Your search keyword '"Bacterial identification"' showing total 22 results

1. Integrating rapid pathogen identification and antimicrobial susceptibility testing through multiplex TaqMan qPCR assay.

Author

Xie, Libo, Yang, Min, Liu, Min, Li, Qianyuan, Luo, Chunhua, and Luo, Jun

Subjects

*ACINETOBACTER baumannii, *MICROBIAL sensitivity tests, *POLYMERASE chain reaction, *DNA folding, *NUCLEOTIDE sequence, *KLEBSIELLA pneumoniae

Abstract

Timely bacterial identification (ID) and antimicrobial susceptibility testing (AST) are of significance for therapy of bacteria-infected patients. In the present study, we developed a multiplex TaqMan qPCR assay for rapid and accurate ID and AST of three common hospital acquired pneumonia species, namely Acinetobacter baumannii , Klebsiella pneumoniae and Staphylococcus aureus. In this assay, DNA extraction and bacterial co-incubation with antibiotics are accomplished based on a common PCR instrument. ID of three bacteria is based on specific conserved DNA sequence fragment (gltA for A. baumannii , phoE for K. pneumoniae and nuc for S. aureus) detection through multiplex TaqMan qPCR assay within 80 min. AST of three bacteria could be acquired within 200 min based on genomic DNA fold change detection after 2 h of antibiotic exposure. Testing of 23 bronchoalveolar lavage fluid samples spiked by different A. baumannii isolates, 20 bronchoalveolar lavage fluid samples spiked by different K. pneumoniae isolates, and 14 bronchoalveolar lavage fluid samples spiked by different S. aureus isolates showed that the multiplex TaqMan qPCR assay had 100% (95% CI: 85.69–100), 100% (95% CI: 83.89–100) and 100% (95% CI:78.47–100) identification agreement with the initial spiked bacteria. Subsequent AST results compared with the standard broth microdilution method showed an overall agreement of 91.30% (95% CI: 73.20 to 97.58) for A. baumannii , 90% (95% CI: 69.90 to 97.21) for K. pneumoniae and 92.86% (95% CI: 68.53 to 98.73) for S. aureus based on the current multiplex TaqMan assay. Due to the high rapidity, good agreement, simplicity, and high throughput, this multiplex TaqMan assay could be helpful for ID and broad-spectrum AST in A. baumannii , K. pneumoniae and S. aureus , as well as potentially applicable for other clinical bacteria by changing the primers and probes. • DNA extraction by thermo-cold lysis reduces time, cost and contamination. • The assay has many advantages including rapidity, good agreement and simplicity. • The multiplex TaqMan assay is helpful for bacterial ID and broad-spectrum AST. • By changing primers and probes, the methodology could be applied broadly. [ABSTRACT FROM AUTHOR]

Published

2024

2. Identification of bacterial isolates from a public hospital in Australia using complexity-reduced genotyping.

Author

Talamantes-Becerra, Berenice, Carling, Jason, Kennedy, Karina, Gahan, Michelle E., and Georges, Arthur

Subjects

*BACTERIAL genomes, *PUBLIC hospitals, *DNA analysis, *HOSPITAL utilization, *DNA data banks, *NUCLEOTIDE sequencing

Abstract

Abstract Bacterial identification methods used in routine identification of pathogens in medical microbiology include a combination approach of biochemical tests, mass spectrometry or molecular biology techniques. Extensive publicly-available databases of DNA sequence data from pathogenic bacteria have been amassed in recent years; this provides an opportunity for using bacterial genome sequencing for identification purposes. Whole genome sequencing is increasing in popularity, although at present it remains a relatively expensive approach to bacterial identification and typing. Complexity-reduced bacterial genome sequencing provides an alternative. We evaluate genomic complexity-reduction using restriction enzymes and sequencing to identify bacterial isolates. A total of 165 bacterial isolates from hospital patients in the Australian Capital Territory, between 2013 and 2015 were used in this study. They were identified and typed by the Microbiology Department of Canberra Public Hospital, and represented 14 bacterial species. DNA extractions from these samples were processed using a combination of the restriction enzymes Pst I with Mse I, Pst I with Hpa II and Mse I with Hpa II. The resulting sequences (length 30–69 bp) were aligned against publicly available bacterial genome and plasmid sequences. Results of the alignment were processed using a bioinformatics pipeline developed for this project, Currito3.1 DNA Fragment Analysis Software. All 165 samples were correctly identified to genus and species by each of the three combinations of restriction enzymes. A further 35 samples typed to the level of strain identified and compared for consistency with MLST typing data and in silico MLST data derived from the nearest sequenced candidate reference. The high level of agreement between bacterial identification using complexity-reduced genome sequencing and standard hospital identifications indicating that this new approach is a viable alternative for identification of bacterial isolates derived from pathology specimens. The effectiveness of species identification and in particular, strain typing, depends on access to a comprehensive and taxonomically accurate bacterial genome sequence database containing relevant bacterial species and strains. Graphical abastract Unlabelled Image Highlights • All complexity-reduced methods identified correctly all samples up to strain level. • Mse I- Hpa II complexity-reduced genotyping method provides better genome coverage. • Strain typing is effective with comprehensive bacterial genome database. [ABSTRACT FROM AUTHOR]

Published

2019

3. Application of the biocopolymer preparation system, rapid BACpro® II kit, for mass-spectrometry-based bacterial identification from positive blood culture bottles by the MALDI Biotyper system.

