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首页> 外文期刊>Journal of immunoassay >The optimisation of a murine TNF-alpha ELISA and the application of the method to other murine cytokines.
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The optimisation of a murine TNF-alpha ELISA and the application of the method to other murine cytokines.

机译:鼠TNF-αELISA的优化及其在其他鼠细胞因子中的应用。

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Cytokines occur in biological systems at low levels of concentration, therefore assays developed to measure them must be very sensitive. Enzyme linked immunosorbent assays (ELISA's) developed using manufacturers recommended end points can detect cytokines to picogram levels but the lower parts of their standard curves can be unreliable. In this study the relative merits of different substrate systems - 2,2'-azino-bis(3-ethylbenzthiazoline-6-sulfonic acid) (ABTS) and 2 forms of tetramethyl benzidine (TMB), were investigated with regard to assay sensitivity. Further, a signal amplification method involving biotinylated tyramine has been used to increase the absorbance signal and thus the assay sensitivity and to achieve a sigmoidal standard curve. The amplified assay approach has been applied successfully to achieve more sensitive detection of TNF-alpha and improve the sensitivity of assays for a wide range of other cytokines. The optimised amplification method is the same for all the cytokine ELISA's performed in this work and this enables them to be performed
机译:细胞因子以低水平的浓度出现在生物系统中,因此开发的用于测量细胞因子的测定必须非常敏感。使用制造商推荐的终点开发的酶联免疫吸附测定(ELISA),可以检测到皮克水平的细胞因子,但其标准曲线的下部可能不可靠。在这项研究中,研究了不同底物系统-2,2'-叠氮基双(3-乙基苯并噻唑啉-6-磺酸)(ABTS)和2种形式的四甲基联苯胺(TMB)的相对优点,以提高测定灵敏度。此外,已经使用涉及生物素化酪胺的信号放大方法来增加吸光度信号,从而增加测定灵敏度并获得S形标准曲线。放大的测定方法已成功应用,以实现对TNF-α的更灵敏检测,并提高了对多种其他细胞因子的测定灵敏度。对于这项工作中进行的所有细胞因子ELISA,优化的扩增方法都是相同的,这使它们能够进行

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