dc-bTBI

The experimental protocol was approved by the Institutional Animal Care and Use Committee of the University of Maryland, with IACUC No. 0912012. In all, 30 adult male Long-Evans rats (300 ± 20 gm) were subjected to dc-bTBI using a Cranium-Only Blast Injury Apparatus (COBIA), as described in Keuhn et al. [5]. Briefly, the rats were anesthetized (60 mg/kg ketamine plus 7.5 mg/kg xylazine, IP), intubated with an endotracheal tube, and allowed to breath room air spontaneously. Although focal blast injury per se is not painful, Buprenorphine (0.05 mg/kg) was given s.c. prior to the procedure as preemptive analgesia and every 12 hours for 48 hours after the procedure for relief of potential pain that could arise from the periosteum at the site of the injury. For dc-bTBI, the occipital region of the head was exposed to a blast wave generated by detonating a .22 caliber smokeless powder cartridge, which generated a peak overpressure of~517 kPa (blast dissipation chamber, 24.5 cm; see [5]). Because COBIA is designed to deliver a 25.4 mm collimated blast wave selectively to the occipital region, there is no “exhaust” or “blast wind” injury due to inhalation of hot gases, and there is no transthoracic, transvascular mechanism of injury [6]. All rats subjected to dc-bTBI experienced apnea immediately after blast, but with lethal dc-bTBI, apnea was persistent and was followed within 30–45 seconds by cardiac arrest, while animals were under anesthesia. dc-bTBI resulted in~33% mortality, similar to previous observations [5]. Survivors were nursed on the heating pad until they recovered spontaneous movements. After the recovery from anesthesia (~ 1 hour) rats that underwent dc-bTBI did not exhibit distressful or abnormal behavior different from the behavior of the sham injury animals. Of the 20 surviving post- dc-bTBI rats, 10 underwent serial MR imaging and 10 were used for neurofunctional testing. As controls for neurofunctional testing, an additional 10 rats underwent sham injury, with the entire procedure performed as described above except that the cartridge was not detonated.

Serial MR imaging (see below) was carried out on 10 rats starting from 1 day before the dc-bTBI injury as baseline. Only rats that completed all imaging time points up to 28 days were included for imaging data analysis (n = 6). MR imaging finding of injured rats were compared to a separate group of sham injured rats (n = 6) who went through the same injury preparation without the actual injury, as well as the imaging procedures. Due to concerns regarding the potentially confounding effects of repeated anesthesia used for serial MR imaging, neurofunctional testing (see below) was conducted on a separate group of rats (n = 10) with dc-bTBI that did not undergo serial anesthesia. Neurofunctional performance in dc-bTBI rats was compared to neurofunctional performance in sham injured rats (n = 10). After MR imaging or neurobehavioral testing rats were euthanized with an overdose of sodium pentobarbital (> 100 mg/kg).

MR Imaging

MR imaging was performed under isoflurane anesthesia before dc-bTBI then at 1, 7, 14 and 28 days after injury. All experiments were performed on a Bruker Biospec 7.0 Tesla 30 cm horizontal bore scanner (Bruker Biospin MRI GmbH, Germany) equipped with a BGA12S gradient system capable of producing pulse gradients of 400 mT/m in each of the three axes, with AVANCE III electronics and interfaced to a Bruker Paravision 5.0 console. A Bruker 4-channel surface coil array was used as the receiver and a Bruker 72 mm linear-volume coil as the transmitter. At all times during the experiment, the animal was under 1–2% isoflurane anesthesia and 1 L/min oxygen administration. An MR compatible small-animal monitoring and gating system (SA Instruments, Inc., New York, USA) was used to monitor the animal’s respiration rate and body temperature. The animal body temperature was maintained at 36–37°C using a warm water bath circulation device. Ear pins were inserted in the rats’ ears to fix their head position in order to reduce head motion. The total duration of the whole imaging experiment was approximately 2 hours.

A three-slice (axial, mid-sagittal, and coronal) scout using rapid acquisition with fast low angle shot (FLASH) was used to localize the rat brain. A fast shimming procedure (Fastmap) was used to improve the B₀ homogeneity covering the brain. Both proton density (PD) and T₂-weighted images were obtained using 2D rapid acquisition with fast spin echo sequence in both the axial and coronal planes. Imaging was performed over a 3 cm field of view (FOV) in the coronal plane with an in-plane resolution of 117μm using 24 slices at 1 mm thickness, at an effective echo-time of 18.9 ms for the proton density weighted images and an effective echo-time of 56.8 ms for the T₂-weighted images. The echo-train length for the fast spin echo sequence was 4, the repeat time (TR) was 5500 ms, and the total acquisition time was ~12 minutes using two averages.

