使用戊二醛和四氧化锇或铁氰化钾还原锇同时固定用于保存单殖吸虫扁虫:对伊科帕梅里佐吸虫的评估
Simultaneous fixation using glutaraldehyde and osmium tetroxide or potassium ferricyanide-reduced osmium for the preservation of monogenean flatworms: an assessment for Merizocotyle icopae.
作者信息
Cribb Bronwen, Armstrong Wendy, Whittington Ian
机构信息
Centre for Microscopy and Microanalysis, The University of Queensland, Brisbane, Queensland 4072, Australia.
出版信息
Microsc Res Tech. 2004 Feb 1;63(2):102-10. doi: 10.1002/jemt.20015.
Simultaneous fixation was investigated for a marine organism: the monogenean flatworm ectoparasite Merizocotyle icopae. Four protocols for primary fixation were compared: 3% glutaraldehyde alone in 0.1M cacodylate buffer for a minimum of 2 hours; 1% glutaraldehyde in combination with 1% osmium tetroxide, both in 0.1M cacodylate buffer, until tissues darkened (5-20 minutes); 1% glutaraldehyde in 0.1M cacodylate buffer in combination with 0.5% potassium ferricyanide-reduced osmium until tissues darkened (5-20 minutes); 1% glutaraldehyde in combination with 1% osmium tetroxide, both in 0.1M cacodylate buffer, for 30 minutes. The study confirms that the standard method for transmission electron microscopic fixation (first listed protocol) routinely applied to platyhelminths is optimal for ultrastructural preservation, but some simultaneous fixation methods (second and third listed protocols) are acceptable when rapid immobilization is needed. Scanning electron microscopic preparations may be improved using simultaneous primary fixation.
对一种海洋生物——单殖吸虫外寄生虫伊氏梅里吸虫进行了同步固定研究。比较了四种初次固定方案:在0.1M二甲胂酸钠缓冲液中单独使用3%戊二醛至少2小时;在0.1M二甲胂酸钠缓冲液中1%戊二醛与1%四氧化锇混合,直至组织变黑(5 - 20分钟);在0.1M二甲胂酸钠缓冲液中1%戊二醛与0.5%亚铁氰化钾还原锇混合,直至组织变黑(5 - 20分钟);在0.1M二甲胂酸钠缓冲液中1%戊二醛与1%四氧化锇混合30分钟。该研究证实,常规应用于扁形虫的透射电子显微镜固定标准方法(第一个列出的方案)对于超微结构保存是最佳的,但在需要快速固定时,一些同步固定方法(第二个和第三个列出的方案)是可以接受的。使用同步初次固定可以改善扫描电子显微镜标本制备。
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