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冷却可提高取自大鼠外周和中枢神经系统的切断轴突的体外存活率及融合修复能力。

Cooling enhances in vitro survival and fusion-repair of severed axons taken from the peripheral and central nervous systems of rats.

作者信息

Marzullo Timothy C, Britt Joshua M, Stavisky Ronda C, Bittner George D

机构信息

School of Biological Sciences (Neurobiology Section), The University of Texas at Austin, Austin, TX 78712, USA.

出版信息

Neurosci Lett. 2002 Jul 12;327(1):9-12. doi: 10.1016/s0304-3940(02)00378-6.

Abstract

Severed segments of rat peripheral (PNS; sciatic) and central nervous system (CNS; spinal) axons continue to conduct action potentials when maintained in vitro at 6-9 degrees C for up to 7 (sciatic axons) and 2 days (spinal axons), compared with only 36 h at 37-38 degrees C for sciatic axons and 6 h for spinal axons. These PNS and CNS axonal segments can be crushed and then treated with polyethylene glycol (PEG), resulting in a rapid reconnection (fusion) of the surviving axons at the crush site, as assessed by conduction of action potentials through the crush site within minutes after PEG administration. Severed PNS or CNS axons maintained in vitro at 6-9 degrees C prior to crushing can be successfully PEG-fused for up to 4 and 1.5 days, respectively, compared with only 24 (sciatic) and 3 h (spinal) at 37-38 degrees C. These data demonstrate that cooling significantly increases both the survival time of severed mammalian PNS and CNS axons and the time that severed axons can still be PEG-fused (rejoined) to rapidly re-establish axonal continuity in vitro.

摘要

当在6 - 9摄氏度的体外环境中维持时,大鼠外周(PNS;坐骨神经)和中枢神经系统(CNS;脊髓)轴突的切断片段能够持续传导动作电位,坐骨神经轴突可达7天,脊髓轴突可达2天,而在37 - 38摄氏度时,坐骨神经轴突仅能维持36小时,脊髓轴突仅能维持6小时。这些外周和中枢神经系统的轴突片段可以被挤压,然后用聚乙二醇(PEG)处理,通过在给予PEG后几分钟内动作电位通过挤压部位的传导来评估,结果显示在挤压部位存活的轴突会迅速重新连接(融合)。与在37 - 38摄氏度时分别仅能成功PEG融合24小时(坐骨神经)和3小时(脊髓)相比,在挤压前于6 - 9摄氏度的体外环境中维持的切断的外周或中枢神经系统轴突,分别可以成功PEG融合长达4天和1.5天。这些数据表明,冷却显著延长了切断的哺乳动物外周和中枢神经系统轴突的存活时间,以及切断的轴突仍能进行PEG融合(重新连接)以在体外快速重建轴突连续性的时间。

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