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大鼠和人血液中毒死蜱、毒死蜱氧磷及3,5,6-三氯-2-吡啶醇的测定

Determination of chlorpyrifos, chlorpyrifos oxon, and 3,5,6-trichloro-2-pyridinol in rat and human blood.

作者信息

Brzak K A, Harms D W, Bartels M J, Nolan R J

机构信息

Health and Environmental Research Laboratories, Dow Chemical Company, Midland, Michigan 48674, USA.

出版信息

J Anal Toxicol. 1998 May-Jun;22(3):203-10. doi: 10.1093/jat/22.3.203.

Abstract

Analytical methods to quantitate chlorpyrifos and two potential metabolites, chlorpyrifos oxon (oxon) and 3,5,6-trichloro-2-pyridinol (TCP), in human and rat blood are described. Chlorpyrifos and the oxon were extracted simultaneously with a methanol/hexane mixture from 0.5 mL blood that was deactivated with an acidic salt solution. The extract was then concentrated and analyzed by negative-ion chemical ionization gas chromatography-mass spectrometry (NCI-GC-MS). TCP was extracted from a separate 0.1-mL aliquot of blood, also deactivated by the addition of acid. The t-butyldimethylsilyl derivative of TCP was formed using MTBSTFA, and the analysis was performed by NCI-GC-MS. Stable isotope analogues of chlorpyrifos (-13C2-15N), oxon (-13C2-15N), and TCP (-13C2) were used as internal standards. Oxon was observed to partially degrade to TCP during the sample analysis. Accurate oxon and TCP measurements were obtained with the use of oxon-13C2-15N, TCP-13C2, and TCP-13C2-15N internal standards, which compensated for both the degradation of oxon and the formation of artifactual TCP during analysis. The limits of quantitation were 1 ng/mL blood for both chlorpyrifos and oxon and 10 ng/mL for TCP. Calibration curves were linear over the concentration range of 2.5-2500 ng/mL solvent for chlorpyrifos and oxon and between 5 and 1060 ng/mL solvent for TCP. Taking concentration factors and extraction efficiencies into account, these linear ranges represent blood concentrations of approximately 0.3-300 ng/mL blood for chlorpyrifos and the oxon and 6-1300 ng/mL blood for TCP. The lowest spike level for chlorpyrifos and the oxon was 1 ng/mL blood, and the lowest spike level for TCP was 10 ng/mL blood. Recoveries from rat blood were as follows: 106-119% for chlorpyrifos, 94-104% for oxon, and 85-102% for TCP. In addition, chlorpyrifos and oxon were incubated with rat and human blood for various time intervals before deactivation to determine precautions that needed to be taken when collecting and handling specimens. No change in chlorpyrifos concentration was observed in rat blood up to 180 min at 37 degrees C. In contrast, the oxon was rapidly hydrolyzed to TCP in both rat (t 1/2 approximately 10 s) and human (t 1/2 approximately 55 s) blood held at 37 degrees C. The hydrolysis rate for the oxon was independent of whether a rat had been administered chlorpyrifos previously, the initial oxon concentration, the presence of chlorpyrifos, and the age or gender of the human volunteers. These results suggest rapid sample preparation is critical for accurate determinations of the oxon metabolite of chlorpyrifos. These methods provide excellent tools for use in chlorpyrifos pharmacokinetic modeling studies.

摘要

本文描述了定量测定人血和大鼠血中毒死蜱及其两种潜在代谢物——毒死蜱氧磷(氧磷)和3,5,6 - 三氯 - 2 - 吡啶醇(TCP)的分析方法。毒死蜱和氧磷用甲醇/己烷混合物从0.5 mL用酸性盐溶液灭活的血液中同时萃取。提取物随后浓缩,并通过负离子化学电离气相色谱 - 质谱联用仪(NCI - GC - MS)进行分析。TCP从另一单独的0.1 mL血液等分试样中萃取,该试样同样通过添加酸进行灭活。使用MTBSTFA形成TCP的叔丁基二甲基甲硅烷基衍生物,并通过NCI - GC - MS进行分析。毒死蜱(-¹³C₂ - ¹⁵N)、氧磷(-¹³C₂ - ¹⁵N)和TCP(-¹³C₂)的稳定同位素类似物用作内标。在样品分析过程中观察到氧磷会部分降解为TCP。使用氧磷 - ¹³C₂ - ¹⁵N、TCP - ¹³C₂和TCP - ¹³C₂ - ¹⁵N内标可获得准确的氧磷和TCP测量值,这补偿了氧磷的降解以及分析过程中人为产生的TCP的形成。毒死蜱和氧磷的定量限均为1 ng/mL血液,TCP为10 ng/mL。毒死蜱和氧磷在2.5 - 2500 ng/mL溶剂浓度范围内校准曲线呈线性,TCP在5 - 1060 ng/mL溶剂浓度范围内校准曲线呈线性。考虑到浓缩因子和萃取效率,这些线性范围分别代表毒死蜱和氧磷在血液中的浓度约为0.3 - 300 ng/mL血液,TCP为6 - 1300 ng/mL血液。毒死蜱和氧磷的最低加标水平为1 ng/mL血液,TCP的最低加标水平为10 ng/mL血液。大鼠血液中的回收率如下:毒死蜱为106 - 119%,氧磷为94 - 104%,TCP为85 - 102%。此外,在灭活前将毒死蜱和氧磷与大鼠和人血在不同时间间隔下孵育,以确定采集和处理标本时所需采取的预防措施。在37℃下,大鼠血液中高达180分钟时未观察到毒死蜱浓度变化。相反,在37℃下,氧磷在大鼠(半衰期约10秒)和人(半衰期约55秒)血液中均迅速水解为TCP。氧磷的水解速率与大鼠之前是否施用毒死蜱、初始氧磷浓度、毒死蜱的存在以及人类志愿者的年龄或性别无关。这些结果表明,快速样品制备对于准确测定毒死蜱的氧磷代谢物至关重要。这些方法为毒死蜱药代动力学建模研究提供了出色的工具。

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