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用于检测血浆、血清和尿液中普鲁卡因胺和N - 乙酰普鲁卡因胺的更灵敏的酶倍增免疫分析技术。

More-sensitive enzyme-multiplied immunoassay technique for procainamide and N-acetylprocainamide in plasma, serum, and urine.

作者信息

Henry P R, Dhruv R A

机构信息

Squibb Institute for Medical Research, New Brunswick, NJ 08903.

出版信息

Clin Chem. 1988 May;34(5):957-60.

PMID:2453309
Abstract

A commercially available (Syva Co.) enzyme-multiplied immunoassay technique (EMIT) for the quantitative determination of procainamide (PA) and N-acetylprocainamide (NAPA) was modified to allow automated quantitative analysis of approximately 100 samples per day, in a working range of 0.1 to 2.0 micrograms/mL. Such a test was needed to evaluate the pharmacokinetic characteristics of controlled-release dosage forms characterized by long half-lives at low plasma concentration. Analytical recovery of PA and NAPA from serum, plasma, and urine was satisfactory, but at extreme ratios for PA:NAPA the accuracy of determining the lower-concentration component became unsatisfactory. In fact, however, we found no such ratios in 5400 clinical samples assayed by this procedure.

摘要

一种市售的(Syva公司)用于定量测定普鲁卡因胺(PA)和N-乙酰普鲁卡因胺(NAPA)的酶放大免疫分析技术(EMIT)经过改进,可实现每天约100个样品的自动定量分析,工作范围为0.1至2.0微克/毫升。需要这样一种检测来评估控释剂型的药代动力学特征,其特点是在低血浆浓度下具有长半衰期。PA和NAPA从血清、血浆和尿液中的分析回收率令人满意,但在PA:NAPA的极端比例下,测定低浓度成分的准确性变得不尽人意。然而,实际上,我们在用此方法检测的5400份临床样品中未发现这样的比例。

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