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原位评估微生物中的DNA片段化。

DNA fragmentation in microorganisms assessed in situ.

作者信息

Fernández José Luis, Cartelle Mónica, Muriel Lourdes, Santiso Rebeca, Tamayo María, Goyanes Vicente, Gosálvez Jaime, Bou Germán

机构信息

INIBIC-Genética, Complejo Hospitalario Universitario Juan Canalejo, As Xubias 84, 15006-A Coruña, Spain.

出版信息

Appl Environ Microbiol. 2008 Oct;74(19):5925-33. doi: 10.1128/AEM.00318-08. Epub 2008 Aug 8.

Abstract

Chromosomal DNA fragmentation may be a direct or indirect outcome of cell death. Unlike DNA fragmentation in higher eukaryotic cells, DNA fragmentation in microorganisms is rarely studied. We report an adaptation of a diffusion-based assay, developed as a kit, which allows for simple and rapid discrimination of bacteria with fragmented DNA. Intact cells were embedded in an agarose microgel on a slide, incubated in a lysis buffer to partially remove the cell walls, membranes, and proteins, and then stained with a DNA fluorochrome, SYBR Gold. Identifying cells with fragmented DNA uses peripheral diffusion of DNA fragments. Cells without DNA fragmentation show only limited spreading of DNA fiber loops. These results have been seen in several gram-negative and gram-positive bacteria, as well as in yeasts. Detection of DNA fragmentation was confirmed by fluoroquinolone treatment and by DNA breakage detection-fluorescence in situ hybridization. Proteus mirabilis with spontaneously fragmented DNA during exponential and stationary growth or Escherichia coli with DNA damaged after exposure to hydrogen peroxide or antibiotics, such as ciprofloxacin or ampicillin, was clearly detected. Similarly, fragmented DNA was detected in Saccharomyces cerevisiae after amphotericin B treatment. Our assay may be useful for the simple and rapid evaluation of DNA damage and repair as well as cell death, either spontaneous or induced by exogenous stimuli, including antimicrobial agents or environmental conditions.

摘要

染色体DNA片段化可能是细胞死亡的直接或间接结果。与高等真核细胞中的DNA片段化不同,微生物中的DNA片段化很少被研究。我们报告了一种基于扩散的检测方法的改进,该方法已开发成试剂盒,可用于简单快速地区分具有DNA片段化的细菌。完整细胞被包埋在载玻片上的琼脂糖微凝胶中,在裂解缓冲液中孵育以部分去除细胞壁、细胞膜和蛋白质,然后用DNA荧光染料SYBR Gold染色。识别具有DNA片段化的细胞利用DNA片段的外周扩散。没有DNA片段化的细胞仅显示DNA纤维环的有限扩散。在几种革兰氏阴性菌和革兰氏阳性菌以及酵母中都观察到了这些结果。通过氟喹诺酮处理和DNA断裂检测-荧光原位杂交证实了DNA片段化的检测。在指数生长期和稳定期自发出现DNA片段化的奇异变形杆菌,或在暴露于过氧化氢或抗生素(如环丙沙星或氨苄青霉素)后DNA受损的大肠杆菌,都能被清楚地检测到。同样,在两性霉素B处理后的酿酒酵母中也检测到了片段化的DNA。我们的检测方法可能有助于简单快速地评估DNA损伤与修复以及细胞死亡,无论是自发的还是由包括抗菌剂或环境条件在内的外源性刺激诱导的。

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