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52. Changes in the Matrix Markedly Enhance the Resolution and Accurate Identification of Human Pathogens by MALDI-TOF MS

Author

Shurene Bishop Simon, Min Fang, Lakshani Rajakaruna, Itaru Dekio, Renata Culak, and Haroun N. Shah

Subjects
Matrix (chemical analysis), chemistry.chemical_compound, Analyte, Matrix-assisted laser desorption/ionization, Time of flight, Resolution (mass spectrometry), chemistry, Analytical chemistry, Sinapinic acid, Biomarker discovery, Mass spectrometry
Abstract

The mass spectral profiles of three major/emerging Gram positive pathogens belonging to the genera Clostridium, Listeria and Propionibacterium were investigated using four MALDI-TOF (Matrix-Assisted Laser Desorption/ Ionization- Time of Flight) Mass Spectrometers from Waters, Shimadzu, Bruker and Ciphergen Biosystems. These instruments have been extensively used for developing a diagnostic platform for high throughput, low cost, near sample-free preparation for microbial identification. The results demonstrate the marked effect of spectral quality obtained by altering the matrix and the added value of simple preparative extraction procedures. While microbial spectral data are generally collected in the mass range 2 to 20 kDa for diagnostic signatures, most of the significant mass ions are

Published
2014
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53. The use of a 16S rDNA directed PCR for the detection of endodontopathogenic Bacteria

Author

Saheer E. Gharbia, Kishor Gulabivala, G. Conrads, Haroun N. Shah, and Friedrich Lampert

Subjects
Adult, Male, Fastidious organism, DNA, Ribosomal, Polymerase Chain Reaction, law.invention, Microbiology, law, RNA, Ribosomal, 16S, Humans, General Dentistry, Polymerase chain reaction, Aged, DNA Primers, Bacteriological Techniques, Bacteria, biology, Hybridization probe, Middle Aged, biology.organism_classification, 16S ribosomal RNA, Molecular biology, Female, Dental Pulp Cavity, Bacteroides, Fusobacterium nucleatum, Primer (molecular biology), Streptococcus milleri
Abstract

The study evaluates a 16S rDNA directed polymerase chain reaction (PCR) to detect and differentiate bacteria in necrotic root canal samples. The examination focused on species that are fastidious concerning culture or are difficult to differentiate after culturing by biochemical methods. In the described PCR assay, a universal 16S rDNA directed forward primer in combination with a highly specific reversed one was used to amplify taxon specific gene fragments of 230 to 950 bp length. A similar PCR reaction using a universal 16S rDNA reversed primer was also established to demonstrate bacteria in root canal specimens in general. A first application of this method revealed the presence of Actinomycetales-species, Fusobacterium nucleatum, "Streptococcus milleri," and, presumably for the first time described in infected root canals, Bacteroides forsythus. The identity of amplificons was confirmed by generating sequence information and comparison to gene databanks.

Published
1997
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54. [Rhodococcus equi infection in AIDS patients: retrospective analysis of 13 patients in Argentina]

Author

Marcelo, Corti, Rubén, Solari, Luis, De Carolis, Omar, Palmieri, Raquel, Rollet, and Haroun N, Shah

Subjects
Adult, Male, Young Adult, Delayed Diagnosis, AIDS-Related Opportunistic Infections, Rhodococcus equi, Argentina, Humans, Actinomycetales Infections, CD4 Lymphocyte Count, Retrospective Studies
Abstract

Rhodococcus equi is a gram positive coccoid rod that causes pulmonary infections in immunosuppressed patients.We retrospectively analyzed epidemiological, clinical, microbiological, radiological, and immunological features as well as the outcomes of 13 AIDS patients with R. equi infection.Between January 1994 and December 2012, 13 patients attending the AIDS department of the Infectious Diseases reference hospital in Buenos Aires were diagnosed with R. equi infection. All were men, the median age was 27 years. At the time of diagnosis, the median of CD4+ T cell counts was 11 cells/μl Twelve patients presented pulmonary disease with isolation of the microorganism from sputum or bronchoalveolar lavage; in the other patient the diagnosis was postmortem with positive culture of cerebrospinal fluid. The most frequent clinical manifestations were fever, haemoptysis, and weight loss. The predominant radiological finding was lobe consolidation with cavitation. Nine patients died after a median survival of 5.5 months. In all of them, cultures persisted positive until the last admission. The other 4 patients did continue clinical follow-ups.The insidious course of R. equi disease and the difficulties in the isolation of the microorganism contribute to the delay in the diagnosis and to the high mortality rate of this opportunistic infection.

Published
2013

55. Molecular signatures for Bacillus species: demarcation of the Bacillus subtilis and Bacillus cereus clades in molecular terms and proposal to limit the placement of new species into the genus Bacillus

Author

Vaibhav, Bhandari, Nadia Z, Ahmod, Haroun N, Shah, and Radhey S, Gupta

Subjects
DNA, Bacterial, Genetic Markers, Bacillus cereus, Bacterial Proteins, INDEL Mutation, RNA, Ribosomal, 16S, Molecular Sequence Data, Amino Acid Sequence, Phylogeny, Bacillus subtilis
Abstract

The genus Bacillus is a phylogenetically incoherent taxon with members of the group lacking a common evolutionary history. Comprising aerobic and anaerobic spore-forming bacteria, no characteristics are known that can distinguish species of this genus from other similar endospore-forming genera. With the availability of complete genomic data from over 30 different species from this group, we have constructed detailed phylogenetic trees to determine the relationships among Bacillus and other closely related taxa. Additionally, we have performed comparative genomic analysis for the determination of molecular markers, in the form of conserved signature indels (CSIs), to assist in the understanding of relationships among species of the genus Bacillus in molecular terms. Based on the analysis, we report here the identification of 11 and 6 CSIs that clearly differentiate a 'Bacillus subtilis clade' and a 'Bacillus cereus clade', respectively, from all other species of the genus Bacillus. No molecular markers were identified that supported a larger clade within this genus. The subtilis and the cereus clades were also the largest observed monophyletic groupings among species from the genus Bacillus in the phylogenetic trees based on 16S rRNA gene sequences and those based upon concatenated sequences for 20 conserved proteins. Thus, the relationships observed among these groups of species through CSIs are independently well supported by phylogenetic analysis. The molecular markers identified in this study provide a reliable means for the reorganization of the currently polyphyletic genus Bacillus into a more evolutionarily consistent set of groups. It is recommended that the genus Bacillus sensu stricto should comprise only the monophyletic subtilis clade that is demarcated by the identified CSIs, with B. subtilis as its type species. Members of the adjoining cereus clade (referred to as the Cereus clade of bacilli), although they are distinct from the subtilis clade, will also retain the Bacillus genus name as they contain several clinically important species, and their transfer into a new genus could have serious consequences. However, all other species that are currently part of the genus Bacillus and not part of these two clades should be eventually transferred to other genera. We also propose that all novel species of the genus Bacillus must meet minimal requirements, foremost among which is that the branching of the prospective species with the Bacillus sensu stricto clade or the Cereus clade of bacilli should be strongly supported by 16S rRNA gene sequence trees or trees based upon concatenated protein sequences. Additionally, the presence of one or more of the CSIs that are specific for these clades may be used to confirm molecularly the placement of the species into these clades. The identified CSIs, in addition to their usefulness for taxonomic and diagnostic purposes, also provide novel probes for genetic and biochemical studies of these bacteria.

