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Rapid Fractionation of Wheat Leaf Protoplasts Using Membrane Filtration 1: The Determination of Metabolite Levels in the Chloroplasts, Cytosol, and Mitochondria

机译:使用膜过滤技术快速分离小麦叶片原生质体:叶绿体,胞质溶胶和线粒体中代谢物含量的测定

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摘要

A technique is presented for measuring the in vivo metabolite levels in the chloroplast stroma, the cytosol, and the mitochondrial matrix of wheat (Triticum aestivum, var `Timmo') leaf protoplasts, in which membrane filtration is used to prepare fractions enriched in the different subcellular fractions within 0.1 seconds after disruption of the protoplasts. By closing a syringe, protoplasts are forced through a net and disrupted, diluting the cytosol into the medium and also releasing intact chloroplasts and mitochondria which can then be immediately removed on membrane filters placed behind the nylon net. By varying the membrane filters, different filtrates are obtained corresponding to (a) mainly cytosol, or (b) cytosol and mitochondria with only low levels of chloroplasts; alternatively, (c) the entire protoplast contents are obtained by omitting the filters. The filtrates are immediately split, half flowing into HClO4 where they are immediately quenched for subsequent metabolite analyses; the other half flows into detergent and is used to monitor the exact distribution of marker enzymes in each individual fractionation. Using the measured distributions of metabolite and of marker enzymes in the three filtrates, the subcellular distribution of the metabolite can be algebraically calculated. The method is presented using ATP as an example.
机译:提出了一种用于测量小麦叶片原生质体中叶绿体基质,胞质溶胶和线粒体基质中体内代谢产物水平的技术,其中使用膜过滤来制备富含不同成分的级分原生质体破坏后0.1秒内产生亚细胞级分。通过关闭注射器,原生质体被迫通过网并被破坏,将细胞溶质稀释到培养基中,还释放出完整的叶绿体和线粒体,然后可以立即将其从置于尼龙网后面的滤膜上除去。通过改变膜过滤器,获得对应于(a)主要为细胞质,或(b)仅具有低水平叶绿体的细胞质和线粒体的不同滤液;或者,(c)通过省略过滤器获得全部原生质体含量。滤液立即分流,一半流入HClO4中,然后立即将其淬灭以用于随后的代谢物分析。另一半流入去污剂,并用于监测每个单独分级分离中标记酶的确切分布。使用三种滤液中代谢物和标记酶的测量分布,可以代数计算代谢物的亚细胞分布。以ATP为例介绍了该方法。

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