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9. Unexpected invasion of miniature inverted-repeat transposable elements in viral genomes

Author

Zhang, Hua-Hao, Zhou, Qiu-Zhong, Wang, Ping-Lan, Xiong, Xiao-Min, Luchetti, Andrea, Raoult, Didier, Levasseur, Anthony, Santini, Sebastien, Abergel, Chantal, Legendre, Matthieu, Drezen, Jean-Michel, Béliveau, Catherine, Cusson, Michel, Jiang, Shen-Hua, Bao, Hai-Ou, Sun, Cheng, Bureau, Thomas E., Cheng, Peng-Fei, Han, Min-Jin, Zhang, Ze, Zhang, Xiao-Gu, and Dai, Fang-Yin

Published
2018
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17. Molecular identification of head lice collected in Franceville (Gabon) and their associated bacteria.

Author

Boumbanda-Koyo, Celia Scherelle, Mediannikov, Oleg, Amanzougaghene, Nadia, Oyegue-Liabagui, Sandrine Lydie, Imboumi-Limoukou, Roméo Karl, Raoult, Didier, Lekana-Douki, Jean Bernard, and Fenollar, Florence

Subjects
COXIELLA burnetii, RICKETTSIA, LICE, CYTOCHROME b, YERSINIA pestis, PATHOGENIC bacteria, HUMAN migrations
Abstract

Background: Pediculus humanus, which includes two ecotypes (body and head lice), is an obligate bloodsucking parasite that co-evolved with their human hosts over thousands of years, thus providing a valuable source of information to reconstruct the human migration. Pediculosis due to head lice occurred each year throughout the world and several pathogenic bacteria, which are usually associated with body lice, are increasingly detected in them. In Gabon, where this pediculosis is still widespread, there is a lack of data on genetic diversity of head lice and their associated bacteria. Methods: This study aimed to investigate the phylogeny of head lice collected in Gabon and their associated bacteria, using molecular tools. Between 26 March and 11 April 2018, 691 head lice were collected from 86 women in Franceville. We studied the genetic diversity of these lice based on the cytochrome b gene, then we screened them for DNA of Bartonella quintana, Borrelia spp., Acinetobacter spp., Yersinia pestis, Rickettsia spp., R. prowazekii, Anaplasma spp. and C. burnetii, using real time or standard PCR and sequencing. Results: Overall 74.6% of studied lice belonged to Clade A, 25.3% to Clade C and 0.1% to Clade E. The phylogenetic analysis of 344 head lice yielded 45 variable positions defining 13 different haplotypes from which 8 were novel. Bacterial screening revealed the presence of Borrelia spp. DNA in 3 (0.4%) of 691 head lice belonging to Clade A and infesting one individual. This Borrelia is close to B. theileri (GenBank: MN621894). Acinetobacter spp. DNA has been detected in 39 (25%) of the 156 screened lice; of these 13 (8.3%) corresponded to A. baumannii. Acinetobacter nosocomialis (n = 2) and A. pittii (n = 1) were also recorded. Conclusions: To of our knowledge, this study is the first to investigate the genetic diversity of head lice from Gabon. It appears that Clade C is the second most important clade in Gabon, after Clade A which is known to have a global distribution. The detection of Borrelia spp. DNA in these lice highlight the potential circulation of these bacteria in Gabon. [ABSTRACT FROM AUTHOR]

Published
2020
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18. MALDI-TOF MS as an innovative tool for detection of Plasmodium parasites in Anopheles mosquitoes

Author

Laroche, Maureen, Almeras, Lionel, Pecchi, Emilie, Bechah, Yassina, Raoult, Didier, Viola, Angèle, and Parola, Philippe

Subjects
Mice, Inbred C57BL, Biological Products, Infectious Diseases, Plasmodium berghei, Research, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, parasitic diseases, Anopheles, Animals, Parasitology, Female, Entomology
Abstract

Background Malaria is still a major public health issue worldwide, and one of the best approaches to fight the disease remains vector control. The current methods for mosquito identification include morphological methods that are generally time-consuming and require expertise, and molecular methods that require laboratory facilities with relatively expensive running costs. Matrix-Assisted Laser Desorption Ionization Time-Of-Flight Mass Spectrometry (MALDI-TOF MS) technology, routinely used for bacterial identification, has recently emerged in the field of entomology. The aim of the present study was to assess whether MALDI-TOF MS could successfully distinguish Anopheles stephensi mosquitoes according to their Plasmodium infection status. Methods C57BL/6 mice experimentally infected with Plasmodium berghei were exposed to An. stephensi bites. For the determination of An. stephensi infection status, mosquito cephalothoraxes were dissected and submitted to mass spectrometry analyses and DNA amplification for molecular analysis. Spectra were grouped according to mosquitoes’ infection status and spectra quality was validated based on intensity and reproducibility within each group. The in-lab MALDI-TOF MS arthropod reference spectra database, upgraded with representative spectra from both groups (infected/non-infected), was subsequently queried blindly with cephalothorax spectra from specimens of both groups. Results The MALDI TOF MS profiles generated from protein extracts prepared from the cephalothorax of An. stephensi allowed distinction between infected and uninfected mosquitoes. Correct classification was obtained in blind test analysis for (79/80) 98.75% of all mosquitoes tested. Only one of 80 specimens, an infected mosquito, was misclassified in the blind test analysis. Conclusions Matrix-Assisted Laser Desorption Ionization Time-Of-Flight Mass Spectrometry appears to be a promising, rapid and reliable tool for the epidemiological surveillance of Anopheles vectors, including their identification and their infection status.

Published
2017

19. Accurate identification of Culicidae at aquatic developmental stages by MALDI-TOF MS profiling

Author

Dieme, Constentin, Yssouf, Amina, Vega-Rúa, Anubis, Berenger, Jean-Michel, Failloux, Anna-Bella, Raoult, Didier, Parola, Philippe, Almeras, Lionel, Unité de Recherche sur les Maladies Infectieuses et Tropicales Emergentes (URMITE), Institut de Recherche pour le Développement (IRD)-Aix Marseille Université (AMU)-Institut National de la Santé et de la Recherche Médicale (INSERM)-IFR48, INSB-INSB-Centre National de la Recherche Scientifique (CNRS), Arbovirus et Insectes Vecteurs - Arboviruses and Insect Vectors, Institut Pasteur [Paris], We thank Pr Ousmane Faye (Université Cheikh Anta Diop (UCAD), Dakar, Senegal) for kindly providing An. coluzzii specimens and Christophe Flaudrops (URMITE-IRD198, Marseille, France) for his advice on the analysis of MALDI-TOF MS profiles. We would like to thank Ricardo Lourenço-de-Oliveira for providing mosquitoes from Manaus in Brazil. This manuscript has been reviewed and corrected by American Journal Experts, Institut des sciences biologiques (INSB-CNRS)-Institut des sciences biologiques (INSB-CNRS)-Centre National de la Recherche Scientifique (CNRS), and Institut Pasteur [Paris] (IP)

Subjects
Research, fungi, MALDI-TOF mass spectrometry, Pupa, Vectors, Infectious Diseases, Culicidae, MESH: Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Species Specificity, Larva, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, parasitic diseases, [SDV.MP.VIR]Life Sciences [q-bio]/Microbiology and Parasitology/Virology, MESH: Biomarkers, MESH: Species Specificity, Animals, Parasitology, MESH: Animals, MESH: Pupa, MESH: Culicidae, MESH: Larva, Aquatic stages, Species identification, Biomarkers
Abstract

