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Prion protein and developments in its detection.

机译:on病毒蛋白及其检测的发展。

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The theoretical risk of transmission of variant Creutzfeldt-Jakob disease (vCJD) via blood transfusions has led to replacement of UK-derived plasma for fractionation by plasma sourced outwith the UK and the introduction of leucodepletion of donated blood and its components. Prion protein in an abnormal conformation (PrPsc) has been identified as inextricably linked with the infectivity of transmissible spongiform encephalopathies such as vCJD and in this review some of its properties relevant to its detection are considered. In particular its insolubility in nonionic detergents and its partial resistance to proteinase K digestion have provided methods for separating it from the normal abundant isoform PrPc prior to subsequent detection, usually by means of antibody probes. As yet no antibodies which discriminate between the abnormal and normal isoforms have been identified with the sole exception of one which is not suitable for generally used immunodetection systems. Most detection systems, such as immunohistochemistry or Western blotting, have been optimized for brain or lympho-reticular tissues. Much less information is available for assays applied to blood or plasma, although some recent publications provide indications of their feasibility. However, a number of obstacles remain to be overcome. These include the issues of assay validation, detection of extremely low levels of PrPsc in the presence of large excesses of PrPc, lack of available standardized reagents, assay specificity and practicality for large-scale screening use. Progress towards these goals is reviewed.
机译:通过输血传播变异型克雅氏病(vCJD)的理论风险已导致英国来源的血浆替换为英国来源的血浆进行分级分离,并引入了捐献血液及其成分的全白血球清除术。 identified构蛋白的异常构象(PrPsc)已被确定与传染性海绵状脑病(如vCJD)的传染性密不可分,并且在本综述中考虑了一些与其检测有关的特性。特别地,其在非离子去污剂中的不溶性和对蛋白酶K消化的部分抗性提供了在随后的检测之前通常通过抗体探针将其与正常的丰富同工型PrPc分离的方法。迄今为止,除了一种不适合于通常使用的免疫检测系统的抗体外,还没有鉴定出能够区分异常同种型和正常同种型的抗体。大多数检测系统,例如免疫组织化学或蛋白质印迹,已针对脑或淋巴网状组织进行了优化。尽管适用于血液或血浆的测定方法的信息很少,但是最近的一些出版物提供了其可行性的迹象。但是,仍有许多障碍有待克服。这些问题包括分析验证,在大量过量的PrPc存在下检测极低水平的PrPsc,缺少可用的标准化试剂,分析特异性和大规模筛选用途的实用性等问题。审查了实现这些目标的进展。

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