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* Institute for Vascular Medicine, Friedrich-Schiller-University of
Jena, Nordhäuserstrasse 78, 99089 Erfurt, Germany;
§ Department of Cardio-Thoracic and Vascular Surgery,
Friedrich-Schiller-University of Jena, Bachstrasse 18, 07740 Jena,
Germany; ¶ Department of Pathology, Louisiana
State University Medical Center, New Orleans, LA 70112-1393;
Contributed by Bengt Samuelsson, November 25, 2002
Oxidation products of low-density lipoproteins have been suggested
to promote inflammation during atherogenesis, and reticulocyte-type 15-lipoxygenase has been implicated to mediate this oxidation. In
addition, the 5-lipoxygenase cascade leads to formation of leukotrienes, which exhibit strong proinflammatory activities in
cardiovascular tissues. Here, we studied both lipoxygenase pathways in
human atherosclerosis. The 5-lipoxygenase pathway was abundantly
expressed in arterial walls of patients afflicted with various lesion
stages of atherosclerosis of the aorta and of coronary and carotid
arteries. 5-lipoxygenase localized to macrophages, dendritic cells,
foam cells, mast cells, and neutrophilic granulocytes, and the number
of 5-lipoxygenase expressing cells markedly increased in advanced
lesions. By contrast, reticulocyte-type 15-lipoxygenase was expressed
at levels that were several orders of magnitude lower than
5-lipoxygenase in both normal and diseased arteries, and its expression
could not be related to lesion pathology. Our data support a model of
atherogenesis in which 5-lipoxygenase cascade-dependent inflammatory
circuits consisting of several leukocyte lineages and arterial wall
cells evolve within the blood vessel wall during critical stages of
lesion development. They raise the possibility that antileukotriene
drugs may be an effective treatment regimen in late-stage disease.
arachidonic acid cascade|coronary heart disease
Atherosclerosis, the disease
that gives rise to myocardial infarction, stroke, and vascular
occlusive disease of the extremities, is the principal cause of
mortality in industrialized countries (1, 2). Risk factors for
atherosclerosis have been identified by epidemiological studies, but
disease-initiating mechanisms largely remain elusive (1). The
response to injury hypothesis (3-5) emphasizes that
atherosclerosis is a chronic inflammatory fibroproliferative disease of
the arterial wall that is associated with aberrant immune reactions. In
addition, the lipid oxidation hypothesis (6, 7) proposes
that oxidized low-density lipoproteins (LDL) may trigger arterial wall
injury and facilitate foam cell formation.
The reticulocyte-type 15-lipoxygenase (15-LO), a family member of
non-heme iron-containing dioxygenases, has been implicated in LDL
oxidation (6-17). However, species-dependent, i.e., pro- versus
antiatherogenic, roles of 15-LO family members have been observed (16).
In addition, actions of the enzyme that are independent of LDL
oxidation have been considered (18). However, although its animal
counterparts have been studied in considerable detail, information on
15-LO expression in human atherogenesis is very limited: Analyses of
atherosclerotic lesions of the aorta (AAO) indicated its expression in
foam cells (17), and stereochemical analyses of oxidized cholesteryl
linoleate in lesion lipids (11, 15) were consistent with its presence
in diseased arterial walls. By contrast, the relevance of the 5-LO
cascade (19-24) and leukotriene receptors (LT-Rs) for atherogenesis
has received less attention.
To gain insight into the relation of LOs and human atherosclerosis, we
initiated studies at predilection sites of the disease, i.e., coronary
and carotid arteries and the aorta. We found that 5-LO was abundantly
present in monocytes/macrophages, dendritic cells (DCs), mast cells,
and neutrophilic granulocytes, and that the number of
5-LO+ cells markedly increased in advanced
lesions. By contrast, 15-LO was barely detectable and its expression
was unrelated to atherosclerosis pathology. These data are consistent
with the concept that the 5-LO cascade generates circuits of
inflammation during critical stages of atherogenesis.
Materials.