Author

Tsuchida, Sachio, Murata, Syota, Miyabe, Akiko, Satoh, Mamoru, Takiwaki, Masaki, Ashizawa, Kazuho, Terada, Takashi, Ito, Daisuke, Matsushita, Kazuyuki, and Nomura, Fumio

Subjects

*MEDICAL polymers, *BACTERIAL typing, *MATRIX-assisted laser desorption-ionization, *GRAM-positive bacteria, *POLYSTYRENE

Abstract

Abstract Matrix-assisted laser desorption ionization time-of-flight mass spectrometry (MALDI-TOF MS) is increasingly used for identification of microorganisms from positive blood cultures. Pretreatments to effectively remove non-bacterial components and selectively collect microorganisms are a prerequisite for successful identification, and a variety of home-brew and commercial protocols have been reported. Although commercially available kits, mainly the Sepsityper Kit, are increasingly used, the identification rates reported often are not satisfactory, particularly for Gram-positive isolates. We recently developed a method to collect bacteria from positive blood culture bottles using a polyallylamine-polystyrene copolymer that has been used in wastewater processing. This pretreatment protocol is now commercially available as the rapid BACpro® II kit (Nittobo Medical Co., Tokyo, Japan). The operation time required for processing using this novel kit is approximately 10 min, and the entire procedure can be completed within a biosafety cabinet. Since the performance of the rapid BACpro® II kit has not been tested using the MALDI Biotyper system, we prospectively evaluated the performance of the rapid BACpro® II kit as compared with the Sepsityper® kit. Performance of the rapid BACpro® II kit was evaluated using a total of 193 monomicrobial cases of positive blood culture. Medium from blood culture bottles was pretreated by the rapid BACpro® II kit or the Sepsityper® Kit, and isolated cells were subjected to direct identification by MS fingerprinting in parallel with conventional subculturing for reference identification. The overall MALDI-TOF MS-based identification rates with >1.7 score and >2.0 score obtained using the rapid BACpro® II kit were 99.5% and 80.8%, respectively, whereas those obtained using the Sepsityper® Kit were 89.1% and 68.4%, respectively (P < 0.05 for >1.7 and P < 0.05 for >2.0 by Pearsons's chi-square). In Gram-positive cases, the rapid BACpro® II kit gave identification rate of 100% with >1.7 score and 69.4% with >2.0 score, whereas there were 84.7% and 56.8%, respectively by the Sepsityper® Kit (P < 0.05 for >1.7). These results are preliminary, but considering that this new kit is easy to perform and the identification rates are promising, the rapid BACpro® II kit deserves assessment in a larger-scale study with a variety of platforms for MS-based bacterial identification. Highlights • We prospectively evaluated the performance of the rapid BACpro® II kit. • The kit consists of four simple steps that can be done within a biosafety cabinet. • The kit protocol is a rapid method for collecting bacteria within about 10 min. [ABSTRACT FROM AUTHOR]

Published

2018

4. An improved in-house lysis-filtration protocol for bacterial identification from positive blood culture bottles with high identification rates by MALDI-TOF MS.

Author

Tsuchida, Sachio, Murata, Syota, Miyabe, Akiko, Satoh, Mamoru, Takiwaki, Masaki, Matsushita, Kazuyuki, and Nomura, Fumio

Subjects

*MICROORGANISMS, *MASS spectrometry, *MATRIX-assisted laser desorption-ionization, *AMMONIUM chloride, *GRAM-positive bacteria

Abstract

Matrix-assisted laser desorption ionization–time of flight mass spectrometry (MALDI-TOF MS) is now a well-established method for identification of microorganisms from positive blood cultures. Pretreatments to effectively remove non-bacterial proteins are a prerequisite for successful identification, and a variety of protocols have been reported. Although commercially available kits, mainly the Sepsityper Kit, are increasingly used, the identification rates reported often are not satisfactory, particularly for Gram-positive isolates. We developed a new, in-house lysis-filtration protocol and prospectively evaluated its performance compared to the Sepsityper kit. The in-house protocol consists of three simple steps: lysis by ammonium chloride, aspiration with a syringe fitted with a 0.45-μm membrane, and centrifugation to collect microbes. The novel protocol requires only 20 min. Performance of the in-house protocol was evaluated using a total of 117 monomicrobial cases of positive blood culture. Medium from blood culture bottles was pretreated by the in-house protocol or the commercial kit, and isolated cells were subjected to direct identification by mass spectrometry fingerprinting in parallel with conventional subculturing for reference identification. The overall MALDI-TOF MS-based identification rates with score > 1.7 and > 2.0 obtained using the in-house protocol were 99.2% and 85.5%, respectively, whereas those obtained using the Sepsityper Kit were 85.4% and 61.5%, respectively. For Gram-positive cases, the in-house protocol yielded scores >1.7 and > 2.0 at 98.5% and 76.1%, respectively, whereas the commercial kit yielded these scores at 76.1% and 43.3%, respectively. Although these are preliminary results, these values suggest that this easy lysis-filtration protocol deserves assessment in a larger-scale test. [ABSTRACT FROM AUTHOR]

