Abstract
BackgroundTraumatic brain injury (TBI) patients in military settings can be exposed to prolonged periods of hypobaria (HB) during aeromedical evacuation. Hypobaric exposure, even with supplemental oxygen to prevent hypoxia, worsens outcome after experimental TBI, in part by increasing neuroinflammation. Cell cycle activation (CCA) after TBI has been implicated as a mechanism contributing to both post-traumatic cell death and neuroinflammation. Here, we examined whether hypobaric exposure in rats subjected to TBI increases CCA and microglial activation in the brain, as compared to TBI alone, and to evaluate the ability of a cyclin-dependent kinase (CDK) inhibitor (CR8) to reduce such changes and improve behavioral outcomes.MethodsAdult male Sprague Dawley rats were subjected to fluid percussion-induced injury, and HB exposure was performed at 6 h after TBI. Western blot and immunohistochemistry (IHC) were used to assess cell cycle-related protein expression and inflammation at 1 and 30 days after injury. CR8 was administered intraperitoneally at 3 h post-injury; chronic functional recovery and histological changes were assessed.ResultsPost-traumatic hypobaric exposure increased upregulation of cell cycle-related proteins (cyclin D1, proliferating cell nuclear antigen, and CDK4) and microglial/macrophage activation in the ipsilateral cortex at day 1 post-injury as compared to TBI alone. Increased immunoreactivity of cell cycle proteins, as well as numbers of Iba-1+ and GFAP+ cells in both the ipsilateral cortex and hippocampus were found at day 30 post-injury. TBI/HB significantly increased the numbers of NADPH oxidase 2 (gp91phox) enzyme-expressing cells that were co-localized with Iba-1+. Each of these changes was significantly reduced by the administration of CR8. Unbiased stereological assessment showed significantly decreased numbers of microglia displaying the highly activated phenotype in the ipsilateral cortex of TBI/HB/CR8 rats compared with TBI/HB/Veh rats. Moreover, treatment with this CDK inhibitor also significantly improved spatial and retention memory and reduced lesion volume and hippocampal neuronal cell loss.ConclusionsHB exposure following TBI increases CCA, neuroinflammation, and associated neuronal cell loss. These changes and post-traumatic cognitive deficits are reduced by CDK inhibition; such drugs may therefore serve to protect TBI patients requiring aeromedical evacuation.
Highlights
Traumatic brain injury (TBI) patients in military settings can be exposed to prolonged periods of hypobaria (HB) during aeromedical evacuation
Post-traumatic hypobaria exposure increases CCA as compared to TBI alone To evaluate the effect of HB on cell cycle activation, we first examined cell cycle pathway changes in the ipsilateral cortex at day 1 after TBI
We examined immunoreactivity of cyclin D1, proliferating cell nuclear antigen (PCNA), and CDK4 in the ipsilateral cortex and hippocampus from sham (n = 4), TBI alone (n = 6), TBI + Veh + HB (n = 6), and TBI + CR8 + HB (n = 6) rats at 30 days postinjury
Summary
Traumatic brain injury (TBI) patients in military settings can be exposed to prolonged periods of hypobaria (HB) during aeromedical evacuation. Patients can be exposed to long periods of hypobaria (HB), as military flights are often pressurized only to 8000 ft, substantially different from commercial air travel [3, 4] It has been recently shown in a rat TBI model that hypobaria during simulated AE worsens cognitive and pathological outcomes [5]; this report and an earlier one using a mouse TBI model suggest that hypobaria can increase posttraumatic inflammatory responses [6]. Cell cycle activation (CCA) occurs after TBI in both neurons and glial cells and contributes to secondary injury [8,9,10]. Administration of cell cycle inhibitors after TBI increases neuronal survival and reduces both microglial and astroglial activation; the latter includes multiple studies utilizing the rat LFP injury model [11,12,13,14,15]
Sign-in/Register to view highlights & summary 
Published Version (
Free)
Talk to us
Join us for a 30 min session where you can share your feedback and ask us any queries you have
Schedule a call