For the DKI acquisition, diffusion weighted images were acquired with a single shot, spin-echo echo-planar imaging (EPI) sequence. An encoding scheme of 30 gradient directions was used with the duration of each of the diffusion gradients (δ) being 4 ms with a temporal spacing of 23 ms (Δ) between the two diffusion gradients. Three b-values (1000 s/mm², 1500 s/mm² and 2000 s/mm²) were acquired for each direction following the acquisition of 5 images acquired with b = 0 s/mm². The DKI images were obtained using 2 averages over the same FOV as the axial PD/T₂ images but at an in-plane resolution of 0.234 mm at a TR/TE of 6000/50ms respectively for a total acquisition time of ~21 min.

For ¹H MRS, adjustments of all first- and second-order shims over the voxel of interest were accomplished with the FASTMAP procedure. The in vivo shimming procedure resulted in full width half maximum (FWHW) ranging from 7.8–10.9 Hz for the unsuppressed water peak in the spectroscopy voxel of the rat brain. This value is comparable with a Bruker spherical quality assurance phantom which typically results in a 5 Hz FWHM. The water signal was suppressed by variable power radiofrequency (RF) pulses with optimized relaxation delays (VAPOR). Outer volume suppression (OVS) combined with point-resolved spectroscopy (PRESS) sequence from a 3 x 3 x 3 mm³ voxel was used for signal acquisition, with TR/TE = 2500/20 ms, spectral bandwidth = 4 kHz, number of data points = 2048, number of averages = 300. Spectral data were obtained from two voxels that covered bi-lateral internal capsule, and two other voxels that covered the center of the hippocampus and the cerebellum respectively (Fig 1).

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Fig 1. Placement of the MRS voxels (white contours) on (a) cerebellum, (b) hippocampus, and (c) bi-lateral internal capsule on representative MR images of a rat.

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Image Analysis

The DKI data were first smoothed using 3D Gaussian smoothing with FWHM = 0.3 mm to improve the signal-to-noise ratio (SNR). DKI reconstruction was performed on each voxel using in-house MATLAB program (Mathworks, Natick, MA), as described by Zhuo et al. [20]. The standard most-widely used DTI model uses the following equation (Eq 1) to arrive at the tensor: (1) Where D_app is the apparent diffusion coefficient (mm²/s)in a given diffusion direction, S(b) is the diffusion weighted signal along that direction, b is the diffusion sensitivity parameter (s/mm²), and S_o is the MR signal intensity when no diffusion-weighting is applied. On the other hand, the DKI model uses the following equation [19]: (2) where K_app is the kurtosis along a certain diffusion direction. In probability theory, kurtosis is a term to describe the “peakness” of a probability distribution, as compared to a Gaussian “bell shaped” distribution. In the DKI model (Eq 2) the extra b² term and K_app captures the deviation of the water diffusion from a mono-exponential form as predicted by the theoretical Gaussian model (as in DTI), especially when higher b-values are used.

Maps of MD, FA, and mean kurtosis (MK) were generated using Eq 2. MK was calculated as the average of K_app along all measured diffusion directions. Manually drawn regions of interest (ROI) were placed bi-laterally in the internal capsule, hippocampus and cerebellum, corresponding to the regions where MRS data were obtained. The DKI ROIs were drawn on 2–3 consecutive slices on FA images in combination with MD images to ensure no CSF area was included. In addition, T2w images were used as anatomical references guided by the rat brain atlas (Pixnos and Watson, 1986) (Fig 2). Mean MD, FA, MK values from each of the ROIs were measured. Post-injury MRI data were normalized by the corresponding baseline data for each rat.

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Fig 2. Placement of DKI ROIs (white contours) on coronal FA maps for bi-lateral hippocampus (1), internal capsule (2), and cerebellum (3).

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¹H MRS data were fitted using the LC Model package [38]. Cramér-Rao lower bounds (CRLB), as reported from the LCModel analysis, were used to assess the reliability of measures of transmitters and the major metabolites. Metabolites having CRLB values less than 20% were further analyzed. The in vivo mean metabolite concentrations relative to total creatine (tCr) at each time point were computed.