Published

2018

5. Applications of copolymer for rapid identification of bacteria in blood culture broths using matrix-assisted laser desorption ionization time-of-flight mass spectrometry.

Author

Ashizawa, Kazuho, Murata, Syota, Terada, Takashi, Ito, Daisuke, Bunya, Masaru, Watanabe, Koji, Teruuchi, Yoko, Tsuchida, Sachio, Satoh, Mamoru, Nishimura, Motoi, Matsushita, Kazuyuki, Sugama, Yuji, and Nomura, Fumio

Subjects

*BLOOD testing, *BLOOD microbiology, *BLOOD sampling, *COPOLYMERS, *MATRIX-assisted laser desorption-ionization

Abstract

Matrix-assisted laser desorption ionization time-of-flight mass spectrometry (MALDI-TOF MS) can be used to identify pathogens in blood culture samples. However, sample pretreatment is needed for direct identification of microbes in blood culture bottles. Conventional protocols are complex and time-consuming. Therefore, in this study, we developed a method for collecting bacteria using polyallylamine–polystyrene copolymer for application in wastewater treatment technology. Using representative bacterial species Escherichia coli and Staphylococcus capitis , we found that polyallylamine–polystyrene can form visible aggregates with bacteria, which can be identified using MALDI-TOF MS. The processing time of our protocol was as short as 15 min. Hemoglobin interference in MALDI spectra analysis was significantly decreased in our method compared with the conventional method. In a preliminary experiment, we evaluated the use of our protocol to identify clinical isolates from blood culture bottles. MALDI-TOF MS-based identification of 17 strains from five bacterial species ( E. coli , Klebsiella pneumoniae , Enterococcus faecalis , S. aureus , and S. capitis ) collected by our protocol was satisfactory. Prospective large-scale studies are needed to further evaluate the clinical application of this novel and simple method of collecting bacteria in blood culture bottles. [ABSTRACT FROM AUTHOR]

Published

2017

6. Identification of microorganisms grown on chromogenic media by MALDI-TOF MS.

Author

Lüthje, Petra, Pranada, Arthur B., Carruthers-Lay, Duncan, Desjardins, Marc, Gaillot, Olivier, Wareham, David, Ciesielczuk, Holly, and Özenci, Volkan

Subjects

*CHROMOGENIC bacteria, *MEDICAL microbiology, *PATHOGENIC bacteria, *MATRIX-assisted laser desorption-ionization, *TIME-of-flight mass spectrometry

Abstract

Matrix-assisted laser desorption ionization-time of flight mass spectrometry (MALDI-TOF MS) and chromogenic media are widely used in clinical microbiology laboratories to facilitate the rapid selection and identification of pathogens. The aim of this study was to evaluate whether usage of chromogenic media limits the diagnostic performance of MALDI-TOF MS for microbial identification. A total of 386 microorganisms collected and analyzed at five laboratories were included. Isolates were cultured on relevant chromogenic media and non-selective agar plates in parallel and identified using the Bruker MALDI-TOF MS. Among the tested isolates, no misidentification was recorded and there was no medium-related difference in the identification level. However, score values were overall slightly but significantly lower for isolates grown on chromogenic media. In conclusion, the use of chromogenic culture media tested here had no relevant impact on MALDI-TOF MS performance for diagnostic purposes. [ABSTRACT FROM AUTHOR]

Published

2017

7. Optimal turnaround time for direct identification of microorganisms by mass spectrometry in blood culture.

Author

Randazzo, Adrien, Simon, Marc, Goffinet, Pierre, Classen, Jean-François, Hougardy, Nicolas, Pierre, Pascal, Kinzinger, Philippe, Mauel, Etienne, and Goffinet, Jean-Sébastien

Subjects

*MASS spectrometry, *DETECTION limit, *AGAR, *ENTEROBACTER cloacae, MICROORGANISM identification

