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采用快速冷冻和深度蚀刻法对培养肝细胞中过氧化物酶体进行的三维和组织化学研究。

Three-dimensional and histochemical studies of peroxisomes in cultured hepatocytes by quick-freezing and deep-etching method.

作者信息

Ohno S, Fujii Y

机构信息

Department of Anatomy, Shinshu University School of Medicine, Matsumoto, Japan.

出版信息

Histochem J. 1990 Mar;22(3):143-54. doi: 10.1007/BF01003534.

Abstract

Primary cultured mouse hepatocytes were treated with clofibric acid to induce peroxisome proliferation. They were briefly fixed with paraformaldehyde and centrifuged to prepare pellets. The hepatocytes were split open to remove cytoplasmic soluble proteins and fixed with glutaraldehyde. They were routinely incubated for catalase enzyme cytochemistry and fixed in osmium tetroxide. The specimens were quickly frozen, deeply etched and rotary shadowed by platinum and carbon. Peroxisomes were identified as osmium reaction products on replica membranes. In treated hepatocytes, the number of peroxisomes was considerably increased and smooth membranous structures resembling sER (referred to as 'peroxisome-forming sheets') showed hypertrophy. The rER associated with intermediate filaments was significantly decreased and 'peroxisome-forming sheets' appeared, being accompanied with budding and fragmentation of peroxisomes.

摘要

原代培养的小鼠肝细胞用氯贝酸处理以诱导过氧化物酶体增殖。将它们用多聚甲醛短暂固定并离心以制备沉淀。肝细胞被裂解以去除细胞质可溶性蛋白,并用戊二醛固定。它们常规用于过氧化氢酶细胞化学孵育并用四氧化锇固定。标本快速冷冻、深度蚀刻并用铂和碳进行旋转投影。过氧化物酶体在复膜上被鉴定为锇反应产物。在处理过的肝细胞中,过氧化物酶体的数量显著增加,类似于滑面内质网(称为“过氧化物酶体形成片层”)的光滑膜结构出现肥大。与中间丝相关的粗面内质网显著减少,“过氧化物酶体形成片层”出现,并伴有过氧化物酶体的出芽和碎片化。

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