Cell culture

Human umbilical vein endothelial cells (HUVEC) were isolated by collagenase type II (Biochrom KG, Berlin, Germany) digestion of human umbilical veins by standard techniques and cultured in EC medium (MCDB 131; Gibco-BRL, Life Technologies GmbH, Karlsruhe, Germany) at 37°C in a humidified atmosphere of 5 % CO₂ and 95 % air as described previously (Stangl et al. Reference Stangl, Gunther, Jarrin, Bramlage, Moobed, Staudt, Baumann and Stangl2001). All experiments were performed with HUVEC from passages one to three. HUVEC were seeded at 1 × 10⁴ cells/well in ninety-six-well plates. After 3 d, the medium was replaced by fresh EC medium before treatment.

Cell viability assay using 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium bromide

Cell viability was measured by 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium bromide (MTT) assay (Chen et al. Reference Chen, Lin, Chen, Ku and Chen2002). The principle of this assay is that mitochondria dehydrogenase in viable cells reduces MTT to a blue formazan. Briefly, cells were grown in ninety-six-well plates and incubated with various concentrations of EA (which was dissolved in dimethyl sulphoxide) for 24 h; 100 μl MTT (0·5 mg/ml) were then added to each well and incubation continued at 37°C for an additional 4 h. The medium was then carefully removed, so as not to disturb the formazan crystals which had formed. Dimethyl sulphoxide (100 μl), which solubilizes formazan crystals, was added to each well and the absorbance of the solubilized blue formazan was read at 530 nml/l (reaction) and 690 nml/l (background) using a DIAS Microplate Reader (Dynex Technologies, Chantilly, VA, USA). The reduction in optical density caused by EA was used as a measurement of cell viability, normalized to cells incubated in control medium, which were considered 100 % viable.

Estimation of the production of reactive oxygen species

The production of intracellular reactive oxygen species (ROS) induced by IL-1β was estimated by a fluorometric assay using 2′,7′-dichlorofluorescein-diacetate (DCFH-DA) as a probe according to the method reported by Bass et al. (Reference Bass, Parce, Decharelet, Szejda, Seeds and Thomas1983). HUVEC (1 × 10⁶) were incubated with IL-1β and EA, suspended in PBS containing 2 % fetal calf serum, and then incubated again with 5 mmol/l 2′,7′-dichlorofluorescein-diacetate for 30 min at 37°C. The formation of 2′,7′-dichlorofluorescein was determined by flow cytometry. The excitation wavelength was 488 nm, and green fluorescence collected through a 530 nm band-pass filter was measured on a logarithmic scale. The formation of ROS was expressed as relative fluorescence intensity.

Real-time PCR for vascular cell adhesion molecule-1, intercellular adhesion molecule-1 and endothelial leucocyte adhesion molecule

The real-time PCR assay for adhesion molecules was conducted according to the method reported by Li & Wang (Reference Li and Wang2002). Total cellular RNA was isolated from samples (HUVEC) using the Trizol reagent according to the manufacturer's instructions (Gibco BRL). RT reactions were carried out for each RNA sample in thin-welled PCR tubes using the First-Strand Synthesis System (Invitrogen, Carlsbad, CA, USA). Each reaction tube contained 4·2 μg total RNA in a volume of 21 μg containing 1 ×  RT buffer, 5·5 mmol/l MgCl₂, 500 μmol/l of each dNTP, 2·5 μmol/l of oligo-d(T)_12–18 primers, 40 U/μl RNase inhibitor, 2 U/μl Escherichia coli RNaseH and 50 U/μl of SuperScript II RT. RT reaction was carried out at 65°C for 5 min, 42°C for 50 min and 70°C for 15 min. The RT reaction mixture was then placed at 4°C for immediate PCR amplification or stored at − 20°C for later use. Real-time PCR was performed in optical real-time PCR tubes. The following primers were used: VCAM-1: forward 5′-AAGCGGAGACAGGAGACAC-3′, reverse 5′-TGGCAGGTATTATTAAGGAGGATG-3′; ICAM-1: forward 5′-TGGTTCACAGGTTCAGATTAC-3′, reverse 5′-GACAAGAGGACAAGGCATAGC-3′; E-selectin: forward 5′-TGTGAGATGCGATGCTGTC-3′, reverse 5′-AACCTCTTCTGTCCATTGTCC-3′; glyceraldehyde-3-phosphate dehydrogenase: forward 5′-CCCACTCCTCCACCTTTG-3′, reverse 5′-CTTCCTCTTGTGCTCTTGC-3′.

