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Preparation of enriched fractions from cerebral cortex containing isolated metabolically active neuronal and glial cells

机译:从大脑皮层制备富含分离的代谢活跃的神经元和神经胶质细胞的富集级分

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1. A procedure has been developed for the separation of intact metabolically active neuronal and glial cells in bulk from rat cerebral cortex. Separation depended on dispersion of the tissue in a Ficoll medium followed by centrifugation on a discontinuous Ficoll gradient. Up to 1·5×107 neuronal cells could be collected from 12 brains within 3hr. The morphological appearance of these cells seemed good, and the fraction was 8·5-fold purified in terms of dry weight. Average dry weight per neuron was 2300μμg. Maximum glial contamination of the neuronal fraction was 11% as determined by carbonic anhydrase measurements. The glial fraction was free from neurons but contained various subcellular contaminants. 2. Concentrations of nucleic acids, phospholipid, protein and phosphoprotein were determined in the separated fractions. The neuronal fraction was richer than the glial in all except phospholipid. Succinate dehydrogenase was equally distributed between neurons and glia but the neuronal fraction was 1·8-fold enriched in cytochrome oxidase. 3. Measurement of respiration by the cells showed an endogenous uptake of 117mμmoles of oxygen/mg./hr. in neurons, and 173mμmoles of oxygen/mg./hr. in glia. Addition of substrate at 10mm stimulated uptake to similar values in both fractions. With glucose it was 390, with pyruvate 355, and with glutamate 215mμmoles of oxygen/mg./hr. This represented a larger stimulation of neuronal than of glial respiration compared with the basal level. 4. Respiration in cell suspensions was 70–80% of that of slices, whereas fractionated tissue homogenates had respiratory rates of only one-third those of the cell suspensions. Lactate dehydrogenase content of cell suspensions was maintained during gradient centrifugation and washing. 5. The possible uses of isolated cell preparations are discussed.
机译:1.已经开发出一种从大鼠大脑皮层中分离完整的代谢活性神经元和神经胶质细胞的程序。分离取决于组织在Ficoll培养基中的分散,然后在不连续的Ficoll梯度上离心。在3小时内,可以从12个大脑中收集到多达1·5×10 7 个神经元细胞。这些细胞的形态学外观似乎良好,并且以干重计该级分是纯化的8·5倍。每个神经元的平均干重为2300μμg。通过碳酸酐酶测量确定,神经元部分的最大神经胶质污染为11%。胶质细胞没有神经元,但含有各种亚细胞污染物。 2.在分离的级分中测定核酸,磷脂,蛋白质和磷蛋白的浓度。除磷脂外,所有神经元部分均比神经胶质丰富。琥珀酸脱氢酶平均分布在神经元和神经胶质之间,但神经元部分富含1-8倍的细胞色素氧化酶。 3.细胞呼吸的测量显示出内源性摄取117mμmoles的氧气/mg./hr。神经元中的173mμmoles/ mg。/ hr。在胶质细胞。在10mm处添加底物会刺激两个部分的吸收达到相似的值。葡萄糖为390,丙酮酸为355,谷氨酸为215mμmoles的氧气/ mg / hr。与基础水平相比,这表示对神经元的刺激比对神经胶质呼吸的刺激更大。 4.细胞悬液的呼吸是切片的呼吸的70-80%,而分级组织匀浆的呼吸率仅为细胞悬液的呼吸率的三分之一。在梯度离心和洗涤过程中保持细胞悬浮液的乳酸脱氢酶含量。 5.讨论了分离细胞制备的可能用途。

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