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Simultaneous assembly of two target proteins using split inteins for live cell imaging

机译:使用分裂内含子同时组装两个靶蛋白,用于活细胞成像

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摘要

Inteins are protein elements that covalently reassemble proteins from two precursor fragments in a process known as protein splicing. They are commonly used to reassemble a single target protein by protein splicing, but a second target protein can potentially reassemble by intein dimerization. Here, we use the naturally occurring split DnaE intein from Nostoc punctiforme (NpuDnaE) to demonstrate the simultaneous assembly of two target proteins in several examples studied with live cell imaging: yellow fluorescent protein (YFP) with monomeric red fluorescent protein (mRFP), dominant positive mutant of RhoA GTPase with YFP and GCaMP2 Ca2+ indicator with mRFP. These examples showed the versatility of the strategy along with some interesting attributes: first, the two target proteins are in equal stoichiometry; second, the extent of protein splicing can be reported by a fluorescent protein. In particular, the split GCaMP2 with mRFP could find applications in tissue-specific Ca2+ imaging in transgenic organisms, where mRFP could control for motion-related intensity changes.
机译:内含肽是在称为蛋白质剪接的过程中从两个前体片段共价重组蛋白质的蛋白质元素。它们通常用于通过蛋白剪接重组单个靶蛋白,但是第二个靶蛋白可能通过内含肽二聚化重组。在这里,我们使用点状鼻菜的天然存在的DnaE内含子(NpuDnaE)来演示在活细胞成像研究的几个示例中两个靶蛋白的同时组装:黄色荧光蛋白(YFP)与单体红色荧光蛋白(mRFP),显性YFP的RhoA GTPase阳性突变体和mRFP的GCaMP2 Ca2 +指示剂。这些例子显示了该策略的多功能性以及一些有趣的属性:首先,两个靶蛋白的化学计量相等;第二,蛋白的剪接程度可以通过荧光蛋白来报告。尤其是,将带有mRFP的GCaMP2拆分物可以在转基因生物的组织特异性Ca2 +成像中找到应用,其中mRFP可以控制运动相关的强度变化。

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