Background The identification of mosquito vectors is generally based on morphological criteria, but for aquatic stages, morphological characteristics may be missing, leading to incomplete or incorrect identification. The high cost of molecular biology techniques requires the development of an alternative strategy. In the last decade, matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF MS) profiling has proved to be efficient for arthropod identification at the species level. Methods To investigate the usefulness of MALDI-TOF MS for the identification of mosquitoes at aquatic stages, optimizations of sample preparation, diet, body parts and storage conditions were tested. Protein extracts of whole specimens from second larval stage to pupae were selected for the creation of a reference spectra database. The database included a total of 95 laboratory-reared specimens of 6 mosquito species, including Anopheles gambiae (S form), Anopheles coluzzi (M form), Culex pipiens pipiens, Culex pipiens molestus, Aedes aegypti and 2 colonies of Aedes albopictus. Results The present study revealed that whole specimens at aquatic stages produced reproducible and singular spectra according to the mosquito species. Moreover, MS protein profiles appeared weakly affected by the diet provided. Despite the low diversity of some MS profiles, notably for cryptic species, clustering analyses correctly classified all specimens tested at the species level followed by the clustering of early vs. late aquatic developmental stages. Discriminant mass peaks were recorded for the 6 mosquito species analyzed at larval stage 3 and the pupal stage. Querying against the reference spectra database of 149 new specimens at different aquatic stages from the 6 mosquito species revealed that 147 specimens were correctly identified at the species level and that early and late developmental stages were also distinguished. Conclusions The present work highlights that MALDI-TOF MS profiling may be useful for the rapid and reliable identification of mosquito species at aquatic stages. With this proteomic tool, it becomes now conceivable to survey mosquito breeding sites prior to the mosquitoes’ emergence and to adapt anti-vectorial measures according to the mosquito fauna detected. Electronic supplementary material The online version of this article (doi:10.1186/s13071-014-0544-0) contains supplementary material, which is available to authorized users.

Published
2014

20. Repertoire of the gut microbiota from stomach to colon using culturomics and next-generation sequencing.

Author

Mailhe, Morgane, Ricaboni, Davide, Vitton, Véronique, Gonzalez, Jean-Michel, Bachar, Dipankar, Dubourg, Grégory, Cadoret, Frédéric, Robert, Catherine, Delerce, Jérémy, Levasseur, Anthony, Fournier, Pierre-Edouard, Angelakis, Emmanouil, Lagier, Jean-Christophe, and Raoult, Didier

Subjects
GUT microbiome, NUCLEOTIDE sequencing, STOMACH, ADENOMATOUS polyps, COLON (Anatomy), GASTROINTESTINAL system, HUMAN microbiota
Abstract

Background: Most studies on the human microbiota have analyzed stool samples, although a large proportion of the absorption of nutrients takes place in upper gut tract. We collected samples from different locations along the entire gastrointestinal tract from six patients who had simultaneously undergone upper endoscopy and colonoscopy, to perform a comprehensive analysis using culturomics with matrix assisted laser desorption ionisation - time of flight (MALDI-TOF) identification and by metagenomics targeting the 16S ribosomal ribonucleic acid (rRNA) gene. Results: Using culturomics, we isolated 368 different bacterial species, including 37 new species. Fewer species were isolated in the upper gut: 110 in the stomach and 106 in the duodenum, while 235 were isolated from the left colon (p < 0.02). We isolated fewer aero-intolerant species in the upper gut: 37 from the stomach and 150 from the left colon (p < 0.004). Using metagenomics, 1,021 species were identified. The upper gut microbiota was revealed to be less rich than the lower gut microbiota, with 37,622 reads from the stomach, 28,390 from the duodenum, and 79,047 from the left colon (p < 0.009). There were fewer reads for aero-intolerant species in the upper gut (8,656 in the stomach, 5,188 in the duodenum and 72,262 in the left colon, p < 0.02). Patients taking proton pump inhibitors (PPI) were then revealed to have a higher stomach pH and a greater diversity of species in the upper digestive tract than patients not receiving treatment (p < 0.001). Conclusion: Significant modifications in bacterial composition and diversity exist throughout the gastrointestinal tract. We suggest that the upper gut may be key to understanding the relationship between the gut microbiota and health. [ABSTRACT FROM AUTHOR]

Published
2018
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21. Correction to: Non contiguous-finished genome sequence and description of Bacillus timonensis sp. nov.

Author

Kokcha, Sahare, Mishra, Ajay Kumar, Lagier, Jean-Christophe, Million, Matthieu, Leroy, Quentin, Raoult, Didier, and Fournier, Pierre-Edouard

Subjects
BACILLUS (Bacteria)
Abstract

The online version of the original article can be found at https://doi.org/10.4056/sigs.2776064. References 1 Kokcha, S, Mishra, A.K, Lagier, J.C. et al non contiguous-finished genome sequence and description of Bacillus timonensis sp. nov. Following publication of the original article [[1]], the authors flagged the following errors: The original version of this article unfortunately contained two mistakes: (1) the authors had omitted to mention 10403188T as type strain name of the new species I Bacillus timonensis i (MM10403188T had been written instead), and (2) in the last paragraph of the protologue, DSM 253720 had been written in place of DSM 25372. [Extracted from the article]

Published
2023
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22. A modified multilocus sequence typing protocol to genotype Kingella kingae from oropharyngeal swabs without bacterial isolation.

Author

El Houmami, Nawal, Bzdrenga, Janek, Pons, Jean-Christophe, Minodier, Philippe, Durand, Guillaume André, Oubraham, Anis, Ceroni, Dimitri, Yagupsky, Pablo, Raoult, Didier, Bidet, Philippe, and Fournier, Pierre-Edouard

Abstract

Background: Outbreaks of Kingella kingae infection are an emerging public health concern among daycare attendees carrying epidemic clones in the oropharynx. However, genotyping of such epidemic clones from affected cases is limited by the low performance of current methods to detect K. kingae from blood samples and lack of specimens available from infected sites. We aimed at developing a modified multilocus sequence typing (MLST) method to genotype K. kingae strains from oropharyngeal samples without prior culture. We designed in silico MLST primers specific for K. kingae by aligning whole nucleotide sequences of abcZ, adk, aroE, cpn60, recA, and gdh/zwf genes from closely related species belonging to the Kingella and Neisseria genera. We tested our modified MLST protocol on all Kingella species and N. meningitidis, as well as 11 oropharyngeal samples from young children with sporadic (n = 10) or epidemic (n = 1) K. kingae infection. Results: We detected K. kingae-specific amplicons in the 11 oropharyngeal samples, corresponding to sequence-type 6 (ST-6) in 6 children including the epidemic cases, ST-25 in 2 children, and 3 possible novel STs (ST-67, ST-68, and ST-69). No amplicon was obtained from other Kingella species and N. meningitidis. Conclusions: We herein developed a specific MLST protocol that enables genotyping of K. kingae by MLST directly from oropharyngeal samples. This discriminatory tool, with which we identified the first K. kingae outbreak caused by ST-6 in Europe, may be used in further epidemiological investigations. [ABSTRACT FROM AUTHOR]

Published
2017
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23. Molecular investigation and phylogeny of Anaplasmataceae species infecting domestic animals and ticks in Corsica, France.

Author

Dahmani, Mustapha, Davoust, Bernard, Tahir, Djamel, Raoult, Didier, Fenollar, Florence, and Mediannikov, Oleg

Subjects
ANAPLASMATACEAE, PHYLOGENY, DOMESTIC animal diseases, TICK-borne diseases in animals, DISEASE prevalence
Abstract

Backgrounds: Corsica is a French island situated in the Mediterranean Sea. The island provides suitable natural conditions to study disease ecology, especially tick-borne diseases and emerging diseases in animals and ticks. The family Anaplasmataceae is a member of the order Rickettsiales; it includes the genera Anaplasma, Ehrlichia, Neorickettsia and Wolbachia. Anaplasmosis and ehrlichiosis traditionally refer to diseases caused by obligate intracellular bacteria of the genera Anaplasma and Ehrlichia. The aim of this study was to identify and estimate the prevalence of Anaplasmataceae species infecting domestic animals and ticks in Corsica. Methods: In this study, 458 blood samples from sheep, cattle, horses, goats, dogs, and 123 ticks removed from cattle, were collected in Corsica. Quantitative real-time PCR screening and genetic characterisation of Anaplasmataceae bacteria were based on the 23S rRNA, rpoB and groEl genes. Results: Two tick species were collected in the present study: Rhipicephalus bursa (118) and Hyalomma marginatum marginatum (5). Molecular investigation showed that 32.1% (147/458) of blood samples were positive for Anaplasmataceae infection. Anaplasma ovis was identified in 42.3% (93/220) of sheep. Anaplasma marginale was amplified from 100% (12/12) of cattle and two R. bursa (2/123). Several potentially new species were also identified: Anaplasma cf. ovis, "Candidatus Anaplasma corsicanum", "Candidatus Anaplasma mediterraneum" were amplified from 17.3% (38/220) of sheep, and Anaplasma sp. marginale-like was amplified from 80% (4/5) of goats. Finally, one R. bursa tick was found to harbour the DNA of E. canis. All samples from horses and dogs were negative for Anaplasmataceae infection. Conclusions: To our knowledge, this study is the first epidemiological survey on Anaplasmataceae species infecting animals and ticks in Corsica and contributes toward the identification of current Anaplasmataceae species circulating in Corsica. [ABSTRACT FROM AUTHOR]

Published
2017
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24. Identification of constraints influencing the bacterial genomes evolution in the PVC super-phylum.