5-LO activating protein (FLAP) antiserum was a kind gift of J. Evans
(Merck); SYBR Green and avian myeloblastosis virus reverse transcriptase was from Roche Diagnostics; platinumTaq
(Thermus aquaticus) DNA polymerase was from Invitrogen; and
all other reagents were from Sigma unless otherwise stated.
Patient Details.
Information on patients is reported in Supporting Text and
Table 1, which are published as supporting information on the PNAS web
site, www.pnas.org. Specimens from the Pathobiological
Determinants of Atherosclerosis in Youth (PDAY)
program were obtained from the Department of Pathology, Louisiana State
University Medical Center, New Orleans.
Cell Culture and Assays.
Immunoblots and real-time RT-PCR analyses were determined as reported
in Supporting Text (and see Table 2, which is published as
supporting information on the PNAS web site). Morphometry was performed
at ×200 magnification in sections that had been graded according to
the American Heart Association (AHA) system (25, 26), adjacent to
sections used for RT-PCR analyses. Cells were recorded positive when
antigen could be associated with a nucleus (hematoxylin) by using a
Sony XC-711P video camera and the Q500/W image analysis system (Leica,
Bensheim, Germany). Data were analyzed using the one-sided
Mann-Whitney U test.
Immunohistochemistry.
Analyses and specificity tests were performed on 8-µm cryostat
sections with LO and leukocyte marker antisera as described in
Supporting Text (and see Table 3, which is published as
supporting information on the PNAS web site) and as reported (27-29).
For localization of 5-LO in foam cells and for morphometry, alkaline phosphatase-labeled streptavidin-biotin was used. AHA classification was performed on parallel sections stained with Oil red O and hematoxylin/eosin. Three-dimensional reconstruction of 5-LO protein was
done using 3D FOR LSM software (Zeiss).
Expression of LO Transcripts and Protein in Human Atherosclerotic
Lesions.
We determined absolute transcript levels of both LOs at three
predilection sites of the disease, i.e., AAO, carotid artery disease
(CAD), and coronary heart disease (CHD), by using real-time RT-PCR
analyses. We also graded lesion stages according to the AHA system (25,
26) to determine expression levels of LOs in atherosclerotic plaques of
individual patients. However, we excluded type VI lesions that are
associated with plaque rupture, hemorrhage, and thrombosis (26),
because these transcripts may originate from trapped leukocytes rather
than from leukocytes that had infiltrated the arterial wall during bona
fide atherogenesis. 5-LO transcripts were readily observed, whereas,
surprisingly, reticulocyte-type 15-LO transcripts were either
undetectable or found at low levels (Fig.
1a; see below). Real-time PCR
analyses provided quantitative information on LO transcripts in CAD
lesions. Because we found 18,900 ± 12,300 5-LO transcripts per
105 GAPDH transcripts (n = 7),
and because the lowest point of the linear portion of the LO standard
curve represented eight cDNA standard molecules (see Fig. 5, which is
published as supporting information on the PNAS web site), 5-LO mRNA
may constitute an abundant mRNA in advanced CAD lesions. Although below
detection limits or barely detectable in most of our RT-PCR assays of
40 specimens (38 patients), 15-LO transcripts were readily found in
human bronchial epithelium (27), trachea, human lung (Fig. 2), and IL-4-stimulated monocytes and DCs
(28, 29). 5-LO transcripts in CAD lesions (type V lesions;
n = 7) exceeded those of 15-LO transcripts by more than
three orders of magnitude (Fig. 1a; and see Fig. 5). When 5- and 15-LO transcripts were compared across all lesions (type 0-V) of
all specimens (n = 40), 5-LO transcripts exceeded 15-LO
transcripts by a factor of
Medical Sciences
Expanding expression of the 5-lipoxygenase pathway within the
arterial wall during human atherogenesis
,
,,,
,,
,
,, and Institute for Atherosclerosis Research, Domagkstrasse 3, 48149 Münster, Germany; ** Department of Medicine, Division of
Cardiology, University of Heidelberg Medical School, Bergheimerstrasse
58, 69115 Heidelberg, Germany; Institute of
Biochemistry, Humboldt University Berlin, Monbijoustrasse 2, 10115 Berlin, Germany; and Karolinska
Institute, Department of Medical Biochemistry and Biophysics,
Division of Chemistry II, S-171 77 Stockholm,
Sweden
Abstract
Top
Abstract
Introduction
Methods
Results
Discussion
References
Introduction
Top
Abstract
Introduction
Methods
Results
Discussion
References
Methods
Top
Abstract
Introduction
Methods
Results
Discussion
References
Results
Top
Abstract
Introduction
Methods
Results
Discussion
References
600. Transcripts of additional
constituents of the 5-LO cascade (19), i.e., LTA4 hydrolase, FLAP, LTC4 synthase, and four LT-Rs
(30-33), were identified by RT-PCR in AAO, CAD, and CHD (Fig.
