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Folding aggregated proteins into functionally active forms

机译:将聚集的蛋白质折叠成功能活跃的形式

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The successful expression and purification of proteins in an active form is essential for structural and biochemical studies. With rapid advances in genome sequencing and high-throughput structural biology, an increasing number of proteins are being identified as potential drug targets but are difficult to obtain in a form suitable for structural or biochemical studies. Although prokaryotic recombinant expression systems are often used, proteins obtained in this way are typically found to be insoluble. Several experimental approaches have therefore been developed to refold these aggregated proteins into a biologically active form, often suitable for structural studies. The major refolding strategies adopt one of two approaches - chromatographic methods or refolding in free solution - and both routes have been successfully used to refold a range of proteins. Future advances are likely to involve the development of automated approaches for protein refolding and purification.
机译:活性形式蛋白质的成功表达和纯化对于结构和生化研究至关重要。随着基因组测序和高通量结构生物学的飞速发展,越来越多的蛋白质被确定为潜在的药物靶标,但很难以适合结构或生化研究的形式获得。尽管经常使用原核重组表达系统,但是通常发现以这种方式获得的蛋白质是不溶的。因此,已经开发出几种实验方法来将这些聚集的蛋白质重新折叠成生物活性形式,通常适合于结构研究。主要的重折叠策略采用两种方法之一-色谱法或在游离溶液中重折叠-两种途径均已成功用于重折叠一系列蛋白质。未来的进展可能涉及蛋白质重折叠和纯化的自动化方法的开发。

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