Development of polymerase chain reaction primer sets for diagnosis of Lyme disease and for species-specific identification of Lyme disease isolates by 16S rRNA signature nucleotide analysis.

R T Marconi; C F Garon

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Development of polymerase chain reaction primer sets for diagnosis of Lyme disease and for species-specific identification of Lyme disease isolates by 16S rRNA signature nucleotide analysis.

机译：通过16S rRNA标记核苷酸分析开发用于诊断莱姆病和用于莱姆病分离株物种特异性鉴定的聚合酶链反应引物组。

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We have determined and compared partial 16S rRNA sequences from 23 Lyme disease spirochete isolates and aligned these with 8 sequences previously presented. The 16S rRNA signature nucleotide compositions were defined for each isolate and compared with the genomic species signature nucleotide sets previously established. To identify positions truly indicative of species classification which could serve as targets for polymerase chain reaction species-specific identification primers, 16S rRNA-based phylogenetic analyses were conducted. On the basis of the identified signature nucleotides, we designed polymerase chain reaction primer sets which (i) amplify all spirochete species associated with Lyme disease and (ii) differentiate between these species. The primer sets were tested on 38 Borrelia isolates associated with Lyme disease and were found to be sensitive and specific. All Lyme disease isolates tested were amplification positive. These primers allow for the rapid species identification of Lyme disease isolates.

机译：我们已经确定并比较了来自23个莱姆病螺旋体分离株的16S rRNA的部分序列，并将其与先前提出的8个序列进行比对。为每个分离物定义了16S rRNA签名核苷酸组成，并与先前建立的基因组物种签名核苷酸集进行了比较。为了鉴定真正指示物种分类的位置，这些位置可以用作聚合酶链反应物种特异性鉴定引物的靶标，进行了基于16S rRNA的系统发育分析。基于鉴定出的特征核苷酸，我们设计了聚合酶链反应引物组，该组（i）扩增与莱姆病相关的所有螺旋体物种，以及（ii）在这些物种之间进行区分。在38个与莱姆病相关的疏螺旋体分离株上测试了引物对，发现它们具有敏感性和特异性。测试的所有莱姆病分离株均为扩增阳性。这些引物可快速鉴定莱姆病分离株。

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《Journal of Clinical Microbiology》 |1992年第11期|共5页
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R T Marconi; C F Garon;
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中图分类医学微生物学（病原细菌学、病原微生物学）;
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1. Rapid diagnosis of lyme disease: Flagellin gene-based nested polymerase chain reaction for identification of causative Borrelia species [J] . Yukita Sato, Tatsuya Konishi, Yoshio Hashimoto, International journal of infectious diseases : . 1998,第2期

机译：莱姆病的快速诊断：基于鞭毛蛋白基因的嵌套式聚合酶链反应，鉴定致病性疏螺旋体
2. Improving the specificity of 16S rDNA-based polymerase chain reaction for detecting Borrelia burgdorferi sensu lato-causative agents of human Lyme disease [J] . Cyr TL, Jenkins MC, Hall RD, Journal of applied microbiology . 2005,第4期

机译：提高基于16S rDNA的聚合酶链反应检测人莱姆病致病性伯氏疏螺旋体致病菌的特异性
3. Polymerase chain reaction primers and probes derived from flagellin gene sequences for specific detection of the agents of Lyme disease and North American relapsing fever. [J] . R N Picken Journal of Clinical Microbiology . 1992,第1期

机译：源自鞭毛蛋白基因序列的聚合酶链反应引物和探针，用于特异性检测莱姆病和北美复发性发热。
4. Quantitation of Three Outer Surface Proteins From The Lyme Disease Spirochete, Borrelia Burgdorferi By Nanoparticle Capture / Multiple Reaction Monitoring-Mass Spectrometry. [C] . Paul Russo, Davide Tamburro, Claudia Fredolini, American Society for Mass Spectrometry Conference on Mass Spectrometry and Allied Topics . 2012

机译：荔枝疾病三种外表面蛋白的定量，培斯基捕获/多反应监测质谱法通过培养基菌螺旋体，Borrelia Burgdorferi。
5. Study of Lyme neuroborreliosis using polymerase chain reaction. [D] . Keller, Tracy L. 1996

机译：使用聚合酶链反应研究莱姆神经支原体病。
6. Development of polymerase chain reaction primer sets for diagnosis of Lyme disease and for species-specific identification of Lyme disease isolates by 16S rRNA signature nucleotide analysis. [O] . R T Marconi, C F Garon 1992

机译：通过16S rRNA标记核苷酸分析开发用于诊断莱姆病和用于莱姆病分离株物种特异性鉴定的聚合酶链反应引物组。
7. Rapid diagnosis of lyme disease: Flagellin gene-based nested polymerase chain reaction for identification of causative Borrelia species [O] . Sato Yukita, Konishi Tatsuya, Hashimoto Yoshio, 1997

机译：莱姆病的快速诊断：基于鞭毛蛋白基因的嵌套式聚合酶链反应，用于鉴定致病性疏螺旋体
8. Images in Health Surveillance: Tickborne Disease Vectors and Lyme Disease Clinical Diagnosis. [R] . 2012

机译：健康监测中的图像：蜱传疾病媒介和莱姆病临床诊断。

Development of polymerase chain reaction primer sets for diagnosis of Lyme disease and for species-specific identification of Lyme disease isolates by 16S rRNA signature nucleotide analysis.

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