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使用液相色谱-串联质谱法对感染小鼠组织中的铜绿假单胞菌烷基喹诺酮信号分子进行生物分析;及其在MvfR抑制药效学评价中的应用。

Bioanalysis of Pseudomonas aeruginosa alkyl quinolone signalling molecules in infected mouse tissue using LC-MS/MS; and its application to a pharmacodynamic evaluation of MvfR inhibition.

作者信息

Turnpenny Paul, Padfield Anthony, Barton Patrick, Teague Joanne, Rahme Laurence G, Pucci Michael J, Zahler Robert, Rubio Aileen

机构信息

Evotec, Drug Metabolism and Pharmacokinetics Department, Abingdon, Oxon, United Kingdom.

Evotec, Drug Metabolism and Pharmacokinetics Department, Abingdon, Oxon, United Kingdom.

出版信息

J Pharm Biomed Anal. 2017 May 30;139:44-53. doi: 10.1016/j.jpba.2017.02.034. Epub 2017 Feb 28.

DOI:10.1016/j.jpba.2017.02.034
PMID:28273650
Abstract

Alkyl quinolone molecules 2-heptyl-4-quinolone (HHQ) and 2-heptyl-3-hydroxy-4(1H)-quinolone (PQS) are important quorum sensing signals, which play a mediatory role in the pathogenesis of acute and chronic Pseudomonas aeruginosa infection. A targeted approach inhibiting the bacterial 'multiple virulence factor regulon' (MvfR) protein complex, offers the possibility to block the synthesis of MvfR-dependant signal molecules. Here, a high throughput bioanalytical method was developed using LC-MS/MS detection for the selective determination of HHQ and PQS in mouse tissue homogenate, over a sensitive range of 1-5000 and 10-5000pg/mL, respectively. Chromatographic peak distortion of the iron chelator PQS was overcome with the applied use of a bidentate chelator mobile phase additive 2-Picolinic acid at 0.2mM concentration, giving an improved separation and response for the analyte, whilst maintaining overall MS system robustness. Following thigh infection with P. aeruginosa strain 2-PA14 in mice, the concentration and time course of HHQ and PQS (4-hydroxy-2-alkyl-quinolone (HAQ) biomarkers) residing in the biophase were evaluated, and exhibited a low level combined with a substantial inter-individual variability. Quantifiable levels could be obtained from approximately 15h post infection, to the study termination at 21-22h. A dose dependant reduction in HAQ tissue concentrations at selected time points were obtained following MvfR inhibitor administration versus drug vehicle (p<0.01, Kruskal-Wallis-one way ANOVA) and meta -analyses of several studies enabled an inhibitory concentration (IC) of 80nM free drug to be determined. However, due to the experimental limitations a defined time profile for in-vivo HAQ production could not be characterised. Microsomal stability measurements demonstrated a rapid metabolic clearance of both alkyl quinolone biomarkers in the bacterial host, with a hepatic extraction ratio greater than 0.96 (the measurable assay limit). High clearance underpinned the low concentrations present in the well-perfused thigh tissue. Along with method development and validation details, this paper considers the kinetics of in-vivo HAQ bio-synthesis during Pseudomonas infection; and risks of biomarker over-estimation from samples which contain an exogenous population of bacteria.

摘要

烷基喹诺酮分子2-庚基-4-喹诺酮(HHQ)和2-庚基-3-羟基-4(1H)-喹诺酮(PQS)是重要的群体感应信号,在急性和慢性铜绿假单胞菌感染的发病机制中起介导作用。一种靶向抑制细菌“多毒力因子调节子”(MvfR)蛋白复合物的方法,为阻断MvfR依赖性信号分子的合成提供了可能性。在此,开发了一种高通量生物分析方法,使用LC-MS/MS检测在小鼠组织匀浆中选择性测定HHQ和PQS,其灵敏范围分别为1-5000和10-5000 pg/mL。通过使用浓度为0.2 mM的双齿螯合剂流动相添加剂2-吡啶甲酸,克服了铁螯合剂PQS的色谱峰变形问题,改善了分析物的分离和响应,同时保持了整个质谱系统的稳健性。在用铜绿假单胞菌菌株2-PA14感染小鼠大腿后,评估了生物相中HHQ和PQS(4-羟基-2-烷基喹诺酮(HAQ)生物标志物)的浓度和时间进程,结果显示其水平较低且个体间差异较大。从感染后约15小时到21-22小时研究结束,均可获得可量化的水平。与药物载体相比,给予MvfR抑制剂后,在选定时间点HAQ组织浓度呈剂量依赖性降低(p<0.01,Kruskal-Wallis单因素方差分析),对多项研究的荟萃分析确定了游离药物的抑制浓度(IC)为80 nM。然而,由于实验限制,无法确定体内HAQ产生的明确时间分布。微粒体稳定性测量表明,在细菌宿主中,两种烷基喹诺酮生物标志物均有快速的代谢清除,肝脏提取率大于0.96(可测量的分析极限)。高清除率是灌注良好的大腿组织中低浓度存在的原因。除了方法开发和验证细节外,本文还考虑了铜绿假单胞菌感染期间体内HAQ生物合成的动力学;以及含有外源细菌群体的样本中生物标志物高估的风险。

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