首页> 外文期刊>The Tohoku Journal of Experimental Medicine >Rapid and large-scale isolation of microsomal fraction of mouse liver by lyophilization and low speed centrifugation.
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Rapid and large-scale isolation of microsomal fraction of mouse liver by lyophilization and low speed centrifugation.

机译:冻干和低速离心小鼠肝脏微粒微粒体馏分的快速和大规模分离。

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摘要

We could prepare the microsomal fraction of mouse liver, without using an ultracentrifuge but with a low speed centrifuge. The procedure includes 1) lyophilization of post-mitochondrial fraction (9,000 x g supernatant) of mouse liver, 2) powdering of the lyophilized sample, 3) the addition of 1.15 per cent potassium chloride solution or distilled water, which afforded microsomal aggregates, 4) sedimentation of microsomal fraction by low-speed centrifugation (20,000 x g, 20 min). The sedimented microsomal fraction showed normal contents of cytochrome P-450 and cytochrome b5, and gave a normal pattern on SDS polyacrylamide gel electrophoresis and normal electron microscopic feature. This method should be convenient for rapid and large-scale preparation of microsomes, especially for the preparation of cytochrome b5 and cytochrome P-450.
机译:我们可以制备小鼠肝脏的微粒体级分,而无需使用超速纤维,而是用低速离心机。 该方法包括1)小鼠肝脏后线粒体馏分(9,000×g上清液)的冻干,2)冻干样品的粉末,3)加入1.15%的氯化钾溶液或蒸馏水,得到微粒聚集体,4) 低速离心微粒体馏分(20,000×g,20分钟)沉淀。 沉积的微粒体馏分显示细胞色素P-450和细胞色素B5的正常含量,并对SDS聚丙烯酰胺凝胶电泳和正常电子显微镜特征进行了正常的图案。 该方法应方便地对微粒体的快速和大规模制备,特别是用于制备细胞色素B5和细胞色素P-450。

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