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首页> 外文期刊>Journal of Clinical Microbiology >Detection of the pathogenic parasite Toxoplasma gondii by specific amplification of ribosomal sequences using comultiplex polymerase chain reaction.
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Detection of the pathogenic parasite Toxoplasma gondii by specific amplification of ribosomal sequences using comultiplex polymerase chain reaction.

机译:通过使用共多重聚合酶链反应的核糖体序列的特异性扩增来检测病原性弓形虫。

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Amplification of DNA sequences from ribosomal DNA (rDNA) was tested as a specific and sensitive method for the detection of small numbers of Toxoplasma gondii tachyzoite cells. We applied the polymerase chain reaction (PCR) on the basis of detection of the 110-fold repetitive rDNA as a target by using (i) DNA sequences within the small ribosomal subunit known to be universal and conserved in all eukaryotes and (ii) small ribosomal subunit and intergenic spacer rDNA sequences known to be T. gondii species specific. The level of sensitivity obtained from a crude cell lysate allowed the detection of as few as one parasite visualized directly as a specific PCR product in agarose gels. By using a combination of universal and T. gondii species-specific primers, we propose a comultiplex-based PCR approach as a new diagnostic tool. The combination of sensitivity, specificity, and built-in positive and negative PCR controls should make detection of the rDNA sequences by comultiplex PCR a useful clinical test for the diagnosis of toxoplasmosis and for epidemiological studies. Finally, the idea of a built-in positive control to support or counter the T. gondii-specific PCR result is novel and is a notable advance.
机译:测试了从核糖体DNA(rDNA)扩增DNA序列的特异性和灵敏方法,用于检测少量的弓形虫速殖子细胞。我们在检测110倍重复rDNA作为靶标的基础上应用了聚合酶链反应(PCR),方法是:(i)使用已知在所有真核生物中都是保守的小核糖体亚基内的DNA序列,以及核糖体亚基和基因间隔垫片rDNA序列已知为弓形虫物种特异性。从粗制细胞裂解物中获得的敏感性水平允许检测到仅在琼脂糖凝胶中直接可视化为特异性PCR产物的一种寄生虫。通过使用通用和弓形虫物种特异性引物的组合,我们提出了一种基于共多重PCR的PCR方法作为一种新的诊断工具。灵敏度,特异性以及内置的阳性和阴性PCR对照的结合,应使通过共多重PCR检测rDNA序列成为诊断弓形虫病和进行流行病学研究的有用临床方法。最后,内置阳性对照来支持或对抗弓形虫特异性PCR结果的想法是新颖的,并且是一个显着的进步。

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