Abstract

Introduction During the past few years, several studies describing direct identification of bacteria from blood culture using mass spectrometry have been published. These methods cannot, however, be easily integrated into a common laboratory workflow because of the high hands-on time they require. In this paper, we propose a new method of identification with a short hands-on time and a turnaround time shorter than 15 min. Materials and methods Positive blood bottles were homogenised and 600 μL of blood were transferred to an Eppendorf tube where 600 μL of lysis buffer were added. After homogenisation, a centrifugation step of 4 min at 10,500 g was performed and the supernatant was discarded. The pellet was then washed and loaded in quadruplicate into wells of a Vitek® MS-DS plate. Each well was covered with a saturated matrix solution and a MALDI-TOF mass spectrometry analysis was performed. Species were identified using the software Myla 3.2.0-2. Results We analysed 266 positive blood culture bottles. A microorganism grew in 261 cultures, while five bottles remained sterile after 48 h of incubation in subculture. Our method reaches a probability of detection at the species level of 77.8% (203/261) with a positive predictive value of 99.5% (202/203). Conclusion We developed a new method for the identification of microorganisms using mass spectrometry, directly performed from a positive blood culture. This method has short hands-on time and turnaround time and can easily take place in the workflow of a laboratory, with comparable results in performance with other methods reported in the literature. [ABSTRACT FROM AUTHOR]

Published

2016

8. MALDI-TOF MS database expansion for identification of Bacillus and related genera isolated from a pharmaceutical facility.

Author

Costa, Luciana Veloso da, Miranda, Rebeca Vitoria da Silva Lage de, Reis, Cristhiane Moura Falavina dos, Andrade, Joyce Modesto de, Cruz, Fernanda Ventura, Frazão, Adriana Marques, Fonseca, Erica Louro da, Ramos, Juliana Nunes, Brandão, Marcelo Luiz Lima, and Vieira, Verônica Viana

Subjects

*BACILLUS (Bacteria), *SPOREFORMING bacteria, *AEROBIC bacteria, *MASS spectrometry, *DATABASES

Abstract

Bacillus and related genera are among the main bacterial groups isolated from pharmaceutical production areas. The identification of Bacillus species and related genera by classical methods is particularly difficult, due to similarities between closely related species. The Matrix-Assisted Laser Desorption Ionization-Time of Flight Mass Spectrometry (MALDI-TOF MS) is one of the most promising techniques for chemotaxonomic characterization of microorganisms, being an alternative to genotypic methods. This study aimed to identify Bacillus strains and related genera isolated from immunobiological production areas by phylogenetic analysis of housekeeping genes and expand the database associated with MALDI-TOF MS to improve their identification. In a previous study, 97 aerobic endospore-forming bacteria isolated from a pharmaceutical facility were analyzed by MALDI-TOF MS and 16S rRNA gene full-length sequencing. All strains were identified as Bacillus and related genera by the latest methodology. Among the 97 strains, 22 were unidentified and 2 strains were misidentified by MALDI-TOF MS. In the present study, these 24 strains were subjected to 16S rRNA gene phylogenetic analysis. Strains not identified at species level by this methodology were submitted to rpoB gene phylogenetic analysis. After identifying the strains, 19 of the 24 strains were incubated for 24, 48, and 72 h on Tryptic Soy Agar and Sheep Blood Agar and subjected to analysis by MALDI-TOF MS. A SuperSpectrum for each strain was created and entered into the equipment database. Finally, the 24 strains were again submitted to proteomic analysis by MALDI-TOF MS, and, at this time, all were correctly identified. The genotypic identification of in-house isolated strains and the introduction of these spectra in MALDI-TOF MS, in order to obtain a customized database, proved to be an extremely effective tool in the identification of Bacillus and related genera from pharmaceutical industry origin. [Display omitted] • MALDI-TOF MS customized database was effective for spore-formers identification. • rpoB gene sequencing was not effective for all spore-formers species. • Species-level identification methodologies are necessary in pharmaceutical industry. • Nine isolates belonging to five possible new species were identified. • MALDI-TOF database must be improved to include pharmaceutical facilities species. [ABSTRACT FROM AUTHOR]

Published

2022

9. Systematic review and critical reflection on the isolation and identification methods for spoilage associated bacteria in fresh marine fish.

Author

Saelens, Ganna and Houf, Kurt

Subjects

*MARINE fishes, *CRITICAL thinking, *FISH microbiology, *IDENTIFICATION of fishes, *MARINE bacteria, *BACTERIAL diversity

