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Blood, Vol. 94 No. 6 (September 15), 1999:
pp. 2020-2028
By
From the Laboratoire de Biologie Vasculaire et Cellulaire,
Unité de Formation et de Recherche Lariboisière-St Louis,
Paris 7, INTS, Paris, France; the Département de
Radiologie Interventionnelle, Hôpital Lariboisière, Paris,
France; and the Institute of Pathology, University of Bonn, Bonn,
Germany.
Vascular malformations are frequent in newborns, and they persist
throughout life, which differentiates them from vascular tumors (eg,
hemangiomas). Arteriovenous malformations are high-flow vascular
malformations. They are considered nonmalignant but can expand and
become a significant clinical risk when extensive. To characterize
endothelial cells from arteriovenous malformations (AMEC), we cultured
cells obtained from surgical specimens and studied their properties.
After selection, the cells that grew out from explants had phenotypic
and antigenic features (platelet endothelial cell adhesion molecule,
von Willebrand factor) of human endothelial cells. Their spontaneous
proliferation rate was higher (1.8 to 6.4 times) than that of human
umbilical vein, arterial, or microvascular endothelial cells. The
proliferation rate of AMEC was not sensitive to the inhibitory activity
of various cytokines (interleukin-1
ANGIOGENESIS and vasculogenesis, which
are observed during embryogenesis and body growth, are essential for
organogenesis and tissue nutrition.1 Frequently, angiogenic
abnormalities are observed in newborns. They are classified according
to their anatomical location and angiographic and developmental
characteristics. In the classification proposed by Mulliken and
Glowacki,2 hemangiomas are different from vascular
malformations. Hemangiomas are involutive tumors, whereas vascular
malformations are composed of dysplastic vessels. Arteriovenous
malformations are high-flow vascular abnormalities, which usually
exhibit a slow rate of expansion. Growth can be acutely accelerated,
however, depending on factors such as puberty, pregnancy, and trauma.
The tumor mass produced may alter the contiguous tissues. Such
arteriovenous malformations represent a critical risk when located in
the head and cervicocephalic region. They are not responsive to
pharmacologic treatment, (eg, corticosteroid or interferon This study was conducted in accordance with the principles of the
Declaration of Helsinki and the 1975 Declaration of Tokyo. Surgical
excisions were performed in 11 consecutive patients with arteriovenous
malformations, and samples were collected (Fig
1A). Cells were successfully cultured from
the surgical biopsies of 6 patients. Because a limited number of cells
grew in culture, a complete characterization could only be achieved in
4 cases. In the other 5 cases, the tissues were either necrotic after
embolization, infected, or did not grow in in vitro conditions. The
main clinical features of the patients are summarized in Table
1. The hemostatic parameters were normal
and there was no evidence of intravascular coagulation.
Materials
Cytokine Growth Factors and Other Reagents
Culture Media and Sera
Antibodies Specific anti-vascular cell adhesion molecule-1 (VCAM-1) and anti-intercellular adhesion molecule-1 (ICAM-1) antibodies were obtained from British Biotechnologies (Abingdon, UK); the antibody directed against E-selectin (H18/7) and the isotype-matched nonbinding E1A monoclonal antibody (MoAb) were a gift from MP Bevilacqua (La Jolla, CA). The 125I-labeled sheep antimouse IgG F(ab')2 fragment was from Amersham; bis Benzimide (Hoechst 33258) was from Sigma.
