Molano Monica, Meijer Chris J L M, Morré Servaas A, Pol Rene, van den Brule Adriaan J C
Department of Pathology, Vrije Universiteit Medical Center, Amsterdam, The Netherlands.
J Clin Microbiol. 2004 Jul;42(7):2935-9. doi: 10.1128/JCM.42.7.2935-2939.2004.
In this study we developed and evaluated a new PCR-based typing assay, directed to the VD2 region of the omp1 gene, for the detection and typing of urogenital Chlamydia trachomatis infections. A nested VD2 PCR-reverse line blot (RLB) assay was developed for the typing of nine different urogenital serovars of C. trachomatis. The assay developed was tested with reference strains of C. trachomatis serovars and cervical scrapes of 86 Colombian women previously found to be positive for C. trachomatis by using plasmid PCR. Two sets of primers directed to the VD2 region of the omp1 gene of C. trachomatis were designed, and fragments of 220 and 166 bp were generated in the primary and nested PCRs, respectively. In addition, an RLB assay was developed to identify nine different urogenital serovars of C. trachomatis (Ba, D, E, F, G, H, I, J, and K) and group controls, including group B (Ba, D, and E), group C (I, J, K, and H), and an intermediate group (F and G). Using this assay, we were able to type 81 of the 86 samples (94.2%). Of these samples, 91.3% were single C. trachomatis infections, and 8.7% were multiple infections. The most common serovars identified were serovars D (22.2%), F (18.5%), G (13.6%), and E (12.3%). Of the women with multiple C. trachomatis infections, >50% contained both serovars D and E. The nested VD2 PCR-RLB developed is a simple, fast, and specific method for the identification of individual urogenital C. trachomatis serovars previously detected by using plasmid PCR. Moreover, it is an appropriate method for studying multiple C. trachomatis infections and for use in large epidemiological studies.
在本研究中,我们开发并评估了一种基于PCR的新型分型检测方法,该方法针对omp1基因的VD2区域,用于泌尿生殖道沙眼衣原体感染的检测和分型。我们开发了一种巢式VD2 PCR-反向线印迹(RLB)检测方法,用于对沙眼衣原体的九种不同泌尿生殖道血清型进行分型。使用开发的检测方法对沙眼衣原体血清型参考菌株以及86名哥伦比亚女性的宫颈刮片进行了检测,这些女性先前通过质粒PCR检测发现沙眼衣原体呈阳性。设计了两组针对沙眼衣原体omp1基因VD2区域的引物,在初次PCR和巢式PCR中分别产生了220 bp和166 bp的片段。此外,还开发了一种RLB检测方法,以鉴定沙眼衣原体的九种不同泌尿生殖道血清型(Ba、D、E、F、G、H、I、J和K)以及分组对照,包括B组(Ba、D和E)、C组(I、J、K和H)和中间组(F和G)。使用该检测方法,我们能够对86个样本中的81个(94.2%)进行分型。在这些样本中,91.3%为单一沙眼衣原体感染,8.7%为多重感染。鉴定出的最常见血清型为血清型D(22.2%)、F(18.5%)、G(13.6%)和E(12.3%)。在患有多重沙眼衣原体感染的女性中,超过50%同时含有血清型D和E。开发的巢式VD2 PCR-RLB是一种简单、快速且特异的方法,用于鉴定先前通过质粒PCR检测到的个体泌尿生殖道沙眼衣原体血清型。此外,它是研究多重沙眼衣原体感染以及用于大型流行病学研究的合适方法。