1a). In view of this unexpected divergence between
expression levels of both LOs, a detailed evaluation of RT-PCR was
performed. This included sequencing of PCR products of all 5-LO cascade
constituents from RNA extracts of AAO, CAD, and CHD, as well as the PCR
product of 15-LO from human lung; similar sensitivities of both LO
real-time RT-PCR assays were established. We excluded the possibility
of inhibitors in tissue RNA extracts of the 15-LO amplification
reaction and determined integrities of RNAs and correlated RNA
integrity to the number of 15- and 5-LO transcripts. Each of these
analyses supported the conclusion of undetectable or low expression of
the 15-LO gene throughout (lesion stages 0-V) human atherogenesis.
Moreover, when we determined 5- and 15-LO mRNA degradation kinetics in
human lung (see Fig. 6, which is published as supporting information on
the PNAS web site), there was no evidence for differential 5- and 15-LO
mRNA degradation. When the mean of 15-LO transcripts across all lesion
stages of atherosclerosis were compared with 15-LO transcripts in human
tissue RNA extracts, 15-LO expression in several tissues other than
trachea and lung exceeded that in cardiovascular tissues (Fig. 2).
View larger version (44K):
[in a new window]
Fig. 1.
Expression of LO in atherosclerotic lesions. (a) LO
transcripts in AAO, CAD, and CHD lesions. First column, transcript
species; cycle numbers of samples in third through sixth columns are
indicated in brackets; second row, sizes of PCR products in bp; third
through sixth columns, ethidium bromide-stained PCR products of AAO,
CAD, CHD lesions, and amplified external standards (eSt); seventh
column, numbers of standard cDNA molecules added to PCR buffer before
amplification (n[eSt]). (b) LO and FLAP immunoblots of
CAD type V lesions. For controls, 2 ng of each 5- and 15-LO proteins
was applied; for FLAP, an unspecified amount of leukocyte membrane
protein was applied. Positions of MW standards are indicated by arrows
at right.
View larger version (19K):
[in a new window]
Fig. 2.
Comparison of 15-LO transcripts in human tissue RNA extracts.
Multiple-tissue RNAs or tracheal and bronchial ring RNA were subjected
to 15-LO and GAPDH real-time RT-PCR analyses. Data for cardiovascular
tissues represent the mean of real-time RT-PCR assays performed
on tissues of 38 patients (42 cardiovascular specimens) afflicted
with all lesion types of atherosclerosis.
In view of abundant 5-LO and FLAP transcripts in CAD lesions, we determined whether these transcripts were translated into their corresponding proteins. When 10 µg of total CAD lesion protein extract was subjected to immunoblot analyses, each of four CAD lesions contained significant amounts of 5-LO and FLAP proteins (Fig. 1b). Although our anti-15-LO antisera detected similar amounts of 15-LO standard, this LO protein remained undetectable in immunoblots of CAD lesions (Fig. 1b). These data indicated that 5-LO and FLAP proteins, but not 15-LO protein, were present in type V CAD lesions.
Identification of 5-LO+ Leukocytes in Atherosclerotic Lesions.
We determined the lineage(s) and phenotypes of
5-LO+ cells and searched for
15-LO+ cells. A large number of cells stained for
5-LO in advanced CAD lesions (Fig. 3
A-D). The majority of
5-LO+ cells were CD68+
indicating 5-LO expression in macrophages and/or DCs (Figs.