Cell Culture Equipment T25 culture flasks (25 cm2), 35-mm plastic dishes, and tissue culture trays (96 wells or 24 wells) were all from Costar (Cambridge, MA).Methods Cell Culture Human umbilical vein endothelial cells (HUVEC). HUVEC were grown as previously described.4 Cells were cultured in M199 medium supplemented with glutamine, HEPES buffer, amphotericin B, and gentamicin and containing human serum AB (15% vol/vol). Cells were tested after 1 to 3 passages. Human arterial endothelial cells (HAEC). HAEC were cultured from human umbilical cords according to a previously described technique.5 After digestion with collagenase at 37°C for 10 minutes, endothelial cells were centrifuged, and the cell pellet was resuspended in M199 medium supplemented with glutamine, HEPES buffer, amphotericin B, and gentamicin and containing human serum AB (15% vol/vol). Arterial endothelial cells were seeded on gelatin (0.2% wt/vol) precoated dishes at a concentration of 40,000 per square centimeter. The medium was changed 3 or 4 hours later (when the cells were attached) and every 2 days, until the cells reached confluence (6 or 7 days). Cells were tested after 1 to 3 passages. Human microvascular endothelial cells (HMEC). Because in prior experiments we observed unexpected results with HMEC, as reported by Xu et al,6 we tested in parallel 2 types of human microvascular endothelial cells from different origins and cultured them according to the techniques described by the manufacturer. The HMEC-1 cell line was obtained from the Center for Disease Control (Atlanta, GA) and passaged in medium MCDB131, which was supplemented with hydrocortisone (1 µg/mL), EGF (10 ng/mL), and 15% FCS. Arteriovenous malformation-derived endothelial cells (AMEC). During the surgical operation, a specimen of the arteriovenous malformation was dissected and put into a container filled with gentamicin and amphotericin diluted in HBSS. The surgical explants were cut into pieces of 1 mm2 and plated on gelatin (0.2%) precoated 35-mm plastic dishes; 0.8 mL of medium M199 with 20% FCS was then added. After 4 to 6 weeks of culture, the selection of endothelial cells growing out from explants was performed in several steps. First, cell colonies, which did not have the gross morphology of endothelial cells (under inverted phase contrast microscopy), were detached by scraping and removed from the dish by aspiration. The colonies that exhibited the characteristic cobblestone morphology of endothelial cells were allowed to proliferate in the dish for 1 week, selected as before, and then subcultured. Cells generated from this selection were called AMEC. AMEC were obtained from 4 different patients (no. 1 to 4). The flow cytometry analysis (FACS) was performed on cells after 2 or more passages. FACS analysis, the proliferation assay, and adhesion molecule expression measurements were performed on the same passage. Monocytes, smooth muscle cells, and fibroblasts. Monocytes were isolated from normal human blood. Smooth muscle cells (SMC) isolated from human uterine arteries, and fibroblasts derived from human skin were kindly provided by INSERM U.353 (Paris, France). Flow Cytometry Analysis After harvesting, cells in suspension were washed, incubated for 30 minutes with the antibodies, and then washed again. The binding of antibodies was shown by incubating the cells with FITC-conjugated antimouse or antirabbit polyclonal antibodies at a dilution giving a negative signal when tested with cells in absence of the first antibody. The immunofluorescence was quantified by FACS (FacScan; Becton Dickinson, Mountain View, CA). For each antibody, 5,000 events were recorded. The cell population was analyzed, and the results were expressed as a percentage of fluorescent cells and the mean fluorescence intensity in arbitrary units of fluorescence (AUF). The forward side scatter (FSC) versus side scatter (SSC) dot plot of HUVEC or AMEC are shown in Fig 2.
In Situ Hybridization With c-ets-1 Riboprobes Immediately after biopsy, the material was fixed in paraformaldehyde (4%) for 24 hours at 4°C, dehydrated through graded alcohols, and embedded in paraffin. Five-micrometer-thick transverse sections were transferred to slides coated with 3-aminopropyl-triethoxysilane. In situ hybridization protocols with 35S-labeled c-ets-1 riboprobes were performed as described elsewhere.7,8 The slides were dipped in the NTB2 nuclear track emulsion and exposed for 10 to 15 days in sealed boxes with dessicator at 4°C. In all experiments, the antisense and the sense probes were hybridized on neighboring sections. The control c-ets-1 sense probe gave no signal. Under darkfield illumination, endothelial cells could be unambiguously identified by comparison with neighboring cells stained conventionally with hematoxylin and eosin.Proliferation Assay Cell proliferation was assayed in triplicate by incorporation of [methyl-3H]thymidine into acid-insoluble DNA of cultured endothelial cells (HUVEC, HAEC, HMEC, and AMEC) as previously described.9 Cells were seeded into 96-well plates, and 2 or 3 hours later (when the cells were adherent), the cultures were incubated for 24 hours with or without cytokines (20 U/mL IL-1 , 500 U/mL TNF- , 250 U/mL IFN- , 2 ng/mL TGF-) in medium M199 with
10% FCS. In previous work,9 we determined the cytokine
concentration that produced 50% inhibition of HUVEC
proliferation. The cells were then pulsed with
[methyl-3H]thymidine for 16 hours and harvested
using an automatic cell harvester (Skatron, Lier, Norway) on glass
fiber filters. Incorporated radioactivity was counted in a
beta counter (Beckman, Fullerton, CA). Percentage of inhibition
of proliferation was determined for each cytokine by comparison
of incorporation of radioactivity expressed in counts per minute in
cytokine-treated endothelial cells and in untreated control cells.
Determination of Adhesion Molecules Expression Confluent HUVEC, HMEC, or AMEC monolayers in microplates were stimulated with IL-1 (100 U/mL) or TNF- (500 U/mL) for 4, 16, or
24 hours before the measurement of E-selectin (CD62E), VCAM-1 (CD106),
and ICAM-1 (CD54) expression. After 2 washes, the monolayers were
incubated for 1 hour on ice in RPMI medium plus 10% FCS containing
specific antibodies (anti-E-selectin [H18/7], anti-VCAM-1, or
anti-ICAM-1). The binding was shown with a second antibody,
125I-labeled sheep antimouse IgG F(ab')2
fragment. The cells were washed, solubilized with sodium dodecyl
sulfate (SDS) (0.1%)-NaOH (25 mmol/L) solution, and then collected.
