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用于增强结直肠癌甲基化分析的带有可延伸封闭探针的创新型半巢式实时PCR检测法

Innovative Semi-Nested Realtime PCR Assay with Extendable Blocking Probe for Enhanced Analysis of Methylation in Colorectal Cancer.

作者信息

Duong Linh Thuy, Dao Trang Thuy, Bui Hoai Thi, Nguyen Ung Dinh, Hoang Ung Tien, Tran Duc Viet, Nguyen Ba Van, Ho Tho Huu

机构信息

Oncology Center, 103 Military Hospital, Vietnam Military Medical University, Hanoi 10000, Vietnam.

Department of Genomics and Cytogenetics, Institute of Biomedicine and Pharmacy (IBP), Vietnam Military Medical University, Hanoi 10000, Vietnam.

出版信息

Biomedicines. 2024 Jul 1;12(7):1458. doi: 10.3390/biomedicines12071458.

Abstract

(1) Background: The detection of methylated (m) in plasma is a promising approach to non-invasive colorectal cancer (CRC) screening. Traditional approaches have limitations in sensitivity and cost-effectiveness, particularly in resource-limited settings. (2) Methods: We developed a semi-nested realtime PCR assay utilizing extendable blocking probes (ExBP) to enhance the detection of low-level m based on DNA melting. This assay allows for the discrimination of m in the presence of high concentrations of non-methylated (up to 100,000 times higher). (3) Results: The assay demonstrated a sensitivity of 73.91% and specificity of 80%, showcasing its ability to detect very low levels of methylated DNA effectively. The innovative use of ExBP without costly modified probes simplifies the assay setup and reduces the overall costs, enhancing its applicability in diverse clinical settings. (4) Conclusions: This novel assay significantly improves the detection of m, offering a potential advance in CRC screening and monitoring. Its cost-efficiency and high sensitivity make it particularly suitable for the early detection and management of CRC, especially in settings with limited resources. Future studies are encouraged to validate this assay in larger populations to establish its clinical benefits and practical utility.

摘要

(1) 背景:检测血浆中的甲基化(m)是一种很有前景的非侵入性结直肠癌(CRC)筛查方法。传统方法在灵敏度和成本效益方面存在局限性,尤其是在资源有限的环境中。(2) 方法:我们开发了一种利用可延伸阻断探针(ExBP)的半巢式实时PCR检测方法,以基于DNA熔解增强对低水平m的检测。该检测方法能够在存在高浓度非甲基化(高达100,000倍)的情况下区分甲基化。(3) 结果:该检测方法的灵敏度为73.91%,特异性为80%,展示了其有效检测极低水平甲基化DNA的能力。ExBP的创新性使用无需昂贵的修饰探针,简化了检测设置并降低了总体成本,增强了其在不同临床环境中的适用性。(4) 结论:这种新型检测方法显著提高了甲基化的检测水平,为CRC筛查和监测带来了潜在进展。其成本效益和高灵敏度使其特别适合CRC的早期检测和管理,尤其是在资源有限的环境中。鼓励未来的研究在更大规模人群中验证该检测方法,以确定其临床益处和实际效用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7d69/11274708/98848c627ef5/biomedicines-12-01458-g001.jpg

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