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Touchdown Enzyme Time Release-PCR for Detection and Identification of Chlamydia trachomatis C. pneumoniae and C. psittaci Using the 16S and 16S-23S Spacer rRNA Genes

机译：使用16S和16S-23S间隔rRNA基因检测和鉴定沙眼衣原体肺炎衣原体和鹦鹉热衣原体的着陆酶时间释放PCR

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摘要

Three touchdown enzyme time release (TETR)-PCR assays were used to amplify different DNA sequences in the variable regions of the 16S and 16S-23S spacer rRNA genes specific for Chlamydia trachomatis, Chlamydia pneumoniae, and Chlamydia psittaci as improved tests for sensitive diagnosis and rapid species differentiation. The TETR-PCR protocol used 60 cycles of amplification, which provided improved analytical sensitivity (0.004 to 0.063 inclusion-forming unit of Chlamydia species per PCR). The sensitivity of TETR-PCR with primer set CTR 70-CTR 71 was 96.7%, and the specificity was 99.6%, compared to those of the AMPLICOR PCR for the detection of C. trachomatis in vaginal swab samples. TETR-PCR for C. pneumoniae with primer set CPN 90-CPN 91 was 90% sensitive and 93.3% specific compared with a nested PCR with primer set CP1/2-CPC/D for clinical respiratory samples. TETR-PCR for C. psittaci with primer set CPS 100-CPS 101 showed substantial agreement with cell culturing (κ, 0.78) for animal tissue samples. Primer sets were then combined into a single multiplex TETR-PCR test. The respective 315-, 195-, and 111-bp DNA target products were precisely amplified when DNA from each of the respective Chlamydia species or combinations of them was used. Multiplex chlamydia TETR-PCR correctly identified one strain of each of the 15 serovars of C. trachomatis, 22 isolates of C. pneumoniae, and 20 isolates of C. psittaci. The primer sets were specific for each species. No target products were amplified when DNA from C. pecorum or a variety of other microorganisms was tested for specificity. TETR-PCR with primers selected for specific sequences in the 16S and 16S-23S spacer rRNA genes is a valuable test that could be used either with individual primers or in a multiplex assay for the identification and differentiation of Chlamydia species from culture isolates or for the detection of chlamydiae in clinical samples.

机译：使用三种着陆酶释放（TETR）-PCR分析法扩增沙眼衣原体，肺炎衣原体和鹦鹉热衣原体特异的16S和16S-23S间隔rRNA基因可变区中的不同DNA序列，作为敏感诊断和诊断的改进测试。物种快速分化。 TETR-PCR方案使用了60个扩增循环，从而提高了分析灵敏度（每个PCR衣原体物种包涵形成单位为0.004至0.063）。与使用AMPLICOR PCR检测阴道拭子样本中的沙眼衣原体相比，使用引物对CTR 70-CTR 71进行TETR-PCR的敏感性为96.7％，特异性为99.6％。带有引物组CP1 / 2-CPC / D的巢式PCR与临床呼吸道标本相比，带有引物组CPN 90-CPN 91的肺炎衣原体的TETR-PCR具有90％的敏感性和93.3％的特异性。带有引物对CPS 100-CPS 101的鹦鹉热衣原体的TETR-PCR与动物组织样品的细胞培养（κ，0.78）表现出基本一致。然后将引物组合成一个多重TETR-PCR测试。当使用来自各个衣原体物种或其组合的DNA时，分别精确扩增了315、195和111 bp的DNA靶产物。多重衣原体TETR-PCR正确地鉴定了沙眼衣原体的15种血清型中的一种菌株，肺炎衣原体的22种分离株和鹦鹉热衣原体的20种分离株。引物对每种物种而言都是特异性的。当测试来自谷氨酸棒杆菌或其他多种微生物的DNA的特异性时，没有扩增目标产物。使用针对16S和16S-23S间隔rRNA基因中特定序列选择的引物进行的TETR-PCR是一项有价值的测试，可以与单个引物一起使用，也可以在多重分析中用于从培养分离株中鉴定或区分衣原体物种或用于检测临床样本中的衣原体。

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期刊名称 Journal of Clinical Microbiology
作者
Guillermo Madico; Thomas C. Quinn; Jens Boman; Charlotte A. Gaydos;
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作者单位

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年(卷),期 2000(38),3
年度 2000
页码 1085–1093
总页数 9
原文格式 PDF
正文语种
中图分类微生物学;
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专利

1. Touchdown Enzyme Time Release-PCR for Detection and Identification of Chlamydia trachomatis, C. pneumoniae, and C. psittaci Using the 16S and 16S-23S Spacer rRNA Genes [J] . Guillermo Madico, Thomas C. Quinn, Jens Boman, Journal of Clinical Microbiology . 2000,第3期

机译：使用16S和16S-23S间隔rRNA基因检测和鉴定沙眼衣原体，肺炎衣原体和鹦鹉热衣原体的着陆酶时间释放PCR
2. A 28 kDa major immunogen of Chlamydia psittaci shares identity with Mip proteins of Legionella spp. and Chlamydia trachomatis - cloning and characterization of the C. psittaci mip-like gene [J] . Daniel D. Rockey, Brian B. Chesebro, Robert A. Heinzen, Microbiology . 1996,第4期

机译：Chlamydia Psittaci的28 kda主要免疫原与军团菌SPP的MIP蛋白共享身份。和衣原体的衣原体 - 克隆和表征C.psittaci mip基因
3. RNA polymerase beta subunit (rpoB) gene and the 16S-23S rRNA intergenic transcribed spacer region (ITS) as complementary molecular markers in addition to the 16S rRNA gene for phylogenetic analysis and identification of the species of the family Mycoplasmataceae [J] . Volokhov D.V., Simonyan V., Davidson M.K., Molecular phylogenetics and evolution . 2012,第1期

机译：除了16S rRNA基因外，RNA聚合酶β亚基（rpoB）基因和16S-23S rRNA基因间转录间隔区（ITS）作为互补分子标记，可用于系统分析和鉴定支原体科的物种
4. Identification of an Alga-Lysing bacteria isolated from TaiHu Lake by the analysis of 16S rRNA and 16S-23S rRNA intergenic spacer region [C] . LI Yun-hui, PU Yue-pu, YIN Li-hong International Forum on Progress on Post-Genome Technologies(5'IFPT); 20070910-11; Suzhou(CN) . 2007

机译：通过16S rRNA和16S-23S rRNA基因间隔区分析鉴定从太湖分离的溶藻细菌。
5. Identification of Pathogenic Nocardia Species by Reverse Line Blot Hybridization Targeting the 16S rRNA and 16S-23S rRNA Gene Spacer Regions [O] . Meng Xiao, Fanrong Kong, Tania C. Sorrell, 2010

机译：靶向16S rRNA和16S-23S rRNA基因间隔区的反向印迹杂交鉴定致病性诺卡氏菌。
6. Touchdown Enzyme Time Release-PCR for Detection and Identification of Chlamydia trachomatis , C. pneumoniae , and C. psittaci Using the 16S and 16S-23S Spacer rRNA Genes [O] . Guillermo Madico, Thomas C. Quinn, Jens Boman, 2000

机译：用于使用16S和16S-23S间隔rRNA基因的用于检测和鉴定C.肺组合，C.Pneumoniae和C.Psittaci的用于检测和鉴定的触地得键酶释放PCR

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Touchdown Enzyme Time Release-PCR for Detection and Identification of Chlamydia trachomatis C. pneumoniae and C. psittaci Using the 16S and 16S-23S Spacer rRNA Genes

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