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采用毛细管电泳-激光诱导荧光偏振检测法的环孢素竞争性免疫测定

Competitive immunoassay for cyclosporine using capillary electrophoresis with laser induced fluorescence polarization detection.

作者信息

Ye L, Le X C, Xing J Z, Ma M, Yatscoff R

机构信息

Department of Public Health Sciences, Faculty of Medicine and Oral Health Sciences, University of Alberta, Edmonton, Canada.

出版信息

J Chromatogr B Biomed Sci Appl. 1998 Aug 28;714(1):59-67. doi: 10.1016/s0378-4347(98)00091-7.

Abstract

Frequent monitoring of immunosuppressive drug cyclosporine A (CsA) in blood samples of tissue transplant patients is required in clinical practice because of the narrow therapeutic range between the immunosuppressive effect and the toxic effect of this drug. We describe a competitive immunoassay capillary electrophoresis (CE) with laser induced fluorescence polarization detection method, which is rapid and sensitive for the determination of CsA. The method is based on the competitive immunochemical reaction between the analyte and fluorescent hapten (CsA*) with the antibody, CE separation of the antibody bound and free fluorescent CsA*, followed by the laser induced fluorescence polarization detection (LIFP) of the fluorescent species. The method detection limit is governed by the stability of the antibody-CsA* complex rather than by the detector noise. The use of post-column sheath flow cuvette LIFP detection resulted in excellent detection limit, typically 0.9 nM (or 9.10(-19) mol for 1 nl injection) of CsA. CsA in whole blood samples from organ transplant patients were measured and results agreed well with those obtained by using a standard fluorescence polarization immunoassay. Each determination took less than 3 min. The CsA metabolites AM9 and AM19 were also determined by using this technique, and their cross-reactivities with the antibody were 13% and 2%, respectively.

摘要

由于组织移植患者血液样本中免疫抑制药物环孢素A(CsA)的免疫抑制作用和毒性作用之间的治疗范围狭窄,临床实践中需要对其进行频繁监测。我们描述了一种采用激光诱导荧光偏振检测的竞争性免疫分析毛细管电泳(CE)方法,该方法对CsA的测定快速且灵敏。该方法基于分析物与荧光半抗原(CsA*)与抗体之间的竞争性免疫化学反应,通过CE分离结合抗体的和游离的荧光CsA*,然后对荧光物质进行激光诱导荧光偏振检测(LIFP)。该方法的检测限取决于抗体 - CsA*复合物的稳定性,而非检测器噪声。采用柱后鞘流比色皿LIFP检测具有出色的检测限,通常CsA的检测限为0.9 nM(对于1 nl进样量相当于9.1×10⁻¹⁹ mol)。对器官移植患者全血样本中的CsA进行了测定,结果与使用标准荧光偏振免疫分析获得的结果吻合良好。每次测定耗时不到3分钟。还使用该技术测定了CsA代谢物AM9和AM19,它们与抗体的交叉反应率分别为13%和2%。

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