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      Cutibacterium acnes (Propionibacterium acnes ) and acne vulgaris: a brief look at the latest updates

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          Time series community genomics analysis reveals rapid shifts in bacterial species, strains, and phage during infant gut colonization

          The gastrointestinal microbiome undergoes shifts in species and strain abundances, yet dynamics involving closely related microorganisms remain largely unknown because most methods cannot resolve them. We developed new metagenomic methods and utilized them to track species and strain level variations in microbial communities in 11 fecal samples collected from a premature infant during the first month of life. Ninety six percent of the sequencing reads were assembled into scaffolds of >500 bp in length that could be assigned to organisms at the strain level. Six essentially complete (∼99%) and two near-complete genomes were assembled for bacteria that comprised as little as 1% of the community, as well as nine partial genomes of bacteria representing as little as 0.05%. In addition, three viral genomes were assembled and assigned to their hosts. The relative abundance of three Staphylococcus epidermidis strains, as well as three phages that infect them, changed dramatically over time. Genes possibly related to these shifts include those for resistance to antibiotics, heavy metals, and phage. At the species level, we observed the decline of an early-colonizing Propionibacterium acnes strain similar to SK137 and the proliferation of novel Propionibacterium and Peptoniphilus species late in colonization. The Propionibacterium species differed in their ability to metabolize carbon compounds such as inositol and sialic acid, indicating that shifts in species composition likely impact the metabolic potential of the community. These results highlight the benefit of reconstructing complete genomes from metagenomic data and demonstrate methods for achieving this goal.
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            The natural history of cutaneous propionibacteria, and reclassification of selected species within the genus Propionibacterium to the proposed novel genera Acidipropionibacterium gen. nov., Cutibacterium gen. nov. and Pseudopropionibacterium gen. nov.

            The genus Propionibacterium in the family Propionibacteriaceaeconsists of species of various habitats, including mature cheese, cattle rumen and human skin. Traditionally, these species have been grouped as either classical or cutaneous propionibacteria based on characteristic phenotypes and source of isolation. To re-evaluate the taxonomy of the family and to elucidate the interspecies relatedness we compared 162 public whole-genome sequences of strains representing species of the family Propionibacteriaceae. We found substantial discrepancies between the phylogenetic signals of 16S rRNA gene sequence analysis and our high-resolution core-genome analysis. To accommodate these discrepancies, and to address the long-standing issue of the taxonomically problematic Propionibacterium propionicum, we propose three novel genera, Acidipropionibacterium gen. nov., Cutibacterium gen. nov. and Pseudopropionibacterium gen. nov., and an amended description of the genus Propionibacterium. Furthermore, our genome-based analyses support the amounting evidence that the subdivision of Propionibacterium freudenreichii into subspecies is not warranted. Our proposals are supported by phylogenetic analyses, DNA G+C content, peptidoglycan composition and patterns of the gene losses and acquisitions in the cutaneous propionibacteria during their adaptation to the human host.
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              What is new in the pathophysiology of acne, an overview

              B. Dreno (2017)
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                Author and article information

                Journal
                Journal of the European Academy of Dermatology and Venereology
                J Eur Acad Dermatol Venereol
                Wiley
                09269959
                June 2018
                June 2018
                June 12 2018
                : 32
                : 5-14
                Affiliations
                [1 ]Department of Dermatology; CIC 1413; CRCINA Inserm 1232; CHU Nantes; Nantes France
                [2 ]Laboratoire de Génie Chimique; UMR 5503, Faculty of Pharmacy; Université de Toulouse; Université Paul Sabatier; Toulouse Cedex 9 France
                [3 ]CHU Toulouse; Hôpital Purpan; Service de Bactériologie-Hygiène; Toulouse France
                [4 ]Department of Bacteriology; CRCINA Inserm 1232; CHU Nantes; Nantes France
                [5 ]Department of Pathophysiology and Transplantation; Università degli Studi di Milano; I.R.C.C.S. Foundation; Cà Granda Ospedale Maggiore Policlinico; Milan Italy
                Article
                10.1111/jdv.15043
                29894579
                fbfd4697-42fa-4101-801b-6ca2dfc55e75
                © 2018

                http://doi.wiley.com/10.1002/tdm_license_1.1

                http://onlinelibrary.wiley.com/termsAndConditions#vor

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