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Blood, Vol. 95 No. 10 (May 15), 2000:
pp. 3232-3241
RED CELLS
From the Cox Laboratory for Biomedical Engineering, Rice University,
and the Department of Medicine, Baylor College of Medicine, Houston,
TX.
Sickle cell anemia is characterized by periodic vasoocclusive
crises. Increased adhesion of sickle erythrocytes to vascular endothelium is a possible contributing factor to vasoocclusion. This
study determined the effect of sickle erythrocyte perfusion at a venous
shear stress level (1 dyne/cm2) on endothelial cell (EC)
monolayers. Sickle erythrocytes up-regulated intercellular adhesion
molecule-1 (ICAM-1) gene expression in cultured human
endothelial cells. This was accompanied by increased cell surface
expression of ICAM-1 and also elevated release of soluble
ICAM-1 molecules. Expression of vascular cell adhesion molecule-1
(VCAM-1) messenger RNA (mRNA) was also strikingly elevated in cultured
ECs after exposure to sickle cell perfusion, although increases in
membrane-bound and soluble VCAM-1 levels were small. The presence of
cytokine interleukin-1
Sickle cell anemia is a genetic disorder of red blood
cells (RBCs) characterized by chronic hemolysis and episodic
vasoocclusive crises. Abnormally high adhesion of sickle erythrocytes
to vascular endothelial cells (ECs) is hypothesized to be a
contributing factor to the initiation and progression of vascular
occlusion.1 Several plasma proteins and receptors expressed
on erythrocyte membranes and EC surfaces have been shown to be involved
in the receptor-mediated adhesion of sickle cells to the
endothelium.2,3 In this study we examined the role of
contact with flowing sickle erythrocytes on the production of cell
adhesion molecules by endothelial cells.
Intercellular adhesion molecule-1 (ICAM-1) and vascular cell adhesion
molecule-1 (VCAM-1) are cytokine-inducible, single-chain glycoproteins
belonging to the immunoglobulin superfamily. ICAM-1 is constitutively
expressed on vascular endothelium and is up-regulated in response to
various stimuli, including cytokines during
inflammation.4,5 It plays an important role in leukocyte
adhesion to endothelial cells. Lymphocyte function-associated
antigen-1 (LFA-1) (CD11a/CD18, VCAM-1 is present in activated ECs after stimulation with cytokines
such as interleukin-1 In this study we investigated the effects of perfusion with sickle
erythrocytes on the production of ICAM-1 and VCAM-1 by cultured human
endothelial cells. A flow apparatus was developed to perfuse sickle
cells over cultured human ECs under well-characterized flow conditions
for times of up to 24 hours. Endothelial cell surface expression and
release of soluble forms of both ICAM-1 and VCAM-1 were examined after
exposure to sickle cell perfusion at 1 dyne/cm2.
Quantitative reverse transcriptase-polymerase chain reaction (RT-PCR)
combined with high pressure liquid chromatography (HPLC) analysis was
used to determine the amounts of ICAM-1 and VCAM-1 messenger RNA (mRNA)
in endothelial cells.
In sickle cell disease, inflammation often precedes or is associated
with pain crises.30 Levels of cytokines, such as IL-1 and
TNF- Endothelial cell culture
Isolation of RBCs
Flow apparatus For flow studies, the flow system was assembled as shown in Figure 1. The flow apparatus consisted of a parallel plate flow chamber, a reciprocating dual syringe pump (New Harvard `33' Double Syringe Pump; Harvard Apparatus, Holliston, MA), and a glass reservoir. The confluent ECs were mounted in the flow chamber by applying vacuum to hold the glass slide, gasket (SF Medical, Hudson, MA), and polycarbonate base together and to form a flow channel of parallel plate geometry. The wall shear stress ( ) can be determined as = 6 µQ/h2w, as
previously described by Frangos et al,35 where µ is the viscosity of the circulating media (1.1 cP), Q is the volumetric flow
rate (4.8 mL/min), h is the height of the flow channel (0.046 cm), and
w is the width (2.49 cm). For all experiments, was 1 dyne/cm2, a venous shear stress level. The flow rate was
controlled by the syringe pump, which drove RBC suspension to
recirculate in the flow loop. We installed 4 polypropylene 1-way check
valves (Cole-Parmer, Vernon Hills, IL) to maintain the unidirectional flow into the flow chamber in spite of the reciprocating movement of
the syringe pump. Stir bars were placed inside the syringes and stirred
at 150-250 rpm at a 20-minute on/20-minute off cycle (Fisher Lab
Controller/Timer, Fisher Scientific Laboratories) to avoid RBC
sedimentation inside the syringes. The glass reservoir was connected to
a humidified mixture of 95% air and 5% CO2 to control the
pH of the circulating media and to keep the media oxygenated.
