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Multiplex bead array assays: performance evaluation and comparison of sensitivity to ELISA.

机译:多重珠阵列测定:性能评估和对ELISA敏感性的比较。

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摘要

The measurement of soluble cytokines and other analytes in serum and plasma is becoming increasingly important in the study and management of many diseases. As a result, there is a growing demand for rapid, precise, and cost-effective measurement of such analytes in both clinical and research laboratories. Multiplex bead array assays provide quantitative measurement of large numbers of analytes using an automated 96-well plate format. Enzyme-linked immunosorbent assay (ELISAs) have long been the standard for quantitative analysis of cytokines and other biomarkers, but are not well suited for high throughput multiplex analyses. However, prior to replacement of ELISA assays with multiplex bead array assays, there is a need to know how comparable these two methods are for quantitative analyses. A number of published studies have compared these two methods and it is apparent that certain elements of these assays, such as the clones of monoclonal antibodies used for detection and reporting, are pivotal in obtaining similar results from both assays. By careful consideration of these variables, it should be possible to utilize multiplex bead array assays in lieu of ELISAs for studies requiring high throughput analysis of numerous analytes.
机译:在许多疾病的研究和管理中,血清和血浆中可溶性细胞因子和其他分析物的测量变得越来越重要。结果,在临床和研究实验室中,对这种分析物的快速,精确和经济有效的测量的需求不断增长。多重珠阵列测定法使用自动96孔板形式对大量分析物进行定量测量。长期以来,酶联免疫吸附测定(ELISA)是细胞因子和其他生物标记物定量分析的标准,但不适用于高通量多重分析。然而,在用多重磁珠阵列测定法代替ELISA测定法之前,需要知道这两种方法在定量分析中的可比性。许多已发表的研究已经比较了这两种方法,很明显,这些测定的某些元素,例如用于检测和报告的单克隆抗体的克隆,对于从两种测定中获得相似的结果至关重要。通过仔细考虑这些变量,应该有可能使用多重磁珠阵列测定法代替ELISA用于需要对多种分析物进行高通量分析的研究。

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