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用二亚胺酯替代醛进行组织固定。II. 用亚氨代辛二酸二甲酯固定的大鼠肝脏的细胞化学和生物化学研究

Tissue fixation with diimidoesters as an alternative to aldehydes. II. Cytochemical and biochemical studies of rat liver fixed with dimethylsuberimidate.

作者信息

Hand A R, Hassell J R

出版信息

J Histochem Cytochem. 1976 Sep;24(9):1000-11. doi: 10.1177/24.9.61239.

Abstract

Rat liver fixed with dimethylsuberimidate (DMS) was studied to investigate the use of diimidoesters as dixatives for light and electron microscopic cytochemistry. Paraffin sections of liver fixed with DMS at pH 9.5 were weakly stained with the ninhydrin-Schiff procedure, indicating extensive reaction of NH3+ groups with the fixative. Nuclei were strongly strained by the Feulgen procedure, with no background [corrected] reaction. In contrast, glutaraldehyde fixation resulted in a significant background reaction in the cytoplasm and nuclei in controls for the Schiff-based stains. DMS-fixed liver stained intensely for glycogen with the Periodic acid-Schiff procedure, and biochemical analysis of glycogen retention and extractability indicated that DMS retained considerably more glycogen in sections than glutaraldehyde. DMS-fixed liver incubated for thiamine pyrophosphatase activity revealed reaction product in ER cisternae, Goli saccules and bile canaliculi. Peroxisomes were strongly reactive for catalase activity after incubation in diaminobenzidine medium, and reaction product of glucose-6-phosphatase activity was considerably greater following DMS fixation than after glutaraldehyde. Biochemical studies revealed up to twice as musch residual activity of glucose-6-phosphatase after DMS fixation. These results suggest that DMS may be useful as a primary fixative for certain cytochemical procedures.

摘要

研究了用亚辛二酸二甲酯(DMS)固定的大鼠肝脏,以探讨二亚胺酯作为光镜和电镜细胞化学固定剂的用途。用pH 9.5的DMS固定的肝脏石蜡切片,经茚三酮-席夫氏法染色较弱,表明NH3+基团与固定剂发生了广泛反应。福尔根氏法对细胞核染色强烈,无背景[校正后]反应。相比之下,戊二醛固定导致基于席夫氏染色的对照中细胞质和细胞核出现明显的背景反应。用高碘酸-席夫氏法对DMS固定的肝脏进行糖原染色,糖原保留和可提取性的生化分析表明,DMS固定的切片中保留的糖原比戊二醛固定的切片多得多。对DMS固定的肝脏进行硫胺素焦磷酸酶活性孵育,在内质网池、高尔基体囊泡和胆小管中发现反应产物。在二氨基联苯胺培养基中孵育后,过氧化物酶体对过氧化氢酶活性反应强烈,DMS固定后葡萄糖-6-磷酸酶活性的反应产物比戊二醛固定后明显更多。生化研究表明,DMS固定后葡萄糖-6-磷酸酶的残留活性高达戊二醛固定后的两倍。这些结果表明,DMS可能作为某些细胞化学程序的主要固定剂有用。

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