Kaiting Xiao , Yanming Lai , Xingxing Liu, Shengjie Li, Wenxu Yuan, Ziyun Wang, Pan Pan, Yongkui Li, Heng Xiao
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Consequently, there is an urgent need for a portable, user-friendly 8-oxoguanine DNA glycosylase assay that offers swift results and supports real-time testing.</p></div><div><h3>Results</h3><p>We've developed a PERFUME method that combines <strong>p</strong>rimer <strong>e</strong>xchange <strong>r</strong>eaction and <strong>f</strong>unctionalized G-q<strong>u</strong>adruplex/he<strong>m</strong>in DNAzym<strong>e</strong> for sensitive detection of Fpg, a typical 8-oxoguanine DNA glycosylase. Utilizing a single probe and T4 Polynucleotide Kinase (PNK) simplifies the experiment to a one-step reaction at 37 °C in 3 h, reducing sample consumption and improving sensitivity. We chose functionalized hemin cofactors, significantly improving catalytic efficiency and enhancing detection capability. This biosensor detects Fpg activity with a sensitivity as low as 0.11 U mL<sup>−1</sup>, displaying exceptional sensitivity, selectivity, and interference resistance in human serum and bacterial cell extracts under isothermal conditions. The biosensor demonstrates remarkable selectivity and ability for Fpg inhibitors screening. In addition, this biosensor enables reading the sample's RGB values using a smartphone, facilitating accurate quantification of Fpg activity without the necessity for specialized equipment.</p></div><div><h3>Significance</h3><p>PERFUME simplifies Fpg detection by using a single hairpin and PNK in a one-step process. We utilize FUME to enhance catalytic efficiency, it surpassing the performance of traditional G-quadruplex/hemin DNAzyme methods. This approach excels in analyzing Fpg in human serum and bacterial extracts. 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引用次数: 0
摘要
背景8-氧鸟嘌呤 DNA 糖基化酶可以维持基因组的稳定性和完整性。然而,当它的活性出现异常时,会干扰正常的 DNA 损伤修复过程,可能导致癌症和其他各种人类疾病的发生。目前检测 8-氧鸟嘌呤 DNA 糖基化酶活性的方法往往存在灵敏度低、程序耗时、劳动密集型要求以及需要专业设备和训练有素的专业人员来执行等问题。结果我们开发了一种 PERFUME 方法,该方法结合了引物交换反应和功能化 G-四链/海明 DNA 酶,可灵敏检测典型的 8-氧鸟嘌呤 DNA 糖基化酶 Fpg。利用单一探针和 T4 多核苷酸激酶(PNK)将实验简化为 37°C 下一步反应,只需 3 小时,从而减少了样品消耗,提高了灵敏度。我们选用了功能化的海明辅助因子,大大提高了催化效率和检测能力。在等温条件下,该生物传感器检测 Fpg 活性的灵敏度低至 0.11 U mL-1,在人血清和细菌细胞提取物中显示出卓越的灵敏度、选择性和抗干扰性。该生物传感器在筛选 Fpg 抑制剂方面具有显著的选择性和能力。此外,该生物传感器还能使用智能手机读取样品的 RGB 值,从而无需专业设备即可准确量化 Fpg 活性。我们利用 FUME 提高了催化效率,其性能超过了传统的 G-四链/hemin DNA 酶方法。这种方法在分析人血清和细菌提取物中的 Fpg 方面表现出色。它可以在等温条件下利用紫外可见光和智能手机对 Fpg 进行定量检测,因此在临床诊断中很有价值。
NNNPERFUME: Detection of 8-oxoguanine DNA glycosylase activity based on primer exchange reaction and functionalized hemin/G-quadruplex DNAzyme
Background
8-oxoguanine DNA glycosylase can maintain genomic stability and integrity. However, it can interfere with the regular DNA damage repair process, possibly leading to the development of cancer and various other human diseases when its activity becomes abnormal. Current methods for detecting 8-oxoguanine DNA glycosylase activity often suffer from low sensitivity, time-consuming procedures, labor-intensive requirements, and the need for specialized equipment and trained professionals for execution. Consequently, there is an urgent need for a portable, user-friendly 8-oxoguanine DNA glycosylase assay that offers swift results and supports real-time testing.
Results
We've developed a PERFUME method that combines primer exchange reaction and functionalized G-quadruplex/hemin DNAzyme for sensitive detection of Fpg, a typical 8-oxoguanine DNA glycosylase. Utilizing a single probe and T4 Polynucleotide Kinase (PNK) simplifies the experiment to a one-step reaction at 37 °C in 3 h, reducing sample consumption and improving sensitivity. We chose functionalized hemin cofactors, significantly improving catalytic efficiency and enhancing detection capability. This biosensor detects Fpg activity with a sensitivity as low as 0.11 U mL−1, displaying exceptional sensitivity, selectivity, and interference resistance in human serum and bacterial cell extracts under isothermal conditions. The biosensor demonstrates remarkable selectivity and ability for Fpg inhibitors screening. In addition, this biosensor enables reading the sample's RGB values using a smartphone, facilitating accurate quantification of Fpg activity without the necessity for specialized equipment.
Significance
PERFUME simplifies Fpg detection by using a single hairpin and PNK in a one-step process. We utilize FUME to enhance catalytic efficiency, it surpassing the performance of traditional G-quadruplex/hemin DNAzyme methods. This approach excels in analyzing Fpg in human serum and bacterial extracts. It allows quantitative Fpg detection using UV–Vis and smartphones under isothermal conditions, making it valuable for clinical diagnosis.
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