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蛋白质等电点的估计方法。

Method for estimation of protein isoelectric point.

机构信息

Laboratory of Biophysics and Medicity Research Laboratory, University of Turku, Tykistökatu 6A, FI-20520 Turku, Finland.

出版信息

Anal Chem. 2012 Oct 2;84(19):8253-8. doi: 10.1021/ac301569b. Epub 2012 Sep 18.

Abstract

Adsorption of sample protein to Eu(3+) chelate-labeled nanoparticles is the basis of the developed noncompetitive and homogeneous method for the estimation of the protein isoelectric point (pI). The lanthanide ion of the nanoparticle surface-conjugated Eu(3+) chelate is dissociated at a low pH, therefore decreasing the luminescence signal. A nanoparticle-adsorbed sample protein prevents the dissociation of the chelate, leading to a high luminescence signal. The adsorption efficiency of the sample protein is reduced above the isoelectric point due to the decreased electrostatic attraction between the negatively charged protein and the negatively charged particle. Four proteins with isoelectric points ranging from ~5 to 9 were tested to show the performance of the method. These pI values measured with the developed method were close to the theoretical and experimental literature values. The method is sensitive and requires a low analyte concentration of submilligrams per liter, which is nearly 10000 times lower than the concentration required for the traditional isoelectric focusing. Moreover, the method is significantly faster and simpler than the existing methods, as a ready-to-go assay was prepared for the microtiter plate format. This mix-and-measure concept is a highly attractive alternative for routine laboratory work.

摘要

样品蛋白吸附到 Eu(3+)螯合物标记的纳米颗粒上是开发非竞争均相方法估计蛋白质等电点(pI)的基础。纳米颗粒表面共轭 Eu(3+)螯合物中的镧系离子在低 pH 下解离,从而降低了发光信号。纳米颗粒吸附的样品蛋白阻止了螯合物的解离,导致发光信号高。由于带负电荷的蛋白质和带负电荷的颗粒之间的静电吸引力降低,在等电点以上,样品蛋白的吸附效率降低。用该方法测试了四种等电点从~5 到 9 的蛋白质,以显示该方法的性能。用开发的方法测量的这些 pI 值与理论和实验文献值接近。该方法灵敏,所需分析物浓度低至亚毫克/升,比传统等电聚焦所需的浓度低近 10000 倍。此外,与现有的方法相比,该方法显著更快更简单,因为已经为微孔板格式制备了即用型测定。这种混合和测量的概念是常规实验室工作的极具吸引力的替代方案。

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