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Defining Genetic Fitness Determinants and Creating Genomic Resources for an Oral Pathogen

机译:定义遗传适应性决定因素并创建口腔病原体的基因组资源

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Periodontitis is a microbial infection that destroys the structures that support the teeth. Although it is typically a chronic condition, rapidly progressing, aggressive forms are associated with the oral pathogen Aggregatibacter actinomycetemcomitans. One of this bacterium's key virulence traits is its ability to attach to surfaces and form robust biofilms that resist killing by the host and antibiotics. Though much has been learned about A. actinomycetemcomitans since its initial discovery, we lack insight into a fundamental aspect of its basic biology, as we do not know the full set of genes that it requires for viability (the essential genome). Furthermore, research on A. actinomycetemcomitans is hampered by the field's lack of a mutant collection. To address these gaps, we used rapid transposon mutant sequencing (Tn-seq) to define the essential genomes of two strains of A. actinomycetemcomitans, revealing a core set of 319 genes. We then generated an arrayed mutant library comprising >1,500 unique insertions and used a sequencing-based approach to define each mutant's position (well and plate) in the library. To demonstrate its utility, we screened the library for mutants with weakened resistance to subinhibitory erythromycin, revealing the multidrug efflux pump AcrAB as a critical resistance factor. During the screen, we discovered that erythromycin induces A. actinomycetemcomitans to form biofilms. We therefore devised a novel Tn-seq-based screen to identify specific factors that mediate this phenotype and in follow-up experiments confirmed 4 mutants. Together, these studies present new insights and resources for investigating the basic biology and disease mechanisms of a human pathogen.
机译:牙周炎是一种微生物感染,会破坏支撑牙齿的结构。虽然它通常是一种慢性疾病,但快速进展的侵袭性形式与口腔病原体放线菌聚合菌有关。这种细菌的关键毒力特征之一是它能够附着在表面并形成强大的生物膜,抵抗宿主和抗生素的杀伤。尽管自最初发现以来,人们对放线菌的了解很多,但我们缺乏对其基础生物学基本方面的了解,因为我们不知道它生存所需的全套基因(基本基因组)。此外,由于该领域缺乏突变体收集,对放线菌的研究受到阻碍。为了解决这些差距,我们使用快速转座子突变测序(Tn-seq)来定义两种放线菌菌株的基本基因组,揭示了一组319个核心基因。然后,我们生成了一个包含 >1,500 个独特插入的阵列突变体文库,并使用基于测序的方法来定义每个突变体在文库中的位置(孔和板)。为了证明其实用性,我们筛选了对亚抑制性红霉素耐药性较弱的突变体,揭示了多药外排泵 AcrAB 作为关键耐药因子。在筛选过程中,我们发现红霉素诱导放线菌形成生物膜。因此,我们设计了一种基于 Tn-seq 的新型筛选来鉴定介导这种表型的特定因素,并在后续实验中确认了 4 个突变体。总之,这些研究为研究人类病原体的基本生物学和疾病机制提供了新的见解和资源。

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