Author

Pinos, Sandrine, Pontarotti, Pierre, Raoult, Didier, and Merhej, Vicky

Subjects
BACTERIAL genomes, BACTERIAL evolution, BACTERIAL ecology, PROTEOBACTERIA, ORIGIN of life, BACTERIAL DNA
Abstract

Background: Horizontal transfer plays an important role in the evolution of bacterial genomes, yet it obeys several constraints, including the ecological opportunity to meet other organisms, the presence of transfer systems, and the fitness of the transferred genes. Bacteria from the Planctomyctetes, Verrumicrobia, Chlamydiae (PVC) super-phylum have a compartmentalized cell plan delimited by an intracytoplasmic membrane that might constitute an additional constraint with particular impact on bacterial evolution. In this investigation, we studied the evolution of 33 genomes from PVC species and focused on the rate and the nature of horizontally transferred sequences in relation to their habitat and their cell plan. Results: Using a comparative phylogenomic approach, we showed that habitat influences the evolution of the bacterial genome's content and the flux of horizontal transfer of DNA (HT). Thus bacteria from soil, from insects and ubiquitous bacteria presented the highest average of horizontal transfer compared to bacteria living in water, extracellular bacteria in vertebrates, bacteria from amoeba and intracellular bacteria in vertebrates (with a mean of 379 versus 110 events per species, respectively and 7.6% of each genomes due to HT against 4.8%). The partners of these transfers were mainly bacterial organisms (94.9%); they allowed us to differentiate environmental bacteria, which exchanged more with Proteobacteria, and bacteria from vertebrates, which exchanged more with Firmicutes. The functional analysis of the horizontal transfers revealed a convergent evolution, with an over-representation of genes encoding for membrane biogenesis and lipid metabolism, among compartmentalized bacteria in the different habitats. Conclusions: The presence of an intracytoplasmic membrane in PVC species seems to affect the genome's evolution through the selection of transferred DNA, according to their encoded functions. [ABSTRACT FROM AUTHOR]

Published
2017
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25. Use of MALDI-TOF MS and culturomics to identify mosquitoes and their midgut microbiota.

Author

Tandina, Fatalmoudou, Almeras, Lionel, Koné, Abdoulaye K., Doumbo, Ogobara K., Raoult, Didier, and Parola, Philippe

Subjects
VIRUS diseases, MOSQUITO vectors, ANOPHELES gambiae, PROTEOBACTERIA, BACTEROIDETES, ACTINOBACTERIA
Abstract

Background: Mosquitoes transmit a wide range of human parasitic and viral diseases. In recent years, new techniques such as MALDI-TOF MS have been developed to identify mosquitoes at the species level, which is key for entomological surveys. Additionally, there is increasing interest in the mosquito microbiota and its role in vector capacity. Methods: The culturomics approach previously used in our laboratory to study human gut microbiota was applied to evaluate the midgut bacterial diversity of Anopheles gambiae (wild and laboratory strains), Aedes albopictus (wild and laboratory strains) and Culex quinquefasciatus (wild strains) in order to determine the influence of the environmental status on the midgut microbiota of the mosquitoes. Results: Mosquitoes collected in the field were accurately identified by MALDI-TOF MS analysis of their legs. Adult mosquito midgut microbiota was composed of four phyla, including Proteobacteria, Bacteroidetes, Actinobacteria and Firmicutes. The majority of the bacteria detected in the microbiota of mosquitoes were gram-negative and belong to the phylum Proteobacteria. MALDI-TOF MS identified for the first time a new bacterial species from An. gambiae midgut microbiota. Conclusion: In this study, the culturomics approach was found to be a reliable technique for exploring the diversity of the mosquito microbiota. MALDI-TOF MS was confirmed as a promising technique to identify mosquitoes collected in the field. Culturomics allowed the isolation of a new bacterial species not previously associated with mosquito vectors. The environment plays a role in the bacterial diversity of the microbiota, which could enable the development of new control strategies for mosquito-borne disease. [ABSTRACT FROM AUTHOR]

Published
2016
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26. Malaria in urban, semi-urban and rural areas of southern of Gabon: comparison of the Pfmdr 1 and Pfcrt genotypes from symptomatic children.

Author

Maghendji-Nzondo, Sydney, Kouna, Lady-Charlène, Mourembou, Gaël, Boundenga, Larson, Imboumy-Limoukou, Romeo-Karl, Matsiegui, Pierre-Blaise, Manego-Zoleko, Rella, Mbatchi, Bertrand, Raoult, Didier, Toure-Ndouo, Fousseyni, and Lekana-Douki, Jean Bernard

Subjects
MALARIA treatment, ARTEMISININ, COMBINATION drug therapy, HAPLOTYPES, DRUG resistance, AMODIAQUINE, PLASMODIUM falciparum
Abstract

Background: Artesunate-amodiaquine (AS-AQ) and artemether-lumefantrine (AL) are first- and second-line treatments for uncomplicated Plasmodium falciparum malaria in Gabon. AL remains highly efficacious, but its widespread use has led to molecular selection of the NFD haplotype on Pfmdr1 and K76 in Pfcrt. In this study, plasmodial infection characteristics and the distribution of the Pfmdr1 and Pfcrt genotypes involved in reduced efficacy of artemisininbased combination therapy (ACT) were investigated in four Gabonese localities. Methods: A cross-sectional study was conducted in the paediatric units of rural (Lastourville and Fougamou), semiurban (Koula-Moutou) and urban (Franceville) areas. Malaria was diagnosed with the rapid diagnostic test Optimal-IT® and confirmed by blood smear. Pfmdr1 codons 86, 184 and 1246 and Pfcrt codon 76 were genotyped by PCR-RFLP and sequencing. Results: Among 1129 included children, the prevalence of plasmodial infection was 79.5 % at Lastourville, 53.6 % at Fougamou, 36.1 % at Koula-Moutou, and 21.2 % at Franceville. The prevalence was significantly higher among children over 60 months of age in both semi-urban (p = 0.01) and urban (p = 0.004) areas. The prevalence of Pfmdr1 wild-type N86 differed significantly between Lastourville (57.8 %) and Koula-Moutou (45.4 %) (p = 0.039). No difference in 184F-carrying parasites was found between Lastourville (73.8 %), Fougamou (81.6 %), Koula-Moutou (83.2 %), and Franceville (80.6 %) (p = 0.240). The prevalence of wild-type D1246 was significantly different between Lastourville (94.1 %), Koula-Moutou (85.6 %) and Franceville (87.3 %) (p = 0.01). The frequency of wild-type K76 was not significantly different across the four sites: Lastourville (16.5 %), Fougamou (27.8 %), Koula-Moutou (17.4 %), and Franceville (29.4 %) (p = 0.09). The mixed genotypes were only found in Lastourville and Franceville. The NFD, YFD and NYD haplotypes were mainly Lastourville (46.6, 25.8, 14.0 %), Fougamou (45.5, 9.1, 42.4 %), Koula-Moutou (35, 6.7, 40.4 %), and Franceville (40.0, 16.0, 32.0 %). Conclusion: This study shows an increase in the prevalence of childhood plasmodial infection in Gabon according to the low socio-economic level, and a high frequency of markers associated with AL treatment failure. Close monitoring of ACT use is needed. [ABSTRACT FROM AUTHOR]

Published
2016
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27. Compartmentalization in PVC super-phylum: evolution and impact.

