首页> 外国专利> Spectrophotometric method for kinetic absorbance measurements in two- phase enzyme immunoassay and apparatus therefor

Spectrophotometric method for kinetic absorbance measurements in two- phase enzyme immunoassay and apparatus therefor

机译:分相光度法在两相酶免疫测定中的动力学吸收测定及其装置

摘要

A method is described for kinetic measurement of enzyme activity bound to a solid matrix which improves both the sensitivity and speed of one immunoassay method. The immunoassay typically consists of reaction of the analyte with two specific antibodies, one fixed to the surface of a polymeric bead or wall of a test tube, the other added in solution and labeled by covalent coupling to an enzyme. By reaction between analyte and both antibodies, the enzyme-labeled antibody becomes fixed to the surface in a quantity proportional to the quantity of the analyte. After washing sufficiently to remove unreacted enzyme-labeled antibody, fixed enzyme activity is measured by incubation with a substrate and measurement of the rate of the reaction catalyzed. Fixation of the enzyme causes the reaction products to be localized near the surface. To measure the concentration of reactant or product repeatedly during the reaction, the solution must be mixed before each measurement, which can interfere with the measurement. In the prior art, the reaction is stopped after incubation and the product measured once. The method and apparatus disclosed here provides stirring and measurement away from the surface, and thus permits repeated measurement during the reaction. This kinetic assay can be performed more rapidly and sensitively than assays based on a single measurement.
机译:描述了一种用于动力学测量结合到固体基质上的酶活性的方法,该方法提高了一种免疫测定方法的灵敏度和速度。免疫测定通常包括分析物与两种特异性抗体的反应,一种固定在聚合物珠或试管壁的表面,另一种固定在溶液中并通过与酶的共价偶联进行标记。通过分析物和两种抗体之间的反应,酶标记的抗体以与分析物的量成比例的量固定在表面上。充分洗涤以除去未反应的酶标记的抗体后,通过与底物孵育并测量催化的反应速率来测量固定的酶活性。酶的固定导致反应产物位于表面附近。为了在反应过程中重复测量反应物或产物的浓度,必须在每次测量之前将溶液混合,这会干扰测量。在现有技术中,温育后停止反应,并且仅测量产物一次。这里公开的方法和设备提供了远离表面的搅拌和测量,因此允许在反应期间重复测量。与基于单个测量的测定相比,该动力学测定可以更快,更灵敏地进行。

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