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Toward development of a screen to identify randomly encoded, foldable sequences

机译:致力于开发屏幕以识别随机编码的可折叠序列

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The ability to identify sequences in a randomly encoded polypep-tide library that are capable of acquiring unique and stably folded structures would be valuable in the examination of protein-folding issues. The quality control system of the yeast secretory pathway prevents the release of incompletely folded polypeptides. Earlier work has shown that this feature can be used in a screen to identify mutations that increase the stability of a protein. We sought to extend this strategy for use with random sequence libraries by combining a quality-control system-based screen with generic tag-based immunodetection that can be applied to any sequence. To test this method, we screened a library encoding random mutations in a bovine pancreatic trypsin inhibitor variant containing a small generic tag. Initial on-plate screening resulted in a large number of false positives: sequences that were secreted but not foldable. These false positives were excluded successfully in additional screening steps that used a liquid-culture secretion screen and a gel electrophoresis assay. Three positive clones were obtained that showed midpoint thermal denaturation temperatures 10-16℃ higher than the original bovine pancreatic trypsin inhibitor variant. Thus, this multistep screening method may be useful for finding novel, foldable sequences.
机译:在随机编码的多肽文库中鉴定能够获得独特且稳定折叠的结构的序列的能力在检查蛋白质折叠问题中将是有价值的。酵母分泌途径的质量控制系统防止释放不完全折叠的多肽。早期的工作表明,可以在屏幕上使用此功能来识别可增加蛋白质稳定性的突变。我们试图通过将基于质量控制系统的筛选与可应用于任何序列的基于通用标签的免疫检测相结合,来扩展该策略以用于随机序列文库。为了测试此方法,我们筛选了一个编码带有小通用标签的牛胰胰蛋白酶抑制剂变异体中的随机突变的文库。最初的板上筛选导致大量的假阳性:被分泌但无法折叠的序列。这些假阳性在使用液体培养物分泌物筛选和凝胶电泳分析的其他筛选步骤中被成功排除。获得了三个阳性克隆,它们的中点热变性温度比原始的牛胰胰蛋白酶抑制剂变异体高10-16℃。因此,这种多步筛选方法可能对发现新颖的可折叠序列很有用。

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