Since the blast wave was directed to impact mid-sagittally with no lateral preference, the MRS and DKI data from bilateral regions were averaged to improve signal sensitivity.

Neurofunctional Tests

Vestibulomotor functions were assessed on days 1–14 following dc-bTBI using the beam walk test, the beam balance test, and the accelerating RotaRod test [39–41]. In the beam walk test, the rat was timed as it walked a 90 × 2 cm beam to a darkened box, while a loud noise was created behind it. In the beam balance test, the ability of the rat to balance on a 30 × 1.5 cm beam was scored for each trial, based on criteria described by Petullo et al. [39] Baseline values were collected after 2 days of training, which consisted of 3 trials per day. In the accelerating RotaRod test, rats were placed on the drum of the accelerating RotaRod (IITC, Life Science, Woodland Hills, CA), starting at 4 rpm, accelerating at a rate of 2 rpm every 5 sec up to a maximum of 45 rpm; 3 trials separated by 20 min were administered on each day of testing, with the average latency to falling off of the drum being reported.

Exploratory behavior was measured by assessing spontaneous rearing using the cylinder test [42–45]. Rats were placed in a plexiglass cylinder (10 cm diameter, 20 cm height) for 3 min. The time spent rearing and exploring the walls with their vibrissae and forelimbs was recorded.

Incremental and rapid spatial learning were measured using the Morris Water Maze (MWM) after testing vestibulomotor function to ensure that deficits observed in dc-bTBI animals early after injury minimally interfere with behavior in MWM as significant motor deficits prevent objective assessment of the performance in MWM. The MWM device and the specific paradigms used in this laboratory have been described in detail [46,47]. Learning the location of the hidden platform from distant visual cues during 5 successive days of training, which is referred to as “incremental spatial learning”, took place on days 14–18 after dc-bTBI or sham-injury. On the following day, day 19 after dc-bTBI or sham-injury, rats were tested for memory retention during a probe trial because probe trial performance has been shown to be a more accurate measure of cognitive function than the incremental learning trials [48]. Then, on day 21, rapid learning was tested by moving the hidden platform to a new quadrant and giving the rats a single learning trial before the probe trial. The time spent in the correct (new) quadrant, which should be more than 25% based on chance alone, is taken as a measure of their ability to rapidly learn the new position. The ability for one-trial rapid learning is a hippocampus-specific cognitive function requiring place information to traverse the full trisynaptic pathway (entorhinal cortex → DG → CA3 →CA1 → entorhinal cortex) [49]. In addition, the feed-forward pathway from the entorhinal cortex to the DG and on to CA3 is needed for pattern separation [50].

Histochemistry

For the dc-bTBI and sham-injured animals that underwent neurofunctional testing, rats were euthanized on day 28 using a lethal dose of pentobarbital IP(> 100mg/kg), and the brains were perfusion-fixed with 10% neutral buffered formalin. After fixation, the brains were cryoprotected using 30% sucrose in PBS for 48 hr at 4°C.

For immunolabelling, coronal cryosections (10 μm), obtained at –5.5 to –6 mm from bregma, were blocked with 5% goat serum (G-9023; Sigma Aldrich, St. Louis, MO) plus 0.2% Triton X-100 (T8787; Sigma-Aldrich) for 1 hour at room temperature. Sections were then incubated overnight at 4°C with rabbit anti-ionized calcium binding adaptor molecule 1 (Iba1) (1:1000; 019–19741; Wako Chemicals, Richmond, VA). After several rinses in phosphate buffered saline, the slides were incubated for one hour with fluorescent-labeled anti-rabbit secondary antibody (1:500; A-11034; Alexa Flour 488; Invitrogen, Molecular Probes, Eugene, OR) at room temperature. Omission of primary antibody was used as a negative control. The sections were cover-slipped with polar mounting medium containing antifade reagent, ProLong Gold AntifadeMoutant with 4’,6-diamidino-2-phenylindole (DAPI; P36931; Invitrogen, Eugene, OR), and were examined using epifluorescence microscopy (Nikon Eclipse 90i; Nikon Instruments Inc., Melville, NY).

