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使用单叠氮碘化丙啶结合定量PCR对消毒效果进行分子监测。

Molecular monitoring of disinfection efficacy using propidium monoazide in combination with quantitative PCR.

作者信息

Nocker Andreas, Sossa Katherine E, Camper Anne K

机构信息

Center for Biofilm Engineering, Montana State University, Bozeman, Montana 59717, USA.

出版信息

J Microbiol Methods. 2007 Aug;70(2):252-60. doi: 10.1016/j.mimet.2007.04.014. Epub 2007 May 1.

Abstract

One of the major drawbacks of DNA-based microbial diagnostics is its inability to discriminate between live and dead bacteria. Due to the persistence of DNA in the environment after cells have lost their viability, DNA-based assays cannot assess pathogenic risk since signals can originate from both live and dead cells. Presented here is a potential application of the novel chemical propidium monoazide (PMA), which results in the selective suppression of DNA detection from dead cells. PMA can only penetrate dead cells with permeabilized cell membranes. Upon intercalation into the DNA, covalent crosslinkage of PMA to DNA is achieved through light exposure. This modification prevents the DNA from being amplified by PCR. The method, in combination with quantitative PCR as a diagnostic tool, successfully monitored the disinfection efficacy of hypochlorite, benzalkonium and heat on several model pathogens. Threshold cycle numbers increased with increasing disinfection strength after PMA treatment of samples compared to non-PMA treated samples. With some disinfectant-specific differences, monitoring viability loss with membrane integrity as an indicator seemed to be more conservative than monitoring viability loss with plate counts. Loss of viability after short UV-exposure could not be monitored with PMA as UV light affects viability by inducing DNA damage without directly affecting membrane permeability.

摘要

基于DNA的微生物诊断的主要缺点之一是无法区分活细菌和死细菌。由于细胞失去活力后DNA仍会在环境中持续存在,基于DNA的检测方法无法评估致病风险,因为信号可能来自活细胞和死细胞。本文介绍了新型化学物质单叠氮丙锭(PMA)的一种潜在应用,它能选择性抑制对死细胞DNA的检测。PMA只能穿透细胞膜通透性增加的死细胞。插入DNA后,通过光照可实现PMA与DNA的共价交联。这种修饰可防止DNA通过聚合酶链式反应(PCR)进行扩增。该方法与作为诊断工具的定量PCR相结合,成功监测了次氯酸盐、苯扎氯铵和热对几种模式病原体的消毒效果。与未用PMA处理的样品相比,对样品进行PMA处理后,随着消毒强度的增加,阈值循环数增加。尽管存在一些消毒剂特异性差异,但以膜完整性为指标监测活力丧失似乎比以平板计数监测活力丧失更为保守。由于紫外线通过诱导DNA损伤影响活力而不直接影响膜通透性,因此PMA无法监测短时间紫外线照射后的活力丧失情况。

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