Development of a specific and sensitive diagnostic PCR for rapid molecular authentication of the medicinal plant Portulaca oleracea

IF 2.3 3区 生物学 Q3 BIOCHEMICAL RESEARCH METHODS
Mo-Rong Xu , Meng-Shiou Lee , Bo-Cheng Yang , Hsiu-Chi Chang , Chao-Lin Kuo , Chia-Hsin Lin , Hsi-Jien Chen , Jai-Hong Cheng , Fang-Chun Sun
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引用次数: 0

Abstract

Adulteration by Bacopa monnieri (BM) in Portulaca oleracea (PO) plants frequently occurs; it decreases the efficacy of traditional Chinese medicine (TCM) and leads to fraud in the herbal marketplace. In this study, a diagnostic PCR assay was established for the rapid authentication of PO and BM in the herbal market. The sequence divergences in internal transcribed spacer 2 (ITS2) between PO and its adulterant species were used to design diagnostic PCR primers. The specific designed primer sets were evaluated and show that the diagnostic PCR assay can be used to verify the authenticity of PO and BM. The detection limits of the primer set for PO and BM identification were 10 pg and 1 pg, respectively. The reactivity of diagnostic PCR was 0.1% PO genomic DNA and 0.01% BM genomic DNA in the test sample during DNA amplification. In addition, multiplex PCR (mPCR) for PO and BM identification was also established. The samples were more susceptible to the effect of steaming in authentication by singleplex PCR and mPCR than boiling and drying treatment. Furthermore, commercial samples from the market were used to demonstrate the applicability of the developed diagnostic PCR for PO authentication and diagnose BM adulteration, and the investigation found that approximately 72.2% (13/18) of PO plants in the herbal market were adulterated. In conclusion, the diagnostic PCR assay was successfully developed and its specificity, sensitivity and reactivity for PO and BM authentication were proven. These developed PCR-based molecular methods can be applied as an identification tool for PO authenticity and can be practically applied for inspection of BM adulteration in the herbal market in the future.

用于药用植物马齿苋快速分子鉴定的特异灵敏诊断性PCR的建立
在马齿苋(PO)植株中,常发生圆斑菌(BM)的掺混;它降低了中药的疗效,并导致草药市场上的欺诈。在本研究中,建立了一种诊断性PCR检测方法,用于草药市场中PO和BM的快速鉴定。利用PO与其混淆种之间的内部转录间隔区2(ITS2)序列差异设计诊断性PCR引物。对设计的特异性引物组进行了评价,表明诊断性PCR检测可用于验证PO和BM的真实性。用于PO和BM鉴定的引物组的检测限分别为10pg和1pg。在DNA扩增过程中,诊断性PCR的反应性为测试样品中0.1%的PO基因组DNA和0.01%的BM基因组DNA。此外,还建立了用于PO和BM鉴定的多重PCR(mPCR)。与煮沸和干燥处理相比,单重PCR和mPCR鉴定样品更容易受到蒸汽处理的影响。此外,使用市场上的商业样本来证明所开发的诊断PCR用于PO认证和诊断BM掺假的适用性,调查发现,草药市场上约72.2%(13/18)的PO植物掺假。总之,成功开发了诊断性PCR检测方法,并证明了其对PO和BM鉴定的特异性、敏感性和反应性。这些开发的基于PCR的分子方法可以作为PO真实性的鉴定工具,并可在未来的草药市场中实际应用于BM掺假的检测。
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来源期刊
Molecular and Cellular Probes
Molecular and Cellular Probes 生物-生化研究方法
CiteScore
6.80
自引率
0.00%
发文量
52
审稿时长
16 days
期刊介绍: MCP - Advancing biology through–omics and bioinformatic technologies wants to capture outcomes from the current revolution in molecular technologies and sciences. The journal has broadened its scope and embraces any high quality research papers, reviews and opinions in areas including, but not limited to, molecular biology, cell biology, biochemistry, immunology, physiology, epidemiology, ecology, virology, microbiology, parasitology, genetics, evolutionary biology, genomics (including metagenomics), bioinformatics, proteomics, metabolomics, glycomics, and lipidomics. Submissions with a technology-driven focus on understanding normal biological or disease processes as well as conceptual advances and paradigm shifts are particularly encouraged. The Editors welcome fundamental or applied research areas; pre-submission enquiries about advanced draft manuscripts are welcomed. Top quality research and manuscripts will be fast-tracked.
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