Published
2013

56. Correlation between Phylogroups and Intracellular Proteomes of Propionibacterium acnes and Differences in the Protein Expression Profiles between Anaerobically and Aerobically Grown Cells

Author

Graham Ball, Haroun N. Shah, Renata Culak, Itaru Dekio, Saheer E. Gharbia, and Min Fang

Subjects
Proteome, Article Subject, Virulence, lcsh:Medicine, Group A, General Biochemistry, Genetics and Molecular Biology, Microbiology, Propionibacterium acnes, Bacterial Proteins, Anaerobiosis, Gene, Regulation of gene expression, General Immunology and Microbiology, biology, Strain (chemistry), lcsh:R, General Medicine, Gene Expression Regulation, Bacterial, biology.organism_classification, Molecular biology, Aerobiosis, Oxygen, Intracellular, Research Article
Abstract

Propionibacterium acnesis one of the dominant commensals on the human skin and also an opportunistic pathogen in relation to acne, sarcoidosis, prostate cancer, and various infections. Recent investigations using housekeeping and virulence genes have revealed that the species consists of three major evolutionary clades (types I, II, and III). In order to investigate protein expression differences between these phylogroups, proteomic profiles of 21 strains ofP. acneswere investigated. The proteins extracted from cells cultured under anaerobic and aerobic conditions were analysed using a SELDI-TOF mass spectrometer, high-resolution capillary gel electrophoresis, and LC-MS/ MS. The SELDI spectral profiles were visualised as a heat map and a dendrogram, which resulted in four proteomic groups. Strains belonging to type I were represented in the proteome Group A, while Group B contained type III strains. Groups C and D contained mixtures of types I and II. Each of these groups was not influenced by differences in culture conditions. Under anoxic growth conditions, a type IB strain yielded high expressions of some proteins, such as methylmalonyl-CoA epimerase and the Christie-Atkins-Munch-Petersen (CAMP) factor. The present study revealed good congruence between genomic and proteomic data suggesting that the microenvironment of each subtype may influence protein expression.

Published
2013
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58. A Retrospective Review of Cases of Anaerobic Empyema and Update of Bacteriology

Author

L. Borenstein, Hannele Jousimies-Somer, Sydney M. Finegold, M. Marina, R. Civen, and Haroun N. Shah

Subjects
Adult, Male, Microbiology (medical), Microbial Sensitivity Tests, Microbiology, Bacteria, Anaerobic, stomatognathic system, Bacteriology, Prevotella, medicine, Humans, Empyema, Aged, Retrospective Studies, Aged, 80 and over, biology, Bacterial Infections, Middle Aged, biology.organism_classification, Peptostreptococcus, Bacteria, Aerobic, Penicillin, stomatognathic diseases, Infectious Diseases, Viridans streptococci, Bacteroides fragilis, Fusobacterium nucleatum, Actinomyces, medicine.drug
Abstract

We conducted a retrospective study to update the bacteriology of 46 cases of anaerobic empyema that were originally studied between 1976 and 1993 at the Wadsworth Anaerobic Bacteriology Clinical Research Laboratory (Los Angeles). Anaerobic bacteriologic studies were completed for all 46 pleural fluid specimens, and aerobic bacteriologic studies were completed for 41 of these specimens. Thirty-seven clinical charts were available for review. A total of 161 anaerobic isolates (3.5 per patient) representing 64 species or groups were recovered. The most common isolates were as follows: Fusobacterium nucleatum (19); Prevotella oris-buccae group (13, 9 of which were P. oris); Bacteroides fragilis group (11, 4 of which were B. fragilis); pigmented Prevotella species (17, 8 of which were in the Prevotella intermedia-nigrescens group); Peptostreptococcus species (17, 9 of which were Peptostreptococcus micros); Eubacterium species (7); Lactobacillus species (8); Actinomyces species (7); and Clostridium species (7). Nineteen if the cases were of purely anaerobic etiology; of these, eight were caused by a single organism: F. nucleatum (five cases); B. fragilis (two cases); and Prevotella mangus (one case). Of the 45 aerobic isolates (1.1 per patient), viridans streptococci were most common (21 isolates), followed by group D nonenterococcal streptococcus (four isolates). Only nine gram-negative rods (six enteric and three nonenteric organisms) and one Staphylococcus aureus isolate were recovered. The susceptibility to penicillin of 64 isolates was examined with the use of the spiral gradient method; 21 (33%) of these isolates were beta-lactamase positive (MICs ranged from 1.1 toor = 54 micrograms/mL vsor = 0.27 micrograms/mL for beta-lactamase-negative strains).

Published
1995
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59. The Biochemical Milieu of the Host in the Selection of Anaerobic Species in the Oral Cavity

Author

SE Gharbia and Haroun N. Shah

Subjects
Microbiology (medical), Mouth, Flora, Sequence analysis, Host (biology), Microorganism, Biology, Ribosomal RNA, Substrate (biology), Microbiology, Isotopic labeling, Bacteria, Anaerobic, A-site, Infectious Diseases, Endopeptidases, Humans, Treponema, Amino Acids, Porphyromonas gingivalis, Ecosystem, Periodontal Diseases, Phylogeny
Abstract

The periodontal pocket provides a unique structural site for studies on host/bacterial interactions. The pocket is colonized by a complex but characteristic anaerobic bacterial flora. Many new taxa have been described that have now been supported by comparative rRNA sequence analysis. Within recent years, several molecular approaches have been used to describe both cultivable and noncultivable species, and new genotypes have been reported. Microbial activity rather than the mere presence of microorganism at a site must be a major factor in the process of disease development. Information on metabolic activities of species and identification of substrates are therefore essential to elucidate the complex interactions that are likely to occur in vivo. We have been using a variety of analytical procedures such as 13 C substrate-enrichment nuclear magnetic resonance, 14 C isotopic labeling experiments, enzyme assays, impedance measurements, and various chromatographic and electrophoretic procedures to study key species of this predominantly asaccharolytic flora. Results have so far indicated a major role for cationic and anionic acids as sources of energy, but the mechanisms of substrate processing may differ significantly between species. In this ecosystem, crevicular fluid is the likely source of nutrients for species. Components of this fluid appear to have a role in the selection of species in subgingival sites.