3B and 4). Moreover, a
subpopulation of CD68+ cells also stained
positive for the DC (Langerhans phenotype) marker antigen, CD1a (ref.
34; Fig. 3H). This indicated the presence of two
5-LO+/CD68+ cell
populations, one resembling a macrophage phenotype and the other a DC
phenotype (35). Another marker of DCs, i.e., DC lysosomal-associated membrane protein (36), was found less frequently, whereas the Langerhans cell marker, langerin (37), remained undetectable. Most
5-LO+ cells strongly stained for HLA-DR,
indicating that the majority of 5-LO+ cells were
activated macrophages and/or DCs capable of antigen presentation (Fig.
3G). Many 5-LO+ cells in CAD
accumulated lipid droplets (Fig. 3 I and K).
Because 5-LO was coexpressed with CD1a and CD68, we designate the two lipid-accumulating cell populations 5-LO+
macrophage foam cells and 5-LO+ DC foam cells.
Three-dimensional construction of 5-LO immunohistochemical positivity
indicated that the bulk of 5-LO protein resided in the nuclear envelope
rather than in the chromatin (Fig. 3 L and M). In
a subpopulation of cells, however, 5-LO was also significantly expressed in the cytosol (Fig. 3 N and O, arrow).
5-LO+ cells were often found in proximity of
5-LO
/CD3+ T lymphocytes
(Fig. 3P). This cellular microenvironment of activated 5-LO+ cells raises the possibility that they
interact with T cells and thereby execute a T cell-dependent immune
reaction. It also became apparent that neither endothelial cells (ECs)
nor smooth muscle cells (SMCs) expressed 5-LO, although both were
strongly MHC-II+. Another
5-LO+ cell population consisted of mast cells
(Fig. 3R) whose number was most prominent in the lamina
adventitia, but mast cells were also found in the lamina intima, and a
minor population of 5-LO+ cells were neutrophilic
CD66b+ granulocytes (not shown). Similar results
were obtained in CHD and AAO (not shown). We next attempted to identify
15-LO+ cells. Our 15-LO antisera specifically
stained bronchial epithelial cells (Fig. 3S), and double LO
staining of human lung revealed that alveolar and subepithelial
5-LO+ macrophages lacked 15-LO, whereas 15-LO
immunostaining in human lung other than bronchial epithelium was
invariably associated with eosinophil peroxidase staining (Fig.
3S; see Fig. 7, which is published as supporting information
on the PNAS web site). By contrast to abundant
5-LO+ cells in all arterial wall laminae (with
the exception of rare eosinophils in the lamina adventitia), no
15-LO+ cells could be detected throughout
atherogenesis (Fig. 3T) in 67 patients (CHD,
n = 39; AAO, n = 22; CAD,
n = 6; see Table 1, which is published as supporting
information on the PNAS web site). However, we identified seven
cases of 15-LO+ cells in the lamina adventitia.
In three patients, aortae contained 15-LO+/keratin+/vimentin+
cell tubes adjacent to a distant portion of the lamina adventitia (Fig.
7). In another aorta specimen, we found eosinophils within a leukocyte
infiltrate located in the lamina adventitia and portions of the outer
lamina media (AHA type V lesion) that thus was classified periarteriitis; additional specimens showed rare eosinophils in the lamina adventitia and, in exceptional cases, in the lamina intima.
Because 15-LO protein remained undetectable in the lamina intima in
each of 78 patients with the exception of very rare eosinophils, 15-LO
could not be associated with atherosclerosis lesion pathology. These
data revealed absence or very low expression of 15-LO and abundant
5-LO+ leukocytes in atherosclerotic lesions.
|
|
5-LO+ Cells Increase in CHD During Transition from Early to Advanced Lesions.