To identify degenerating neurons, cryosections (10 μm) were labeled with Fluoro-Jade C histo-fluorescent stain [51] according to the manufacturer’s protocol (1FJC; Histo-Chem, Jefferson, AR). Sections were cover-slipped with non-polar mounting medium (8312–4; Cytoseal XYL, Richard-Allan Scientific, Kalamazoo, MI), and were examined using epifluorescence microscopywith a fluorescein isothiocyanate (FITC) filter, with care being taken to limit the time of exposure in order to reduce photo bleaching.

Unbiased measurements of specific labeling within an ROI were obtained using NIS-Elements AR software (Nikon Instruments, Melville, NY) from sections immune-labeled or stained in a single batch, as previously described [46,52]. All ROI images for a given signal were captured using uniform parameters of magnification, area, exposure, and gain, and were applied to multiple sections. The following ROIs were defined: (i) for Iba1 in the hippocampus, a rectangular ROI, 450 ☓ 360 μm, was positioned on the perforant pathway; (ii) for Fluoro-Jade C in the hippocampus, a rectangular ROI, 450 ☓ 360 μm, was positioned at the hilus of the dentate gyrus. Segmentation analysis was performed by computing a histogram of pixel intensity for a particular ROI. Specific labeling was defined as pixels with signal intensity greater than 2☓ that of background (standard threshold based on the analysis of the intensity histograms of the ROI’s with no labeling). For both Iba1 and Fluoro-Jade C, the area occupied by pixels with specific labeling was used to determine the percent area with specific labeling (% ROI).

Statistical Analysis

Statistical calculations were carried out using either SPSS (IBM SPSS, version 21) or OriginPro8 (OriginLab Corp., Northampton, MA, USA). MRI data from the two groups of TBI and the sham at 5 time points and neurofunctional data were analyzed using a two-way repeated measure ANOVA with Fisher’s LSD post-hoc comparisons (6 rats/group for MRI, 10 rats/group for neurofunctional, for a balanced design). Non-parametric datasets (beam walk scores) were rank-transformed prior to the application of parametric statistical analysis. Histochemical data were analyzed using an unpaired t-test. Statistical significance was accepted if p<0.05.

MR Imaging

Fig 3 shows representative in vivo T2w, DKI, FA and MK images (Fig 3A) and MRS spectrum (Fig 3B) for a representative dc-bTBI rat at all imaging points from baseline to 28 days post injury. The location of the dc-bTBI injury was visible at Day1 on T2w images, which appeared to be fully resolved by Day7. No other abnormalities within the brain parenchyma were observed at any imaging time point.

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Fig 3. MRI data of a representative dc-bTBI rat at different time points from baseline to 28 days post injury.

(a) T2w images, FA and MK maps from DKI for a coronal slice. Arrow indicated soft tissue contusion from the injury, which were apparent at Day1 on T2w images but has fully resolved by Day7. (b) In vivo proton MRS acquired in the hippocampus. alanine (Ala), asparttate (Asp), g-aminobutyric acid (GABA), glucose (Glc), glutamine (Gln), glutamate (Glu), glutathione (GSH), myo-inositol (Ins), lactate (Lac), N-acetylaspartate (NAA), N-acetylaspartylglutamate (NAAG), taurine (Tau), total creatine (tCr), choline compounds (tCho), glutamate/glutamine complex (Glx), and macromolecules (MM).

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In the hippocampus (Fig 4A), no abnormalities were observed in T2w images. However, DKI results indicated significant group effect between dc-bTBI and sham rats for MK (F = 11.384, p = 0.007). Significant group-by-time interaction was found for MK (F = 6.424, p = 0.0004) and MD (F = 3.07, p = 0.027). Post-hoc tests indicated that dc-bTBI rats had significantly higher MK at 7 days (p = 0.0006), 14 days (p < 0.0001) and 28 days (p = 0.004), with a clear trend of maximum difference at 14 days and recovery at 28 days. Reduced MD was accompanied by MK increase, although MD was only significant at 14 days (p = 0.005). MRS results showed significant group difference between dc-bTBI and sham rats in Tau (F = 6.7, p = 0.027) and Ins (F = 5.4, p = 0.042) levels. Significant group-by-time interaction was found in Tau (F = 3.0, p = 0.029). Post-hoc tests indicated that dc-bTBI rats had significantly lower Tau level at 7 days (p = 0.004) and 14 days (p = 0.011), as well as lower Ins level at 14 days (p = 0.020).

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Fig 4. Changes of DKI and MRS parameters in the sham and dc-bTBI rats in the hippocampus (a) and internal capsule (b) from baseline to 28 days post injury.