Author

Pinos, Sandrine, Pontarotti, Pierre, Raoult, Didier, Baudoin, Jean Pierre, and Pagnier, Isabelle

Subjects
BACTERIOPHAGES, BACTERIAL DNA, MICROMETRY, GENOMES, MICROSCOPY
Abstract

Background: The PVC super-phylum gathers bacteria from seven phyla (Planctomycetes, Verrucomicrobiae, Chlamydiae, Lentisphaera, Poribacteria, OP3, WWE2) presenting different lifestyles, cell plans and environments. Planctomyces and several Verrucomicrobiae exhibit a complex cell plan, with an intracytoplasmic membrane inducing the compartmentalization of the cytoplasm into two regions (pirellulosome and paryphoplasm). The evolution and function of this cell plan is still subject to debate. In this work, we hypothesized that it could play a role in protection of the bacterial DNA, especially against Horizontal Genes Transfers (HGT). Therefore, 64 bacterial genomes belonging to seven different phyla (whose four PVC phyla) were studied. We reconstructed the evolution of the cell plan as precisely as possible, thanks to information obtained by bibliographic study and electronic microscopy. We used a strategy based on comparative phylogenomic in order to determine the part occupied by the horizontal transfers for each studied genomes. Results: Our results show that the bacteria Simkania negevensis (Chlamydiae) and Coraliomargarita akajimensis (Verrucomicrobiae), whose cell plan were unknown before, are compartmentalized, as we can see on the micrographies. This is one of the first indication of the presence of an intracytoplasmic membrane in a Chlamydiae. The proportion of HGT does not seems to be related to the cell plan of bacteria, suggesting that compartmentalization does not induce a protection of bacterial DNA against HGT. Conversely, lifestyle of bacteria seems to impact the ability of bacteria to exchange genes. Conclusions: Our study allows a best reconstruction of the evolution of intracytoplasmic membrane, but this structure seems to have no impact on HGT occurrences. [ABSTRACT FROM AUTHOR]

Published
2016
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28. Non contiguous-finished genome sequence and description of Microbacterium gorillae sp. nov.

Author

Hadjadj, Linda, Rathored, Jaishriram, Keita, Mamadou Bhoye, Michelle, Caroline, Levasseur, Anthony, Raoult, Didier, Fournier, Pierre-Edouard, Rolain, Jean-Marc, and Bittar, Fadi

Subjects
MICROBACTERIUM, GORILLA (Genus), NUCLEOTIDE sequencing, GRAM-positive bacteria, PHENOTYPES, NUCLEIC acid hybridization
Abstract

Strain G3T (CSUR P207 = DSM 26203) was isolated from the fecal sample of a wild gorilla (Gorilla gorilla subsp gorilla) from Cameroon. It is a Gram-positive, facultative anaerobic short rod. This strain exhibits a 16S rRNA sequence similarity of 98.2% with Microbacterium thalassium, the closest validly published Microbacterium species and member of the family Microbacteriaceae. Moreover, it shows a low MALDI-TOF-MS score (1.1 to 1.3) that does not allow any identification. Thus, it is likely that this strain represents a new species. Here we describe the phenotypic features of this organism, the complete genome sequence and annotation. The 3,692,770 bp long genome (one chromosome but no plasmid) contains 3,505 protein-coding and 61 RNA genes, including 4 rRNA genes. In addition, digital DNA-DNA hybridization values for the genome of the strain G3T against the closest Microbacterium genomes range between 19.7 to 20.5, once again confirming its new status as a new species. On the basis of these polyphasic data, consisting of phenotypic and genomic analyses, we propose the creation of Microbacterium gorillae sp. nov. that contains the strain G3T. [ABSTRACT FROM AUTHOR]

Published
2016
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29. High-quality draft genome sequence and description of Haemophilus massiliensis sp. nov.

Author

Lo, Cheikh Ibrahima, Sankar, Senthil Alias, Fall, Bécaye, Sambe-Ba, Bissoume, Diawara, Silman, Gueye, Mamadou Wague, Mediannikov, Oleg, Blanc-Tailleur, Caroline, Wade, Boubacar, Raoult, Didier, Fournier, Pierre-Edouard, and Fenollar, Florence

Subjects
HAEMOPHILUS, NUCLEOTIDE sequencing, ASCITIC fluids, RIBOSOMAL RNA, PASTEURELLACEAE, MATRIX-assisted laser desorption-ionization, WOMEN patients
Abstract

Strain FF7T was isolated from the peritoneal fluid of a 44-year-old woman who suffered from pelvic peritonitis. This strain exhibited a 16S rRNA sequence similarity of 94.8% 16S rRNA sequence identity with Haemophilus parasuis, the phylogenetically closest species with a name with standing in nomenclature and a poor MALDI-TOF MS score (1.32 to 1.56) that does not allow any reliable identification. Using a polyphasic study made of phenotypic and genomic analyses, strain FF7T was a Gram-negative, facultatively anaerobic rod and member of the family Pasteurellaceae. It exhibited a genome of 2,442,548 bp long genome (one chromosome but no plasmid) contains 2,319 protein-coding and 67 RNA genes, including 6 rRNA operons. On the basis of these data, we propose the creation of Haemophilus massiliensis sp. nov. with strain FF7T (= CSUR P859 = DSM 28247) as the type strain. [ABSTRACT FROM AUTHOR]

Published
2016
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30. Identification of blood meal sources in the main African malaria mosquito vector by MALDI-TOF MS.

Author

Niare, Sirama, Berenger, Jean-Michel, Dieme, Constentin, Doumbo, Ogobara, Raoult, Didier, Parola, Philippe, and Almeras, Lionel

Subjects
BLOOD meal as feed, MOSQUITO vectors, MALARIA, ANOPHELES gambiae, EPIDEMIOLOGICAL research
Abstract

Background: The identification of blood meal sources in malaria vectors is critical to better understanding host/vector interactions and malaria epidemiology and control. Currently, the identification of mosquito blood meal origins is based on time-consuming and costly techniques such as precipitin tests, ELISA and molecular tools. Although these tools have been validated to identify the blood meal and trophic preferences of female Anopheles mosquitoes, they present several limitations. Recently, matrix-assisted, laser desorption/ionization time-of-light mass spectrometry (MALDI-TOF MS) was successfully used as a quick and accurate tool for arthropod identification, including mosquitoes. The aim of the present work was to test whether MALDI-TOF MS could also be applied to identification of blood meal sources from engorged mosquitoes. Methods: Abdomen proteins extracted from Anopheles gambiae (stricto sensu, S molecular form) that were either unengorged or artificially engorged on seven distinct types of vertebrate blood (human, horse, sheep, rabbit, mouse, rat, dog) were submitted for MALDI-TOF MS. Results: The comparison of mass spectrometry (MS) spectra from mosquito abdomens collected 1 h post-feeding, were able to discriminate blood meal origins. Moreover, using Aedes albopictus specimens, abdominal protein MS spectra from engorged mosquitoes were found specific to host blood source and independent of the mosquito species. A sequential analysis revealed stability of mosquito abdominal protein spectra up to 24 h post-feeding. Conclusions: These results indicate that MALDI-TOF MS could determine feeding patterns of freshly engorged mosquitoes up to 24 h post-blood meal. The MALDI-TOF MS technique appears to be an efficient tool for large epidemio-logical surveillance of vector-borne diseases and outbreak source identification. [ABSTRACT FROM AUTHOR]

Published
2016
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31. Detection of Bartonella tamiae, Coxiella burnetii and rickettsiae in arthropods and tissues from wild and domestic animals in northeastern Algeria.

