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通过生物发光法对内源性脑ATP进行的图像表示。

A pictorial representation of endogenous brain ATP by a bioluminescent method.

作者信息

Kogure K, Alonso O F

出版信息

Brain Res. 1978 Oct 13;154(2):273-84. doi: 10.1016/0006-8993(78)90700-x.

Abstract

The layering of a luciferin-luciferase solution on brain slices makes endogenous ATP visible. Rat brains, frozen in situ and sliced at 16 micrometer thickness at a temperature of--15 degrees C, were fixed by a ternary mixture of ethanol, formalin and dioxane at--20 degrees C for 15 min, and dried at 40 degrees C for 12 h. Luciferin, luciferase and a small quantity of magnesium sulfate were dissolved into an arsenate buffer solution containing 1% polyvinylpyrrolidone, 2% gelatin and 1% glycerol. The solution was then frozen into a column, sliced at 40 micrometer thickness at--15 degrees C and placed on the precooled brain slice. A luminiferous luciferin-ATP reaction begins when the brain slice reaches room temperature and persists for more than 10 min. This technique therefore makes possible the optical and/or photographic determination of the endogenous concentration of brain ATP. Capability of the technique is also demonstrated.

摘要

在脑片上分层放置荧光素 - 荧光素酶溶液可使内源性ATP可见。将大鼠脑原位冷冻,在-15℃下切成16微米厚的切片,于-20℃用乙醇、福尔马林和二氧六环的三元混合物固定15分钟,然后在40℃干燥12小时。将荧光素、荧光素酶和少量硫酸镁溶解于含有1%聚乙烯吡咯烷酮、2%明胶和1%甘油的砷酸盐缓冲溶液中。然后将该溶液冻成柱状,在-15℃切成40微米厚的切片,并置于预冷的脑片上。当脑片达到室温时,发光的荧光素 - ATP反应开始,并持续超过10分钟。因此,该技术使得对脑ATP内源性浓度进行光学和/或摄影测定成为可能。该技术的能力也得到了证明。

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