Cytochemical demonstration of glutaraldehyde-resistant NADH-ferricyanide oxido-reductase activities in rat-liver plasma membranes and Golgi apparatus.

Cytobiologie Pub Date : 1978-12-01
D J Morré, E L Vigil, C Frantz, H Goldenberg, F L Crane
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Abstract

NADH-ferricyanide reductase activity was demonstrated in rat liver endomembranes by cytochemical procedures. The activity observed in plasma membrane and mature portions of the Golgi apparatus resisted fixation in 0.1% glutaraldehyde, a characteristic which permitted differentiation of the NADH-ferricyanide reductase of plasma membranes and mature Golgi apparatus elements from those of mitochondria, microbodies, endoplasmic reticulum and nuclear envelope. With the latter membranes, activity could be demonstrated only with unfixed material or following brief glutaraldehyde fixation and was greatest with broken cells or isolated fractions due to problems of penetration of reagents. Biochemical studies paralleled cytochemical findings with respect to glutaraldehyde fixation and sensitivity to other metabolic inhibitors. The findings provide evidence that a NADH-ferricyanide reductase may be among the membrane constituents conserved and/or modified during flow differentiation of membranes. The basis for a method to evaluate plasma membrane contamination of endoplasmic reticulum fractions and to differentiate among mature and immature secretory vesicles of the Golgi apparatus is also indicated.

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大鼠肝质膜和高尔基体抗戊二醛nadh -铁氰化物氧化还原酶活性的细胞化学证明。
通过细胞化学方法证实了nadh -铁氰还原酶在大鼠肝内膜中的活性。在质膜和高尔基体成熟部分中观察到的活性抵抗0.1%戊二醛的固定,这一特征使得质膜和成熟高尔基体元件的nadh -铁氰化还原酶与线粒体、微体、内质网和核膜的nadh -铁氰化还原酶分化。对于后一种膜,只有在未固定的材料或短暂的戊二醛固定后才能显示活性,并且由于试剂的渗透问题,当细胞破裂或分离组分时活性最大。关于戊二醛固定和对其他代谢抑制剂的敏感性,生化研究与细胞化学研究结果相一致。这些发现提供了证据,表明nadh -铁氰化物还原酶可能是在膜流动分化过程中保守和/或修饰的膜成分之一。为评价内质网部分质膜污染和区分高尔基体成熟和未成熟分泌囊泡的方法奠定了基础。
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