Author

Leulmi, Hamza, Aouadi, Atef, Bitam, Idir, Bessas, Amina, Benakhla, Ahmed, Raoult, Didier, and Parola, Philippe

Subjects
BARTONELLA, RICKETTSIA, COXIELLA burnetii, TICKS, FLEA control, ALGERIAN economy
Abstract

Background: In recent years, the scope and importance of emergent vector-borne diseases has increased dramatically. In Algeria, only limited information is currently available concerning the presence and prevalence of these zoonotic diseases. For this reason, we conducted a survey of hematophagous ectoparasites of domestic mammals and/or spleens of wild animals in El Tarf and Souk Ahras, Algeria. Methods: Using real-time PCR, standard PCR and sequencing, the presence of Bartonella spp., Rickettsia spp., Borrelia spp. and Coxiella burnetii was evaluated in 268/1626 ticks, 136 fleas, 11 Nycteribiidae flies and 16 spleens of domestic and/or wild animals from the El Tarf and Souk Ahras areas. Results: For the first time in Algeria, Bartonella tamiae was detected in 12/19 (63.2 %) Ixodes vespertilionis ticks, 8/11 (72.7 %) Nycteribiidae spp. flies and in 6/10 (60 %) bat spleens (Chiroptera spp.). DNA from Coxiella burnetii, the agent of Q fever, was also identified in 3/19 (15.8 %) I. vespertilionis from bats. Rickettsia slovaca, the agent of tick-borne lymphadenopathy, was detected in 1/1 (100 %) Haemaphysalis punctata and 2/3 (66.7 %) Dermacentor marginatus ticks collected from two boars (Sus scrofa algira) respectively. Ri. massiliae, an agent of spotted fever, was detected in 38/94 (40.4 %) Rhipicephalus sanguineus sensu lato collected from cattle, sheep, dogs, boars and jackals. DNA of Ri. aeschlimannii was detected in 6/20 (30 %) Hyalomma anatolicum excavatum and 6/20 (30 %) Hy. scupense from cattle. Finally, Ri. felis, an emerging rickettsial pathogen, was detected in 80/110 (72.7 %) Archaeopsylla erinacei and 2/2 (100 %) Ctenocephalides felis of hedgehogs (Atelerix algirus). Conclusion: In this study, we expanded knowledge about the repertoire of ticks and flea-borne bacteria present in ectoparasites and/or tissues of domestic and wild animals in Algeria. [ABSTRACT FROM AUTHOR]

Published
2016
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32. Draft genome of Gemmata massiliana sp. nov, a water-borne Planctomycetes species exhibiting two variants.

Author

Aghnatios, Rita, Cayrou, Caroline, Garibal, Marc, Robert, Catherine, Azza, Said, Raoult, Didier, and Drancourt, Michel

Subjects
GENOMES, PEPTIDOGLYCANS, CHROMOSOMES, RIBOSOMAL RNA, HYPOTHETICAL particles, CULTURE media (Biology)
Abstract

Gemmata massiliana is a new Planctomycetes bacterium isolated from a hospital water network in France, using a new culture medium. It is an aerobic microorganism with optimal growth at pH 8, at 30 °C and salinity ≤ 1.25 % NaCl. G. massiliana is resistant to β-lactam antibiotics, due to lack of peptidoglycan in its cell wall. G. massiliana shares a 97 % 16S rRNA gene sequence similarity with the nearest species, Gemmata obscuriglobus; and 99 % similarity with unnamed soil isolates . Its 9,249,437-bp genome consists in one chromosome and no detectable plasmid and has a 64.07 % G + C content, 32.94 % of genes encoding for hypothetical proteins. The genome contains an incomplete 19.6-kb phage sequence, 26 CRISPRs, 3 CAS and 15 clusters of secondary metabolites. G. massiliana genome increases knowledge of a poorly known world of bacteria. [ABSTRACT FROM AUTHOR]

Published
2015
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33. Genome sequence and description of Pantoea septica strain FF5.

Author

Lo, Cheikh, Padhmanabhan, Roshan, Mediannikov, Oleg, Nguyen, Thi, Raoult, Didier, Fournier, Pierre-Edouard, and Fenollar, Florence

Subjects
ENTEROBACTERIACEAE, PANTOEA, GENOMES, GENES, CHROMOSOMES
Abstract

Strain FF5 was isolated from the skin flora of a healthy Senegalese 35-year-old woman. This strain was identified as belonging to the species Pantoea septica based on rpoB sequence identity of 99.7 % with Pantoea septica strain LMG 5345 and a highest MALDI-TOF-MS score of 2.3 with Pantoea septica. Like P. septica, this FF5 strain is a Gram-negative, aerobic, motile, and rod-shaped bacterium. Currently, 17 genomes have been sequenced within the genus Pantoea but none for Pantoea septica. Herein, we compared the genomic properties of strain FF5 to those of other species within the genus Pantoea. The genome of this strain is 4,548,444 bp in length (1 chromosome, no plasmid) with a G + C content of 59.1 % containing 4125 protein-coding and 68 RNA genes (including 2 rRNA operons). We also performed an extensive phenotypic analysis showing new phenotypic characteristics such as the production of alkaline phosphatase, acid phosphatase and naphthol-AS-BI-phosphohydrolase. [ABSTRACT FROM AUTHOR]

Published
2015
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34. Genome sequence of Oceanobacillus picturae strain S1, an halophilic bacterium first isolated in human gut.

Author

Lagier, Jean-Christophe, Khelaifia, Saber, Azhar, Esam, Croce, Olivier, Bibi, Fehmida, Jiman-Fatani, Asif, Yasir, Muhammad, Helaby, Huda, Robert, Catherine, Fournier, Pierre-Edouard, and Raoult, Didier

Subjects
HALOBACTERIUM, BACTERIAL genomes, GUT microbiome, MATRIX-assisted laser desorption-ionization, MEDICAL microbiology, GENETIC code
Abstract

Oceanobacillus picturae is a strain of a moderately halophilic bacterium, first isolated from a mural painting. We demonstrate, for the first time, the culture of human Oceanobacillus picturae, strain S1, whose genome is described here, from a stool sample collected from a 25-year-old Saoudian healthy individual. We used a slightly modified standard culture medium adding 100 g/L of NaCl. We provide a short description of this strain including its MALDI-TOF spectrum, the main identification tool currently used in clinical microbiology. The 3,675,175 bp long genome exhibits a G + C content of 39.15 % and contains 3666 protein-coding and 157 RNA genes. The draft genome sequence of Oceanobacillus picturae has a similar size to the Oceanobacillus kimchii (respectively 3.67 Mb versus 3.83 Mb). The G + C content was higher compared with Oceanobacillus kimchii (respectively 39.15 % and 35.2 %). Oceanobacillus picturae shared almost identical number of genes (3823 genes versus 3879 genes), with a similar ratio of genes per Mb (1041 genes/Mb versus 1012 genes/Mb). The genome sequencing of Oceanobacillus picturae strain S1 isolated for the first time in a human, will be added to the 778 genome projects from the gastrointestinal tract listed by the international consortium Human Microbiome Project. [ABSTRACT FROM AUTHOR]

Published
2015
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35. Screen-and-treat program by point-of-care of Atopobium vaginae and Gardnerella vaginalis in preventing preterm birth (AuTop trial): study protocol for a randomized controlled trial.

