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Blood, Vol. 96 No. 1 (July 1), 2000:
pp. 176-181
HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY
From the Tumor Angiogenesis Laboratory, Department of
Internal Medicine, University Hospital Maastricht, Maastricht,
The Netherlands; and the Department of Biochemistry, Molecular Biology
and Biophysics, University of Minnesota Health Sciences Center,
Minneapolis, Minnesota.
Bactericidal/permeability-increasing protein (BPI) has been known
for some time to function in killing bacteria and in neutralizing the
effects of bacterial endotoxin lipopolysaccharide. In the present
study, BPI is found to be a novel endogenous inhibitor of angiogenesis.
Within the sub-µM range, BPI shows a
concentration-dependent inhibition of endothelial cell (EC)
proliferation that is mediated by cell detachment and subsequent
induction of apoptosis. As measured by flow cytometric analysis of the
percentage of subdiploid cells, apoptosis induction was half-maximal at
about 250 nmol/L BPI. Apoptosis was confirmed by quantification of
cells with nuclear fragmentation. Apoptosis was found to be EC
specific. In an in vitro collagen gel-based angiogenesis assay, BPI at
1.8 µmol/L inhibited tube formation by 81% after only 24 hours.
Evidence for in vivo inhibition of angiogenesis was obtained, using the chorioallantoic membrane assay in which BPI was seen to be
significantly effective at concentrations as low as 180 nmol/L. This
newly discovered function of BPI might provide a possible therapeutic
modality for the treatment of various pathologic disorders that depend on angiogenesis.
(Blood. 2000;96:176-181)
The 55-kd bactericidal protein produced by human
neutrophils is most well known as the
bactericidal/permeability-increasing factor (BPI),1,2 but
it is also known as the cationic antibacterial protein of 57 kd
(CAP57)3 and as the bactericidal protein of 55 kd molecular
mass (BP55).4,5 BPI is most bactericidal against
gram-negative bacteria1 and has been shown to neutralize both the pyrogenicity of bacterial lipopolysaccharide (LPS) in rabbits
and the ability of LPS to initiate the coagulation pathway of the
Limulus amoebocyte lysate or to cause tumor necrosis factor (TNF) release from human monocytes.6 BPI functions by
binding to the lipid A moiety of LPS,7 whereby neutralizing
the ability of this endotoxin to up-regulate the expression of
complement receptors on neutrophils and to cause a systemic
inflammatory response during bacterial infection. Lipid A consists of a
phosphorylated diglucosamine moiety attached to 2 fatty acyl chains.
Because BPI is cationic and is known to bind the polysulfated
glycosaminoglycan heparin,8 it may function by effectively
interacting with the anionic phosphate groups on LPS. Relatedly, many
proteins isolated from blood are cationic and bind heparin. One of
these proteins, platelet factor-4 (PF4), is a potent
anticoagulant, perhaps the strongest binder of heparin, is
antiangiogenic, and is also known to be bactericidal.9,10
Until now, aside from its antibacterial effects, no other activities
for BPI have been reported. Given chemical similarities between BPI and
PF4 and the fact that they share at least some biological activities,
it was postulated that they may display other functional similarities.
Probably the most clinically important activity of PF4 is its ability
to inhibit angiogenesis.11,12 Angiogenesis, or the
outgrowth of capillaries from existing vasculature, occurs during
physiological processes, such as embryogenesis, the menstrual cycle,
and wound healing, but it is also involved in numerous pathologic
disorders requiring vascular outgrowth, such as cancer, arthritis, and
atherosclerosis. A major interest in angiogenesis has developed in the
field of oncology because it has been recognized that tumors, which are
dependent on angiogenesis for outgrowth and metastasis, can be treated
by attacking their blood supply.13,14
Here it is reported that BPI, like PF4, is indeed an effective
inhibitor of angiogenesis. We found that BPI inhibits endothelial cell
(EC) growth at low doses, leading to the inhibition of angiogenesis both in vitro and in vivo. The commonality between antiangiogenic and
antibacterial proteins and the role of angiogenesis during inflammation
are discussed. The fact that BPI is now found to be an endogenous
inhibitor of angiogenesis makes it an important pharmacologic candidate
for future antiangiogenic therapy in the clinic.
Purification of BPI
Cell culture
Proliferation assay HUVECs were seeded in a 96-well culture plate coated with 1 mg/mL fibronectin (2 hours at 20°C) at a concentration of 3000 cells per well in a volume of 50 µL. The cells were allowed to adhere for 3 hours at 37°C at 5% CO2, and subsequently, 50 µL culture medium with 20 ng/mL basic fibroblast growth factor (bFGF), with or without BPI, was added. The cells were cultured for 72 hours. During the last 6 hours of the assay, the culture was pulsed with 0.5 µCi [methyl-3H]-thymidine (Amersham Life Science) per well. Activity was measured using liquid scintillation. Measurements were done in triplicate.Apoptosis assay HUVECs were seeded at a concentration of 3000 cells per well in a 1 mg/mL, fibronectin-coated, 96-well culture plate. The cells were cultured during 72 hours either in normal culture medium; in the presence of BPI, PF4, and BSA at different concentrations, or under serum deprivation. In some experiments, cells were cultured with or without 5 IU heparin (Leo Pharmaceutical Products, Weesp, The Netherlands). After 72 hours of culture, the cells were harvested with 0.125% trypsin. Part of the cells was used to make cytospin preparations on glass slides for determination of cell morphology after haematoxillin/eosin staining. The remaining cells were centrifuged at 1500 rpm for 5 minutes, washed once with PBS, and subsequently fixed in 70% ethanol at 20°C for 2 hours. The cells were pelleted at
1500 rpm and resuspended in DNA extraction buffer (90 volumes 0.05 mol/L Na2HPO4.2H2O, 10 volumes of
0.025 mol/L citric acid, and 1 volume of 10% Triton-X100 [in
distilled water, pH7.4]) and incubated at 37°C for 20 minutes.
