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General qPCR and Plate Reader Methods for Rapid Optimization of Membrane Protein Purification and Crystallization Using Thermostability Assays

机译:使用热稳定性测定法快速优化膜蛋白纯化和结晶的通用qPCR和酶标仪方法

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摘要

This unit describes rapid and generally applicable methods to identify conditions that stabilize membrane proteins using temperature-based denaturation measurements as a proxy for target time-dependent stability. Recent developments with thiol-reactive dyes sensitive to the unmasking of cysteine residues upon protein unfolding have allowed for routine application of thermostability assays to systematically evaluate the stability of membrane protein preparations after various purification procedures. Test conditions can include different lipid cocktails, lipid-detergent micelles, pH, salts, osmolytes, and potential active-site ligands. Identification and use of conditions that stabilize the structure have proven successful in enabling the structure determination of numerous families of membrane proteins that otherwise were intractable.
机译:本单元介绍了快速且普遍适用的方法,这些方法可使用基于温度的变性测量值作为目标时间依赖性稳定性的代用品来鉴定稳定膜蛋白的条件。对蛋白质解折叠后对半胱氨酸残基的暴露敏感的硫醇反应性染料的最新发展已允许常规应用热稳定性测定法,以系统地评估各种纯化程序后膜蛋白制品的稳定性。测试条件可以包括不同的脂质混合物,脂质洗涤剂胶束,pH,盐,渗透液和潜在的活性部位配体。稳定结构的条件的鉴定和使用已被证明能够成功确定许多原本难以处理的膜蛋白家族的结构。

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