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血浆中血栓素B2的放射免疫测定:方法学改进

Radioimmunoassay of thromboxane B2 in plasma: methodological modifications.

作者信息

Rogasi P G, Paniccia R, Coppo M, Prisco D, Boddi M, Chen J, Gensini G F, Abbate R

机构信息

Clinica Medica I, University of Florence, Italy.

出版信息

Thromb Res. 1988 Sep 1;51(5):533-41. doi: 10.1016/0049-3848(88)90118-1.

Abstract

Thromboxane B2 (TxB2) determination is usually performed by using commercial 3H-RIA kits. However, the low amounts of TxB2 present in plasma are not detectable without previous extraction. The aim of this study is the evaluation of 1) plasma protein interferences on the binding and separation steps of bound from free analyte and 2) charcoal efficacy in different experimental conditions. Our results indicate that plasma proteins do not influence the antibody binding, but significantly reduce the efficacy of precipitation of kit dextran-charcoal, so that the supernate radioactivity rises with the protein amount increase (r = 0.99 p less than 0.001). Such greater number of counts in the samples determines a lower estimation of TxB2 concentration in plasma when the calibration curve is set up in buffer. Our findings suggest that, in order to measure low amounts of plasma TxB2 without extraction, it is useful: 1) to refer to a calibration curve set up in buffer-diluted plasma, 2) to use the uncoated charcoal concentration allowing the lowest stripping and 3) to perform all steps at 4 degrees C.

摘要

血栓素B2(TxB2)的测定通常使用商用3H-RIA试剂盒进行。然而,血浆中存在的少量TxB2在未经预先提取的情况下是无法检测到的。本研究的目的是评估1)血浆蛋白对结合与游离分析物分离步骤的干扰,以及2)不同实验条件下活性炭的效能。我们的结果表明,血浆蛋白不影响抗体结合,但会显著降低试剂盒葡聚糖-活性炭沉淀的效能,从而使上清液放射性随蛋白量增加而升高(r = 0.99,p小于0.001)。当在校准曲线在缓冲液中建立时,样品中如此大量的计数会导致血浆中TxB2浓度的估计值较低。我们的研究结果表明,为了在不进行提取的情况下测量少量血浆TxB2,以下方法是有用的:1)参考在缓冲液稀释血浆中建立的校准曲线,2)使用能实现最低洗脱的未包被活性炭浓度,以及3)在4℃下进行所有步骤。

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