Published
1995
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60. Molecular Analysis of Surface-Associated Enzymes of Porphyromonas gingivalis

Author

Haroun N. Shah and SE Gharbia

Subjects
DNA, Bacterial, Microbiology (medical), Clostridium symbiosum, Molecular Sequence Data, Mutagenesis (molecular biology technique), Biology, Bacterial Proteins, Amino Acid Sequence, Amino Acids, Gene, Porphyromonas gingivalis, chemistry.chemical_classification, Base Sequence, Membrane Proteins, biology.organism_classification, Molecular biology, Cysteine protease, Cysteine Endopeptidases, Open reading frame, Infectious Diseases, Enzyme, Biochemistry, chemistry, Codon usage bias, Mutagenesis, Site-Directed, Glutamate Dehydrogenase (NADP+)
Abstract

There is now increasing evidence that surface-associated enzymes, previously considered to be involved in intermediary metabolism or virulence, play a role in physiological reactions such as signal transduction, transport systems, and metabolic processes. Herein we report the molecular aspects of two such enzymes, the cysteine proteinase gingivain and NAD-dependent glutamate dehydrogenase of Porphyromonas gingivalis. The gdh gene comprises an open reading frame of 1,335 base pairs that encodes a 49,000-M(r) protein of 445 amino acids. The gdh gene showed high homology (78.3%) with that of Clostridium symbiosum. Optimal codons accounted for 35.9% of the total codon usage, indicating high expression of this enzyme. These data are currently being used to carry out targeted mutagenesis, which was established here for gingivain. Conditions for targeted mutagenesis within the histidine domain of the catalytic site of gingivain using Tn 4351 was successfully achieved. Consequently, the catalytic functions, such as gingivain's capacity to hydrolyze the synthetic substrate alpha-benzoyl-arginine-4-nitroanilide, were disrupted.

Published
1995
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61. The Application of Matrix-Assisted Laser Desorption/Ionisation Time of Flight Mass Spectrometry to Profile the Surface of Intact Bacterial Cells

Author

Ian Brookhouse, Saheer E. Gharbia, Frank Trundle, Haroun N. Shah, Kathryn Ralphson, Carrina J. Keys, and Martin A. Claydon

Subjects
Chromatography, Ecology, Biology, Laser, biology.organism_classification, law.invention, Agar plate, Matrix (chemical analysis), law, Ionization, Desorption, Time-of-flight mass spectrometry, Bacteroides fragilis, Clonal diversity
Abstract

Matrix-Assisted Laser Desorption/lonisation Time of Flight Mass Spectrometry (MALDI-TOF-MS) as a tool for differentiating bacterial species was examined using reference strains representing gram-positive and gram-negative taxa. Initially, the effect of differences in medium composition on spectral profile was examined. The results indicated that growth on Columbia blood agar resulted in a larger spectrum of ionized residues and was therefore used for the cultivation of all strains in the rest of the study. The stability of the obtained mass spectral profiles against differences in batch and media processing suggested that no significant alterations to the profiles occurred in response to changes in media sources. The established conditions from these initial experiments were used to standardize subsequent experiments. The MALDI-TOF-MS profiles of 15 reference strains were compared and species characteristic markers were identified. The potential of using MALDI-TOF-MS as a tool for probing clonal diversity was examined using well characterized but clonally variable isolates of Bacteroides fragilis . Comparative analysis of the profiles of 20 strains revealed 5 clusters within the species but compared to other taxa such as Bacteroides merdae and Salmonella arizonae they form a closely related lineage. These results obtained strongly support the potential to use MALDI-TOF-MS as a tool for exploring bacterial surfaces for characteristic biomarkers and species-specific signatures.

Published
2011

62. Enzymes of Diagnostic Importance Within the Bacteroidaceae; Use as Possible Ecological Markers

Author

Saheer E. Gharbia, T. A. R. Al-Jalili, Haroun N. Shah, S. V. Seddon, and R. A. Nash

Subjects
chemistry.chemical_classification, Leptotrichia buccalis, biology, Ecology, Glutamate dehydrogenase, Dehydrogenase, biology.organism_classification, Malate dehydrogenase, Enzyme assay, Microbiology, Enzyme, chemistry, Biochemistry, biology.protein, Bacteroides fragilis, Bacteroidaceae
Abstract

Cell free extracts from a wide variety of Gram-negative, anaerobic, non-sporeforming rods were screened for dehydrogenase enzymes of carbohydrate and nitrogen metabolism. Four enzymes, malate dehydrogenase, glutamate dehydrogenase, glucose-6-phosphate dehydrogenase and 6-phosphogluconate dehydrogenase, were found to be of diagnostic importance. The ‘Bacteroides fragilis’ group possessed all four enzymes whereas the ‘B. melaninogenicus-B. oralis’ group and the asaccharolytic, pigmented species were characterised by the presence of only malate and glutamate dehydrogenases. The saccharolytic and asaccharolytic pigmented species could be differentiated by the wide difference in pH optimum for malate dehydrogenase. Fusobacterium species and Leptotrichia buccalis both possessed only glutamate dehydrogenase, but there were differences in enzyme activity between both taxa. Other genera such as Anaerorhabdus, Megamonas, Mitsuokella. Rikenella, Sebaldella and Tissierella had characteristic enzyme profiles. These enzymatic data are of diagnostic value within the Bacteroidaceae and may serve as useful markers for studying the ecological interrelationships of these bacteria.Keywords: Bacteroidaceae; Dehydrogenases; Enzyme patterns.