There is little information on the kinetics of leukocyte infiltration
of arterial wall laminae during human atherogenesis (38-40). To
determine these kinetics and those of 5-LO+
cells, we performed morphometric analyses of patients afflicted with
CHD AHA stages 0-V. We first determined cell numbers of
CD68+, mast cell tryptase+,
and CD66b+, and 5-LO+ cells
per length (mm) of internal elastic lamina in a defined area of the
left descending circumflex coronary artery of 29 patients. In
preliminary analyses, we found that 98% of all
5-LO+ cells were CD68+
macrophages/foam cells/DCs in both laminae media and intima of stage
IV-V CAD lesions (n = 7; Fig. 4). However, another
sizable population of 5-LO+ cells in CHD were
adventitial mast cells (9.3% tryptase+ mast
cells, 89.4% CD68+ cells, 1.3%
CD66b+ neutrophils, and negligible numbers of
eosinophils). Mast cells (40) were also found in both laminae intima
and media, although to a much lesser extent (<2%), and
CD66b+ neutrophilic granulocytes represented a
still smaller population (<1.5%) in these compartments. To examine
the possibility that 5-LO expression was related to disease
development, we compared 5-LO+ cells of AHA
lesion stages 0-I with those of AHA stages II-III and IV-V. Most
5-LO+ cells in subclinical stages (0-I and
II-III) resided in the lamina adventitia (Fig. 4), although in each of
the lesions, smaller numbers of 5-LO+ macrophages
were found in the lamina intima. However, as atherogenesis progresses,
marked increases were observed in both laminae intima and media (Fig.
4). When 5-LO+ cells in individual laminae in
stages 0-III (clinically silent) were correlated with lesion stages
IV-V (clinically overt), significant differences became apparent in
each case, i.e., 5-LO+ cells increased 13.5-,
13-, and 3-fold in laminae intima, media, and adventitia, respectively.
These data indicated that the net 5-LO+ cell
influx into arterial walls increases during the time window when
clinically silent lesions develop into clinically apparent lesions, and
that, unlike early lesions, the majority of 5-LO+
leukocytes per total arterial wall resides in the lamina intima in
late-stage disease. The data also revealed that clinically significant
atherosclerosis resembles panarteriitis. Major constituents of
atherosclerotic plaques are SMCs, T cells, collagen, extracellular lipid, and calcified as well as necrotic tissue (3-5), none of which
harbor 5-LO. In view of this heterogeneity, we determined whether the
density of 5-LO+ cells (calculated per
mm2 lesion area) increased during atherogenesis.
We found that this density increased 19-fold in the lamina media
(P < 0.001, n = 7) and 3-fold in
laminae intima and adventitia (P < 0.01, n = 22) when subclinical (0-III) and clinical (IV-V)
stages were compared. These numbers represent averages of
5-LO+ cells per tissue volume
that incompletely reflect the precise cell distribution within the
arterial wall. Thus, 5-LO+ leukocytes are not
distributed uniformly but accumulate at distinct sites such as the
shoulder region below the fibrous cap, thereby forming foci leaving
other areas largely devoid of 5-LO+ cells.
Indeed, inspection of advanced lesions revealed that the density of
5-LO+ cells was found to be very high, sometimes
occupying the majority of the total surface area of a given focus (Fig.
3 D, G, H, and K). The
morphology of atherosclerotic lesions of CHD and extracardial lesions
of muscular arteries are similar; we found that absolute densities of
5-LO+ cells in laminae intimae of type V CHD and
CAD lesions were not very different: CAD, 191 ± 37, n = 6; CHD, 74 ± 23, n = 6 (P = 0.026; means ± SEM; two-sided Mann-Whitney
U test).
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Discussion |
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Abstract
Introduction
Methods
Results
Discussion
References
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Mechanisms of arterial wall inflammation in atherogenesis are poorly understood. Our data reveal expression of the entire 5-LO cascade and of four LT-Rs in AAO, CAD, and CHD. By contrast, reticulocyte-type 15-LO remains undetectable or low with no apparent association to atherosclerosis pathology. That 5-LO+ cells sharply increase during transition from silent to advanced disease is consistent with formation of increasing numbers of circuits of inflammation consisting of 5-LO cascade-expressing leukocytes and LT-R-expressing ECs, SMCs, macrophages, mast cells, and T cells during clinically significant stages of lesion development. This proposition is supported by the many activities that LTs can exert in intact cardiovascular tissues (see below), and by our unpublished data that reveal that each of the cell types that form atherosclerotic lesions show a distinctive LT-R expression pattern as evidenced by both LT-R transcript determination and pharmacological profiles using LT-R antagonists (K.L., R.S., M.H., R. Heller, E. Bretschneider, H. Galczenski, J. F. Evans, and A.J.R.H.).