Abstract

Consumers demand more fresh, safe, and high-quality food. As this is partiallycorrelated to the microbial profile, several microbiological examination tools are available. Incontrast to meat, no microbiological normalized methods to assess the microbiological quality of fresh marine fish have been agreed on. As a result, studies on the detection and diversity of spoilage associated organisms (SAOs) in fish often apply various detection, isolation, and identification techniques. This complicates the comparison and interpretation of data reported, and often results in different or inconclusive results. Therefore, the present review aimed to present a critical overview of the isolation/cultivation and detection techniques currently applied in fish microbiology. After a comprehensive search in the PubMed, Web of Science and Scopus databases, a total of 111 studies fulfilled the review selection criteria. Results revealed that when relying on culture media for the isolation of SAOs in fish, it is essential to include a salt-containing medium next to plate count agar that is currently used as the reference medium for the enumeration of bacteria on fish. In terms of identification, MALDI-TOF MS and 16S rRNA gene sequencing are currently the most promising tools, though other housekeeping genes should be targeted as well, and, the biggest challenge at this point is still the lack of comprehensive proteomic and sequence databases for SAOs. A full replacement of cultivation by next generation sequencing is difficult to recommend due to the absence of a standardized experimental methodology, especially for fish, and the relatively high sequencing costs. Additionally, a discrepancy between culture-dependent and independent methods in revealing the bacterial diversity, and abundancy, from marine fish was demonstrated by several authors. It is therefore recommended to consider both approaches as complements of one another, rather than substitutes, and to include them simultaneously to yield more complete results regarding the SAOs in fresh marine fish. As such, a thorough understanding of the biology of spoilage organisms and process will be obtained to prolong the shelf-life and deliver a high-quality product. • Spoilage associated organisms (SAOs) are the main cause of fish deterioration. • No guidelines on isolation and identification of SAOs in fresh marine fish. • Salt-containing agar media are essential for the growth of SAOs. • There is a discrepancy between culture-dependent and -independent approaches. • Recommendations for the detection and identification of SAOs in fish are provided. [ABSTRACT FROM AUTHOR]

Published

2022

10. Efficient differentiation of Corynebacterium striatum, Corynebacterium amycolatum and Corynebacterium xerosis clinical isolates by multiplex PCR using novel species-specific primers.

Author

Santos, Carolina S., Ramos, Juliana N., Vieira, Veronica V., Pinheiro, Carina S., Meyer, Roberto, Alcantara-Neves, Neuza M., Ramos, Rommel T., Silva, Artur, Jr.Hirata, Raphael, Felicori, Liza, de Alegría Puig, Carlos Ruiz, Navas, Jesús, Azevedo, Vasco, Mattos-Guaraldi, Ana L., and Pacheco, Luis G.C.

Subjects

*CORYNEBACTERIUM, *DNA primers, *POLYMERASE chain reaction, *RIBOSOMAL RNA, *NUCLEOTIDE sequencing

Abstract

A multiplex-PCR (mPCR) assay was designed with species-specific primers which generate amplicons of 226 bp, 434 bp and 106 bp for differentiating the species C . striatum , C . amycolatum , and C . xerosis , respectively. mPCR results were 100% in agreement with identifications achieved by 16S rRNA and rpoB gene sequencing and by VITEK-MS. [ABSTRACT FROM AUTHOR]

Published

2017

11. Robustness of two MALDI-TOF mass spectrometry systems for bacterial identification

Author

Carbonnelle, Etienne, Grohs, Patrick, Jacquier, Hervé, Day, Nesrine, Tenza, Sylvie, Dewailly, Alexandra, Vissouarn, Odile, Rottman, Martin, Herrmann, Jean-Louis, Podglajen, Isabelle, and Raskine, Laurent

Subjects

*MATRIX-assisted laser desorption-ionization, *TIME-of-flight mass spectrometry, *DETECTION of microorganisms, *ROBUST control, *MOLECULAR biology, *BACTERIA

Abstract

Abstract: MALDI-TOF-MS systems (Microflex-Bruker Daltonics/BioTyper™ and Axima-Assurance-Shimadzu/SARAMIS-AnagnosTec) were assessed for bacterial identification. Focusing on bacteria difficult to identify routinely, 296 strains were identified by molecular biology techniques as gold standard. MALDI-TOF-MS identification provided correct results at genus and species level for 94.9%, 83.4% and 83.8%, 65.9% with Biotyper and Saramis respectively. [Copyright &y& Elsevier]

Published

2012

12. Bacterial classification using genomic fingerprints obtained by virtual hybridization

Author

Jaimes-Díaz, Hueman, García-Chéquer, Adda Jeanette, Méndez-Tenorio, Alfonso, Santiago-Hernández, Juan Carlos, Maldonado-Rodríguez, Rogelio, and Beattie, Kenneth Loren

Subjects

*BACTERIA classification, *GENOMES, *MOLECULAR probes, *PHYLOGENY, *CORYNEBACTERIUM, *NUCLEOTIDE sequence, *BIOINFORMATICS

Abstract

Abstract: In silico genomic fingerprints were produced by virtual hybridization of 191 fully sequenced bacterial genomes using a set of 15,264 13-mer probes specially designed to produce universal whole genome fingerprints. A novel approach for constructing phylogenetic trees, based on comparative analysis of genomic fingerprints, was developed. The resultant bacterial phylogenetic tree had strong similarities to those produced from the alignment of conserved sequences. Notably, the trees derived from the alignment of other conserved COG genes divided the Bacillus and Corynebacterium genera into the same subgroups produced by the novel bacterial tree. A number of discrepancies between both techniques were observed for the grouping of some Lactobacillus species. However, a detailed analysis of the alignment of these genomes using other bioinformatics tools revealed that the grouping of these organisms in the novel tree was more satisfactory than the groupings from previous classifications, which used only a few conserved genes. All these data suggest that the bacterial taxonomy produced by genomic fingerprints is satisfactory, but sometimes different from classical taxonomies. Discrepancies probably arise because the fingerprinting technique analyzes genomic sequences and reveals more information than previously used approaches. [Copyright &y& Elsevier]

Published

2011

13. Assessment of VITEK® 2, MALDI-TOF MS and full gene 16S rRNA sequencing for aerobic endospore-forming bacteria isolated from a pharmaceutical facility.