After this incubation period, propidium iodide was added at a
concentration of 20 µg/mL, and the DNA profile of the HUVECs was
analyzed on the flow cytometer (FACS Calibur; Becton Dickinson). In
some experiments, the caspase inhibitor z-VAD.FMK (Alexis Biochemicals)
was used (100 µmol/L) to inhibit apoptosis.17 Statistical
significance was determined using the Mann-Whitney U test.
In vitro angiogenesis Sprouting and tube formation of ECs were studied with the use of cytodex-3 beads overgrown with ECs in a 3-dimensional gel.18,19 Bovine microvascular ECs (BCEs) were mixed with gelatin-coated cytodex-3 microcarrier beads (Sigma, The Netherlands) at a concentration of 25 cells per bead and cultured for 72 hours in a tissue culture plate in RPMI-1640, supplemented with 20% HS, 2 mmol/L L-glutamine, 50 ng/mL streptomycin, and 50 U/mL penicillin. The beads were spun down and resuspended in a concentration of 25 beads per 100 µL, in 8 volumes of vitrogen-100 (Collagen, Fremont, CA), 1 volume 10 × concentrated -MEM (Life Technologies, Breda, The
Netherlands), 1 volume 11.76 mg/mL sodium bicarbonate, and 20 ng/mL
bFGF. This mixture (100 µL) was suspended to each well of a 96-well
culture plate, after which gelation was allowed to take place at
37°C. After gelation medium was applied on top of the gel
containing 20 ng/mL bFGF with or without BPI at concentrations as
indicated and with or without 5 IU/mL heparin. After 24 hours,
photographs were made. For quantification, these images were analyzed
using NIH image computer software. Statistical analysis was done using the Mann-Whitney U test.
Chorioallantoic membrane assay Fertilized white leghorn chicken eggs were incubated for 3 days at 37°C and 60% humidity. On the third day, a hatch was made in the eggshell. The eggs were further incubated at 37°C and 60% humidity until day 7. On this day, a silicone ring was placed directly onto the chorioallantoic membrane (CAM) and was left to stabilize for 2 hours. Subsequently, the treatment of the CAMs started by daily addition of 65 µL of either vehicle (saline), 180 nmol/L or 540 nmol/L BPI dissolved in saline. On day 10, the CAMs were photographed. Quantification of vascularization was performed by enumeration of intersections with 3 concentric rings that were superimposed on the photographs.
BPI inhibits EC growth Potential angiogenic effects from BPI were first investigated in vitro with the use of an EC proliferation assay with cultured HUVECs. EC proliferation was measured using a [3H]-thymidine incorporation assay and by enumeration of living cells following 3 days of culture of HUVECs in the presence of various concentrations of BPI. Both bFGF-induced (20 ng/mL) (Figure 1) and spontaneous (not shown) EC proliferation were inhibited by BPI in a similar concentration-dependent fashion. BPI inhibited 80% proliferation at 1.8 µmol/L, whereas the half-maximal response was observed at about 250 nmol/L (Figure 1A). To discriminate between cytostatic and cytotoxic effects, proliferation was also investigated by quantifying the number of living cells, using the trypan blue dye-exclusion method. Similar results were found in both assays. In these experiments, BSA was used as a negative control, and the angiogenesis inhibitor PF411 was used as a positive control. The dye-exclusion method indicated that BPI is cytotoxic for ECs, whereas PF4 has been recognized as being cytostatic and not cytotoxic20 (Figure 1B). Figure 1C demonstrates that HUVECs are at least an order of magnitude more sensitive to BPI than to PF4, in the [3H]-thymidine incorporation assay.
BPI induces apoptosis in ECs
Heparin blocks the apoptosis inducing activity of BPI
BPI inhibits in vitro angiogenesis
BPI inhibits angiogenesis in vivo
A novel biological activity for BPI has been reported in
this study. BPI has joined the list of antiangiogenic agents that include PF4, angiostatin,22 and endostatin.23
More and more angiogenesis inhibitors are continually being discovered,
and only a few will ever be used in therapeutic applications.
BPI, aside from providing a potential treatment against sepsis, might also be used in the treatment of cancer and/or other
angiogenesis-related pathological disorders. In its capacity as an
antiangiogenic agent, BPI works specifically on and is cytotoxic to
ECs, whereas both PF4 and endostatin, for example, are cytostatic,
arresting ECs in the cell cycle.11,20 The concentration at
which BPI is half-maximally effective at inhibiting in vitro
angiogenesis, 80 nmol/L, is considered to be quite low relative to that
of many other inhibitors of angiogenesis,22,23 like
PF411 that demonstrates a similar effectivity at a
concentration about 10-fold higher in inhibiting proliferation;
however, the antiangiogenic effects in the in vitro assay were quite
similar.20
Submitted September 21, 1999; accepted February 23, 2000.
Reprints: Daisy W. J. van der Schaft, Tumor Angiogenesis
Laboratory, Department of Internal Medicine, University Hospital Maastricht, P.O. Box 5800, 6202 AZ Maastricht, The Netherlands; e-mail:
DvdSchaft{at}hotmail.com.
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.
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Abstract
Introduction
3-integrin antibody,
which binds the EC surface 
