Bosin E, Monji N
Anal Biochem. 1983 Sep;133(2):283-7. doi: 10.1016/0003-2697(83)90084-2.
An enzyme-linked immunosorbent technique for human serum retinol-binding protein (RBP) was developed. The assay detects RBP via a double-antibody (rabbit anti-human RBP) sandwich technique. The antibody is immobilized by passive adsorption to a polystyrene tube; the assay is then carried out by successive additions containing known and unknown amounts of RBP (antigen), alkaline phosphatase linked to the same antibody, and p-nitrophenyl phosphate (substrate). Colorimetric analysis of the hydrolysis of the substrate by the enzyme (indirectly) attached to the antigen is used for RBP quantitation. The intra- and interassay coefficients of variation ranged between 4 and 7 and 9 and 12%, respectively. The assay can be performed in less than 7 h and has a sensitivity in the nanogram range (3-48 ng/ml). RBP content was analyzed in serum and urine samples of 20 healthy donors and 17 patients with renal failure and in 20 serum specimens of patients with liver cirrhosis. Renal patients had higher serum (mean 150, range 50-398 micrograms/ml) and urine RBP levels (mean 14, range 1-80 micrograms/ml) than normal donors (mean serum 43, range 30-60 micrograms/ml; mean urine RBP 0.06, range 0.04-0.13 microgram/ml). Liver disease patients had lower than normal serum RBP values (mean 22, range 10-43 micrograms/ml).
开发了一种用于检测人血清视黄醇结合蛋白(RBP)的酶联免疫吸附技术。该检测方法通过双抗体(兔抗人RBP)夹心技术检测RBP。抗体通过被动吸附固定在聚苯乙烯管上;然后依次加入已知和未知量的RBP(抗原)、与同一种抗体连接的碱性磷酸酶和对硝基苯磷酸(底物)来进行检测。通过与抗原相连的酶(间接)对底物水解的比色分析来定量RBP。批内和批间变异系数分别在4%至7%和9%至12%之间。该检测可在不到7小时内完成,灵敏度在纳克范围内(3 - 48纳克/毫升)。对20名健康供体、17名肾衰竭患者的血清和尿液样本以及20名肝硬化患者的血清标本进行了RBP含量分析。肾衰竭患者的血清(平均150,范围50 - 398微克/毫升)和尿液RBP水平(平均14,范围1 - 80微克/毫升)高于正常供体(血清平均43,范围30 - 60微克/毫升;尿液RBP平均0.06,范围0.04 - 0.13微克/毫升)。肝病患者的血清RBP值低于正常水平(平均22,范围10 - 43微克/毫升)。