Author

Bretelle, Florence, Fenollar, Florence, Baumstarck, Karine, Fortanier, Cécile, Cocallemen, Jean François, Serazin, Valérie, Raoult, Didier, Auquier, Pascal, and Loubière, Sandrine

Subjects
MEDICAL screening, POINT-of-care testing, GARDNERELLA, PREMATURE labor prevention, RANDOMIZED controlled trials, BACTERIAL vaginitis, COST effectiveness, MOLECULAR diagnosis, ANTIBIOTICS, COMMUNICABLE disease diagnosis, BACTERIAL vaginitis diagnosis, CLINICAL medicine, MEDICAL databases, INFORMATION storage & retrieval systems, BACTERIAL growth, BACTERIOLOGY technique, COMMUNICABLE diseases, COMPARATIVE studies, DNA, EXPERIMENTAL design, GESTATIONAL age, HOSPITAL costs, PREMATURE infants, RESEARCH methodology, MEDICAL care costs, MEDICAL cooperation, RESEARCH protocols, MICROBIOLOGICAL techniques, POLYMERASE chain reaction, RESEARCH, PREGNANCY complications, EVALUATION research, TREATMENT effectiveness, PREDICTIVE tests, ACTINOBACTERIA, ECONOMICS, DIAGNOSIS, PREVENTION
Abstract

Background: International recommendations in favor of screening for vaginal infection in pregnancy are based on heterogeneous criteria. In most developed countries, the diagnosis of bacterial vaginosis is only recommended for women with high-risk of preterm birth. The Nugent score is currently used, but molecular quantification tools have recently been reported with a high sensitivity and specificity. Their value for reducing preterm birth rates and related complications remains unexplored. This trial was designed to assess the cost-effectiveness of a systematic screen-and-treat program based on a point-of-care technique for rapid molecular diagnosis, immediately followed by an appropriate antibiotic treatment, to detect the presence of abnormal vaginal flora (specifically, Atopobium vaginae and Gardnerella vaginalis) before 20 weeks of gestation in pregnant women in France. We hypothesized that this program would translate into significant reductions in both the rate of preterm births and the medical costs associated with preterm birth.Methods/design: A multicenter, open-label randomized controlled trial (RCT) will be conducted in which 20 French obstetrics and gynecology centers will recruit eligible pregnant women at less than 20 weeks gestation with singleton pregnancy and with a low-risk factor for preterm birth. Interventions will include a) an experimental group that will receive a systematic rapid screen-and-treat program from a point-of-care analysis using a molecular quantification method and b) a control group that will receive usual care management. Randomization will be in a 1:1 allocation ratio. The primary endpoint that will be assessed over a period of 12 months will be the incremental cost-effectiveness ratio (ICER) expressed as cost per avoided preterm birth before 37 weeks. Secondary endpoints will include ICER per avoided preterm birth before 24, 28 and 32 weeks, obstetrical outcomes, neonatal outcomes, rates of treatment failure and recurrence episodes for positive women. Uncertainty surrounding these estimates will be addressed using nonparametric bootstrapping and represented using cost-effectiveness acceptability curves. A total of 6,800 pregnant women will be included.Discussion: This appropriate randomized controlled design will provide insight into the cost-effectiveness and therefore the potential cost savings of a rapid screen-and-treat strategy for molecular abnormal vaginal flora in pregnant women. National and international recommendations could be updated based on the findings of this study.Trial Registration: ClinicalTrials.gov: NCT02288832 (registration date: 30 October 2014); Eudract: 2014-001559-22. [ABSTRACT FROM AUTHOR]

Published
2015
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36. Pan-genomic analysis to redefine species and subspecies based on quantum discontinuous variation: the Klebsiella paradigm.

Author

Caputo, Aurélia, Merhej, Vicky, Georgiades, Kalliopi, Fournier, Pierre-Edouard, Croce, Olivier, Robert, Catherine, and Raoult, Didier

Subjects
CLADISTIC analysis, NUCLEIC acid hybridization, KLEBSIELLA pneumoniae, TAXONOMY
Abstract

Background: Various methods are currently used to define species and are based on the phylogenetic marker 16S ribosomal RNA gene sequence, DNA-DNA hybridization and DNA GC content. However, these are restricted genetic tools and showed significant limitations. Results: In this work, we describe an alternative method to build taxonomy by analyzing the pan-genome composition of different species of the Klebsiella genus. Klebsiella species are Gram-negative bacilli belonging to the large Enterobacteriaceae family. Interestingly, when comparing the core/pan-genome ratio; we found a clear discontinuous variation that can define a new species. Conclusions: Using this pan-genomic approach, we showed that Klebsiella pneumoniae subsp. ozaenae and Klebsiella pneumoniae subsp. rhinoscleromatis are species of the Klebsiella genus, rather than subspecies of Klebsiella pneumoniae. This pan-genomic analysis, helped to develop a new tool for defining species introducing a quantic perspective for taxonomy. Reviewers: This article was reviewed by William Martin, Pierre Pontarotti and Pere Puigbo (nominated by Dr Yuri Wolf). [ABSTRACT FROM AUTHOR]

Published
2015
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37. Non-contiguous finished genome sequence and description of Clostridium ihumii sp. nov.

Author

Merhej, Vicky, Pfleiderer, Anne, Ramasamy, Dhamodharan, Lagier, Jean-Christophe, Michelle, Caroline, Raoult, Didier, and Fournier, Pierre-Edouard

Abstract

Clostridium ihumii strain AP5 sp. nov. is a new species within the genus Clostridium. This strain, whose genome is described here, was isolated from the stool sample of a 21-year-old French Caucasian female with anorexia nervosa. C. ihumii is a Gram-positive, anaerobic bacillus. Here we describe the features of this organism, together with the complete genome sequence and annotation. The 4,433,668 bp long genome contains 4,076 protein-coding and 85 RNA genes, including 9 rRNA genes. [ABSTRACT FROM AUTHOR]

Published
2015
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38. Non contiguous-finished genome sequence and description of Bacillus jeddahensis sp. nov.

Author

Bittar, Fadi, Bibi, Fehmida, Ramasamy, Dhamodharan, Lagier, Jean-Christophe, Azhar, Esam I., Jiman-Fatani, Asif A., Al-Ghamdi, Ahmed K., Ti Thien Nguyen, Yasir, Muhammad, Fournier, Pierre-Edouard, and Raoult, Didier

Subjects
BACILLUS genetics, OVERWEIGHT men, FECAL analysis, NUCLEIC acid hybridization, NUCLEOTIDE sequencing
Abstract

Strain JCET was isolated from the fecal sample of a 24-year-old obese man living in Jeddah, Saudi Arabia. It is an aerobic, Gram-positive, rod-shaped bacterium. This strain exhibits a 16S rRNA nucleotide sequence similarity of 97.5% with Bacillus niacini, the phylogenetically closest species with standing nomenclature. Moreover, the strain JCETpresents many phenotypic differences, when it is compared to other Bacillus species, and shows a low MALDI-TOF Mass Spectrometry score that does not allow any identification. Thus, it is likely that this strain represents a new species. Here we describe the features of this organism, together with the complete genome sequence and annotation. The 4,762,944 bp long genome (1 chromosome but no plasmid) contains 4,654 protein-coding and 98 RNAs genes, including 92 tRNA genes. The strain JCETdiffers from most of the other closely Bacillus species by more than 1% in G + C content. In addition, digital DNA-DNA hybridization values for the genome of the strain JCET against the closest Bacillus genomes range between 19.5 to 28.1, that confirming again its new species status. On the basis of these polyphasic data made of phenotypic and genomic analyses, we propose the creation of Bacillus jeddahensis sp. nov. that contains the strain JCET. [ABSTRACT FROM AUTHOR]

Published
2015
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39. Influenza-attributable deaths in south-eastern France (1999 to 2010): mortality predictions were undependable.

Author

Thiberville, Simon-Djamel, Gaudart, Jean, Raoult, Didier, and Charrel, Remi N.