When considering our observation of low 15-LO expression in human lesions, several caveats deserve attention: (i) Human atherosclerosis requires years to decades to develop into clinically acute disease; expression of 15-LO during a narrow time window (not represented in the lesions studied here) may have escaped detection. (ii) 15-LO expression does not necessarily coincide with predominance of 13(S)-hydroxyoctadecanoic acid (HODE) in lesion lipids (11, 15); thus, 13(S)-HODE may persist longer than 15-LO mRNA or protein. (iii) The lack of selective LO mRNA stability in human lung can only provide presumptive evidence for LO stability in lesion macrophages. (iv) Lesion macrophages represent heterogeneous cell populations (35, 38, 39); 15-LO may be expressed in a small subtype of macrophages. (v) The absolute levels of 15-LO transcripts per total arterial wall RNA may be misleadingly low, because RNA derived from 15-LO-negative cells may be a dilution factor. (vi) Atherosclerosis is an ill defined combination of various chronic inflammatory arterial wall pathologies (3-7); hence, 15-LO may be expressed in some but not all forms of atherosclerosis. Also, 12/15-LO/apo-E double-deficient mice, 12/15-LO/LDL receptor double-deficient mice, and 12/15-LO/apolipoprotein B mRNA editing catalytic polypeptide-1/LDL receptor triple-deficient mice have been shown to develop fewer aorta lesions than apoE-deficient control mice (9, 10, 18). This may be due to reduced LDL oxidation, but also to effects of the enzyme on targets yet to be defined (18). When taken together, it cannot be excluded that there is a role of 15-LO in human atherogenesis.
A salient feature of our data is that 5-LO-dependent inflammatory
circuits expand within the arterial wall notably during late stage
atherogenesis. Participants of these circuits may be LT-forming
leukocytes and LT-R-expressing arterial wall cells, and possibly other
hematopoietic cell lineages. Moreover, release of intermediates
of the 5-LO pathway, i.e., LTA4, from
macrophages/DCs/foam cells/mast cells and its subsequent uptake and
conversion to LTs by neighboring cells may provide mechanisms for
augmented, i.e., transcellular, LT synthesis (41-45). In
this regard, it is of interest that both SMCs and ECs express
LTA4 hydrolase and that ECs express LTC4 synthase and an additional microsomal
glutathione S-transferase, both of which have been
implicated in transcellular LT formation (45). LTs are long known to
exert powerful effects when added to cardiovascular preparations.
