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利用实时荧光定性和定量 PCR 鉴定污染工业粗制猪肝素的反刍动物成分的种属特异性。

Species-specific identification of ruminant components contaminating industrial crude porcine heparin using real-time fluorescent qualitative and quantitative PCR.

机构信息

Department of Laboratory Medicine, Southwest Hospital, Third Military Medical University, Chongqing 400038, China.

出版信息

Anal Bioanal Chem. 2012 Feb;402(4):1625-34. doi: 10.1007/s00216-011-5590-2. Epub 2011 Dec 7.

DOI:10.1007/s00216-011-5590-2
PMID:22147273
Abstract

Ever since the emergence of bovine spongiform encephalopathy, the source of pharmaceutical heparin has been restricted to porcine intestinal mucosa. In this project, two real-time fluorescent PCR methods were developed to assist with quality control analysis. The first is a qualitative method which relies on SYBR Green I chemistry to confirm the porcine origin of industrial crude porcine heparin (ICPH), identify any ruminant contaminants, and generally control purity. The second is based on TaqMan chemistry and is able to quantitatively identify porcine, bovine, caprine, and ovine components and contaminants in ICPH. By targeting mitochondrial DNA, both PCR systems showed a detection limit of 1 pg DNA and amplification efficiencies ranging between 96% and 102%. Moreover, quantitative PCR showed a detection limit of 0.02 ppm in samples comprising porcine, bovine, caprine, and ovine DNA. The results of qualitative PCR over 27 ICPH samples showed that all samples were porcine in origin and that 17 had ruminant contaminants. The results of quantitative PCR further showed that out of all 17 samples with ruminant contaminants, seven samples had bovine, ovine, and caprine contaminants, two samples had bovine and ovine contaminants, and eight samples had only ovine contaminants. In conclusion, the qualitative PCR system was found to be a relatively inexpensive, rapid, and flexible method of identifying the porcine origin of and ruminant contaminants in ICPH, while the quantitative PCR was found suitable to accurately analyze the components and contaminants in detail. Both methods are suitable for routine control assays for the evaluation of ICPH purity and origins of contaminants.

摘要

自牛海绵状脑病出现以来,制药肝素的来源一直局限于猪肠黏膜。在这个项目中,开发了两种实时荧光 PCR 方法来辅助质量控制分析。第一种是定性方法,它依赖于 SYBR Green I 化学来确认工业粗制猪肝素(ICPH)的猪源,识别任何反刍动物污染物,并通常控制纯度。第二种方法基于 TaqMan 化学,能够定量识别 ICPH 中的猪、牛、山羊和绵羊成分和污染物。通过靶向线粒体 DNA,这两种 PCR 系统的检测限均为 1 pg DNA,扩增效率在 96%至 102%之间。此外,定量 PCR 在包含猪、牛、山羊和绵羊 DNA 的样品中的检测限为 0.02 ppm。对 27 个 ICPH 样本进行定性 PCR 的结果表明,所有样本均源自猪,且 17 个样本有反刍动物污染物。定量 PCR 的结果进一步表明,在所有 17 个有反刍动物污染物的样本中,有 7 个样本含有牛、羊和山羊污染物,2 个样本含有牛和羊污染物,8 个样本仅含有羊污染物。总之,定性 PCR 系统被发现是一种相对廉价、快速和灵活的方法,可用于识别 ICPH 的猪源和反刍动物污染物,而定量 PCR 则适合于准确分析成分和污染物的详细情况。这两种方法均适用于 ICPH 纯度和污染物来源的常规控制分析。

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