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C-reactive protein (CRP) aptamer binds to monomeric but not pentameric form of CRP

机译:C反应蛋白(CRP)适体结合单体但不是五聚体形式的CRP

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摘要

Native C-reactive protein (CRP) is composed of five identical subunits arranged in a pentameric structure (pCRP). Binding of pCRP to damaged cell membranes produces a second isoform, modified CRP, which has similar antigenicity to isolated monomeric subunits of CRP (mCRP). Emerging evidence indicates that modified CRP plays a role in inflammation and atherosclerosis, however, there are very few techniques that can distinguish the different isoforms of CRP. Here we show that an RNA aptamer binds specifically to mCRP and not to pCRP. Using this aptamer, we describe a simple, fast, and sensitive assay to detect nanomolar concentrations of mCRP using fluorescence anisotropy. In addition, we show that this aptamer can be used to detect mCRP in polyacrylamide gels and bound to a surface using total internal reflection fluorescence microscopy. The biological activity of the mCRP we prepared by heating pCRP with 0.1% sodium dodecyl sulfate was confirmed by observing binding to the complement protein, C1q. This probe provides an important tool for CRP research and has the potential to improve clinical diagnostics that predict risk for cardiovascular disease. [Figure not available: see fulltext.]
机译:天然C反应蛋白(CRP)由以五聚体结构(pCRP)排列的五个相同亚基组成。 pCRP与受损细胞膜的结合产生了第二种亚型,即修饰的CRP,它具有与CRP(mCRP)分离的单体亚基相似的抗原性。越来越多的证据表明,修饰的CRP在炎症和动脉粥样硬化中起作用,但是,几乎没有什么技术可以区分CRP的不同亚型。在这里,我们显示RNA适体特异性结合mCRP,而不结合pCRP。使用这种适体,我们描述了一种简单,快速,灵敏的测定方法,可使用荧光各向异性检测纳摩尔浓度的mCRP。此外,我们表明,这种适体可用于检测聚丙烯酰胺凝胶中的mCRP,并使用全内反射荧光显微镜结合到表面。通过观察与补体蛋白C1q的结合,证实了我们通过将pCRP与0.1%十二烷基硫酸钠加热制备的mCRP的生物活性。该探针为CRP研究提供了重要工具,并具有改善可预测心血管疾病风险的临床诊断的潜力。 [图不可用:请参见全文。]

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