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一个最小复制子使沙眼衣原体的有效、种属特异性基因缺失成为可能,并使用鼠型沙眼衣原体将基因敲除研究扩展到感染的动物模型。

A Minimal Replicon Enables Efficacious, Species-Specific Gene Deletion in Chlamydia and Extension of Gene Knockout Studies to the Animal Model of Infection Using Chlamydia muridarum.

机构信息

Department of Microbiology, Immunology & Molecular Genetics, University of Kentuckygrid.266539.d College of Medicine, Lexington, Kentucky, USA.

Division of Immunity and Pathogenesis, Burnett School of Biomedical Sciences, College of Medicine, University of Central Floridagrid.170430.1, Orlando, Florida, USA.

出版信息

Infect Immun. 2022 Dec 15;90(12):e0045322. doi: 10.1128/iai.00453-22. Epub 2022 Nov 9.

Abstract

The genus Chlamydia consists of diverse, obligate intracellular bacteria that infect various animals, including humans. Although chlamydial species share many aspects of the typical intracellular lifestyle, such as the biphasic developmental cycle and the preference for invasion of epithelial cells, each chlamydial strain also employs sophisticated species-specific strategies that contribute to an extraordinary diversity in organ and/or tissue tropism and disease manifestation. In order to discover and understand the mechanisms underlying how these pathogens infect particular hosts and cause specific diseases, it is imperative to develop a mutagenesis approach that would be applicable to every chlamydial species. We present functional evidence that the region between Chlamydia trachomatis and Chlamydia muridarum and , containing four 22-bp tandem repeats that are present in all chlamydial endogenous plasmids, represents the plasmid origin of replication. Furthermore, by introducing species-specific regions into an engineered 5.45-kb pUC19-based plasmid, we generated vectors that can be successfully transformed into and propagated under selective pressure by C. trachomatis serovars L2 and D, as well as C. muridarum. Conversely, these vectors were rapidly lost upon removal of the selective antibiotic. This conditionally replicating system was used to generate a deletion mutant by fluorescence-reported allelic exchange mutagenesis in both C. trachomatis serovar D and C. muridarum. The strains were analyzed using invasion and fitness assays. The virulence of the C. muridarum strains was then assessed in a murine infection model. Our approach represents a novel and efficient strategy for targeted genetic manipulation in Chlamydia beyond C. trachomatis L2. This advance will support comparative studies of species-specific infection biology and enable studies in a well-established murine model of chlamydial pathogenesis.

摘要

衣原体属包含多种专性细胞内细菌,可感染包括人类在内的各种动物。尽管衣原体物种在典型的细胞内生活方式方面有许多共同之处,如两相发育周期和偏好入侵上皮细胞,但每种衣原体菌株也采用了复杂的种特异性策略,导致其在器官和/或组织嗜性和疾病表现方面具有非凡的多样性。为了发现和理解这些病原体感染特定宿主和引起特定疾病的机制,开发一种适用于每种衣原体物种的突变体生成方法是至关重要的。我们提供了功能证据,证明衣原体属和衣原体属之间的区域 和 ,包含四个存在于所有衣原体内源性质粒中的 22 个碱基对串联重复序列,代表质粒复制起点。此外,通过将种特异性 区域引入工程化的基于 5.45-kb pUC19 的质粒中,我们生成了可以成功转化并在衣原体属血清型 L2 和 D 以及衣原体属 选择压力下进行复制的载体。相反,在去除选择抗生素后,这些载体迅速丢失。这个条件复制系统用于通过荧光报告等位基因交换突变在衣原体属血清型 D 和衣原体属 中生成 缺失突变体。使用入侵和适应性测定对这些菌株进行了分析。然后在小鼠感染模型中评估了 缺失突变体的毒力。我们的方法代表了一种新颖而有效的靶向遗传操作策略,可用于衣原体属,超越了衣原体属 L2。这一进展将支持针对物种特异性感染生物学的比较研究,并能够在成熟的小鼠衣原体发病机制模型中进行研究。

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