用于口腔鳞状细胞癌组织 qPCR 分析的 DNA 合成比较评估 - 一种用于基因表达研究的快速、稳健的分离技术

Ramya Mahalingam , Vivek Narayanan , Magesh Karuppur Thiagarajan , T. Jayaprakash , K.V. Leela
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引用次数: 0

摘要

背景从生物材料中分离 DNA 是包括聚合酶链反应 (PCR) 在内的多个生物分析过程的第一步。这一过程的最佳条件是DNA纯净,没有潜在的扩增反应抑制剂。由于生物样本的数量和质量有限,因此必须从原始样本中提取尽可能多的 DNA。固相萃取技术常用于纯化 DNA。在这一过程中,DNA 被吸附在固体支持物上,通过洗涤去除反应中的污染物,然后从支持物中洗脱出纯化的 DNA。DNA 的质量和浓度对基因分析程序有直接影响。因此,在解释基于 PCR 的诊断检测结果之前,必须确认 DNA 的制备和完整性,尤其是在未鉴定出病原体 DNA 的情况下。方法:我们使用两种标准化的 DNA 合成方案与使用病毒检测试剂盒中的载体 RNA 和蛋白酶 K 的测试方案进行了比较研究。通过对转移抑制基因 NDRG1、RhoGDI 和 KISS 1 的基因扩增进行 qPCR 分析,评估合成 DNA 的质量和数量。通过 q PCR 分析得出的基因表达浓度验证了 DNA 的浓度。采用测试方案合成 DNA 时,基因表达量明显更高。因此,这项研究验证了核酸载体 RNA 分子在改进用于基因分析程序的组织样本 DNA 提取过程方面的潜力。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Comparative evaluation of DNA synthesis for qPCR analysis from oral squamous cell carcinoma tissues - A rapid and robust isolation technique for gene expression studies

Background

DNA isolation from biological materials is the initial step in several bioanalytical processes, including the polymerase chain reaction (PCR). This procedure works best with pure DNA devoid of potential amplification reaction inhibitors. Since the quantity and quality of biological samples are limited, it is essential to extract as much DNA as possible from the original sample. The solid-phase extraction technique is frequently used to purify DNA. In this process, the DNA is adsorbed onto a solid support, any contaminants from the reaction are eliminated by washing, and the purified DNA is then eluted from the support. The quality and concentration of DNA have a direct effect on the gene analysis procedure. Therefore, before interpreting the results of PCR-based diagnostic assays, it is imperative to confirm the DNA preparation and integrity, particularly if no pathogenic DNA is identified.

Methods

A comparative study was carried out using two standardized protocols for DNA synthesis in comparison with a test protocol incorporating carrier RNA and proteinase K from a viral detection kit. The quality and quantity of the synthesized DNA are assessed by qPCR analysis for gene amplification of metastasis suppressor genes NDRG1, RhoGDI, and KISS 1.

Results and conclusion

The test protocol showed higher yields of DNA in comparison to the standard protocol. The concentration of DNA obtained was validated by the concentration of gene expressed from q PCR analysis. The gene expression was significantly higher when the test protocol method was followed for DNA synthesis. Thus the study validates the potential of nucleic acid carrier RNA molecules to improve DNA extraction processes used in tissue samples for gene analysis procedures.
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