Characterization of the trigeminovascular actions of several adenosine A_2A receptor antagonists in an in vivo rat model of migraine

Fifty seven normotensive male Sprague-Dawley rats (300–400 g), purchased from Harlan (Horst, The Netherlands), were maintained at a 12/12-h light-dark cycle (with light beginning at 7 a.m.) and housed at a constant temperature (22 ± 2°C) and humidity (50%), with food and water ad libitum. Only male rats were used to avoid crosstalk between CGRP and hormonal fluctuations during the female oestrus cycle [23]. The animals were anaesthetized with an intraperitoneal (i.p.) injection of sodium pentobarbital (60 mg/kg, followed by 18 mg/kg i.v. per hour when necessary). The adequacy of anaesthesia was judged by a negative tail flick test and the absence of ocular reflexes, amongst others. All experimental protocols of this study were approved by our Institutional Ethics Committee [Erasmus MC; permission protocol number EMC 1931 (118–09-04)], in accordance with the NIH guide for the Care and Use of Laboratory Animals in U.S.A. and the ARRIVE guidelines for reporting experiments in animals [24]. All rats were randomly assigned into the different experimental protocols (see experimental protocol section).

After anesthesia, the trachea was cannulated and connected to a pressure ventilator (small animal ventilator SAR-830 series, CWE Inc., Ardmore, PA, U.S.A.). End-tidal pCO₂ was monitored (Capstar-100 CWE Inc., PA, U.S.A.) and kept between 35 and 48 mmHg. The left femoral vein and artery were cannulated for intravenous (i.v.) administration of drugs and continuous monitoring of blood pressure, respectively. Two or three samples of blood (at the beginning and at the end of the experiment) were withdrawn via the femoral artery to monitor blood gases and other parameters, which were kept between normal values (pH: 7.35–7.48; pCO₂: 35–48 mmHg; pO₂: 100–120 mmHg). The body temperature of each rat was monitored via a rectal thermometer and maintained throughout the experiment (36.5 °C–37.5 °C) by a homeothermic blanket system for rodents (Harvard Instruments, Edenbridge, Kent, U.K.). The rats were placed in a stereotaxic frame and the parietal bone overlying a segment of the dural meningeal artery was carefully drilled thin, applying cold saline (4 °C) until the artery was visible. Since skull drilling induces vasodilation, we allowed the animal to recover for 1 h before the experimental protocol. The drilled area was covered with mineral oil to prevent drying and to facilitate visualization of the meningeal artery. The artery was captured with an intravital microscope (model MZ 16; Leica microsystem Ltd., Heerbrugg, Switzerland) using a cyan blue filter on a cold source of light. A zoom lens (80–450 × magnification) and a camera was used to display images with the blood vessel diameter (30–40 μm at baseline) being continuously monitored and measured with a video dimension analyser (Living Systems Instrumentation Inc., Burlington, VT, U.S.A.). In rats where periarterial electrical stimulation was used to evoke dural vasodilation, a bipolar stimulating electrode (NE 200X, Clark Electromedical, Edenbridge, Kent, U.K.) was placed on the surface of the cranial window approximately within 200 μm from the vessel of interest. The cranial window surface was stimulated at 5 Hz, 1 ms for 10 s (Stimulator model S88, Grass Instruments, West Warwick, RI, U.S.A.). For neurogenic dural vasodilation, we initially started with a current intensity (monitored on an oscilloscope, model 54601A, Hewlett Packard, Palo Alto, CA, U.S.A.) of 100 μA and increased with 50 μA steps until a maximal level of dilatation was achieved, usually at 200 μA. The resulting data were displayed and recorded using a WINDAQ data acquisition system (Version 2.54; DataQ Instruments Inc., Akron, OH, U.S.A.).

First, 6 animals were used to determine the effect of i.v. adenosine and caffeine on the middle meningeal artery diameter. The doses of adenosine (1 mg/kg) and caffeine (40 mg/kg) were based on previously published work [15, 25]. Further, 51 animals were divided into two groups which received, respectively, periarterial electrical stimulation (150–250 μA; n = 27) and the adenosine A₂ receptor agonist CGS21680 (10 μg/kg, i.v., n = 24; the optimal dose as determined in 7 pilot experiments, data not shown). Dural vasodilator responses remained unchanged after repeated treatment for 4 times (data not shown) and in the presence of the vehicle captisol, which was used for dissolving most of the antagonists. Thirty min were allowed between each of these treatments for recovery to the baseline diameter. Subsequently, each of these groups was subdivided into five subgroups (n = 3–6 each) which were given (after 30 min) i.v. bolus injections of, respectively, the adenosine A_2A receptor antagonists JNJ-41942914 (0.3, 1, and 3 mg/kg), JNJ-39928122, JNJ-40529749, JNJ-40064440 and JNJ-41501798 (all 1, 3 and up to 10 mg/kg). Based on their binding affinities (see Table 1), only doses up until significant blockade, were tested for the CGS21580 response. Each antagonist dose was administered 5 min before periarterial electrical stimulation or CGS21680, except for caffeine (15 min) as previously reported [25]. The duration of each experiment was approximately 2.5 h after stabilization.

All data are presented as mean ± SEM. The peak increases in dural meningeal artery diameter are expressed as percent change from baseline. Changes in mean arterial blood pressure (MAP) were expressed as absolute values (mm Hg). The difference between the variables within one group was compared by using a one-way repeated measures analysis of variance followed by Dunnet’s test. Dunnet’s test does not give individual P-values, hence statistical significance was accepted at P < 0.05. When there was only one dose applied (for caffeine), two-tailed paired Student’s T-test was used.

The compounds used in this study were: sodium pentobarbital (Nembutal; Ceva Sante Animale B.V., Maassluis, The Netherlands); caffeine, adenosine and CGS21680 hydrochloride hydrate (2-p-(2-Carboxyethyl)phenethylamino-5′-N-ethylcarboxamido adenosine hydrochloride hydrate) (Sigma Chemicals Co., Steinheim, Germany); JNJ-41942914, JNJ-39928122, JNJ-40064440, JNJ-40529749 and JNJ-41501798 (gift courtesy from Janssen Research & Development, L.L.C., Raritan, NJ, U.S.A.). Caffeine, adenosine, CGS21680 and JNJ-40064440 were dissolved in distilled water, whereas JNJ-39928122, JNJ-41942914, JNJ-40529749 and JNJ-41501798 were dissolved in captisol (sulfobutylether β-cyclodextrin; Ligand Pharmaceuticals, San Diego, U.S.A.). The suspensions of JNJ-40529749 and JNJ-41501798 were sonicated and filtrated. All solutions were further diluted in saline.