Published
2011

63. Identification of a Bacillus anthracis specific indel in the yeaC gene and development of a rapid pyrosequencing assay for distinguishing B. anthracis from the B. cereus group

Author

Nadia Z. Ahmod, Radhey S. Gupta, and Haroun N. Shah

Subjects
Microbiology (medical), Bacillus cereus, Virulence, Microbiology, Polymerase Chain Reaction, Sensitivity and Specificity, law.invention, Bacterial Proteins, INDEL Mutation, law, Animals, Humans, Indel, Molecular Biology, Polymerase chain reaction, DNA Primers, Genetics, Electrophoresis, Agar Gel, Bacteriological Techniques, biology, fungi, Sequence Analysis, DNA, biology.organism_classification, Bacillus anthracis, Cereus, Agarose gel electrophoresis, Pyrosequencing
Abstract

Bacillus anthracis, the causative agent of anthrax, is a potential source of bioterrorism. The existing assays for its identification lack specificity due to the close genetic relationship it exhibits to other members of the B. cereus group. Our comparative analyses of protein sequences from Bacillus species have identified a 24 amino acid deletion in a conserved region of the YeaC protein that is uniquely present in B. anthracis. PCR primers based on conserved regions flanking this indel in the Bacillus cereus group of species (viz. Bacillus cereus, B. anthracis, B. thuringiensis, B. mycoides, B. weihenstephnensis and B. pseudomycoides) specifically amplified a 282 bp fragment from all six reference B. anthracis strains, whereas a 354 bp fragment was amplified from 15 other B. cereus group of species/strains. These fragments, due to large size difference, are readily distinguished by means of agarose gel electrophoresis. In contrast to the B. cereus group, no PCR amplification was observed with any of the non-B. cereus group of species/strains. This indel was also used for developing a rapid pyrosequencing assay for the identification of B. anthracis. Its performance was evaluated by examining the presence or absence of this indel in a panel of 81 B. cereus-like isolates from various sources that included 39 B. anthracis strains. Based upon the sequence data from the pyrograms, the yeaC indel was found to be a distinctive characteristic of various B. anthracis strains tested and not found in any other species/strains from these samples. Therefore, this B. anthracis specific indel provides a robust and highly-specific chromosomal marker for the identification of this high-risk pathogen from other members of the B. cereus group independent of a strain's virulence. The pyrosequencing platform also allows for the rapid and simultaneous screening of multiple samples for the presence of this B. anthracis-specific marker.

Published
2011

64. Measurement of Electrical Bioimpedance for Studying Utilization of Amino Acids and Peptides by Porphyromonas gingivalis, Fusobacterium nucleatum, and Treponema denticola

Author

Saheer E. Gharbia, Haroun N. Shah, and M. I. N. Zhang

Subjects
Microbiology (medical), Casamino acid, Peptide, Microbiology, chemistry.chemical_compound, stomatognathic system, Electric Impedance, Treponema, Amino Acids, Bacteroidaceae, Porphyromonas gingivalis, chemistry.chemical_classification, Bacteriological Techniques, Fusobacterium nucleatum, biology, Treponema denticola, biology.organism_classification, Culture Media, Amino acid, stomatognathic diseases, Infectious Diseases, chemistry, Biochemistry, Peptides
Abstract

The growth response of Porphyromonas gingivalis, Fusobacterium nucleatum, and Treponema denticola to peptides (supplied as trypticase) and amino acids (supplied as casamino acids) was measured over 24 hours by monitoring changes in alternating-current conductivity at 37 degrees C. All species utilized peptides preferentially over amino acids. These results are consistent with those obtained previously with conventional growth-response experiments. The duration of the linear growth response to trypticase of P. gingivalis was 9.7 hours, whereas that of both F. nucleatum and T. denticola was24 hours. By contrast, there was more uniformity in the utilization of amino acids from the casamino acid mixture, which previously has been shown to be a poor growth substrate. Furthermore, subtle differences in growth patterns, such as the ability of F. nucleatum to metabolize its storage glycopolymers before utilizing amino acids, were clearly evident. The present method provides an excellent means of studying bacterial growth kinetics and delineating bacterial/substrate specificities of both synthetic and natural substrates.

Published
1993
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66. Coherent pipeline for biomarker discovery using mass spectrometry and bioinformatics

Author

Haroun N. Shah, Raju Misra, Nadia Z. Ahmod, Ali Al-Shahib, Min Fang, and Saheer E. Gharbia

Subjects
Proteomics, Databases, Factual, In silico, Computational biology, Biology, Bioinformatics, lcsh:Computer applications to medicine. Medical informatics, Sensitivity and Specificity, Biochemistry, Mass Spectrometry, Bacterial Proteins, Species Specificity, Structural Biology, Clostridium botulinum, Database search engine, Biomarker discovery, Molecular Biology, lcsh:QH301-705.5, Conserved Sequence, Applied Mathematics, Computational Biology, Pipeline (software), Computer Science Applications, Identification (information), lcsh:Biology (General), Biomarker (medicine), lcsh:R858-859.7, DNA microarray, Algorithms, Biomarkers, Research Article
Abstract

Background Robust biomarkers are needed to improve microbial identification and diagnostics. Proteomics methods based on mass spectrometry can be used for the discovery of novel biomarkers through their high sensitivity and specificity. However, there has been a lack of a coherent pipeline connecting biomarker discovery with established approaches for evaluation and validation. We propose such a pipeline that uses in silico methods for refined biomarker discovery and confirmation. Results The pipeline has four main stages: Sample preparation, mass spectrometry analysis, database searching and biomarker validation. Using the pathogen Clostridium botulinum as a model, we show that the robustness of candidate biomarkers increases with each stage of the pipeline. This is enhanced by the concordance shown between various database search algorithms for peptide identification. Further validation was done by focusing on the peptides that are unique to C. botulinum strains and absent in phylogenetically related Clostridium species. From a list of 143 peptides, 8 candidate biomarkers were reliably identified as conserved across C. botulinum strains. To avoid discarding other unique peptides, a confidence scale has been implemented in the pipeline giving priority to unique peptides that are identified by a union of algorithms. Conclusions This study demonstrates that implementing a coherent pipeline which includes intensive bioinformatics validation steps is vital for discovery of robust biomarkers. It also emphasises the importance of proteomics based methods in biomarker discovery.