Actions of LTs in intact tissues are as varied as coronary artery
contraction, chronotropic effects on heart rate, and impairment of left
ventricular contractility (20), edema formation in the microcirculation
(21), and mononuclear cell recruitment into tissues (21). LTs also
trigger a variety of activities in cultured arterial wall cells,
including induction of P-selectin, von Willebrand factor (46), and
platelet-activating factor (47) in ECs, and stimulation of SMC
proliferation (48-50). Beyond its established role in inflammation,
the 5-LO pathway has been implicated in the regulation of immune
responses: The 5-LO cascade is expressed in DCs (29, 34), LTs activate
T and B cells (references in ref. 51) and affect DC migration to
regional lymph nodes (52), and most cells that participate in immune
reactions express LT-Rs (29-33, 53). Despite these powerful
activities, the role of 5-LO in the pathogenesis of atherosclerosis has
not received much attention. Because detailed information on the 5-LO
pathway in atherosclerosis has not yet been available, potential
mechanisms of LT formation and LT-R target cells have been difficult to
conceive. Our data suggest that large numbers of
5-LO+ leukocytes may act from within the lesions
rather than from the blood vessel lumen in the proximity of cells that
express LT-Rs during late-stage atherogenesis. Because
5-LO+ macrophages/DCs/foam cells express MHC-II
molecules and localize in the proximity of activated T cells (54), they
may present antigen and thereby establish immune response circuits. In
unpublished studies (K.L., R.S., M.H., R. Heller, E. Bretschneider, H. Galczenski, J. F. Evans, and A.J.R.H.), we have observed
differential LT-R expression in cultured human SMCs and ECs and that
cysLTs induce sustained oscillatory Ca2+
transients in ECs. When previously observed actions of LTs on ECs and
SMCs are considered with our present data, LT-generating leukocytes may
activate arterial wall cell and leukocyte LT-Rs and thus exert a
multitude of actions on blood vessel homeostasis. CysLT-dependent
coronary artery contraction was documented by Corey and colleagues more
than 20 years ago (20). Recently, Allen et al. (24) reported
hypercontractility toward cysLTs in diseased versus normal coronary
arteries. The anatomy, frequency, and kinetics of generation of
5-LO-containing infiltrates observed here are compatible with
participation of LTs to several hallmarks of clinically overt
atherosclerosis, including EC dysfunction, intimal edema, leukocyte
infiltration, aberrant contractility, SMC proliferation, and immune
reactivity. A recent study by Mehrabian et al. (55)
indicates a significant role of the 5-LO gene in atherosclerosis
susceptibility of hyperlipidemic LDL
receptor/ mice providing functional evidence
for an indispensable involvement of 5-LO in the pathogenesis of the
disease in experimental atherosclerosis models. Although these data
require confirmation in additional model systems, deficiency of only
one 5-LO allele surprisingly conferred potent protection against
atherosclerosis development of LDL receptor/
mice. In addition, Aiello et al. (56) demonstrated that
pharmacological BLT-R antagonism was also protective in three
atherosclerosis-susceptible mouse strains. Anti-LT drugs are already in
use for the treatment of bronchial asthma in man (57). Their
availability represents a unique opportunity to test whether
pharmacological inhibition of the 5-LO cascade will beneficially affect
the clinical outcome of the disease.
| |
Acknowledgements |
|---|
B.S. and A.J.R.H. dedicate this article to the memory of Russell Ross. We thank J. Glomset (Howard Hughes Medical Institute Laboratory, University of Washington, Seattle) and D. Steinberg (Department of Medicine, University of California at San Diego, La Jolla) for critical comments, H. Kosmehl (Department of Pathology, University of Jena) for identification of 15-LO-expressing cell structures, Sem Saeland (Schering-Plough, Dardilly, France) for a gift of anti-langerin antiserum, and G. Weber, M. Voigt, C. Ströhl, and M. Franke for expert technical assistance. Antiserum against 5-LO was prepared by Dr. Y.-Y. Zhang and A. Nordberg (Karolinska Institute). This study was supported by Deutsche Forschungsgemeinschaft Grant Ha 1083/13-1/13-2, European Union Research Network Grant QLG1-CT-2001-01521, Interdisziplinäres Zentrum für Klinische Forschung Jena Grants TP4.4 and TP4.9, Swedish Research Council Grant 03X-217, and a grant from the Stiftung für Verhalten und Umwelt.
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Abbreviations |
|---|
AAO, atherosclerosis of the aorta; AHA, American Heart Association; CAD, carotid artery disease; CHD, coronary heart disease; DC, dendritic cell; ECs, endothelial cells; LO, lipoxygenase; FLAP, 5-LO activating protein; GAPDH, glyceraldehyde-3-phosphate dehydrogenase; LDL, low-density lipoprotein; LT, leukotriene; LT-R, LT receptor; SMCs, smooth muscle cells.
| |
Footnotes |
|---|
R.S., R.G., and K.L. contributed equally to this work.
To whom correspondence should be addressed. E-mail:
spanbroek{at}zmkh.ef.uni-jena.de.
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References |
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Abstract
Introduction
Methods
Results
Discussion
References
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