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对用二甲基亚砜冻干的心肌进行扫描电子显微镜检查,以同时显示细胞形态和微血管功能。

Scanning electron microscopy of heart muscle freeze-dried from dimethylsulfoxide for simultaneous demonstration of cell morphology and microvascular function.

作者信息

Sage M D, Gavin J B

出版信息

Stain Technol. 1986 Sep;61(5):261-7. doi: 10.3109/10520298609109951.

Abstract

Scanning electron microscopy was used to examine cryofracture surfaces of ventricular myocardium from glutaraldehyde fixed rat and rabbit hearts subjected to intravascular injection of polymerizing acrylic resin. This allowed simultaneous observation of morphological features of cardiac muscle cells and the functional state of their associated small blood vessels. Because the resin injected to identify capillaries accessible to flow might be soluble in commonly used tissue dehydrating agents, alternative preparation methods using the cryoprotectants dimethylsulfoxide (DMSO) and glycerol were investigated. Provided a high performance backscattered electron detector and simple environmental cell were used to abolish specimen charging and circumvent potential instrument contamination, immersion in 2.82 M DMSO for 12 hr prior to cryofracture and freeze-drying gave the best results. The SEM appearance of specimens dehydrated in this way differed little from that of specimens prepared by ethanol dehydration and freeze-drying or by acetone dehydration and critical-point drying. Tissue shrinkage was 26.5 +/- 9.4%, comparable to that found after standard methods using solvent dehydration and critical-point drying.

摘要

扫描电子显微镜用于检查经戊二醛固定的大鼠和兔心脏的心室心肌冷冻断裂表面,这些心脏经血管内注射聚合丙烯酸树脂。这使得能够同时观察心肌细胞的形态特征及其相关小血管的功能状态。由于注入以识别可流动毛细血管的树脂可能可溶于常用的组织脱水剂,因此研究了使用冷冻保护剂二甲基亚砜(DMSO)和甘油的替代制备方法。如果使用高性能背散射电子探测器和简单的环境室来消除样品充电并避免潜在的仪器污染,在冷冻断裂和冷冻干燥前将样品浸入2.82 M DMSO中12小时可得到最佳结果。以这种方式脱水的样品的扫描电镜外观与通过乙醇脱水和冷冻干燥或丙酮脱水和临界点干燥制备的样品的外观差异不大。组织收缩率为26.5 +/- 9.4%,与使用溶剂脱水和临界点干燥的标准方法后发现的收缩率相当。

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