一种高效、简便的提取胃组织中幽门螺杆菌DNA的方法

Q3 Medicine
Parastoo Saniee, Paria Ghadersoltani, Masoumeh Noroozpour, Alireza Sadjadi
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引用次数: 0

摘要

背景与目的:福尔马林固定石蜡包埋档案组织可用于遗传分析和评估一些患者的病史,包括传染病。然而,目前还没有从存档标本中提取细菌DNA的既定方案。在这项研究中,通过对先前发表的方案进行一些修改,从存档的幽门螺旋杆菌阳性胃活检中提取DNA。通过扩增幽门螺杆菌特异性16S rRNA基因来评估提取DNA的质量。方法:收集2002-2008年间50例幽门螺杆菌阳性胃活检标本,经石蜡块固定包埋。石蜡去除后,同时进行蛋白酶K处理和玻璃微珠机械破坏,对胃组织进行消化。在传统的苯酚-氯仿法基础上,加入一步苯酚处理和两步孵育,进行DNA提取。评估提取的DNA样本的数量和质量。此外,使用针对幽门螺杆菌特异性16S rRNA的引物进行PCR。结果:电泳显示,所有活检标本均恢复完整的dna。扩增519bp大小的PCR产物,证实所有活组织中均存在幽门螺杆菌特异性16S rRNA基因。结论:所有样本的幽门螺杆菌特异性16S rRNA基因扩增成功率均为100%。在这方面,设计的改进方法有效地去除了干扰污染物,提高了从存档组织中提取的细菌DNA的质量。这些修饰可能有助于更好地从人体组织中存在的不同细菌中提取完整的DNA。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
An Efficient and Easy- to- Use Method for Extraction of H. pylori DNA from Archival Formalin-Fixed and Paraffin-Embedded Gastric Tissues
Background & Objective: Formalin-fixed paraffin-embedded archived tissues are useful for the genetic analyses and assessment of some patients’ disease history, including infectious diseases. However, there is no established protocol for extracting bacterial DNA from the archived specimens. In this study DNA was extracted from the archived H. pylori-positive gastric biopsies by some modifications applied to the previously published protocols. The quality of the extracted DNA was assessed by amplifying H. pylori-specific 16S rRNA gene.Methods: Fifty H. pylori-positive gastric biopsies obtained, fixed, and embedded in paraffin blocks during 2002-2008 were recruited. After paraffin removal, simultaneous proteinase K treatment and mechanical disruption using glass beads were used for the digestion of gastric tissues. DNA extraction was performed by adding one step of phenol treatment and two steps of incubation to the conventional phenol-chloroform method. The quantity and quality of the extracted DNA samples were assessed. Also, PCR was performed using primers specific for the H. pylori-specific 16S rRNA.Results: The electrophoresis showed that intact DNAs were recovered from all biopsy samples. Amplification of the PCR products with the size of 519bp confirmed the presence of H. pylori-specific 16S rRNA gene in all the biopsies.Conclusion: A 100% success rate for the amplification of H. pylori-specific 16S rRNA gene was achieved from all the samples. In this regard, the designed modified method resulted in the effective removal of interfering contaminations and enhanced the quality of the extracted bacterial DNA from the archived tissues. These modifications may contribute to better extraction of the intact DNA from different bacteria present in human tissues.
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来源期刊
Iranian Journal of Pathology
Iranian Journal of Pathology Medicine-Pathology and Forensic Medicine
CiteScore
2.00
自引率
0.00%
发文量
99
审稿时长
20 weeks
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