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使用Percoll密度梯度离心法从大鼠脑及其亚区域快速分离代谢活跃的线粒体。

Rapid isolation of metabolically active mitochondria from rat brain and subregions using Percoll density gradient centrifugation.

作者信息

Sims N R

机构信息

Department of Medical Biochemistry, Flinders University of South Australia, Bedford Park.

出版信息

J Neurochem. 1990 Aug;55(2):698-707. doi: 10.1111/j.1471-4159.1990.tb04189.x.

Abstract

Two procedures are described for isolating free (nonsynaptosomal) mitochondria from rat brain. Both procedures employ a discontinuous Percoll gradient and yield well coupled mitochondria which exhibit high rates of respiratory activity and contain little residual contamination by synaptosomes or myelin. The procedures are considerably more rapid than methods described previously for the isolation of brain mitochondria and do not require an ultracentrifuge or swing-out rotor. The first method separates mitochondria by gradient centrifugation from a P2 (crude mitochondrial) fraction and is likely to be widely applicable for studies in which at least 500 mg of tissue are available as starting material. In the second method, the unfractionated homogenate is subjected directly to gradient centrifugation. This method requires the preparation of more gradients (per gram of tissue) than the first method and yields a subcellular fraction with slightly more synaptosomal contamination. However, this second procedure is more rapid, requires less manipulation of the tissue, and is suitable for obtaining mitochondria with well preserved metabolic characteristics from subregions of single rat brains.

摘要

本文描述了两种从大鼠脑中分离游离(非突触体)线粒体的方法。两种方法均采用不连续的Percoll梯度,得到的线粒体偶联良好,呼吸活性高,且几乎没有突触体或髓磷脂的残留污染。这些方法比先前描述的脑线粒体分离方法要快得多,并且不需要超速离心机或甩平式转头。第一种方法通过梯度离心从P2(粗线粒体)组分中分离线粒体,可能广泛适用于至少有500毫克组织作为起始材料的研究。在第二种方法中,未分级的匀浆直接进行梯度离心。该方法(每克组织)比第一种方法需要制备更多的梯度,并且产生的亚细胞组分中突触体污染略多。然而,第二种方法更快,对组织的操作更少,适用于从单个大鼠脑的亚区域获得代谢特征保存良好的线粒体。

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