Experiments were performed in a 37°C room. Media samples were drawn
from the glass reservoir at several time points during 24-hour flow
studies, and equal amounts of fresh media (RBC suspension) were
replenished at the same time of sampling to maintain a 15-mL constant
circulating volume. Media samples were centrifuged at 13 600g
for 10 minutes to remove RBCs and then stored at  80°C until the assays were performed. After being subjected to 24-hour flow
studies, the hematocrit of RBC suspension was measured by capillary
centrifugation and was found to be close to 1%, which was the starting
hematocrit. At the end of each flow study, HUVECs were harvested either
for RNA analysis or to examine cell surface expression of adhesion
molecules.
RNA isolation For RNA analysis, total cellular RNA was isolated from HUVECs at the end of flow studies using a FastRNA GREEN kit (BIO 101, La Jolla, CA). Total RNA was then resuspended in diethylpyrocarbonate-treated (DEPC-treated) (Sigma) water and stored at80°C until the assays were performed. RNA
concentration and purity were determined spectrophotometrically (DU-640 Spectrophotometer; Beckman Instruments, Fullerton, CA).
Synthesis of competitor RNA The competitor RNA (cRNA) for target ICAM-1 mRNA was constructed as an internal control in RT-PCR. The cRNA and target RNA have identical terminal ends to be amplified with the same pair of primers. They also have the same sequence and similar lengths between 2 terminal ends, except that cRNA is 60 nucleotides shorter so that the RT-PCR products from cRNA and target RNA can be distinguished by different molecular weights. The reaction rate of cRNA and target RNA in RT-PCR can be assumed to be equal because they bear great similarity. Target RNA and cRNA were mixed together to perform RT-PCR. When the amount of cRNA (known) and the amount of target RNA (unknown) were the same, the ratio of their RT-PCR products was 1.
Quantitative RT-PCR
HPLC analysis
Flow cytometry For flow cytometric analysis, EC monolayers were washed 3 times with Dulbecco's phosphate-buffered saline (D-PBS, calcium- and magnesium-free [Ca++/Mg2+ free]; Sigma) at the end of flow studies. No significant RBC attachment to EC monolayers was observed by using an inverted phase-contrast microscopy. HUVECs were then removed from the glass slides after incubation with 50 mmol/L ethylenediaminetetraacetic acid (EDTA) for 10 minutes at 37°C followed by centrifugation at 13 600g for 10 minutes. The pellet was washed once and then resuspended in 500 µL D-PBS per 0.25 × 106 cells. Fluorescein isothiocyanate-conjugated (FITC-conjugated) mouse immunoglobulin G (IgG) antihuman ICAM-1 monoclonal antibody (mAb) or FITC-conjugated mouse IgG antihuman VCAM-1 mAb (both from R&D Systems) was added to the cell suspension at a final concentration of 3 µg/mL and incubated for 30 minutes at 4°C. Unbounded antibody was removed by centrifugation at 13 600g for 10 minutes. Labeled cells were fixed in 1% formaldehyde and then analyzed using a FACScan flow cytometer. At least 5000 cells were analyzed, and the results were expressed as geometric mean fluorescence. Background binding was detected using fluorescein-conjugated mouse IgG isotype controls (R&D Systems).Enzyme-linked immunosorbent assay Soluble ICAM-1 and VCAM-1 released into the flow system were measured by sandwich enzyme-linked immunosorbent assay (ELISA) kits (R&D Systems).Lactate dehydrogenase assay The release of lactate dehydrogenase (LDH) into the circulating solution was used as an indicator of the extent of hemolysis during 24-hour flow studies. LDH concentration was measured spectrophotometrically by an LDH-L reagent kit (Ciba-Corning, Oberlin, OH). The percent of lysis was calculated by comparing the LDH concentrations of media samples from flow studies to the LDH concentrations of the media samples from negative control (0% lysis) and positive control (100% lysis). The negative control was fresh RBC suspension not subjected to any experiments. The positive control was fresh RBC suspension sonicated with a sonic dismembrator (Fisher Scientific Laboratories) to produce complete RBC lysis.Data presentation Data are presented as the mean plus or minus SEM, and n represents the number of experiments. Cumulative production levels were determined by a mass balance, which took into account samples withdrawn and fresh RBC suspension replenished. Statistical analysis was done by using 2-tailed t tests for paired samples from 2 groups and by using repeated measures of analysis of variance (ANOVA) to determine the trends from cumulative production between 2 groups over time. ANOVA followed by the Fisher's protected least significant difference (PLSD) was used as appropriate. P < .05 was considered to be statistically significant.