The radioactivity was measured in a gamma counter (Beckman, Fullerton,
CA). The specific binding was calculated by subtracting the nonspecific
radioactivity that was measured in wells labeled with the
isotype-matched nonbinding E1A MoAb.10
Statistical Analysis The results are expressed as mean ± standard deviation. Statistical analysis was performed by using Wilcoxon's rank sum test for paired values for comparison of the effect of the different cytokines (IL-1, TNF-, IFN-, and TGF-) on adhesion molecule expression on the cell surface of HUVEC, HMEC, and AMEC. Comparison of
inhibition of proliferation of AMEC, HMEC, and HAEC to HUVEC by the
different cytokines were performed by using one-way ANOVA followed by
the parametric Dunnett's test.
Morphological Aspect The initial culture from surgical pieces of arteriovenous malformations (Fig 1A) contained heterogeneous populations. Only cultured cells that had the morphological characteristics of endothelial cells were kept. At confluence, HUVEC had a cobblestone aspect when cultured on gelatin-coated plastic dishes with a strict monolayer growth (Fig 1B). At confluence, AMEC cultured on gelatin-coated plastic dishes had an elongated form with an endothelial-like polygonal morphology. They were closely contiguous and grew as a monolayer (Fig 1C).Flow Cytometry Analysis Cultures in which mixed populations were present, ie, either SMCs and endothelial cells, or endothelial cells and fibroblasts, or a pure endothelial cell population (Fig 2D), demonstrated different scatter patterns, when analyzed for size and nuclearity.
Cell Proliferation Studies
C-ets-1 in situ Hybridization
Cytokine Stimulation
Adhesion Molecule Expression
The endothelial cells cultured from explants of arteriovenous
malformations may originate from the vascular malformation or, for a
small proportion, from adjacent vessels. The characteristics of these
cells, compared with endothelial cells from arterial or venous origin
or from normal skin microvessels, are different, which is in favor of
their origin from the arteriovenous malformation.
The authors are grateful to F. Vileyn (INTS) and LPH/Hôpital St
Louis members (Paris) for their help in preparing this manuscript. Pr
J. Levin is acknowledged for helpful reviewing of the manuscript (University of California School of Medicine, San Francisco, CA).
Submitted July 15, 1998; accepted May 18, 1999.
O.C. was a recipient of a fellowship from ADR Biologie vasculaire
cellulaire, Paris, France and N.W. was a recipient of a grant from the
Dr Mildred Scheel Foundation, Germany.
The publication costs of this
article were defrayed in part by
page charge payment. This article
must therefore be hereby marked
"advertisement"
in accordance with 18 U.S.C. section
1734 solely to indicate this fact.
Address reprint requests to Jean-Luc Wautier, MD,
Laboratoire de Biologie Vasculaire et Cellulaire, Institut National de
la Transfusion Sanguine, 6, rue Alexandre Cabanel, 75739 Paris Cedex
15, France; e-mail: wautier{at}ints.fr.
1.
Folkman J, Shing Y:
Angiogenesis.
J Biol Chem
267:10931, 1992
2.
Mulliken JB, Glowacki J:
Hemangiomas and vascular malformations in infants and children, a classification based on endothelial characteristics.
Plast Reconstr Surg
69:412, 1982[Medline]
[Order article via Infotrieve]
3.
Höyhtyä M, Myllylä R, Piuva J, Kivirikko K, Tryggvason K:
Monoclonal antibodies to human prolyl-4-hydroxylase.
Eur J Biochem
141:477, 1984
4.
Wautier JL, Paton C, Wautier MP, Pintigny D, Abadie E, Passa P, Caen JP:
Increased adhesion of erythrocytes to endothelial cells in diabetes mellitus and its relation to vascular complications.
N Engl J Med
305:237, 1981[Abstract]
5.
Weiss R, Sun B, Rodgers BD:
An improved method of human umbilical arterial endothelial cell culture.
Thromb Res
61:171, 1991[Medline]
[Order article via Infotrieve]
6.
Xu Y, Swerlick R, Sepp N, Bosse D, Ades E, Lawley T:
Characterization of expression and a modulation of cell adhesion molecules on an immortalized human dermal microvascular endothelial cell line (HMEC-1).
J Invest Dermatol
102:833, 1994[Medline]
[Order article via Infotrieve]
7.
Vandenbunder B, Pardanaud L, Jaffredo T, Mirabel MA, Stehelin D:
Complementary patterns of expression of c-ets-1, c-myb and c-myc in the blood forming system of the chick embryo.
Differentiation
107:265, 1989
8.
