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首页> 外文期刊>Applied Microbiology and Biotechnology >A novel rapid and continuous procedure for large-scale purification of magnetosomes from Magnetospirillum gryphiswaldense
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A novel rapid and continuous procedure for large-scale purification of magnetosomes from Magnetospirillum gryphiswaldense

机译:一种新颖快速连续的方法,用于从灰螺磁螺菌大规模纯化磁小体

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摘要

A new rapid and continuous procedure was developed for purifying magnetosomes from Magnetospirillum gryphiswaldense MSR-1 cells on a large scale. The procedure included these steps: disruption of cells with a high-pressure homogeniser, isolation of magnetosomes with a continuous magnetism isolation system accompanied by low-power ultrasonication and urea treatment, removal of adsorbed and surface proteins with proteinase K, removal of nucleic acids with electro-elution, and replacement of the PBS buffer with distilled water by a magnetically stirred system. The purified magnetosomes were stored at −20 °C after lyophilized and treated with γ-rays. The time required for purification was reduced from 20–30 to 2–5 days. Evaluation of the purity of the resulting magnetosomes was carried out with SDS-PAGE, PCR, and Fourier-transform infrared spectroscopy. The overall data suggest that the method presented here is a simple, rapid, continuous, and highly efficient procedure for large-scale purification of magnetosomes.
机译:开发了一种新的快速且连续的程序,用于大规模纯化来自Magspirospirillum gryphiswaldense MSR-1细胞的核小体。该程序包括以下步骤:用高压匀浆器破碎细胞,用连续磁分离系统分离磁小体,同时进行低功率超声处理和尿素处理,用蛋白酶K去除吸附的蛋白质和表面蛋白,用蛋白酶K去除核酸。电洗脱,并通过磁力搅拌系统用蒸馏水代替PBS缓冲液。冻干后,将纯化的磁小体保存在-20°C并用γ射线处理。纯化所需的时间从20-30天减少到2-5天。用SDS-PAGE,PCR和傅里叶变换红外光谱法对所得磁小体的纯度进行评估。总体数据表明,此处介绍的方法是用于大规模纯化磁小体的简单,快速,连续且高效的过程。

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