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在比色和荧光酶免疫分析中,常用的标记酶辣根过氧化物酶、碱性磷酸酶或β-半乳糖苷酶,哪种能产生最佳结果?

Which of the commonly used marker enzymes gives the best results in colorimetric and fluorimetric enzyme immunoassays: horseradish peroxidase, alkaline phosphatase or beta-galactosidase?

作者信息

Porstmann B, Porstmann T, Nugel E, Evers U

出版信息

J Immunol Methods. 1985 May 10;79(1):27-37. doi: 10.1016/0022-1759(85)90388-6.

Abstract

Comparing the marker enzymes horseradish peroxidase (HRP), alkaline phosphatase (AP) and beta-galactosidase (beta Gal) in IgG-coupled form with respect to their temperature-dependent kinetics over a period of 22 h the temperature of 37 degrees C warrants highest substrate turnover for all enzymes at all reaction times using fluorogens. Also applying chromogens the optimum temperature for beta Gal is 37 degrees C and depends for HRP and AP on the reaction time. The substrate turnover of HRP using ABTS as chromogen is much higher compared to the other enzymes--both related to mol enzyme (molar activity) and to gram enzyme (specific activity). The turnover decreases for all enzymes in different degrees after coupling to IgG. The turnover of fluorogenic substrates is lower for all enzymes than the turnover of chromogenic substrates but due to the more sensitive detection of fluorogenic products the detection limits for all conjugates were lowered too--especially for beta Gal-IgG by a factor of 333 compared to the colorimetric procedure. In a 2-site binding enzyme immunoassay for alpha-1-fetoprotein (AFP) the detection limit for AFP was reduced by a factor of 2 only by the fluorimetry compared to the colorimetry with all 3 marker enzymes. The HRP-IgG conjugates warranted lowest detection limits for AFP (0.5-1 microgram/1), highest analytical sensitivity (slope of standard curves) at shortest periods of substrate reaction compared to the other enzymes.

摘要

比较辣根过氧化物酶(HRP)、碱性磷酸酶(AP)和β-半乳糖苷酶(βGal)以IgG偶联形式在22小时内的温度依赖性动力学,对于所有酶在所有反应时间使用荧光底物时,37℃的温度保证了最高的底物周转率。使用色原底物时,βGal的最佳温度为37℃,而HRP和AP的最佳温度则取决于反应时间。与其他酶相比,使用ABTS作为色原底物时HRP的底物周转率要高得多——无论是与摩尔酶(摩尔活性)还是与克酶(比活性)相关。与IgG偶联后,所有酶的周转率都有不同程度的下降。所有酶的荧光底物周转率都低于色原底物周转率,但由于荧光产物的检测更灵敏,所有偶联物的检测限也降低了——尤其是βGal-IgG与比色法相比降低了333倍。在α-1-甲胎蛋白(AFP)的双位点结合酶免疫测定中,与比色法相比,使用所有三种标记酶时,荧光法仅将AFP的检测限降低了2倍。与其他酶相比,HRP-IgG偶联物保证了AFP的最低检测限(0.5 - 1微克/升),在最短的底物反应时间内具有最高的分析灵敏度(标准曲线斜率)。

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