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首页> 外文期刊>Plant molecular biology reporter >A Rapid and Sensitive Fuiorimetric Protocol for the Quantification of Green Fluorescent Protein in Soluble Protein Extracts from Transgenic Ambidopsis
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A Rapid and Sensitive Fuiorimetric Protocol for the Quantification of Green Fluorescent Protein in Soluble Protein Extracts from Transgenic Ambidopsis

机译:快速灵敏的荧光定量定量协议,用于定量分析来自转基因两栖动物的可溶性蛋白提取物中的绿色荧光蛋白

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摘要

Green fluorescent protein (GFP) is a popular qualitative reporter protein used to study different aspects of plant biology. However, to be used as a reliable quantitative reporter in expression studies using fluorescence based assays, methods to eliminate interfering endogenous molecules must be considered. Therefore, a standard curve based solid phase fluorescent immunoassay that eliminates the effects of interfering endogenous molecules was developed to quantify the GFP levels in soluble green extracts prepared from plants. Microtiter plates coated with anti-GFP were used to capture GFP from soluble plant extracts, interfering endogenous molecules was eliminated by washing without disturbing the anti-GFP binding of GFP, and then the fluorescence intensity of bound GFP was measured using a spectrofluorometer. We report in this study the use of this method to quantify the expression levels of soluble modified GFP in transgenic Arabidopsis thaliana.
机译:绿色荧光蛋白(GFP)是一种流行的定性报道蛋白,用于研究植物生物学的各个方面。但是,要在基于荧光的测定法的表达研究中用作可靠的定量报告基因,必须考虑消除干扰内源性分子的方法。因此,开发了消除干扰内源性分子影响的基于标准曲线的固相荧光免疫测定法,以定量从植物制备的可溶性绿色提取物中的GFP水平。使用涂有抗GFP的微量滴定板从可溶性植物提取物中捕获GFP,在不干扰GFP的抗GFP结合的情况下通过洗涤除去干扰的内源分子,然后使用分光荧光计测量结合的GFP的荧光强度。我们在这项研究中报告了这种方法的使用,以量化转基因拟南芥中可溶性修饰的GFP的表达水平。

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