Resuscitation speed affects brain injury in a large animal model of traumatic brain injury and shock

After induction of anesthesia, a cutdown technique was used to access the right and left femoral arteries for invasive blood pressure monitoring (Eagle 4000 patient monitor, GE Marquette Piscataway NJ) and blood draw respectively. The left femoral vein was cannulated for fluid administration, whereas the right external jugular vein was used for the insertion of a pulmonary artery (PA) catheter. The PA catheter was used for measurements of cardiac output, pulmonary and central venous pressures as well as mixed venous oxygenation. A distal midline laparotomy was performed for the insertion of a cystostomy tube. Hemodynamic parameters (V9004 SurgiVet, Waukesha, WI), including cardiac output (Vigilance II Monitor, Edwards Lifesciences, Irvine CA), were recorded in five-minute intervals. The animal’s head was fixed in a custom made stereotactic frame with a mouthpiece affixed to the zygoma to prevent movement.

A 20 mm burr hole was made on the right side of the skull, next to the coronal and sagittal sutures over the frontal lobe to expose the dura. Bone was carefully removed so as not to disturb the dura and the underlying brain tissue. A catheter for intracranial pressure monitoring and monitoring of cerebral oxygenation (Integra Lifesciences, Plainsboro, NJ) was inserted through a bolt placed in a 2-mm burr hole on the left side of the skull, 10 mm lateral and 10 mm anterior to the bregma.

A computer-controlled cortical impact device was used for these experiments. Briefly, a 15 mm cylindrical impactor tip was mounted on an electronic motor, and the dynamics were precisely controlled to deliver 4 m/s velocity, 100 ms dwell time and 12 mm depth penetration. After impact, the burr hole was sealed with bone wax to prevent leakage of cerebrospinal fluid, and to eliminate any artifact in ICP monitoring.

Model outline is provided in Figure 1. Total blood volume was estimated, and 40% of it was withdrawn through the femoral arterial catheter using a Masterflex pump, Model L/S Computerized Drive with a MF easy load II Pump-head, Model 77201–60 (Cole-Palmer, Vernon Hills, IL). Bleeding was started concurrent with TBI at a rate of 3.15% total blood volume/min and was captured in a Terumo blood collection bag (CPDA and AS-5). Isoflurane was decreased with the onset of hypotension. If MAP dropped < 30 mmHg, hemorrhage was briefly held and a small volume of saline was infused through the femoral venous line. Once the MAP reached 35 mmHg, saline infusion was stopped and hemorrhage was restarted. Using this protocol, MAP was maintained between 30 mmHg and 35 mm Hg until 40% of the estimated blood volume was withdrawn in a controlled fashion. Following hemorrhage, animals were left in shock for 120 minutes and MAP was maintained between 30–35 mmHg by titrating the dose of inhaled isoflurane. After the 2 hours of shock, animals were resuscitated as follows: Prior to the experiment, animals had been randomly assigned to 1 of 4 resuscitation groups (Figure 1): 1) bolus infusion with FFP 1*shed blood volume (n = 5) at 50 ml/min, 2) Stepwise infusion of FFP 1*shed blood with infusion speeds starting at 2 ml/min and gradually increasing to 50 ml/min (n = 6), 3) stepwise infusion of NS*3 shed blood volume with infusion speeds staring at 6 ml/min and gradually increasing to 165 ml/min (n = 6) and 4) bolus infusion of NS *3 shed blood volume at 165 ml/min (n = 5). Bolus resuscitation protocols were based on previous experiments [9]. The stepwise resuscitation protocols were the result of several pilot experiments suggesting an optimal hemodynamic response while minimizing resuscitation time and the extent of the brain injury. Fluids were infused into the femoral vein using a Masterflex pump. Animals were monitored for six hours post resuscitation and were kept warm (Bair Hugger Model 505; Arizant Healthcare Inc., Eden Praire, MN). Electrolytes were corrected as needed. Following the six-hour observation period, animals were euthanized by intravenous injection of sodium pentobarbital 100 mg/kg (Euthasol, Virbac Corp, Fort Worth, TX).

An arterial blood gas was analyzed at baseline, following 2 hours of shock and the 6-hour observation period.

Normal saline (0.9% NaCl) was obtained from Hospira inc. (Lake Forest, IL) and stored at room temperature. FFP was isolated from healthy porcine donors. Briefly, whole blood was captured in a blood collection bag and centrifuged at 5000 g for 10 minutes at 4°C. The supernatant was further centrifuged at 5000 g for 10 minutes to extract the plasma which was stored at −80°C. It was thawed immediately prior to use.

