Iwata Akira, Stys Peter K, Wolf John A, Chen Xiao-Han, Taylor Andrew G, Meaney David F, Smith Douglas H
Department of Neurosurgery, University of Pennsylvania, Philadelphia, Pennsylvania 19104-6316, USA.
J Neurosci. 2004 May 12;24(19):4605-13. doi: 10.1523/JNEUROSCI.0515-03.2004.
We demonstrated previously that dynamic stretch injury of cultured axons induces structural changes and Ca2+ influx modulated by tetrodotoxin (TTX)-sensitive voltage-gated sodium channels (NaChs). In the present study, we evaluated potential damage to the NaCh alpha-subunit, which can cause noninactivation of NaChs. In addition, we explored the effects of pre-injury and post-injury treatment with TTX and protease inhibition on proteolysis of the NaCh alpha-subunit and intra-axonal calcium levels ([Ca2+]i) over 60 min after trauma. After stretch injury, we found that [Ca2+]i continued to increase in untreated axons for at least 60 min. We also observed that the III-IV intra-axonal loop of the NaCh alpha-subunit was proteolyzed between 5 and 20 min after trauma. Pre-injury treatment of the axons with TTX completely abolished the posttraumatic increase in [Ca2+]i and proteolysis of the NaCh alpha-subunit. In addition, both pre-injury and post-injury inhibition of protease activity attenuated long-term increases in [Ca2+]i as well as mitigating degradation of the NaCh alpha-subunit. These results suggest a unique "feed-forward" deleterious process initiated by mechanical trauma of axons. Na+ influx through NaChs resulting from axonal deformation triggers initial increases in [Ca2+]i and subsequent proteolysis of the NaCh-subunit. In turn, degradation of the alpha-subunit promotes persistent elevations in [Ca2+]i, fueling additional pathologic changes. These observations may have important implications for developing therapeutic strategies for axonal trauma.
我们之前证明,培养轴突的动态拉伸损伤会诱导结构变化以及由河豚毒素(TTX)敏感的电压门控钠通道(NaChs)调节的Ca2+内流。在本研究中,我们评估了对NaChα亚基的潜在损伤,这种损伤可导致NaChs的非失活。此外,我们探讨了在创伤后60分钟内,TTX预处理和后处理以及蛋白酶抑制对NaChα亚基蛋白水解和轴突内钙水平([Ca2+]i)的影响。拉伸损伤后,我们发现未处理的轴突中[Ca2+]i至少持续增加60分钟。我们还观察到,创伤后5至20分钟内,NaChα亚基的轴突内III-IV环被蛋白水解。轴突损伤前用TTX处理完全消除了创伤后[Ca2+]i的增加和NaChα亚基的蛋白水解。此外,损伤前和损伤后蛋白酶活性的抑制均减弱了[Ca2+]i的长期增加,并减轻了NaChα亚基的降解。这些结果表明,轴突机械创伤引发了一个独特的“前馈”有害过程。轴突变形导致通过NaChs的Na+内流触发了[Ca2+]i的初始增加以及随后NaCh亚基的蛋白水解。反过来,α亚基的降解促进了[Ca2+]i的持续升高,加剧了其他病理变化。这些观察结果可能对制定轴突创伤的治疗策略具有重要意义。