Published
2010

71. Bacteroides,Prevotella, andPorphyromonas

Author

Haroun N. Shah, Saheer E. Gharbia, and Ingar Olsen

Subjects
Bacilli, Antibiotic resistance, biology, Prevotella, food and beverages, Porphyromonas, Ribosomal RNA, Bacteroides, biology.organism_classification, Isolation (microbiology), Bacteroides thetaiotaomicron, Microbiology
Abstract

1 Classification 2 Bacteroides 3 Prevotella 4 Porphyromonas 5 The Current Status of Species that Previously Belonged to the Genus Bacteroides 6 Antibiotic Resistance 7 Molecular Analysis 8 Bacteroides, Prevotella, and Porphyromonas in the Normal Flora 9 Antimicrobial Susceptibility 10 Pathogenicity Keywords: Bacteroides, Prevotella, and Porphyromonas; gram-negative, nonsporing, anaerobic bacilli with rounded or pointed ends; isolation and classification of organisms-presenting difficulties; impact of rRNA sequence analysis; genus Bacteroides-small nonmotile gram-negative bacilli and coccobacilli; Bacteroides thetaiotaomicron; Bacteroides putredinis and Bacteroides microfusus; gram-negative anaerobic bacilli-in normal flora of gastrointestinal tract

Published
2010
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72. Biochemical and Chemical Studies on Strains Designated Prevotella intermedia and Proposal of a New Pigmented Species, Prevotella nigrescens sp. nov

Author

Saheer E. Gharbia and Haroun N. Shah

Subjects
DNA, Bacterial, Cellobiose, Immunology, Microbiology, Malate dehydrogenase, Prevotella nigrescens, Prevotella, Bacteroides, Bacteroidaceae, chemistry.chemical_classification, biology, Pigmentation, Glutamate dehydrogenase, Prevotella intermedia, Nucleic Acid Hybridization, biology.organism_classification, Bacterial Typing Techniques, Culture Media, Phenotype, Enzyme, Biochemistry, chemistry, Fermentation, Xylans, Bacteria
Abstract

A total of 31 strains of Prevotella intermedia were subjected to DNA-DNA hybridization and were characterized by performing physiological tests and by performing a multilocus enzyme analysis, using malate dehydrogenase and glutamate dehydrogenase. All of the strains assigned to P. intermedia fermented glucose and sucrose, hydrolyzed starch but not esculin, and produced indole, acetic, isobutyric, isovaleric, and succinic acids as metabolic end products. The results of DNA reassociation experiments performed with the reference probe permitted separation of the strains into two well-defined homology groups. In addition, strains with DNAs that hybridized with DNA from strain ATCC 25611T (T = type strain) had high levels of peptidase activity and cleaved lipid substrates (4-methylumbelliferyl laurate and 4-methylumbellifelyl elaidate). Multilocus enzyme electrophoresis revealed two electromorphic profiles, one characteristic of strain ATCC 25611T and the other characteristic of strain ATCC 33563T. We propose that a new species, Prevotella nigrescens, should be created for the genetically distinct group of strains that hybridized with strain ATCC 33563T. Strain ATCC 33563 is designated the type strain of P. nigrescens.

Published
1992
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73. Multilocus enzyme electrophoretic analysis and DNA-DNA reassociation of strains designated Prevotella intermedia

Author

Haroun N. Shah and Saheer E. Gharbia

Subjects
chemistry.chemical_classification, Hybridization probe, Glutamate dehydrogenase, Prevotella intermedia, Biology, biology.organism_classification, Applied Microbiology and Biotechnology, Malate dehydrogenase, Molecular biology, chemistry.chemical_compound, Enzyme, chemistry, Biochemistry, Prevotella, DNA, Bacteria
Abstract

Strains of Prevotella intermedia which have been characterized previously by a variety of biochemical and chemical techniques were subjected to multilocus enzyme electrophoresis and DNA-DNA reassociation. Two separate groups of strains were discernible. One had high homology with the type strain ATCC 25611 DNA probe and electrophoretically fast migrating malate dehydrogenase (MDH) (3.8–4.0 cm) and glutamate dehydrogenase (GDH) (3.2–3.4 cm) bands. The other group of strains hybridized with the DNA probe of reference strain ATCC 33563 and possessed slower moving enzymes (MDH, 3.0 cm; GDH, 1.4–1.6 cm). These results indicate that strains currently identified as P. intermedia comprise at least two geno-species, and that the criteria used to define this species are inadequate.

Published
1992
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74. Evidence for independent molecular identity and functional interaction of the haemagglutinin and cysteine proteinase (gingivain) of Porphyromonas gingivalis

Author

Haroun N. Shah, Ann Progulske-Fox, Saheer E. Gharbia, and K. Brocklehurst

Subjects
Microbiology (medical), Erythrocytes, Lysis, Hemagglutination, Carbohydrates, Benzoylarginine Nitroanilide, Biology, Hemolysis, Microbiology, Epitope, 2,2'-Dipyridyl, medicine, Animals, Disulfides, Porphyromonas gingivalis, Antiserum, Sheep, Immune Sera, General Medicine, Hydrogen-Ion Concentration, Hemagglutinin, medicine.disease, biology.organism_classification, Cysteine Endopeptidases, Microscopy, Electron, Hemagglutinins, Biochemistry, Bacterial outer membrane
Abstract

Summary The sequence of events involved in haemagglutination and lysis of erythrocytes by washed cells, vesicles and the culture supernate of Porphyromonas gingivalis strain W83 was monitored by 51Cr release and transmission electronmicroscopy. All preparations, except capsular material and lipopolysaccharide, caused haemagglutination and, by a slow process of attachment and specific attack on the surface structures of the red blood cells, produced minute pores and eventual leakage of cellular contents. N-acetylglucosamine, N-acetylgalactosamine and several other sugars such as glucose and sucrose had no effect on haemagglutination. Antiserum raised against a cloned haemagglutinin of P. gingivalis strain 381 inhibited the activity of strain W83 cells, vesicles and supernate. The antiserum-neutralised supernate lost 70–80% of its hydrolytic activity towards α-N-benzoyl-L-arginine-4-nitroanilide but the residual activity behaved in a manner similar to the native supernate in that it was completely inhibited by the addition of 2,2′-dipyridyl disulphide and was fully restored upon addition of a low-Mr mercaptan. Binding of the antiserum to the haemagglutinin epitope of P. gingivalis still permitted titration of the active centre cysteinyl thiol group of the proteinase. Purified gingivain caused lysis of erythrocytes and was not neutralised by antiserum to the haemagglutinin. These results suggest that, although the haemagglutinin and gingivain are probably separate molecules, they are closely associated on the outer membrane of P. gingivalis and may be functionally related.