Author

Costa, Luciana Veloso da, Miranda, Rebeca Vitoria da Silva Lage de, Fonseca, Erica Louro da, Gonçalves, Natalia Pedra, Reis, Cristhiane Moura Falavina dos, Frazão, Adriana Marques, Cruz, Fernanda Ventura, Brandão, Marcelo Luiz Lima, Ramos, Juliana Nunes, and Vieira, Verônica Viana

Subjects

*SPOREFORMING bacteria, *RIBOSOMAL RNA, *AEROBIC bacteria, *PAENIBACILLUS, *GENES

Abstract

VITEK®2, MALDI-TOF MS and 16S rRNA sequencing were evaluated for the identification of aerobic endospore-forming bacteria (AEB) from a pharmaceutical facility. MALDI-TOF MS demonstrated higher accuracy compared to VITEK®2, although both databases were insufficient to identify AEB species. Sequencing was the best methodology, but unable to identify closely related species. [Display omitted] • VITEK® 2 was not effective for AEB identification. • VITEK® 2 and MALDI-TOF MS databases are not updated with most AEB species.1 • 16S rRNA sequencing was the best method for AEB identification. • Bacillus and Paenibacillus were the main isolated genera. • Five possible new species were isolated. [ABSTRACT FROM AUTHOR]

Published

2022

14. Effect of selective growth media on the differentiation of Salmonella enterica serovars by Fourier-Transform Mid-Infrared Spectroscopy

Author

Baldauf, Nathan A., Rodriguez-Romo, Luis A., Männig, Annegret, Yousef, Ahmed E., and Rodriguez-Saona, Luis E.

Subjects

*SALMONELLA, *FOOD pathogens, *SALMONELLA food poisoning, *SALMONELLA diseases, *FOURIER transform spectroscopy

Abstract

Abstract: Salmonella enterica serovars are prevalent foodborne pathogens responsible for high numbers of salmonellosis each year. Complex Fourier-transform infrared (FTIR) spectra offer unique biochemical fingerprints of bacteria with bands due to major cellular components. Growth media effects on discrimination of Salmonella serovars by FTIR spectroscopy were investigated and a novel sample preparation technique was developed. S. enterica strains from six serovars were grown on xylose lysine desoxycholate (XLD), Miller–Mallinson (MM), and plate count (PCA) agar as a control (37 °C, 24 h). Isolated colonies were suspended in 50% acetonitrile and centrifuged; the remaining pellet was placed on an AMTIR (attenuated total reflectance) crystal and dried under vacuum. Classification models (Soft Independent Modeling of Class Analogy, SIMCA), generated from derivatized infrared spectra (1300–900 cm− 1 or 1200–900 cm− 1), successfully discriminated among Salmonella strains with major discrimination from 1000–970 cm− 1 associated to stretching modes of O-specific polysaccharide chains of lipopolysaccharides. Sample treatment with acetonitrile enhanced safe handling of the bacteria, removed interfering signals and improved the discriminating ability of SIMCA. All media were able to discriminate the S. enterica strains studied, varying in discriminating peaks and class distances in SIMCA classification. This methodology, with the production of large libraries of pathogenic bacteria, could be applied for the rapid monitoring of bacterial contamination in food with minimal sample manipulation. [Copyright &y& Elsevier]

Published

2007

15. 16S rRNA sequencing in routine bacterial identification: A 30-month experiment

Author

Mignard, S. and Flandrois, J.P.

Subjects

*BACTERIA, *DIAGNOSTIC microbiology, *NUCLEOTIDE sequence, *MICROORGANISMS

Abstract

Abstract: Accurate identification of bacterial isolates is an essential task in clinical microbiology. Phenotypic methods are time-consuming and either fail to identify some bacteria such as Gram-positive rods entirely or at least fail to do so in some clinical situations. 16S rDNA sequencing is a recent method of identification which offers a useful alternative. In this study, we investigate the usefulness of this method for identifying a range of bacteria in a clinical laboratory under routine conditions. Over a period of 30 months, 683 isolates were obtained from clinical specimens, sequenced and analysed. For 568 of these isolates (83.1%), the sequence provided species level identification. For 108 isolates (15.8%), the identification was limited to the genus level, and for 7 isolates (1%), the sequence remained unidentifiable by 16S rDNA sequence analysis. For the isolates identified only to the genus level, the 16S rDNA approach failed to identify bacteria to the taxonomic level for 3 reasons: failure to differentiate between species in 72 isolates (66%), the lack of any closely related sequence in the database for 15 isolates (13.8%) and the presence of more than 1% of undetermined position in the sequence for 13 isolates (12%). [Copyright &y& Elsevier]