Wernert N, Raes MB, Lassalle P, Dehouck MP, Gosselin B, Vandenbunder B, Sthelin D:
C-ets-1 proto-oncogene is a transcription factor expressed in endothelial cells during tumor vascularization and other forms of angiogenesis in humans.
Am J Pathol
140:119, 1992[Abstract]
9.
Delomenie C, Wautier MP, Chappey O, Wautier JL:
Modulation of human endothelial cell activation by antiproliferative cytokines: Exploration of arachidonic acid and intracellular cytokine pathways as possible mechanisms of action.
Exp Cell Res
207:122, 1993[Medline]
[Order article via Infotrieve]
10.
Pober JS, Bevilacqua MP, Mendrick DL, Lapierre LA, Fiers W, Gimbrone MA Jr:
Two distinct monokines, interleukin 1 and tumor necrosis factor, each independently induce biosynthesis and transient expression of the same antigen on the surface of cultured human vascular endothelial cells.
J Immunol
136:1680, 1986[Abstract]
11.
Fajardo LF:
The complexity of endothelial cells.
Am J Clin Pathol
92:241, 1989[Medline]
[Order article via Infotrieve]
12.
Takahashi K, Mulliken JB, Kozakewich HP, Rogers RA, Folkman J, Ezekowitz RAB:
Cellular markers that distinguish the phases of hemangioma during infancy and childhood.
J Clin Invest
93:2357, 1994
13.
Piali L, Fichtel A, Terpe HJ, Imhof BA, Gisler RH:
Endothelial vascular cell adhesion molecule-1 expression is suppressed by melanoma and carcinoma.
J Exp Med
181:811, 1995
14.
Griffioen AW, Damen CA, Martinotti S, Blijham GH, Groenewegen G:
Endothelial intercellular adhesion molecule-1 expression is suppressed in human malignancies: The role of angiogenic factors.
Cancer Res
56:1111, 1996
15.
Kitayama J, Nagawa H, Yasuhara H, Tsuno N, Kimura W, Shibata Y, Muto T:
Suppressive effect of basic fibroblast growth factor on transendothelial emigration of CD4(+) T-lymphocyte.
Cancer Res
54:4729, 1994
16.
Griffioen AW, Damen CA, Blijham GH, Groenewegen G:
Tumor angiogenesis is accompanied by a decreased inflammatory response of tumor-associated endothelium.
Blood
88:667, 1996
17.
Gimbrone MA Jr, Nagel T, Topper JN:
Biomechanical activation: An emerging paradigm in endothelial adhesion biology.
J Clin Invest
99:1809, 1997[Medline]
[Order article via Infotrieve]
18.
Topper JN, Cai J, Falb D, Gimbrone MA Jr:
Identification of vascular endothelial genes differentially responsive to fluid mechanical stimuli: cycloxygenase-2, manganese superoxide dismutase, and endothelial cell nitric oxide synthase are selectively up-regulated by steady laminar shear stress.
Proc Natl Acad Sci USA
93:10417, 1996
19.
Iwasaka C, Tanaka K, Abe M, Sato Y:
Ets-1 regulates angiogenesis by inducing the expression of urokinase-type plasminogen activator and matrix metalloproteinase-1 and the migration of vascular endothelial cells.
J Cell Physiol
169:522, 1996[Medline]
[Order article via Infotrieve]
20.
Athanassiou M, Mavrothalassitis GJ, Yuan CC, Blair DG:
The Gag-Myb-Ets fusion oncogene alters the apoptotic response and growth factor dependence of interleukin-3 dependent murine cells.
Oncogene
12:337, 1996[Medline]
[Order article via Infotrieve]
21.
Bories JC, Willerford DM, Grevin D, Davidson L, Camus A, Martin P, Stehelin D, Alt FW:
Increased T-cell apoptosis and terminal B-cell differentiation induced by inactivation of Ets-1 proto-oncogene.
Nature
377:635, 1995[Medline]
[Order article via Infotrieve]
22.
Chen HM, Boxer LM:
23.
Nelson B, Tian G, Erman B, Gregoire J, Maki R, Graves B, Sen R:
Regulation of lymphoid-specific immunoglobulin µ heavy chain gene enhancer by ETS domain proteins.
Science
261:82, 1993
24.
Memon SA, Moreno MB, Petrak D, Zacharchuck CM:
Bcl-2 blocks glucocorticoid -but not Fas- or activation-induced apoptosis in a T cell hybridoma.
J Immunol
155:4644, 1995[Abstract]
25.
Tsukada T, Eguchi K, Migita K, Kawabe Y, Kawakami A, Matsuoka N, Takashima H, Mizokami A, Nagataki S:
Transforming growth factor beta 1 induces apoptotic cell death in cultured human umbilical vein endothelial cells with down-regulated expression of bcl-2.
Biochem Biophys Res Commun
210:1076, 1995[Medline]
[Order article via Infotrieve]
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