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一种使脑组织小区域可逆失活的方法。

A method of reversible inactivation of small regions of brain tissue.

作者信息

Malpeli J G, Schiller P H

出版信息

J Neurosci Methods. 1979 Aug;1(2):143-51. doi: 10.1016/0165-0270(79)90011-6.

Abstract

A method is described for reversibly inactivating small, precisely localized regions of brain tissue with injections of nanoliter quantities of the local anesthetic lidocaine hydrochloride. The injections are made through a combined recording-injection probe consisting of a glass micropipette onto whose outer surface is plated a metallic cylinder for recording extracellular action potentials. The recording cylinder for recording extracellular action potentials. The recording cylinder, located a known distance from the pipette tip, picks up a continuous, large-amplitude, multiunit response which can be used to accurately position the tip according to physiological criteria. It also provides a means of determining the duration of the anesthetic block and estimating its spreat. This devise has been used to selectively block 200--400 micrometers regions of individual laminae of the lateral geniculate nucleus centered within 50 micrometers of a retinotopically defined target site. The blocks last from 3 to 10 min and can be repeated many times at the same location.

摘要

本文描述了一种方法,通过注射纳升量的局部麻醉剂盐酸利多卡因,可逆性地使脑组织中微小的、精确定位的区域失活。注射是通过一个组合的记录-注射探针进行的,该探针由一个玻璃微吸管组成,在其外表面镀有一个用于记录细胞外动作电位的金属圆柱体。用于记录细胞外动作电位的记录圆柱体。记录圆柱体位于距吸管尖端已知距离处,可拾取连续的、大幅度的多单位反应,该反应可用于根据生理标准精确地定位尖端。它还提供了一种确定麻醉阻滞持续时间并估计其扩散范围的方法。该装置已用于选择性地阻断外侧膝状体单个层中200-400微米的区域,这些区域以视网膜拓扑定义的靶位点为中心,在50微米范围内。阻滞持续3至10分钟,并且可以在同一位置重复多次。

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