Published

2006

16. Mining fatty acid databases for detection of novel compounds in aerobic bacteria

Author

Dawyndt, Peter, Vancanneyt, Marc, Snauwaert, Cindy, De Baets, Bernard, De Meyer, Hans, and Swings, Jean

Subjects

*FATTY acids, *AEROBIC bacteria, *MICROBIOLOGY, *ANALYTICAL chemistry

Abstract

Abstract: This study examines how the discriminatory power of an automated bacterial whole-cell fatty acid identification system can be significantly enhanced by exploring the vast amounts of information accumulated during 15years of routine gas chromatographic analysis of the fatty acid content of aerobic bacteria. Construction of a global peak occurrence histogram based upon a large fatty acid database is shown to serve as a highly informative tool for assessing the delineation of the naming windows used during the automatic recognition of fatty acid compounds. Along the lines of this data mining application, it is suggested that several naming windows of the Sherlock MIS TSBA50 peak naming method may need to be re-evaluated in order to fit more closely with the bulk of observed fatty acid profiles. At the same time, the global peak occurrence histogram has put forward the delineation of 32 new peak naming windows, accounting for a 26% increase in the total number of fatty acid features taken into account for bacterial identification. By scrutinizing the relationships between the newly delineated naming windows and the many taxonomic units covered within a proprietary fatty acid database, all new naming windows were proven to correspond with stable features of some specific groups of microorganisms. This latter analysis clearly underscores the impact of incorporating the new fatty acid compounds for improving the resolution of the bacterial identification system and endorses the applicability of knowledge discovery in databases within the field of microbiology. [Copyright &y& Elsevier]

Published

2006

17. Effects of varied pH, growth rate and temperature using controlled fermentation and batch culture on Matrix Assisted Laser Desorption/Ionization whole cell protein fingerprints

Author

Wunschel, David S., Hill, Eric A., McLean, Jeffrey S., Jarman, Kristin, Gorby, Yuri A., Valentine, Nancy, and Wahl, Karen

Subjects

*HYDROGEN-ion concentration, *ANTHROPOMETRY, *LEAVENING agents, *MICROBIOLOGY

Abstract

Abstract: Rapid identification of microorganisms using matrix assisted laser desorption/ionization (MALDI) is a rapidly growing area of research due to the minimal sample preparation, speed of analysis and broad applicability of the technique. This approach relies on expressed biochemical markers, often proteins, to identify microorganisms. Therefore, variations in culture conditions that affect protein expression may limit the ability of MALDI-MS to correctly identify an organism. We have expanded our efforts to investigate the effects of culture conditions on MALDI-MS signatures to specifically examine the effects of pH, growth rate and temperature. Continuous cultures maintained in bioreactors were used to maintain specific growth rates and pH for E. coli HB 101. Despite measurable morphological differences between growth conditions, the MALDI-MS data associated each culture with the appropriate library entry (E. coli HB 101 generated using batch culture on a LB media), independent of pH or growth rate. The lone exception was for a biofilm sample collected from one of the reactors which had no appreciable degree of association with the correct library entry. Within the data set for planktonic organisms, variations in growth rate created the largest variation between fingerprints. The effect of varying growth temperature on Y. enterocolitica was also examined. While the anticipated effects on phenotype were observed, the MALDI-MS technique provided the proper identification. [Copyright &y& Elsevier]

Published

2005

18. Fast and reliable bacterial identification direct from positive blood culture using a new TFA sample preparation protocol and the Vitek® MS system.

Author

Monteiro, Jussimara, Inoue, Fernanda Matsiko, Lobo, Ana Paula T., Sugawara, Eduardo K., Boaretti, Fabiana M., and Tufik, Sergio

Subjects

*BLOOD microbiology, *TRIFLUOROACETIC acid, *CHEMICAL sample preparation, *GRAM-positive bacteria, *MASS spectrometry

Abstract

A simple and reliable protocol using 0.1% trifluoroacetic acid (TFA) was developed to identify bacteria directly from blood cultures on the Vitek® MS system. Results presented a correlation of 99% for Gram-negative bacteria at species level, and 86.3% and 82.3% of Gram-positive bacteria at the genus and species levels, respectively. [ABSTRACT FROM AUTHOR]

Published

2015

19. Efficient differentiation of Corynebacterium striatum , Corynebacterium amycolatum and Corynebacterium xerosis clinical isolates by multiplex PCR using novel species-specific primers

Author

Roberto Meyer, Luis G.C. Pacheco, Neuza Maria Alcantara-Neves, Verônica Viana Vieira, Carlos Ruiz de Alegría Puig, Carina S. Pinheiro, Carolina S. Santos, Vasco Azevedo, Jesús Navas, Juliana Nunes Ramos, Rommel Thiago Jucá Ramos, Artur Silva, Raphael Hirata, Liza Felicori, Ana Luíza Mattos-Guaraldi, and Universidad de Cantabria