Published
1992
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76. Assessment of the Relative Cytotoxicity ofPorphyromonas gingivalisCells, Products, and Components on Human Epithelial Cell Lines

Author

Saheer E. Gharbia, Haroun N. Shah, and C.M. O'Toole

Subjects
Lipopolysaccharides, Cell Survival, Virulence, Basement Membrane, Epithelium, Cell Line, 2,2'-Dipyridyl, Bacterial Proteins, Cell Adhesion, medicine, Humans, Cytotoxic T cell, Centrifugation, Disulfides, Cytotoxicity, Porphyromonas gingivalis, Bacterial Capsules, biology, Cytotoxins, Carcinoma, Cell Membrane, Fatty Acids, Volatile, biology.organism_classification, Molecular biology, Squamous carcinoma, Cell biology, Cysteine Endopeptidases, medicine.anatomical_structure, Cell culture, Carcinoma, Squamous Cell, Periodontics
Abstract

Established human cell lines derived from a transitional cell carcinoma (J82), a squamous carcinoma (SCaBER), and a normal urothelium (HCV-29) were used to assess the relative cytotoxicity and tissue specificity of putative virulence determinants of P. gingivalis W83. Intact cells of W83 had no effect on any of the cell lines, whereas disrupted cells caused extensive cytotoxicity particularly to monolayers of HCV-29 and J82. The purified cysteine proteinase, gingivain, caused marked disruption of the basement membrane of the SCaBER monolayers but had no cytotoxic effects. Use of the thiol-inhibitor, 2,2'-dipyridyl disulphide revealed that the effects observed with the vesicles and the culture supernatant were due to the presence of the cysteine proteinase. The attachment of vesicles to the SCaBER cells was evident in electron micrographs. Short-chain volatile fatty acids added in concentrations equivalent to those present in the culture supernatant had no effect on any of the cell lines tested. Culture supernatants obtained from high speed centrifugation (150,000 x g) showed no cytotoxic effects. This was in marked contrast to the supernatant obtained by lower sedimentation (18,000 x g), which damaged all monolayers tested. These results suggest that these cell lines are potentially useful for assessing putative virulence determinants of P. gingivalis and other periodontal pathogens.

Published
1992
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78. Elucidation of the outer membrane proteome of Salmonella enterica serovar Typhimurium utilising a lipid-based protein immobilization technique

Author

Roger Karlsson, Hazel Appleton, Catherine Arnold, Darren Chooneea, Haroun N. Shah, and Vesela Encheva

Subjects
Microbiology (medical), Proteomics, Proteases, Proteome, medicine.medical_treatment, Lipoproteins, lcsh:QR1-502, Carbonates, Cell Fractionation, Microbiology, lcsh:Microbiology, Mass Spectrometry, Surface-Active Agents, Research article, medicine, Protease, biology, Salmonella typhi, biology.organism_classification, Cytosol, Microscopy, Electron, Immobilized Proteins, Membrane protein, Biochemistry, Salmonella enterica, Bacterial outer membrane, Bacterial Outer Membrane Proteins, Chromatography, Liquid
Abstract

Background Salmonella enterica serovar Typhimurium (S. Typhimurium) is a major cause of human gastroenteritis worldwide. The outer membrane proteins expressed by S. Typhimurium mediate the process of adhesion and internalisation within the intestinal epithelium of the host thus influencing the progression of disease. Since the outer membrane proteins are surface-exposed, they provide attractive targets for the development of improved antimicrobial agents and vaccines. Various techniques have been developed for their characterisation, but issues such as carryover of cytosolic proteins still remain a problem. In this study we attempted to characterise the surface proteome of S. Typhimurium using Lipid-based Protein Immobilisation technology in the form of LPI™ FlowCells. No detergents are required and no sample clean up is needed prior to downstream analysis. The immobilised proteins can be digested with proteases in multiple steps to increase sequence coverage, and the peptides eluted can be characterised directly by liquid chromatography - tandem mass spectrometry (LC-MS/MS) and identified from mass spectral database searches. Results In this study, 54 outer membrane proteins, were identified with two or more peptide hits using a multi-step digest approach. Out of these 28 were lipoproteins, nine were involved in transport and three with enzyme activity These included the transporters BtuB which is responsible for the uptake of vitamin B12, LamB which is involved in the uptake of maltose and maltodextrins and LolB which is involved in the incorporation of lipoproteins in the outer membrane. Other proteins identified included the enzymes MltC which may play a role in cell elongation and division and NlpD which is involved in catabolic processes in cell wall formation as well as proteins involved in virulence such as Lpp1, Lpp2 and OmpX. Conclusion Using a multi-step digest approach the LPI™ technique enables the incorporation of a multi-step protease work flow ensuring enough sequence coverage of membrane proteins subsequently leading to the identification of more membrane proteins with higher confidence. Compared to current sub-cellular fractionation procedures and previous published work, the LPI™ technique currently provides the widest coverage of outer membrane proteins identified as demonstrated here for Salmonella Typhimurium.

Published
2009

79. Proteomic analysis of the adaptive response of Salmonella enterica serovar Typhimurium to growth under anaerobic conditions

Author

Vesela Encheva, Saheer E. Gharbia, and Haroun N. Shah

Subjects
Salmonella typhimurium, Proteome, Inositol monophosphatase, Down-Regulation, Microbiology, Superoxide dismutase, Peptide mass fingerprinting, Bacterial Proteins, Malate Dehydrogenase, Electrophoresis, Gel, Two-Dimensional, Anaerobiosis, chemistry.chemical_classification, biology, Permease, Gene Expression Regulation, Bacterial, Fumarate reductase, biology.organism_classification, Adaptation, Physiological, Up-Regulation, Succinate Dehydrogenase, Metabolic pathway, Enzyme, chemistry, Biochemistry, Salmonella enterica, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Fermentation, biology.protein, Carrier Proteins, Metabolic Networks and Pathways
Abstract

In order to survive in the host and initiate infection,Salmonella entericaneeds to undergo a transition between aerobic and anaerobic growth by modulating its central metabolic pathways. In this study, a comparative analysis of the proteome ofS. entericaserovar Typhimurium grown in the presence or absence of oxygen was performed. The most prominent changes in expression were measured in a semiquantitative manner using difference in-gel electrophoresis (DIGE) to reveal the main protein factors involved in the adaptive response to anaerobiosis. A total of 38 proteins were found to be induced anaerobically, while 42 were repressed. The proteins of interest were in-gel digested with trypsin and identified by MALDI TOF mass spectrometry using peptide mass fingerprinting. In the absence of oxygen, many fermentative enzymes catalysing reactions in the mixed-acid or arginine fermentations were overexpressed. In addition, the enzyme fumarate reductase, which is known to provide an alternative electron acceptor for the respiratory chains in the absence of oxygen, was shown to be induced. Increases in expression of several glycolytic and pentose phosphate pathway enzymes, as well as two malic enzymes, were detected, suggesting important roles for these in anaerobic metabolism. Substantial decreases in expression were observed for a large number of periplasmic transport proteins. The majority of these are involved in the uptake of amino acids and peptides, but permeases transporting iron, thiosulphate, glucose/galactose, glycerol 3-phosphate and dicarboxylic acids were also repressed. Decreases in expression were also observed for a superoxide dismutase, ATP synthase, inositol monophosphatase, and several chaperone and hypothetical proteins. The changes were monitored in two different isolates, and despite their very similar expression patterns, some variability in the adaptive response to anaerobiosis was also observed.

