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Molecular Identification of Giardia duodenalis Isolates from Fars Province, Iran.伊朗法尔斯省十二指肠贾第虫分离株的分子鉴定
Iran J Parasitol. 2014 Mar;9(1):70-8.
2
Low risk for transmission of zoonotic Giardia duodenalis from dogs to humans in rural Cambodia.在柬埔寨农村地区,犬源十二指肠贾第虫向人类传播的风险较低。
Parasit Vectors. 2014 Aug 29;7:412. doi: 10.1186/1756-3305-7-412.
3
Molecular identification of Giardia lamblia; is there any correlation between diarrhea and genotyping in Iranian population?蓝氏贾第鞭毛虫的分子鉴定;伊朗人群腹泻与基因分型之间是否存在关联?
Gastroenterol Hepatol Bed Bench. 2014 Summer;7(3):168-72.
4
Identification of genotypes of Giardia duodenalis human isolates in Isfahan, Iran, using polymerase chain reaction - Restriction Fragment Length polymorphism.运用聚合酶链反应-限制性片段长度多态性技术对伊朗伊斯法罕地区人体分离株中的十二指肠贾第虫基因型进行鉴定。
Adv Biomed Res. 2012 Dec 28;1:84. doi: 10.4103/2277-9175.105166. eCollection 2012.
5
Application of HRM assays with EvaGreen dye for genotyping Giardia duodenalis zoonotic assemblages.应用 EvaGreen 染料的 HRM 分析方法进行肠贾第虫人际传播株的基因分型。
Parasitol Res. 2012 Nov;111(5):2157-63. doi: 10.1007/s00436-012-3064-x. Epub 2012 Aug 11.
6
Giardia intestinalis: DNA extraction approaches to improve PCR results.肠道贾第虫:提高 PCR 结果的 DNA 提取方法。
Exp Parasitol. 2011 Jun;128(2):159-62. doi: 10.1016/j.exppara.2011.02.001. Epub 2011 Feb 17.
7
Zoonotic potential and molecular epidemiology of Giardia species and giardiasis.动物源寄生虫种属的动物源性潜力与分子流行病学及贾第虫病。
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8
Multilocus genotyping of Giardia duodenalis reveals striking differences between assemblages A and B.对十二指肠贾第鞭毛虫的多位点基因分型揭示了 A 组和 B 组之间的显著差异。
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Stool-based DNA testing, a new noninvasive method for colorectal cancer screening, the first report from Iran.基于粪便的DNA检测,一种用于结直肠癌筛查的新型非侵入性方法,来自伊朗的首份报告。
World J Gastroenterol. 2007 Mar 14;13(10):1528-33. doi: 10.3748/wjg.v13.i10.1528.
10
Evaluation of the sensitivities of DNA extraction and PCR methods for detection of Giardia duodenalis in stool specimens.粪便标本中检测十二指肠贾第鞭毛虫的DNA提取和PCR方法的敏感性评估。
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针对该基因进行PCR,对从囊肿中提取DNA的四种方法的比较与评估。

Comparison and evaluation of four methods for extracting DNA from cysts for PCR targeting the gene.

作者信息

Sepahvand Akram, Pestehchian Nader, Yousefi Hossein Ali, Gharehbaba Reza Pahlavan

机构信息

Department of Parasitology and Mycology, School of Medicine, Isfahan University of Medical Sciences, Isfahan, Iran.

Infectious Disease and Tropical Medicine Research Center, Isfahan University of Medical Sciences, Isfahan, Iran.

出版信息

J Parasit Dis. 2017 Mar;41(1):263-267. doi: 10.1007/s12639-016-0790-5. Epub 2016 Jun 10.

DOI:10.1007/s12639-016-0790-5
PMID:28316423
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5339212/
Abstract

is an intestinal flagellated protozoan and the common cause of gastrointestinal diseases in human. This parasite can be seen in two different forms in its life cycle including as cyst and trophozoite. Due to presence of resistant cyst wall, DNA extraction inhibitors along with artifact in stool specimens, this study was performed aiming to evaluate four methods for DNA extraction from cysts. Seventy positive stool specimens that were confirmed by light microscope were included in this study. All stool samples were concentrated using four layered discontinuous sucrose flotation technique (0.5, 0.75, 1, and 1.5 M) and single-layered sucrose solution (0.85 M). The isolated cysts were then subjected to DNA extraction by four methods. To remove the artifacts, the extracted DNA were evaluated by PCR. The results of the present study showed the high level of optical density (OD) in the method I ( < 0.01) with the following steps; cysts plus crushed cover glass were vortexed. Then, the samples were boiled and then followed by freeze-thaw cycles, yet this method yielded the lowest concentration. Furthermore, the highest concentration were observed in the method II ( <0.01) with the following steps; cysts plus crushed cover glass and TAE buffer were mixed and then shaken, followed by boiling. Based on the results of the present study, using crushed cover glass, boiling and freeze-thaw cycles can be effective in destruction of cyst wall and have enough efficiency for extracting DNA from cysts.

摘要

是一种肠道鞭毛虫原生动物,是人类胃肠道疾病的常见病因。这种寄生虫在其生命周期中可以以两种不同的形式出现,即包囊和滋养体。由于存在抗性包囊壁、粪便标本中的DNA提取抑制剂以及假象,本研究旨在评估从包囊中提取DNA的四种方法。本研究纳入了70份经光学显微镜确认的阳性粪便标本。所有粪便样本均采用四层不连续蔗糖浮选技术(0.5、0.75、1和1.5M)和单层蔗糖溶液(0.85M)进行浓缩。然后,通过四种方法对分离出的包囊进行DNA提取。为了去除假象,通过PCR对提取的DNA进行评估。本研究结果显示,方法I(<0.01)的光密度(OD)水平较高,步骤如下:将包囊加破碎的盖玻片涡旋。然后,将样品煮沸,接着进行冻融循环,但该方法产生的浓度最低。此外,方法II(<0.01)观察到的浓度最高,步骤如下:将包囊加破碎的盖玻片和TAE缓冲液混合,然后振荡,接着煮沸。根据本研究结果,使用破碎的盖玻片、煮沸和冻融循环可有效破坏包囊壁,并且具有足够的效率从包囊中提取DNA。