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通过激光诱导荧光毛细管电泳检测受损DNA中的标记无碱基位点。

Detection of labeled abasic sites in damaged DNA by capillary electrophoresis with laser-induced fluorescence.

作者信息

Fundador Erwin, Rusling James

机构信息

Department of Chemistry, University of Connecticut, Storrs, CT 06269-3060, USA.

出版信息

Anal Bioanal Chem. 2007 Mar;387(5):1883-90. doi: 10.1007/s00216-006-1041-x. Epub 2007 Jan 6.

Abstract

Removal of nucleobases from the DNA backbone leads to the formation of abasic sites. The rate of abasic site formation is significantly increased for chemically damaged nucleobases. Thus, abasic sites serve as general biomarkers for the quantification of DNA damage. Herein, we show that capillary electrophoresis with laser-induced fluorescence (CE-LIF) can be used to detect the amount of abasic sites with very high sensitivity. For proof of concept, DNA was incubated with methylmethane sulfonate (MMS) and the damaged bases were removed by incubation at 80 degrees C. The resulting abasic sites were then tagged with a fluorescent aldehyde-reactive probe (FARP). The DNA was precipitated with ethanol, and then analyzed by CE-LIF. CE-LIF and HPLC analysis shows that the fluorescently tagged DNA (DNA-FARP) had a peak area directly proportional to the amount of N-7 methyl guanines. The CE-LIF method had a detection limit of 1.2 abasic sites per 1,000,000 bases or ca. 20 attomoles of abasic sites. This provides a general method for detecting DNA damage that is not only faster but also has comparable or better sensitivity than the alternative ELISA-like method.

摘要

从DNA主链上去除核碱基会导致无碱基位点的形成。对于化学损伤的核碱基,无碱基位点的形成速率会显著增加。因此,无碱基位点可作为定量DNA损伤的通用生物标志物。在此,我们表明激光诱导荧光毛细管电泳(CE-LIF)可用于以非常高的灵敏度检测无碱基位点的数量。为了验证概念,将DNA与甲基磺酸甲酯(MMS)孵育,并在80摄氏度下孵育以去除受损碱基。然后用荧光醛反应探针(FARP)标记产生的无碱基位点。用乙醇沉淀DNA,然后通过CE-LIF进行分析。CE-LIF和HPLC分析表明,荧光标记的DNA(DNA-FARP)的峰面积与N-7甲基鸟嘌呤的量成正比。CE-LIF方法的检测限为每1,000,000个碱基1.2个无碱基位点,或约20阿托摩尔的无碱基位点。这提供了一种检测DNA损伤的通用方法,该方法不仅更快,而且与类似ELISA的替代方法相比具有相当或更好的灵敏度。

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