Published
2009

80. Comparison of the amino acid uptake profile of reference and clinical isolates of Fusobacterium nucleatum subspecies

Author

Saheer E. Gharbia and Haroun N. Shah

Subjects
Microbiology (medical), Arginine, Immunology, Gingiva, Subspecies, Microbiology, chemistry.chemical_compound, Glutamates, Species Specificity, stomatognathic system, Cysteine, Amino Acids, General Dentistry, Bacteroidaceae, Histidine, chemistry.chemical_classification, Fusobacterium nucleatum, biology, Ornithine, biology.organism_classification, Amino acid, stomatognathic diseases, chemistry, Biochemistry, Bacteria
Abstract

Human isolates of Fusobacterium nucleatum subspecies appear to colonize different niches in the oral cavity, which may be reflected in their nutritional properties. Consequently the utilization of nitrogenous substrates, their sources of energy (supplied here as amino acids) were compared between the 3 subspecies using the reference strain and fresh clinical isolates of each subspecies. All strains incorporated mainly acidic and basic amino acids but significant differences occurred between subspecies. Both reference and clinical isolates of F. nucleatum subspecies polymorphum utilized all amino acids in the medium but the levels of glutamate, arginine and cysteine were noticeably higher in the reference strain. By contrast, F. nucleatum subspecies fusiforme used a very restricted range of amino acids, of which only glutamate, arginine, histidine and cysteine were taken up at greater than 0.5 mM. F. nucleatum subspecies nucleatum utilized fewer amino acids than F. nucleatum subspecies polymorphum but higher concentrations were taken up by the former. Clinical isolates of F. nucleatum subspecies nucleatum incorporated polar and nonpolar neutral amino acids poorly but their levels increased steadily as a clinical isolate was subcultured over a period of 4 months, and was eventually similar to the reference strain. The effect of adding the key catabolic substrate, glutamate (10 mM), on the amino acid uptake profile of F. nucleatum subspecies nucleatum resulted in the complete suppression of the dibasic amino acids arginine, ornithine and histidine. Strains of this subspecies could grow on glutamate as a major source of carbon and energy but, morphologically, the cells appeared somewhat distended and had a tendency to clump.

Published
1991
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81. Intrageneric Relationships of Members of the Genus Fusobacterium as Determined by Reverse Transcriptase Sequencing of Small-Subunit rRNA

Author

Haroun N. Shah, Duncan R. Clark, Matthew D. Collins, Saheer E. Gharbia, and Paul A. Lawson

Subjects
Genetics, Base Sequence, biology, Molecular Sequence Data, Immunology, RNA-Directed DNA Polymerase, Fusobacterium, Fusobacterium gonidiaformans, biology.organism_classification, Microbiology, Fusobacterium periodonticum, RNA, Bacterial, stomatognathic diseases, Fusobacterium mortiferum, stomatognathic system, Fusobacterium necrogenes, Fusobacterium ulcerans, RNA, Ribosomal, 16S, Fusobacterium nucleatum, Sequence Alignment, Phylogeny, Fusobacterium russii
Abstract

The phylogenetic interrelationships of 14 members of the genus Fusobacterium were investigated by performing a comparative analysis of the 16S rRNA sequences of these organisms. The sequence data revealed considerable intrageneric heterogeneity. The four species Fusobacterium nucleatum (including F. nucleatum subsp. nucleatum, F. nucleatum subsp. polymorphum, "F. nucleatum subsp. fusiforme," and "F. nucleatum subsp. animalis"), Fusobacterium alocis, Fusobacterium periodonticum, and Fusobacterium simiae, which colonize oral cavities, exhibited high levels of sequence homology with each other and formed a distinct group within the genus. Fusobacterium mortiferum, Fusobacterium varium, and Fusobacterium ulcerans also formed a phylogenetically coherent group, as did the two species Fusobacterium gonidiaformans and Fusobacterium necrophorum. Fusobacterium russii and Fusobacterium necrogenes displayed no specific relationship with any of the other fusobacteria. The sequence data are discussed in the context of previous physiological and chemical findings.

Published
1991
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82. Isolation, purification and characterisation of 2-oxoglutarate reductase fromFusobacterium nucleatum

Author

Haroun N. Shah and Saheer E. Gharbia

Subjects
chemistry.chemical_classification, biology, Molecular mass, Glyoxylate cycle, Metabolism, Reductase, biology.organism_classification, Microbiology, Molecular biology, Enzyme, chemistry, Biochemistry, Fusobacterium, Genetics, biology.protein, Citrate synthase, Fusobacterium nucleatum, Molecular Biology
Abstract

2-Oxoglutarate reductase from Fusobacterium nucleatum was isolated by thiol-disulphide interchange covalent chromatography. The enzyme was purified approximately 4000-fold and had a molecular mass of 68 kDa. The Michaelis constants for 2-oxoglutarate and NADH were 6.4 × 10−5 and 0.4 × 10−5, respectively. The involvement of sulphahydryl groups in catalysis was shown from the inhibition of 2-oxoglutarate reduction in the presence of 2,2′-dipyridyl disulphide and reactivation with 2-mercaptoethanol. Allosteric effectors did not alter the rate of the reaction, or the enzyme stability. With the exception of 2-oxoglutarate, none of the other oxo-acids such as oxaloacetate, pyruvate, 2-oxobutyrate and glyoxylate were reduced. Although 2-oxoglutarate oxidised NADPH to a limited extent (3%), the enzyme was almost entirely specific towards NADH. 2-Oxoglutarate reductase was stable at 45°C for 10 min, while incubation at 60°C abolished all activity.