Temporal data in each rat were normalized to its baseline (pre-injury) value. Error bar shows standard error. Comparisons were made between sham and dc-bTBI rats.

https://doi.org/10.1371/journal.pone.0136151.g004

Similar DKI changes were observed in the internal capsule (Fig 4B), although in this typical white matter region, FA showed significant changes concomitant with MK changes, while there were no changes in MD. In this region, MK had both a significant group effect (F = 6.37, p = 0.030), and a significant group-by-time interaction (F = 4.37, p = 0.005). Significant group-by-time interaction was observed for FA (F = 4.62, p = 0.004). Post-hoc tests indicated that dc-bTBI rats had significantly higher MK at 14 days (p < 0.001) and 28 days (p = 0.026); as well as significantly higher FA at 7 days (p = 0.0032) and 14 days (p < 0.001), with both demonstrating a trend for peak increase at 14 days and recovery at 28 days. MRS results showed significant group-by-time interaction in the Gln level (F = 3.89, p = 0.009), where the dc-bTBI rats showed significantly higher Gln level at 1 day post injury (p = 0.016).

There were no significant group effects or group-by-time interactions found in any MRI or MRS measures of the cerebellum. All imaging data are provided in S1 File.

Neurofunction

The rat model of dc-bTBI that we studied was associated with abnormalities in vestibulomotor function, complex neuromotor function, and neurocognition, with vestibulomoter abnormalities being prominent early after injury. Compared to the sham-injured group, dc-bTBI rats performed significantly worse on the beam walk test at 1 and 3 days (p< 0.01), with partial recovery at 7 days (p = 0.014) after injury (Fig 5A). Compared to sham-injured animals, dc-bTBI rats performed significantly worse on the beam balance test at 1, 3 and 7 days (p< 0.01) (Fig 5B), and fell off the accelerating RotaRod sooner at 1, 3 and 7 days (p< 0.05) (Fig 5C). The rearing time was significantly shorter in dc-bTBI rats at 1 and 3 days (p< 0.01), and partially recovered at 7 days after dc-bTBI (Fig 5D).

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Fig 5. dc-bTBI causes abnormalities in vestibulomotor performance.

A–D: performance on beam walk (A), beam balance (B), accelerating RotaRod (C) and spontaneous rearing (D) over the course of 1–14 days; n = 10 sham-injury, 10dc-bTBI; day 0 is baseline before dc-bTBI;*, p< 0.05; **, p<0.01for comparison between sham and dc-bTBI rats.

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Cognitive abnormalities were prominent later after injury (Fig 6). No differences were identified in incremental learning during days 14–18 after dc-bTBI (Fig 6A). However, significant deficits were found on the memory probe on day 19 and on the rapid learning test on day 21 after dc-bTBI (Fig 6B and 6C).

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Fig 6. dc-bTBI causes abnormalities incognitive function measured using Morris Water Maze test.

Performance during incremental learning (A), memory probe test (B), and rapid learning test (C) during days 14–21, as indicated; n = 10 sham-injury, 10 dc-bTBI; in (C), 25% represents chance alone;*, p< 0.05; **, p<0.01 for comparison between sham and dc-bTBI rats.

https://doi.org/10.1371/journal.pone.0136151.g006

Histology

On day 28 after dc-bTBI, the brains of animals that had undergone neurofunctional testing were examined for evidence of hippocampal injury. We focused on the hippocampus because deficits in rapid spatial learning and memory are considered to be hippocampus-specific [49,50,53,54]. Immunolabeling for Iba1 showed significant microglial activation in the hippocampus (Fig 7). Also, staining with Fluoro-Jade C showed significant neurodegeneration in the hippocampus (Fig 7).

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Fig 7. Histochemical findings in the hippocampus in dc-bTBIvs.

sham-injured rats at 28 days.A,B: Iba1 immunolabeling (green) for microglia in a sham-injured and a dc-bTBI rat,respectively. C, D: Fluoro-Jade C (green) for neurodegeneration in a sham-injured and a dc-bTBI rat, respectively. E,F: Quantification of Iba1 immunolabeling and Fluoro-Jade C staining in sham-injured and dc-bTBI rats; in A–D, DAPI (blue) nuclear labeling is also shown; n = 5 per group; **, p<0.01for comparison between sham and dc-bTBI rats.

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