Sleep phenotype in the Townes mouse model of sickle cell disease

Experiments were conducted in adult male 10-to-12-week-old Townes knockout-transgenic SS and AS sickle cell mice on a background strain of B6 and S129. Colonies of Townes SS and AS mice were bred and maintained at the University of Pittsburgh, as previously reported [10]. Mouse genotypes were confirmed either by PCR or Hb gel electrophoresis at 3–4 weeks of age. Mouse phenotypes were confirmed by total Hb concentration (from venous whole blood using a portable Co-oximeter; AVOXImeter 4000) and reticulocyte count (from flow cytometry) at 10 weeks of age. Animal handling and experimentation was conducted ethically and in accordance with approved Institutional Animal Care and Use Committee (IACUC) protocols at the University of Pittsburgh.

All mice underwent surgical implantation of polysomnographic electrodes on day 0 and were tethered to the recording system after 7 days of recovery. On day 11, after 4 days of undisturbed acclimation to the tether, electroencephalographic (EEG) and electromyographic (EMG) signals were recorded for a continuous 24-h period. A subset of mice were subsequently catheterized on day 12, and, after 2 days of recovery, arterial blood was collected under freely behaving conditions for assessment of arterial blood gases.

Animals were anesthetized using 1–2% isoflurane for all surgical procedures, administered pain medication after surgery (0.3 mg/ml buprenorphine for maximum of 3 days), and monitored daily during the post-operative period. EEG electrodes (E363/1, Plastics One, Roanoke, VA) and nuchal EMG electrodes (E363/76, Plastics One) were implanted as previously described [11]. In brief, a midline incision was made to expose the skull and muscles immediately posterior to the skull. The underlying fascia was gently cleared from the skull surface, four small burr holes were drilled through the skull in the frontal and parietal regions, and four EEG electrodes were fastened via jewel screws (diameter of 1.6 mm). The first and second electrodes were placed 2–3 mm caudal to bregma and 1–2 mm lateral of the midsagittal suture. The third and fourth electrodes were placed 2–3 mm rostral to bregma and 1–2 mm lateral of the midsagittal suture. Two nuchal EMG electrodes were stitched flat onto the surface of the neck muscle. The EEG and EMG electrodes were inserted into a pedestal (MS363, Plastics One) and secured to the skull with dental acrylic. After recovery from surgery, a connector cable was placed onto the head pedestal and attached to a low-friction mercury swivel allowing unrestricted movement of the tethered mouse.

In a subset of mice, an arterial catheter was implanted chronically under isoflurane anesthesia, as previously described [12]. The catheter was inserted in the left femoral artery, sutured in place, stabilized with superglue (Henkel Corp., Rocky Hill, CT, USA), and tunneled subcutaneously to the upper back by threading through a blunt needle. The catheter was taped to the connector cable attached to the pedestal and connected to a 360° swivel designed for mice (375/D/22QM; Instech, Plymouth Meeting, PA, USA) that worked in combination with the electrical swivel used to record polysomnography. Catheter patency was maintained by continuously flushing saline containing 20 U ml⁻¹ heparin (Baxter, Deerfield, IL, USA) at a rate of 3 μl h⁻¹ using a multi-syringe pump (R99-EM; Razel Scientific Instruments, St. Albans, VT, USA).

The mice were maintained on a 12:12-h light-dark cycle and were housed in a customized pyramidal cage [7″ (W) × 9″ (H) × 7″ (L)] with continuous access to food and water. The cage was contained inside a light-controlled and sound-dampening chamber [22″ (L) × 16.5″ (H) × 14″ (W)] (BRS/LVE, Laurel, MD). The mice were housed in the same chambers throughout the entire adaptation and experimental period to control for environmental exposure. The polysomnographic tether and arterial catheter (in the subset of instrumented mice) exited through a 1″-diameter hole in the top of the chamber, and connected to an amplifier and a multi-syringe pump, respectively.

A Grass Instruments amplifier (Quincy, MA) was used to record EEG activity (filtered 0.1–30 Hz) and EMG activity (filtered 10–100 Hz). Signals from the Grass recorder were collected using Windaq Pro acquisition software (Dataq Instruments; Akron, OH), were digitized at 300 Hz (DI-720 data acquisition board; Dataq Instruments; Akron, OH), and stored for analyses.

