influence of antithrombin III on coagulation and inflammation in porcine septic shock.
Arterioscler Thromb Vasc Biol.
1999;19:1566-1572 4. Meijer C, Wiezer MJ, Hack CE, et al. Coagulopathy following major liver resection: the effect of and the role of decreased synthesis of regulating proteins by liver. Shock. 2001;15:261-271[Medline] [Order article via Infotrieve]. 5. Inthorn D, Hoffmann JN, Hartl WH, Mühlbayer D, Jochum M. Antithrombin III supplementation in severe sepsis: beneficial effects on organ dysfunction. Shock. 1997;8:238-334. 6. Inthorn D, Hoffmann JN, Hartl WH, Mühlbayer D, Jochum M. Effect of antithrombin III supplementation on inflammatory immune response in patients with severe sepsis. Shock. 1998;10:90-96[Medline] [Order article via Infotrieve]. 7. Eisele B, Larmy M, Thijs LG, et al. Antithrombin III in patients with severe sepsis. A randomized, placebo-controlled, double-blind multicenter trial plus a meta-analysis on all randomized, placebo-controlled, double-blind trials with antithrombin III in severe sepsis. Intensive Care Med. 1998;24:663-672[CrossRef][Medline] [Order article via Infotrieve].
8.
Hoffmann JN, Vollmar B, Inthorn D, Schildberg FW, Menger MD.
Antithrombin reduces leukocyte adhesion during chronic endotoxemia by modulation of the cyclooxygenase pathway.
Am J Physiol Cell Physiol.
2000;279:C98-C107 9. Kurose I, Miura S, Funkumura D, et al. Attenuating effect of antithrombin III on the fibrinolytic activation and microvascular derangement in rat gastric mucosa. Thromb Haemost. 1994;71:119-123[Medline] [Order article via Infotrieve].
10.
Ostrovsky L, Woodman RC, Payne D, Teoh D, Kubes P.
Antithrombin III prevents and rapidly reverses leukocyte recruitment in ischemia/reperfusion.
Circulation.
1997;96:2302-2310
11.
Harada N, Okajima K, Kushimoto S, Isobe H, Tanaka K.
Antithrombin reduces ischemia/reperfusion injury of rat liver by increasing the hepatic level of prostacyclin.
Blood.
1999;93:157-164
12.
Uchiba M, Okajima K, Murakami K, Okabe H, Takatsuki K.
Attenuation of endotoxin-induced pulmonary vascular injury by antithrombin III.
Am J Physiol.
1996;270:L921-L930 13. Totzke G, Smolny M, Seibel M, Czechowski M, Schobersbergher W, Hoffmann G. Antithrombin III enhances inducible NOS gene expression in vascular smooth muscle cells. Cell Immunol. 2001;208:1762-1770.
14.
Dunzendorfer S, Kaneider N, Rabensteiner A, et al.
Cell-surface heparan sulfate proteoglycan-mediated regulation of human neutrophil migration by the serpin antithrombin III.
Blood.
2001;97:1079-1085 15. Souter PJ, Thomas S, Hubbard AR, Poole S, Römisch J, Gray E. Antithrombin inhibits lipopolysaccharide-induced tissue factor and interleukin-6 production by mononuclear cells, human umbilical vein endothelial cells, and whole blood. Crit Care Med. 2001;29:134-139[CrossRef][Medline] [Order article via Infotrieve]. 16. Yamamoto Y, Gaynor RB. Therapeutic potential of inhibition of the NF-kappa B pathway in the treatment of inflammation and cancer. J Clin Invest. 2001;107:135-142[Medline] [Order article via Infotrieve].
17.
Hatata EN, Krappmann D, Scheidereit C.
NF- 18. Peters RT, Maniatis T. A new family of IKK-related kinases may function as I kappa B kinase kinases. Biochim Biophys Acta. 2001;1471:M57-M62[Medline] [Order article via Infotrieve]. 19. Karin M, Delhase M. The I kappa B kinase (IKK) and NF-kappa B: key elements of proinflammatory signalling. Semin Immunol. 2000;12:85-98[CrossRef][Medline] [Order article via Infotrieve].
20.
Hölschermann H, Dürfeld F, Maus U, et al.
Cyclosporine A inhibits tissue factor expression in monocytes/macrophages.
Blood.
1996;88:3837-3845 21. Jaffe EA, Nachman RL, Becker CG, et al. Culture of human endothelial cells derived from umbilical veins: identification of morphologic and immunologic criteria. J Clin Invest. 1973;52:2745-2756[Medline] [Order article via Infotrieve].
22.
Blackburn MN, Smith RL, Carson J, Sibley CC.
The heparin-binding site of antithrombin III. Identification of a critical tryptophan in the amino acid sequence.
J Biol Chem.
1984;259:939-941
23.
Hölschermann H, Rascher C, Oelschläger C, et al.
Opposite regulation of tissue factor by calcineurin in monocytes and endothelial cells.
J Immunol.
2001;166:7112-7120 24. Chomczynski P, Sacchi N. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Anal Biochem. 1987;162:156-159[Medline] [Order article via Infotrieve]. 25. Scarpati EM, Wen D, Broze G, et al. Human tissue factor: cDNA-sequence and chromosome localisation of the gene. Biochemistry. 1987;26:5234-5238[CrossRef][Medline] [Order article via Infotrieve]. 26. Opal SM. Phylogenetic and functional relationships between coagulation and the innate immune response. Crit Care Med. 2000;28(suppl 9):S77-S80[CrossRef][Medline] [Order article via Infotrieve]. 27. Cirino G, Bucci M, Cicala C, Napoli C. Inflammation-coagulation network: are serine protease receptors the knot? Trends Pharmacol Sci. 2000;21:170-172[CrossRef][Medline] [Order article via Infotrieve]. 28. Coughlin SR. Thrombin signalling and protease-activated receptors. Nature. 2000;407:258-264[CrossRef][Medline] [Order article via Infotrieve].
29.
Esmon CT.
Introduction: are natural anticoagulants candidates for modulating the inflammatory response to endotoxin?
Blood.
2000;95:1113-1116 30. Jochum M. Influence of high-dose antithrombin concentrate therapy on the release of cellular proteinases, cytokines, and soluble adhesion molecules in acute inflammation. Semin Hematol. 1995;32(suppl 2):19-32[Medline] [Order article via Infotrieve]. 31. Zuo XJ, Okada Y, Nicolaidou E, et al. Antithrombin III inhibits T- and B-lymphocyte activation in vitro and improves parameters of inflammation in a rat model of acute lung allograft rejection. Transplant Proc. 1999;31:816-817 |
B activation in human
monocytes and vascular endothelial cells
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Abstract
Introduction
, tumor necrosis factor-