Brains were removed following euthanasia and were sliced into 5 mm coronal sections. Slices were incubated in 2% 2,3,5-triphenyltetrazolium chloride (TTC) (SigmaChemical Co., St. Louis, MO) to assess the presence of nonviable tissue. Size of the lesion was measured with computer-assisted image analysis software ImageJ (NIH, Bethesda, MD). Brain swelling was calculated by comparing it to the uninjured hemisphere [(ipsilateral hemisphere’s volume/contralateral hemisphere’s volume) − 1] × 100 . True infarction volumes were corrected by the swelling factor.

Stroke volume (SV) was calculated as Cardiac Output/Heart Rate. Systemic vascular resistance (SVR) was calculated as 80 × (mean arterial pressure-central venous pressure)/Cardiac Output.

Data are presented as mean ± standard error of the mean. Brain lesion size and swelling as well as arterial blood gas parameters were compared using an unpaired t-test.

For the purpose of comparing post-resuscitation hemodynamic variables, following biostatistician consultation we used a linear mixed model to compare value means from end of resuscitation through the 6-hour observation period between groups while correcting for intra-group repeated measures. Based on these measurements, the model calculated an estimated mean value for the 6-hour timeframe in each group.

Sample size calculations were based on previously published data [9],[10] from the same model, and the group sizes were sufficient to detect a 50% difference between the groups for continuous variables (with variance of 25% within the group), with a power (1-β) = 90% and α = 0.05.

All statistical analysis was done using SPSS 20.0 (IBM Corp. Armonk NY).

Statistical significance was defined as p < 0.05.

Arterial blood gas values are listed in Table 1. At the 6-hour observation time point, fast infusion of FFP was associated with higher hemoglobin levels compared with stepwise FFP infusion (6.60 ± 0.44 g/dl vs. 5.12 ± 1.13 g/dl, p = 0.01) as well as higher lactate levels (2.94 ± 0.22 mmol/l vs. 2.04 ± 0.12 mmol/l, p = 0.01). No differences were found in the NS groups.

Hemodynamic variables are shown in Table 2 while Figure 2 depicts selected variables from start of resuscitation and over the course of the 6-hour observation period.

In the FFP groups, fast resuscitation resulted in overall higher mean arterial pressures (MAP, 55.90 ± 0.93 mmHg vs. 53.39 ± 0.86 mmHg, p = 0.05) but similar central venous pressures (CVP). This was, however, associated with a higher systemic vascular resistance in the fast resuscitation group (SVR, 1052.75 ± 65.90 mmHg vs. 761.63 ± 22.42 mmHg, p = 0.04) as well as a lower mean pulmonary artery pressures (MPAP, 15.12 ± 1.26 mmHg vs. 23.11 ± 1.17 mmHg, p < 0.01).

In the NS groups, fast NS resuscitation resulted in an overall higher MAP (52.93 ± 1.41 mmHg vs. 46.92 ± 1.30, p = 0.01), but no difference in CVP. As in the FFP groups, this was associated with a higher SVR (921.40 ± 19.42 mmHg vs. 573.41 ± 17.92 mmHg, p < 0.01).

Cardiac function is summarized in Table 2 and Figure 3. In both FFP and NS groups, fast resuscitation was associated with overall lower cardiac outputs (FFP: 4.81 ± 1.50 l/min vs. 5.45 ± 1.14 l/min, p = 0.03; NS: 4.37 ± 0.12 l/min vs. 6.35 ± 0.10 l/min, p < 0.01). No differences in stroke volume were observed.

ICP and brain pO2 values are shown in Table 2 and Figure 4. Fast resuscitation with FFP resulted higher ICP (9.10 ± 0.72 mmHg vs. 6.36 ± 0.68 mmHg, p = 0.04) but no difference in brain oxygenation compared with stepwise resuscitation. No differences were observed in the NS groups.

Lesion sizes and brain swelling is shown in Figure 4. Fast resuscitation with FFP resulted in increased brain swelling (22.36 ± 1.03% vs. 15.58 ± 2.52%, p = 0.04) but similar lesion sizes (2160.24 ± 202.56 mm³ vs. 2141.32 ± 256.27 mm³, p = 0.96) compared with stepwise FFP resuscitation. Fast resuscitation with normal saline resulted in increased brain swelling (37.24 ± 1.63% vs. 26.74 ± 1.33%, p = 0.05) as well as lesion size (3285.44 ± 130.81 mm³ vs. 2509.41 ± 297.44 mm³, p = 0.04).