Approximately 80 μl of arterial blood was collected and analyzed with a VetScan i-STAT 1 blood gas analyzer (ABAXIS, Union City, CA). Blood samples were withdrawn during the light period with the mouse in quiet wakefulness to determine the partial pressure of arterial oxygen (PaO₂), the partial pressure of arterial carbon dioxide (PaCO₂), and the arterial oxygen saturation (SO₂).

Sleep data were analyzed using a customized program that converted DATAQ digitized data files into Stanford Sleep Structure Scoring System (SSSSS) format for characterization of signals using the rodent software developed by Joel H. Benington [13] and subsequently validated in mice by Veasey et al. [14]. The program utilizes Fourier spectral analysis of the EEG in the delta (0.5–4.0 Hz), sigma (10.0–14.0 Hz), and theta (6.0–9.0 Hz) frequency bands in combination with the moving average of the EMG amplitude to assess sleep/wake states in 10-s epochs (necessary to provide accurate determination of the beginning and end of REM sleep bouts that typically average around 1 min). Twenty-four-hour periods of data were plotted as sigma*theta power from Fourier spectral analysis against EMG, and thresholds for the slope and intercept of the relationship were used to distinguish between sleep and wake. A second plot of the delta/theta power from Fourier spectral analysis against EMG was used to distinguish non-rapid eye movement (NREM) sleep from rapid eye movement (REM) sleep based on a delta/theta threshold.

Total time spent in each of the three sleep states (Awake, NREM, and REM) was calculated as a percentage of the number of epochs of that state over a 24-h period. The number and duration of NREM and REM sleep bouts were determined according to the following criteria: an NREM sleep bout began with three or more consecutive epochs of NREM sleep and ended with three or more consecutive epochs of wake or two or more consecutive epochs of REM sleep; an REM sleep bout started with two or more consecutive epochs of REM sleep and ended with three or more consecutive epochs of wake or NREM sleep. An awake bout began with three consecutive epochs of awake and ended with three consecutive epochs of sleep (any combination of NREM or REM sleep). Time to resume sleep was defined as the length of time from the onset of three or more consecutive epochs of wake to the next combination of any three consecutive epochs of NREM or REM sleep. An arousal was defined as one or more epochs of wake following three or more consecutive periods of either REM or NREM sleep. Arousal frequency per hour of sleep was calculated as total number of arousals/total sleep time in 24 h.

The AS and SS mice were matched for age and weight and arterial blood gas analyses showed no difference in PaO₂, PaCO₂, SO₂, or pH between strains (Table 1). As expected, the SS mice exhibited significantly less (p < 0.01) total hemoglobin compared to AS mice, as well as a significantly higher (p < 0.01) reticulocyte percentage of red blood cells (Table 1).

Over the 24-h sleep/wake cycle, SS mice exhibited a 17% reduction of time in NREM sleep, with a comparable increase in time awake (Fig. 1a, b; p < 0.01) relative to AS mice. The decrease in NREM sleep time was due to a decrease in number, but not the duration, of NREM bouts (Figs. 1a and 2b). Interestingly, when assessing just the dark (active) period, the SS mice did exhibit a significant decrease (p < 0.05) in NREM bout length compared to the AS mice (Table 2; p < 0.05). In contrast to NREM sleep, there were no differences in time spent in REM sleep in either the light or dark period and no differences in number or duration of REM sleep bouts between the SS and AS mice (Figs. 1c and 2c, d and Table 2).

Despite the SS mice spending less time in NREM sleep than AS mice, they exhibited significantly fewer arousals per hour of sleep (Fig. 3a; p < 0.05). A decrease in arousal frequency in the light period primarily accounted for the overall 24-h decrease in arousal frequency (Table 2; p < 0.05). The time to resume sleep after an arousal was significantly increased in SS mice compared to AS mice over the 24-h sleep/wake cycle (Fig. 3b; p < 0.01), a response that was present in both the light and dark periods (Table 2).