Sickle erythrocytes up-regulated ICAM-1 gene expression After exposure to either sickle cell perfusion or normal RBC perfusion at 1 dyne/cm2, ICAM-1 mRNA levels in confluent HUVECs were measured at 3, 6, 12, and 24 hours (Figure 4). At 3 and 6 hours, which were the early time points, perfusion with sickle erythrocytes significantly induced ICAM-1 gene expression. The increases caused by sickle cell perfusion were about 3-fold at 3 hours and 6-fold at 6 hours compared with matched normal RBC perfusion. Beyond 12 hours, ICAM-1 mRNA levels were relatively low and the same in both conditions. ICAM-1 mRNA expression was maximal at 3 hours, and decreased with time, but the expression was still maintained above the baseline for 24 hours. Basal amounts of ICAM-1 mRNA in cultured HUVECs were about 0.5 × 10 18 mole per 0.25 µg total RNA
(data not shown).
Cell surface expression of ICAM-1 The level of membrane-bound ICAM-1 (mbICAM-1) production associated with flow and cytokine stimulation was measured by flow cytometry. As shown in Figure 5, sickle cell perfusion and normal RBC perfusion had the same mbICAM-1 levels at 3 and 6 hours, which were approximately equal to constitutive amounts of mbICAM-1 expressed on cultured HUVECs. Thereafter, the surface expression started to rise in both conditions. Sickle cells caused about 4-fold and 6-fold increases above baseline in EC surface expression of ICAM-1 at 12 hours and 24 hours (P < .05), respectively. Normal erythrocytes elicited a similar pattern, whereas the increased magnitudes were smaller than those caused by sickle erythrocytes. At 12 and 24 hours, HUVECs subjected to sickle cell perfusion had nearly 2-fold increases in mbICAM-1 levels compared with HUVECs exposed to normal RBC perfusion.
Release of soluble ICAM-1 In all experiments, no soluble ICAM-1 (sICAM-1) was detected before 6 hours. As shown in Figure 6, sICAM-1 was first detected at 6 hours in sickle cell perfusion, and the release increased with time. On the other hand, sICAM-1 was not detectable in normal RBC perfusion until 12 hours, when matched sickle cell perfusion induced a 9-fold higher release of sICAM-1 from HUVECs.
Sickle erythrocytes up-regulated VCAM-1 gene expression Basal amounts of VCAM-1 mRNA in cultured HUVECs were about 1 × 1018 mole per 0.25 µg total RNA (data
not shown). After exposure to RBC perfusion at 1 dyne/cm2,
VCAM-1 mRNA amounts in cultured HUVECs were measured at 3-, 6-, 12-, and 24-hour flow studies. In normal RBC perfusion, VCAM-1 mRNA levels were about 8 ± 2 × 1018
moles per 0.25 µg total RNA at 3 and 6 hours, then the levels decreased monotonically and returned to baseline at 24 hours. Similar
to ICAM-1, VCAM-1 gene expression was up-regulated by sickle
cells at early phases of flow studies (Figure
7). At 3 hours, sickle cell perfusion
caused a 2-fold increase in VCAM-1 mRNA amounts compared with normal
RBC perfusion. The induction maximized at 6 hours, when an average
9-fold increase of VCAM-1 transcript was caused by sickle
erythrocytes compared with normal erythrocytes. Thereafter in sickle
cell perfusion, VCAM-1 mRNA levels decreased gradually, but they were
still maintained about 3-fold above baseline until 24 hours.
Cell surface expression of VCAM-1 and release of soluble VCAM-1 The cell surface expression of VCAM-1 on HUVECs was determined by flow cytometry, and the release of soluble VCAM-1 from HUVECs was detected by ELISA. In contrast to ICAM-1, membrane-bound and soluble VCAM-1 levels did not increase greatly in response to the significantly elevated VCAM-1 mRNA amounts.
LDH assays
We observed 3 important phenomena in this study: (1) Sickle erythrocytes have direct effects on gene regulation in cultured human ECs under vascular flow environments, (2) gene expression of ICAM-1 and VCAM-1 in ECs was up-regulated after exposure to sickle cell perfusion at 1 dyne/cm2; and (3) under RBC perfusion, the production of ICAM-1 and VCAM-1 proteins appeared to be regulated via different mechanisms. Sickle erythrocytes increased gene expression and cell surface expression of ICAM-1 in endothelial cells The ICAM-1 molecule consists of 5 extracellular immunoglobulin domains, a hydrophobic transmembrane region, and a short cytoplasmic tail.36,39 ICAM-1 has a great variety of functions. Besides its important role in recruiting white cells to inflammatory sites, ICAM-1 is also involved in the cell-cell interactions in immune response,40 and it is the major human rhinovirus receptor.41,42 Although so far there has been no evidence showing that ICAM-1 is directly involved in sickle cell adhesion to ECs, the up-regulation of ICAM-1 production in HUVECs by sickle erythrocytes may have several physiological effects. For instance, increased ICAM-1 expression reflects an activated endothelium state that may lead to leukocyte adhesion and exacerbate vascular occlusive events. By analysis of over 1000 sickle cell patients, Mansour43 demonstrated that the strongest correlation between hematological variables and the severity of crises was found to be with total leukocyte counts not erythrocyte-related parameters, which suggests an important role of leukocytes in sickle cell disease. Lipowsky et al30 proposed that leukocyte-endothelium adhesion may be a significant determinant in the onset of sequestration and entrapment of RBCs and thus obstruct the microvascular lumen, which will contribute to the initiation of vasoocclusive crises.
