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Low False-Positives in an mLumin-Based Bimolecular Fluorescence Complementation System with a Bicistronic Expression Vector

机译:具有双顺反子表达载体的基于mLumin的双分子荧光互补系统中的低假阳性

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The simplicity and sensitivity of the bimolecular fluorescence complementation (BiFC) assay make it a powerful tool to investigate protein-protein interactions (PPIs) in living cells. However, non-specific association of the fluorescent protein fragments in a BiFC system can complicate evaluation of PPIs. Here, we introduced a bicistronic expression vector, pBudCE4.1, into an mLumin-based BiFC system, denoted as the BEVL-BiFC system. The BEVL-BiFC system achieved a 25-fold contrast in BiFC efficiency between positive (Fos/Jun) and negative (ΔFos/Jun) PPIs. The high BiFC efficiency was due to a low false-positive rate, where less than 2% of cells displayed BiFC in the negative control. K-Ras and its interactive proteins, Ras binding domain (RBD) of Raf-1 and Grb2 were used to confirm the accuracy of the BEVL-BiFC system. The results also provide direct evidence in individual cells that post-translational modification of K-Ras and its localization at the plasma membrane (PM) were not essential for the interaction of K-Ras and Raf-1, whereas the interaction of Grb2 and K-Ras did depend on the PM localization of K-Ras. Taken together, the BEVL-BiFC system was developed to reduce the false-positive phenomenon in BiFC assays, resulting in more robust and accurate measurement of PPIs in living cells.
机译:双分子荧光互补(BiFC)分析的简单性和灵敏度使其成为研究活细胞中蛋白质相互作用的强大工具。但是,BiFC系统中荧光蛋白片段的非特异性结合会使PPI的评估复杂化。在这里,我们将双顺反子表达载体pBudCE4.1引入了基于mLumin的BiFC系统,称为BEVL-BiFC系统。 BEVL-BiFC系统在正(Pos / Jun)和负(ΔFos/ Jun)PPI之间实现了25倍的BiFC效率对比。 BiFC的高效率归因于假阳性率低,在阴性对照中不到2%的细胞显示BiFC。使用K-Ras及其相互作用蛋白Raf-1和Grb2的Ras结合域(RBD)来确定BEVL-BiFC系统的准确性。该结果还提供了直接证据,证明单个细胞中K-Ras的翻译后修饰及其在质膜(PM)的定位对于K-Ras和Raf-1的相互作用不是必需的,而Grb2和K的相互作用-Ras确实取决于K-Ras的PM定位。总而言之,开发了BEVL-BiFC系统以减少BiFC分析中的假阳性现象,从而使活细胞中PPI的测量更加可靠和准确。

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