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Determination of genotypes of Toxoplasma gondii strains isolated from patients with toxoplasmosis.

机译:确定弓形虫病患者分离的弓形虫菌株的基因型。

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摘要

To determine the genotypes of Toxoplasma gondii strains associated with human toxoplasmosis, we developed a sensitive approach for typing parasites grown from clinical samples by short-term in vitro culture. A newly described nested PCR assay was capable of amplifying genomic DNA from as few as five parasites in the presence of host tissues. Typing was based on DNA polymorphisms at the SAG2 locus, encoding tachyzoite surface antigen p22. Restriction fragment length polymorphisms in PCR-amplified SAG2 products were used to classify strains into one of the three major lineages of T. gondii. This approach was successfully used to determine the genotypes of 68 of 72 samples that had been previously isolated from patients with congenital, cerebral, and disseminated toxoplasmosis. Type II strains of T. gondii were found in a majority of the samples, accounting for 55 (81%) of the 68 toxoplasmosis cases. In contrast, type I and III strains were found in only 7 (10%) and 6 (9%) of the 68 cases, respectively. The results of this study support the previous finding that type II strains are most often associated with human toxoplasmosis. Nested PCR analysis at the SAG2 locus provides rapid assignment of T. gondii to a specific genotype that should be useful in analyzing a variety of clinical samples.
机译:为了确定与人类弓形虫病相关的弓形体弓形虫的基因型,我们开发了一种敏感的方法,可以对通过短期体外培养从临床样品中生长的寄生虫进行分型。新近描述的巢式PCR分析能够在宿主组织存在的情况下,从少至五个寄生虫中扩增出基因组DNA。键入是基于SAG2位点的DNA多态性,编码Tachyzoite表面抗原p22。 PCR扩增的SAG2产物中的限制性片段长度多态性用于将菌株分类为弓形虫的三个主要谱系之一。该方法已成功用于确定先前从先天性,脑性和弥漫性弓形虫病患者中分离出的72个样品中的68个的基因型。在大多数样本中发现了弓形虫的II型菌株,占68例弓形虫病病例中的55株(81%)。相比之下,在68例病例中,分别仅发现7例(10%)和6例(9%)I型和III型毒株。这项研究的结果支持先前的发现,即II型毒株最常与人类弓形虫病相关。在SAG2位点的巢式PCR分析可将刚地弓形虫快速分配至特定基因型,该基因型可用于分析各种临床样品。

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