Subjects
PUBLIC health, INFLUENZA A virus, H1N1 subtype, PANDEMICS, MORTALITY, POISSON processes
Abstract

Background: Following the 2009 influenza pandemic, several studies showed that the mortality pattern associated with the A(H1N1)2009 virus primarily affected children and young adults. In this study, we aimed to estimate the influenza-attributable deaths during the periods from 1999 to 2010, in the Provence-Alpes-Côte-d'Azur (PACA) region of south-eastern France in order to corroborate the hypothesis that (i) influenza-attributable deaths caused by A(H1N1)2009 strain were much lower than initially expected. Methods: In order to compare our results with published data, we used the same statistical model of an Austrian team, using a Poisson model adjusted on co-circulating respiratory syncytial virus to explain the weekly mortality. Results: We assessed that 5.7 % of the respiratory deaths were attributable to influenza virus during the 2009-2010 pandemic season. This mortality was lower than that observed during the ten preceding epidemic periods (13.8 % on average). Age group- based analysis revealed that during the pandemic period, the groups under 65 had a systematically higher excess of respiratory mortality while the age group over 65 had a much lower mortality than during the seasonal epidemic seasons. Similarly, among the less specific outcome (non violent and cardiovascular mortality) the age groups over 45 had higher excess of mortality during the seasonal epidemics than during the pandemic period. Conclusions: Since most of the influenza mortality is commonly observed in the elderly group (>65 year-old), the moderate elderly mortality during the 2009 pandemic period has impacted the total mortality, and has resulted in a reduced total mortality despite an increased mortality in the young age group. Despite using identical parameters and the same approach as in a previously published study using an Austrian population sample, we observed a lower excess respiratory mortality in the south-eastern France than in Vienna. Thus, the pandemic virus caused less death than the epidemic viruses that circulated during the preceding years. In contrast with catastrophic predictions made in the early phase of the pandemic, human lives were saved during the circulation period of A(H1N1)2009 virus, resulting in a lower overall mortality. [ABSTRACT FROM AUTHOR]

Published
2015
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40. Positron emission tomography in the diagnosis of Whipple's endocarditis: a case report.

Author

Jos, Sarah-Lyne, Angelakis, Emmanouil, Caus, Thierry, and Raoult, Didier

Subjects
ENDOCARDITIS, FLUORODEOXYGLUCOSE F18, IMMUNOHISTOCHEMISTRY, POSITRON emission tomography, POSITRON emission
Abstract

Background: Whipple's disease is a systemic infection that sometimes is associated with cardiac manifestations. The diagnosis of Tropheryma whipplei endocarditis is still the result of chance because there are no diagnostic criteria and clinical signs are often those of cardiac disease rather than infection. Case presentation: Culture-negative endocarditis was suspected in a non-febrile 77-year-old French woman from North France with a history of a graft replacement 4 years prior. Positron emission tomography revealed intense fluorodeoxyglucose uptake around the metal ring of the aortic graft. The valve was replaced, and T. whipplei was detected in a valve sample by molecular assays. Immunohistochemical staining of the valve for T. whipplei was also positive. Conclusion: The localization of infectious foci by positron emission tomography and systematically testing valve specimens for T. whipplei are promising for diagnosing Whipple's disease. [ABSTRACT FROM AUTHOR]

Published
2015
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41. Babela massiliensis, a representative of a widespread bacterial phylum with unusual adaptations to parasitism in amoebae.

Author

Pagnier, Isabelle, Yutin, Natalya, Croce, Olivier, Makarova, Kira S., Wolf, Yuri I., Benamar, Samia, Raoult, Didier, Koonin, Eugene V., and La Scola, Bernard

Subjects
BIOLOGICAL adaptation, PARASITISM, AMOEBIDA, ARCHAEBACTERIA, METAGENOMICS
Abstract

Background: Only a small fraction of bacteria and archaea that are identifiable by metagenomics can be grown on standard media. Recent efforts on deep metagenomics sequencing, single-cell genomics and the use of specialized culture conditions (culturomics) increasingly yield novel microbes some of which represent previously uncharacterized phyla and possess unusual biological traits. Results: We report isolation and genome analysis of Babela massiliensis, an obligate intracellular parasite of Acanthamoeba castellanii. B. massiliensis shows an unusual, fission mode of cell multiplication whereby large, polymorphic bodies accumulate in the cytoplasm of infected amoeba and then split into mature bacterial cells. This unique mechanism of cell division is associated with a deep degradation of the cell division machinery and delayed expression of the ftsZ gene. The genome of B. massiliensis consists of a circular chromosome approximately 1.12 megabase in size that encodes, 981 predicted proteins, 38 tRNAs and one typical rRNA operon. Phylogenetic analysis shows that B. massiliensis belongs to the putative bacterial phylum TM6 that so far was represented by the draft genome of the JCVI TM6SC1 bacterium obtained by single cell genomics and numerous environmental sequences. Conclusions: Currently, B. massiliensis is the only cultivated member of the putative TM6 phylum. Phylogenomic analysis shows diverse taxonomic affinities for B. massiliensis genes, suggestive of multiple gene acquisitions via horizontal transfer from other bacteria and eukaryotes. Horizontal gene transfer is likely to be facilitated by the cohabitation of diverse parasites and symbionts inside amoeba. B. massiliensis encompasses many genes encoding proteins implicated in parasite-host interaction including the greatest number of ankyrin repeats among sequenced bacteria and diverse proteins related to the ubiquitin system. Characterization of B. massiliensis, a representative of a distinct bacterial phylum, thanks to its ability to grow in amoeba, reaffirms the critical role of diverse culture approaches in microbiology. [ABSTRACT FROM AUTHOR]

Published
2015
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42. Whole-genome assembly of Akkermansia muciniphila sequenced directly from human stool.

Author

Caputo, Aurélia, Dubourg, Grégory, Croce, Olivier, Gupta, Sushim, Robert, Catherine, Papazian, Laurent, Rolain, Jean-Marc, and Raoult, Didier

Subjects
DRUG resistance in bacteria, BACTERIAL population, ANTI-infective agents, BACTERIAL colonies, IMIPENEM, AKKERMANSIA muciniphila, METAGENOMICS, ENTEROCOCCUS
Abstract

Background: Alterations in gut microbiota composition under antibiotic pressure have been widely studied, revealing a restricted diversity of gut flora, including colonization by organisms such as Enterococci, while their impact on bacterial load is variable. High-level colonization by Akkermansia muciniphila, ranging from 39% to 84% of the total bacterial population, has been recently reported in two patients being treated with broad-spectrum antibiotics, although attempts to cultivate this microorganism have been unsuccessful. Results: Here, we propose an original approach of genome sequencing for Akkermansia muciniphila directly from the stool sample collected from one of these patients. We performed and assembly using metagenomic data obtained from the stool sample. We used a mapping method consisting of aligning metagenomic sequencing reads against the reference genome of the Akkermansia muciniphila MucT strain, and a De novo assembly to support this mapping method. We obtained draft genome of the Akkermansia muciniphila strain Urmite with only 56 gaps. The absence of particular metabolic requirement as possible explanation of our inability to culture this microorganism, suggests that the bacterium was dead before the inoculation of the stool sample. Additional antibiotic resistance genes were found following comparison with the reference genome, providing some clues pertaining to its survival and colonization in the gut of a patient treated with broad-spectrum antimicrobial agents. However, no gene coding for imipenem resistance was detected, although this antibiotic was a part of the patient's antibiotic regimen. Conclusions: This work highlights the potential of metagenomics to facilitate the assembly of genomes directly from human stool. [ABSTRACT FROM AUTHOR]

Published
2015
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43. MALDI-TOF mass spectrometry and identification of new bacteria species in air samples from Makkah, Saudi Arabia.

Author

Angelakis, Emmanouil, Yasir, Muhammad, Azhar, Esam I., Papadioti, Anastasia, Bibi, Fehmida, Aburizaiza, Asad S., Metidji, Sarah, Memish, Ziad A., Ashshi, Ahmad M., Hassan, Ahmed M., Harakeh, Steve, Gautret, Philippe, and Raoult, Didier

Subjects
RESPIRATORY diseases, MASS spectrometry, AIR pollution, PILGRIMAGE to Mecca
Abstract

Background During the Hajj season, respiratory symptoms are very common among pilgrims. Here, we investigated the viable bacterial population in air samples collected around the slaughterhouses used during the Hajj. Methods and results We collected air samples on three days from four different sites: slaughterhouses at Al-Kakia, Al-Meaisim and Al-Sharaia, and from a waste disposal area designated for the remnants of slaughter. Samples were cultured on blood agar plates for 48 h, and bacterial isolates were identified using MALDI-TOF MS. A dendrogram using the spectra of the unidentified bacterial species was constructed, and PCR amplification and sequencing of the 16S rRNA gene was performed for one isolate per cluster. In total, 2500 colonies appeared on the nutrient agar plates, and 244 were purified for further analysis. Good identification was obtained for 202 (83%) isolates by MALDI-TOF MS. The most common genera were Bacillus (n = 94, 45%) and Staphyloccocus (n = 55, 26%). Poor identification was obtained for 42 (17%) isolates, and their spectra clustering revealed that these isolates belonged to 10 species. Four of these were considered to be new species. Conclusions During the Hajj, the air was contaminated by many environmental bacterial agents, and MALDI-TOF MS was successfully adapted for their rapid identification. [ABSTRACT FROM AUTHOR]

Published
2014
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44. Non-contiguous finished genome sequence and description of Fenollaria massiliensis gen. nov., sp. nov., a new genus of anaerobic bacterium.