Subjects

0301 basic medicine, Microbiology (medical), 030106 microbiology, Corynebacterium, Microbiology, DNA sequencing, 03 medical and health sciences, RNA, Ribosomal, 16S, Multiplex polymerase chain reaction, Corynebacterium spp, Humans, Bacterial identification, Molecular Biology, Species specific primers, DNA Primers, Vitek-MS, Corynebacterium Infections, biology, DNA-Directed RNA Polymerases, Multiplex PCR, Amplicon, 16S ribosomal RNA, biology.organism_classification, rpoB, Molecular biology, Molecular Typing, Corynebacterium striatum, 030104 developmental biology, Corynebacterium amycolatum, Emerging pathogens, Multiplex Polymerase Chain Reaction

Abstract

A multiplex-PCR (mPCR) assay was designed with species-specific primers which generate amplicons of 226 bp, 434 bp and 106 bp for differentiating the species C. striatum, C. amycolatum, and C. xerosis, respectively. mPCR results were 100% in agreement with identifications achieved by 16S rRNA and rpoB gene sequencing and by VITEK-MS. This work was supported by grants from FAPESB (JCB0031/2013) and CAPES (PROCAD 071/2013).

Published

2017

20. Effect of gamma radiation on the identification of bacterial pathogens by MALDI-TOF MS

Author

Tracz, Dobryan M., McCorrister, Stuart J., Westmacott, Garrett R., and Corbett, Cindi R.

Subjects

*GAMMA rays, *ENZYME-linked immunosorbent assay, *BIOSAFETY, *MASS spectrometry, *MATRIX-assisted laser desorption-ionization, *TIME-of-flight mass spectrometry, *PATHOGENIC bacteria, *RAPID methods (Microbiology)

Abstract

Abstract: MALDI-TOF MS is a well-established method for rapid identification of bacteria; however there are no reports to date on its performance with gamma-irradiated samples typically used in BSL-3 laboratories for sample inactivation. In this report we demonstrate that gamma-irradiated bacteria can be accurately identified by MALDI-TOF MS in most cases, but a decrease in identification scores is observed. [Copyright &y& Elsevier]

Published

2013

21. Application of probabilistic neural network in bacterial identification by biochemical profiles.

Author

Jia, Juntao, Liang, Chengzhu, Cao, Jijuan, and Li, Zhengyi

Subjects

*BACTERIAL typing, *ARTIFICIAL neural networks, *PROBABILITY theory, *BIOCHEMISTRY, *MICROBIOLOGY, *ALGORITHMS

Abstract

Abstract: An algorithm of Probabilistic Neural Network (PNN) for bacterial identification based on the probability matrix of API 20E system as a case study is reported. The PNN shows the correct identification of all the taxa belonging to the training and test sets and possesses merits over the conventional methods. [Copyright &y& Elsevier]

Published

2013

22. A method for the detection of antibiotic resistance markers in clinical strains of Escherichia coli using MALDI mass spectrometry.

Author

Hart PJ, Wey E, McHugh TD, Balakrishnan I, and Belgacem O

Subjects

Amino Acid Sequence, Biomarkers analysis, Databases, Protein, Escherichia coli classification, Escherichia coli genetics, Escherichia coli Proteins isolation & purification, Peptides, Periplasm chemistry, Periplasmic Proteins isolation & purification, Proteomics methods, beta-Lactamases isolation & purification, Drug Resistance, Bacterial, Escherichia coli chemistry, Escherichia coli drug effects, Escherichia coli Proteins analysis, Periplasmic Proteins analysis, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods

Abstract

Matrix-assisted laser-desorption/ionisation time-of-flight mass spectrometry (MALDI-TOF MS) is one of the most widely used mass spectrometry based approaches for bacterial identification and classification. The relatively simple sample preparation requirements and the speed of analysis which can usually be completed within a few minutes have resulted in the adoption and assimilation of MALDI-TOF MS into the routine diagnostic workflow of Clinical microbiology laboratories worldwide. This study describes the facilitation of bacterial discrimination based on antibiotic resistance markers through the implementation of MALDI-TOF MS. The periplasmic compartment of whole bacterial cells contains several proteins which confer antibiotic resistance in the Enterobacteriaceae. In order to reduce the complexity of the sample to be analysed via MALDI-TOF MS, the periplasm was extracted and subjected to in solution tryptic digestion followed by nano-LC separation. This method, established that peptide sequence biomarkers from several classes of antibiotic resistance proteins could be predicted using protein/peptide database tools such as Mascot. Biomarkers for a CTX-M-1 group extended spectrum β-lactamase, CMY-2 an Amp-C β-lactamase, VIM a metallo-β-lactamase, TEM a β-lactamase and KanR an aminoglycoside modifying enzyme were detected. This allowed for discrimination at a species level and at an almost identical strain level where the only difference between strains was the carriage of a modified antibiotic resistance carrying plasmid. This method also was able to detect some of these biomarkers in clinical strains where multiple resistance mechanisms were present., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2015