Sickle erythrocytes increased gene expression of VCAM-1 in endothelial cells The predominant form of VCAM-1 molecules in human ECs contain 7 immunoglobulin domains, a single transmembrane region, and a short cytoplasmic domain.48 Swerlick et al20 and Natarajan et al21 demonstrated that VCAM-1 expressed on HUVECs stimulated with TNF- for 9 hours or
IL-1 for 24 hours may be responsible for binding sickle erythrocytes
to cytokine-treated ECs under venous shear stress environments via
sickle RBC membrane-associated VLA-4.
Effects of IL-1
The release of soluble ICAM-1 and soluble VCAM-1 The existence of soluble ICAM-1 in human serum was first demonstrated in 1991 by Seth et al22 using immunoblotting and by Rothlein et al23 using ELISA. Soluble ICAM-1 contains most of the 5 extracellular immunoglobulin domains of membrane-bound ICAM-1 as well as the ability to bind specifically to LFA-1.23 The mechanism by which sICAM-1 molecules are released into extracellular fluid remains unclear. No alternatively spliced forms of ICAM-1 mRNA lacking the transmembrane domain have been identified yet, and it is therefore probable that the molecules are shed or cleaved from cell surfaces by proteases.49 The physiological role of sICAM-1 remains to be determined. It is possible that the released sICAM-1 is merely destined for clearance or may be regarded as EC markers of the presence of inflammatory states.50 Nonetheless, the ability of sICAM-1 to bind to LFA-1 shows that sICAM-1 may have some biological functions. Marlin et al51 demonstrated that sICAM-1 can inhibit rhinovirus infection, and Becker et al52 showed that sICAM-1 shed from human melanoma cells is able to inhibit cell-mediated cytotoxicity.
Transcriptional regulation of ICAM-1 and VCAM-1 An increasing number of reports have demonstrated that the elevated expression of EC ICAM-1 and VCAM-1 is either wholly or partly due to the up-regulation of genes.59 Our results are consistent with this observation, although detailed mechanisms by which sickle erythrocytes induced ICAM-1 and VCAM-1 gene expression in ECs remain to be determined. However, extensive research that has been done to elucidate the transcriptional regulation of ICAM-1 and VCAM-1 by analysis of their 5' regulatory sequences may provide insights into the possible pathways involved in sickle cell-EC interactions.
The experimental system The flow apparatus described here demonstrated an in vitro model to examine the interactions between sickle cells and ECs under well-characterized flow conditions. The model can be used for investigating the effects of sickle erythrocytes on the function, metabolism, and gene regulation of ECs along with other important factors in the blood stream such as cytokines or protein components. The model can also be used for elucidating the cellular and molecular bases involved. At 24 hours, high hemolysis (about 27%) restricted the useful time frame of this system. The increased hemolysis after long-term exposure to shear and to surfaces of the flow system may be due to inherent characteristics of RBCs because both normal RBCs and sickle cells showed the same extent of hemolysis.Conclusions This study is the first demonstration that sickle erythrocytes have direct effects on gene regulation in cultured human ECs under controlled fluid mechanical environments. The results reveal that sickle erythrocyte perfusion increased the EC production of cell adhesion molecules, which may create a vascular environment that favors adhesion events, lengthens microcirculation transient times, and thus renders sickle cell anemia patients vulnerable to vasoocclusive crises.
The authors thank Cynthia Patton for help in the collection of clinic materials, Dr Susan McCormick for advice on molecular biology protocols, and Dr Thomas Chow for assistance in flow cytometry. The technical assistance of Marcella Estralla, Nancy Turner, and Dick Chronister is gratefully acknowledged.
Supported by grant R01 HL50601 from the National Institutes of Health, Bethesda, MD.
Reprints: Larry V. McIntire, Cox Laboratory for Biomedical Engineering, Institute of Biosciences and Bioengineering, Rice University, Houston, TX 77251-1892; e-mail: mcintire{at}rice.edu.
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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Top
Abstract
Introduction
B) by hydrogen peroxide.
: tissue distribution, biochemistry, and function of a natural adherence molecule (ICAM-1).
J Immunol.
1986;137:245