Author

Pagnier, Isabelle, Croce, Olivier, Robert, Catherine, Raoult, Didier, and Scola, Bernard

Subjects
GENOMES, RIBOSOMAL RNA, GENES, PROTEINS, BIOMOLECULES
Abstract

Fenollaria massiliensis strain 9401234, is the type strain of Fenollaria massiliensis gen. nov., sp. nov., a new species within a new genus Fenollaria. This strain, whose genome is described here, was isolated from an osteoarticular sample. F. massiliensis strain 9401234 is an obligate anaerobic Gram-negative bacillus. Here we describe the features of this organism, together with the complete genome sequence and annotation. The 1.71 Mbp long genome exhibits a G+C content of 34.46% and contains 1,667 protein-coding and 30 RNA genes, including 3 rRNA genes. [ABSTRACT FROM AUTHOR]

Published
2014
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45. Non-contiguous finished genome sequence and description of Bacteroides neonati sp. nov., a new species of anaerobic bacterium.

Author

Cassir, Nadim, Croce, Olivier, Pagnier, Isabelle, Benamar, Samia, Couderc, Carine, Robert, Catherine, Raoult, Didier, and Scola, Bernard

Subjects
BACTEROIDACEAE, BIOLOGICAL classification, GENETICS, BACTEROIDES, GENOMES
Abstract

Bacteroides neonati strain MS4, is the type strain of Bacteroides neonati sp. nov., a new species within the genus Bacteroides. This strain, whose genome is described here, was isolated from a premature neonate stool sample. B. neonati strain MS4 is an obligate anaerobic Gram-negative bacillus. Here we describe the features of this organism, together with the complete genome sequence and annotation. The 5.03 Mbp long genome exhibits a G+C content of 43.53% and contains 4,415 protein-coding and 91 RNA genes, including 9 rRNA genes. [ABSTRACT FROM AUTHOR]

Published
2014
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46. Non-contiguous finished genome sequence and description of Gorillibacterium massiliense gen. nov, sp. nov., a new member of the family Paenibacillaceae.

Author

Keita, Mamadou, Padhmanabhan, Roshan, Caputo, Aurélia, Robert, Catherine, Delaporte, Eric, Raoult, Didier, Fournier, Pierre-Edouard, and Bittar, Fadi

Subjects
GENOMES, TRANSFER RNA, PLASMIDS, CYTOPLASMIC inheritance, GENETIC vectors
Abstract

Strain G5 gen. nov., sp. nov. is the type strain of Gorillibacterium massiliense, a newly proposed genus within the family Paenibacillaceae. This strain, whose genome is described here, was isolated in France from a stool sample of a wild Gorilla gorilla subsp. gorilla from Cameroon. G. massiliense is a facultatively anaerobic, Gram negative rod. Here we describe the features of this bacterium, together with the complete genome sequence and annotation. The 5,546,433 bp long genome (1 chromosome but no plasmid) contains 5,145 protein-coding and 76 RNA genes, including 69 tRNA genes. [ABSTRACT FROM AUTHOR]

Published
2014
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47. Genome sequence and description of Nesterenkonia massiliensis sp. nov. strain NP1.

Author

Edouard, Sophie, Sankar, Senthil, Dangui, Nicole, Lagier, Jean-Christophe, Michelle, Caroline, Raoult, Didier, and Fournier, Pierre-Edouard

Subjects
GENOMES, RIBOSOMAL RNA, GENES, PROTEINS, BIOMOLECULES
Abstract

Nesterenkonia massiliensis sp. nov., strain NP1, is the type strain of Nesterenkonia massiliensis sp. nov., a new species within the genus Nesterenkonia. This strain, whose genome is described here, was isolated from the feces of a 32-year-old French woman suffering from AIDS and living in Marseille. Nesterenkonia massiliensis is a Gram-positive aerobic coccus. Here, we describe the features of this bacterium, together with the complete genome sequencing and annotation. The 2,726,371 bp long genome (one chromosome but no plasmid) contains 2,663 protein-coding and 51 RNA genes, including 1 rRNA operon. [ABSTRACT FROM AUTHOR]

Published
2014
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48. Non-contiguous finished genome sequence of Corynebacterium timonense type strain 5401744.

Author

Roux, Véronique, Robert, Catherine, and Raoult, Didier

Subjects
CORYNEBACTERIACEAE, CORYNEBACTERIUM, GENOMES, GENES, PROTEINS
Abstract

Corynebacterium timonense strain 5401744 is a member of the genus Corynebacterium which contains Gram-positive bacteria with a high G+C content. It was isolated from the blood of a patient with endocarditis. In this work, we describe a set of features of this organism, together with the complete genome sequence and annotation. The 2,553,575 bp long genome contains 2,401 protein-coding genes and 55 RNA genes, including between 5 and 6 rRNA operons. [ABSTRACT FROM AUTHOR]

Published
2014
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49. Non-contiguous finished genome sequence and description of Corynebacterium jeddahense sp. nov.

Author

Edouard, Sophie, Bibi, Fehmida, Dhamodharan, Ramasamy, Lagier, Jean-Christophe, Azhar, Esam, Robert, Catherine, Caputo, Aurelia, Yasir, Muhammad, Jiman-Fatani, Asif, Alawi, Maha, Fournier, Pierre-Edouard, and Raoult, Didier

Subjects
CORYNEBACTERIUM diseases, GENOMES, CHROMOSOMES, RNA, GENES, CATTLE
Abstract

Corynebacterium jeddahense sp. nov., strain JCB, is the type strain of Corynebacterium jeddahense sp. nov., a new species within the genus Corynebacterium. This strain, whose genome is described here, was isolated from fecal flora of a 24-year-old Saudi male suffering from morbid obesity. Corynebacterium jeddahense is a Gram-positive, facultative anaerobic, nonsporulating bacillus. Here, we describe the features of this bacterium, together with the complete genome sequencing and annotation, and compare it to other member of the genus Corynebacterium. The 2,472,125 bp-long genome (1 chromosome but not plasmid) contains 2,359 protein-coding and 53 RNA genes, including 1 rRNA operon. [ABSTRACT FROM AUTHOR]

Published
2014
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50. Non contiguous-finished genome sequence and description of Enorma timonensis sp. nov.

Author

Ramasamy, Dhamodaran, Dubourg, Gregory, Robert, Catherine, Caputo, Aurelia, Papazian, Laurent, Raoult, Didier, and Fournier, Pierre-Edouard

Subjects
GENOMES, RIBOSOMAL RNA, PROTEINS, BIOMOLECULES, GENETICS
Abstract

Enorma timonensis strain GD5 sp. nov., is the type strain of E. timonensis sp. nov., a new member of the genus Enorma within the family Coriobacteriaceae. This strain, whose genome is described here, was isolated from the fecal flora of a 53-year-old woman hospitalized for 3 months in an intensive care unit. E. timonensis is an obligate anaerobic rod. Here we describe the features of this organism, together with the complete genome sequence and annotation. The 2,365,123 bp long genome (1 chromosome but no plasmid) contains 2,060 protein-coding and 52 RNA genes, including 4 rRNA genes. [ABSTRACT FROM AUTHOR]

Published
2014
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