Each tube contained 1 μl of each RT product (200 ng total RNA), 5·5 mmol/l MgCl₂, 400 μm-dNTP, 500 nmol/l primer (forward and reverse), 0·005 U/μl iTaq DNA polymerase and 20 nmol/l SYBR Green I in a total volume of 25 μl. Amplification conditions were 3 min at 95°C for activation, then run for forty cycles at 95°C for 15 s and 60°C for 1 min. All reactions were performed in the Bio-Rad iCycle Sequence Detection System using the iCycle V3.1 program. The threshold cycle (Ct) and melting point (Mt) were obtained during each reaction. The relative quantification was calculated based on its 2^− ΔCt value, ΔCt = Ct (sample) – Ct (control).

Measurement of NF-κB activity

Nuclear extracts were prepared as described previously (Dschietzig et al. Reference Dschietzig, Richter, Pfannenschmidt, Bartsch, Laule, Baumann and Stangl2001). Bradford reagent determined protein concentrations. For analysis of NF-κB activity, a TransAM NF-κB Family kit was used (Active Motif, Rixensart, Belgium). In this assay, ninety-six-well plates were coated with an oligonucleotide containing the consensus binding sequence for NF-κB 5′-GGGACTTTCC-3′. Specific primary antibodies included in the kit detected the binding of NF-κB family transcription factors to their consensus sequence. Experiments were analysed by an ELISA-based assay. A total of 10 μg nuclear extract was used in each experiment and processed according to the manufacturer's protocol. Briefly, nuclear extracts were incubated with the oligonucleotide-coated wells for 60 min. Where indicated a competitor for NF-κB binding (NF-κB wild-type consensus oligonucleotide) was added in molar excess prior to the probe. The wells were then washed and incubated with the primary antibodies for p65, p50, c-Rel, p52 and RelB for 60 min. After incubation with a horseradish peroxidase-conjugated secondary antibody, a substrate was added to produce blue colour and then for quantitation by a standard ELISA reader. The absorbance was read at 450 nm and the blanks were subtracted from all measurements. The data presented are the result of three independent experiments.

Monocyte-endothelial cell adhesion

HUVEC (2 × 10⁵) were distributed into six-well plates and allowed to reach confluence. They were then incubated for 18 h with medium supplemented with EA at concentrations of 25 and 50 μmol/l according to the MTT test, followed by incubation for 6 h with 10 ng/ml IL-1β in the continued presence of EA. U937 cells, originally derived from a human histiocytic lymphoma and used for the monocyte-endothelial cell adhesion assay, were grown in RPMI-1640 medium (Gibco, New York, USA) containing 10 % fetal bovine serum and subcultured at a 1 : 5 ratio three times per week, labelled for 30 min at 37°C with calcein AM (10 nmol/l; Molecular Probe; Invitrogen) in RPMI-1640 medium and washed with PBS to remove free dye, and then resuspended in 10 % M-199 medium. Labelled U937 cells (1 × 10⁶) were added to each HUVEC-containing well and incubated for 1 h. Non-adherent cells were removed by two gentle washes with PBS. Then, adherent U937 cells were determined by a fluorescence plate reader at an excitation wavelength of 485 nm and emission at 530 nm; HUVEC cell monolayers served as the blank.

Statistics

Results are presented as means and standard deviations. Statistical significance was determined by one-way ANOVA. Differences were considered significant at P < 0·05.