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A redox sensitivity-based method to quantify both pentameric and monomeric C-reactive protein in a single assay

机译:基于氧化还原的方法,以在单一测定中量化五聚体和单体C反应蛋白

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摘要

C-reactive protein (CRP) can exist in both pentameric (pCRP) and monomeric conformation (mCRP). Though serum pCRP is an established marker of inflammation, the diagnostic significance of mCRP remains unknown largely due to the lack of a reliable assay. The power and specificity of antibody-based assays are limited by the antibody reagents used and by the degree of cross-reactivity that may exist in detecting each antigen, as mCRP is known to be formed from the pentameric and both conformations usually coexist in clinical samples. Here, we describe an assay that measures both CRP conformations in simple samples in a single assay. This assay depends on the rationale that the intra-molecular disulfide bonds in pCRP resist reduction, while those in mCRP can be readily reduced. The distinct sensitivity of pCRP and mCRP to reduction can be easily detected and separated by electrophoresis. This assay may provide a means to study clinical correlation between pCRP and mCRP in clinical samples in the future and to evaluate their respective significance as disease markers.
机译:在五聚体(PCRP)和单体构象(MCRP)中可以存在C反应蛋白(CRP)。虽然血清PCRP是炎症的既定标志物,但由于缺乏可靠的测定,MCRP对MCRP的诊断意义仍然未知。基于抗体的测定的功率和特异性受到在检测每种抗原中可能存在的交叉反应性的抗体试剂的限制,因为已知MCRP是由五聚体形成的,并且两种构象通常在临床样品中共存。在这里,我们描述了一种测定在单一测定中的简单样品中测量CRP构象。该测定取决于PCRP抗蚀剂中的分子内二硫化键的基本原理,而MCRP中的那些可以容易地降低。通过电泳,可以容易地检测和分离PCRP和MCRP到还原的明显敏感性。该测定可以提供在未来临床样本中PCRP和MCRP之间研究PCRP和MCRP之间的临床相关性的手段,并评估它们作为疾病标志物的各自意义。

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