Hybrid &lt;em&gt;De Novo&lt;/em&gt; Genome Assembly for the Generation of Complete Genomes of Urinary Bacteria using Short- and Long-read Sequencing Technologies

Sharon, Belle M.; Hulyalkar, Neha V.; Nguyen, Vivian; Palmer, Kelli L.; Nisco, Nicole J. De

doi:10.3791/62872

Cited by 9 publications

(9 citation statements)

References 13 publications

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“…The bacterial strains used in this study were originally isolated from clean-catch midstream urine collected from consenting postmenopausal women (age 55-85) who were either healthy (no current UTI), or had active, symptomatic rUTI as part of institutional review board-approved studies STU 032016-006 and MR 17-120. Species identification of the 37 urinary bacterial strains used in this study was performed by 16S rRNA PCR Sanger Sequencing as previously described ( Sharon et al., 2021 ). The species used in this study are listed in Table 1 followed by the number of strains assayed per species.…”

Section: Methodsmentioning

confidence: 99%

A Semi-Quantitative Assay to Measure Glycosaminoglycan Degradation by the Urinary Microbiota

Nguyen

Khan

Shipman

et al. 2022

Front. Cell. Infect. Microbiol.

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Glycosaminoglycans (GAGs) are linear polysaccharides and are among the primary components of mucosal surfaces in mammalian systems. The GAG layer lining the mucosal surface of the urinary tract is thought to play a critical role in urinary tract homeostasis and provide a barrier against urinary tract infection (UTI). This key component of the host-microbe interface may serve as a scaffolding site or a nutrient source for the urinary microbiota or invading pathogens, but its exact role in UTI pathogenesis is unclear. Although members of the gut microbiota have been shown to degrade GAGs, the utilization and degradation of GAGs by the urinary microbiota or uropathogens had not been investigated. In this study, we developed an in vitro plate-based assay to measure GAG degradation and utilization and used this assay to screen a library of 37 urinary bacterial isolates representing both urinary microbiota and uropathogenic species. This novel assay is more rapid, inexpensive, and quantitative compared to previously developed assays, and can measure three of the major classes of human GAGs. Our findings demonstrate that this assay captures the well-characterized ability of Streptococcus agalactiae to degrade hyaluronic acid and partially degrade chondroitin sulfate. Additionally, we present the first known report of chondroitin sulfate degradation by Proteus mirabilis, an important uropathogen and a causative agent of acute, recurrent, and catheter-associated urinary tract infections (CAUTI). In contrast, we observed that uropathogenic Escherichia coli (UPEC) and members of the urinary microbiota, including lactobacilli, were unable to degrade GAGs.

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Section: Methodsmentioning

confidence: 99%

A Semi-Quantitative Assay to Measure Glycosaminoglycan Degradation by the Urinary Microbiota

Nguyen

Khan

Shipman

et al. 2022

Front. Cell. Infect. Microbiol.

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“…Er676 was isolated by plating urine on chromogenic agar (Chromagar Orientation, BD) and picking well-isolated colonies with enterococcal morphology. For species identification, single colonies were selected and subjected to PCR and Sanger sequencing of the conserved 16S rRNA gene as described previously [19,20]. Sequences were queried against the nr/ nt database using megablast (blast v2.10.0) and the species E. raffinosus was confirmed [21].…”

Section: Strain Isolation and Species Identificationmentioning

confidence: 99%

“…In preparation for sequencing, genomic DNA was isolated from overnight cultures of Er676 and ATCC49464 grown in Brain Heart Infusion (BHI) broth at 37 °C using the DNeasy Blood and Tissue kit (Qiagen). To facilitate lysis, 20 mg ml −1 lysozyme and 450 kUml −1 mutanolysin were included in the lysis buffer [19,22]. DNA was quantified via a Qubit fluorometer and quality and integrity were assessed by agarose gel electrophoresis.…”

Section: Genomic Dna Isolation and Sequencingmentioning

confidence: 99%

Inter-species diversity and functional genomic analyses of closed genome assemblies of clinically isolated, megaplasmid-containing Enterococcus raffinosus Er676 and ATCC49464

Sharon

Hulyalkar

Palmer

et al. 2023

Access Microbiology

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Enterococcus raffinosus is an understudied member of its genus possessing a characteristic megaplasmid contributing to a large genome size. Although less commonly associated with human infection compared to other enterococci, this species can cause disease and persist in diverse niches such as the gut, urinary tract, blood and environment. Few complete genome assemblies have been published to date for E. raffinosus . In this study, we report the complete assembly of the first clinical urinary E. raffinosus strain, Er676, isolated from a postmenopausal woman with history of recurrent urinary tract infection. We additionally completed the assembly of clinical type strain ATCC49464. Comparative genomic analyses reveal inter-species diversity driven by large accessory genomes. The presence of a conserved megaplasmid indicates it is a ubiquitous and vital genetic feature of E. raffinosus . We find that the E. raffinosus chromosome is enriched for DNA replication and protein biosynthesis genes while the megaplasmid is enriched for transcription and carbohydrate metabolism genes. Prophage analysis suggests that diversity in the chromosome and megaplasmid sequences arises, in part, from horizontal gene transfer. Er676 demonstrated the largest genome size reported to date for E. raffinosus and the highest probability of human pathogenicity. Er676 also possesses multiple antimicrobial resistance genes, of which all but one are encoded on the chromosome, and has the most complete prophage sequences. Complete assembly and comparative analyses of the Er676 and ATCC49464 genomes provide important insight into the inter-species diversity of E. raffinosus that gives it its ability to colonize and persist in the human body. Investigating genetic factors that contribute to the pathogenicity of this species will provide valuable tools to combat diseases caused by this opportunistic pathogen.

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“…Closed hybrid assemblies were created using the normal mode of Unicycler v0.4.8 ( 6 ), SPAdes v3.13.0 ( 7 ), Racon v1.4.10 ( 8 ), and Pilon v1.2.3 ( 9 , 10 ). The closed genomes were then rotated to the start of either the dnaA or repA gene, when present.…”

Section: Announcementmentioning

confidence: 99%

Complete Genome Sequences of Three Lactobacillus gasseri Urine Isolates Obtained from Postmenopausal Women

Shipman

Nguyen

Sharon

et al. 2022

Microbiol Resour Announc

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Lactobacillus gasseri frequently colonizes the lower urinary tract of healthy women. However, the role of L. gasseri in urinary tract health and the genes required for urinary tract colonization are poorly understood. Herein, we announce the complete genome sequences of three Lactobacillus gasseri isolates collected from the urine of postmenopausal women.

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Hybrid <em>De Novo</em> Genome Assembly for the Generation of Complete Genomes of Urinary Bacteria using Short- and Long-read Sequencing Technologies

Cited by 9 publications

References 13 publications

A Semi-Quantitative Assay to Measure Glycosaminoglycan Degradation by the Urinary Microbiota

A Semi-Quantitative Assay to Measure Glycosaminoglycan Degradation by the Urinary Microbiota

Inter-species diversity and functional genomic analyses of closed genome assemblies of clinically isolated, megaplasmid-containing Enterococcus raffinosus Er676 and ATCC49464

Complete Genome Sequences of Three Lactobacillus gasseri Urine Isolates Obtained from Postmenopausal Women

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