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酶解分离的哺乳动物血管平滑肌细胞对药理和电刺激的反应。

Responses of enzymatically isolated mammalian vascular smooth muscle cells to pharmacological and electrical stimuli.

作者信息

DeFeo T T, Morgan K G

出版信息

Pflugers Arch. 1985 May;404(1):100-2. doi: 10.1007/BF00581502.

Abstract

A modified method for enzymatically isolating mammalian vascular smooth muscle cells has been developed and tested for ferret portal vein smooth muscle. This method produces a high proportion of fully relaxed cells and these cells appear to have normal pharmacological responsiveness. The ED50 values for both alpha stimulation and potassium depolarization are not significantly different in the isolated cells from those obtained from intact strips of ferret portal vein, suggesting that the enzymatic treatment does not destroy receptors or alter the electrical responsiveness of the cells. It was also possible to demonstrate a vasodilatory action of papaverine, nitroprusside and adenosine directly on the isolated cells indicating that the pathways involved are intact in the isolated cells. This method should be of considerable usefulness, particularly in combination with the new fluorescent indicators and cell sorter techniques which require isolated cells.

摘要

已开发出一种改良的酶法分离哺乳动物血管平滑肌细胞的方法,并在雪貂门静脉平滑肌上进行了测试。该方法可产生高比例的完全松弛细胞,且这些细胞似乎具有正常的药理反应性。分离细胞中α刺激和钾去极化的半数有效剂量(ED50)值与从雪貂门静脉完整条带获得的细胞中的值无显著差异,这表明酶处理不会破坏受体或改变细胞的电反应性。还能够直接证明罂粟碱、硝普钠和腺苷对分离细胞具有血管舒张作用,这表明所涉及的途径在分离细胞中是完整的。该方法应具有相当大的实用性,特别是与需要分离细胞的新型荧光指示剂和细胞分选技术相结合时。

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