Published
1991
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83. Utilization of aspartate, glutamate, and their corresponding peptides byFusobacterium nucleatum subspecies andPorphyromonas gingivalis

Author

Haroun N. Shah and Saheer E. Gharbia

Subjects
chemistry.chemical_classification, biology, Polyglutamate, Catabolism, Glutamate receptor, Peptide, General Medicine, Metabolism, biology.organism_classification, Fluorescamine, Applied Microbiology and Biotechnology, Microbiology, Amino acid, chemistry.chemical_compound, chemistry, Biochemistry, Fusobacterium nucleatum
Abstract

Glutamate and aspartate are key amino acids for catabolism byFusobacterium nucleatum subspecies andPorphyromonas gingivalis respectively. However, peptides such as yeast extract are their preferred sources of energy. To determine more precisely the possible nature of these peptides, we examined the utilization of these amino acids and their corresponding peptides by cell suspension experiments with a fluorescamine labeling technique. High molecular weight (M.W.) polyglutamate (>40,000) was poorly utilized by all taxa, whereas 95% of its low-M.W. peptide (2,000–5,000) was used byF. nucleatum subspeciesnucleatum, but the remaining two subspecies utilized 90% polyaspartate within the same period. ForF. nucleatum subspeciesnucleatum as the test organism, T0.5 (the time taken to use 50% of the test substrate) was 1.7 h longer for glutamate than for the homopolymer. Furthermore, in the presence of both substrates, polyglutamate suppressed the uptake of glutamate until about 50% (ca. 1.5 mmol/L) of the peptide was used, after which the incorporation of the free amino acid started. A similar pattern of utilization was observed inP. gingivalis with its preferred peptide polyaspartate, for which the T0.5 was three times shorter than its monomer, aspartate. Both species had the capacity to utilize the heteropolymer, poly aspartate/glutamate, but at a significantly slower rate than the corresponding homopolymer.

Published
1991
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84. The GenusBacteroides

Author

Sally Langham, Wibke Kallow, Rogério C Jacinto, Haroun N. Shah, Saheer E. Gharbia, Nadia Z. Ahmod, and Martin Welker

Subjects
Systematics, Flora, Type species, biology, Genus, Zoology, Obligate anaerobe, Ribosomal RNA, Bacteroides, Bacteroides fragilis, biology.organism_classification
Abstract

The genus Bacteroides has been described over 100 years and comprises a group of small nonmotile, nonsporing, Gram-negative rods; they are obligate anaerobes and form a major part of the bacterial flora of the human intestinal tract. Poor circumscription of this group has led to the genus accumulating a large and diverse collection of species that only superficially resembles this description but could not be accommodated elsewhere. Based largely on chemotaxonomic and genetic criteria the genus was reclassified (Shah and Collins, 1989) to encompass the type species Bacteroides fragilis and members of the ‘B. fragilis group’. This more restricted definition, spurred on mainly by 16S rRNA (ribosomal ribonucleic acid), has encouraged more in-depth analysis of the colonic flora and a large number of new species have been described. Full genomes of four species have been completed. Such studies are providing a better basis for elucidating the biological role of specific species within the intestinal tract and their involvement in a variety of physiological and cellular processes. Keywords: bacteroides; systematics; identification; salient features; biology and pathogenicity

Published
2008
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85. High throughput identification of clinical isolates of Staphylococcus aureus using MALDI-TOF-MS of intact cells

Author

Armine Sefton, Ingrid Innes, Haroun N. Shah, Angela M. Kearns, Graham Ball, Lakshani Rajakaruna, Vesela Encheva, Diane Dare, Renata Culak, Helen Sutton, Linda Molenaar, Melvin Eydmann, and Gillian Hallas

Subjects
Microbiology (medical), Staphylococcus aureus, Cell Culture Techniques, Human pathogen, Biology, Mass spectrometry, medicine.disease_cause, Microbiology, Bacterial Proteins, RNA, Ribosomal, 16S, Genotype, Databases, Genetic, Genetics, medicine, Humans, Sample preparation, Molecular Biology, Ecology, Evolution, Behavior and Systematics, Bacteriological Techniques, Reproducibility of Results, Staphylococcal Infections, 16S ribosomal RNA, Matrix-assisted laser desorption/ionization, Infectious Diseases, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Time-of-flight mass spectrometry
Abstract

Staphylococcus aureus remains an important human pathogen responsible for a high burden of disease in healthcare and community settings. The emergence of multidrug-resistant strains is of increasing concern world-wide. The identification of S. aureus is currently based upon phenotypic and genotypic methods. Here, an alternative approach involving mass spectral analysis of surface-associated proteins of intact bacterial cells by matrix-assisted laser desorption/ionisation time of flight mass spectrometry (MALDI-TOF-MS) was investigated using 95 isolates obtained directly from a clinical laboratory at The Royal London Hospital and 39 isolates from the Staphylococcal Reference Unit, Health Protection Agency, London. Results obtained indicate that clinical isolates share many common mass ions with-type/reference strains which allowed their correct identification when searched against a comprehensive database that has been in the process of development for several years. The existing database contains more than 5000 profiles of various bacterial pathogens, but comprises mainly type or reference strains. The MicrobeLynx software successfully identified all isolates to the correct genus and all but four to the correct species. These were misidentified in the first instance due to contamination or low mass ion intensity but once the cultures were purified and re-analysed they were confirmed as S. aureus by both MALDI-TOF-MS and 16S rRNA sequence analysis. The high percentage of correct identifications coupled with the high speed and the minimal sample preparation required, indicate that MALDI-TOF-MS has the potential to perform high throughput identification of clinical isolates of S. aureus despite the inherent diversity of this species. The method is, however, only reproducible if variable parameters such as sample preparation, media, growth condition, etc. are standardised.

Published
2008

86. Mass Spectrometry for Microbial Proteomics

Author

Haroun N. Shah, Saheer E. Gharbia, Haroun N. Shah, and Saheer E. Gharbia

Subjects
Proteomics--Methodology, Mass spectrometry, Microbial proteins--Spectra
Abstract

New advances in proteomics, driven largely by developments in mass spectrometry, continue to reveal the complexity and diversity of pathogenic mechanisms among microbes that underpin infectious diseases. Therefore a new era in medical microbiology is demanding a rapid transition from current procedures to high throughput analytical systems for the diagnosis of microbial pathogens. This book covers the broad microbiological applications of proteomics and mass spectrometry. It is divided into six sections that follow the general progression in which most microbiology laboratories are approaching the subject –Transition, Tools, Preparation, Profiling by Patterns, Target Proteins, and Data Analysis.

Published
2010

87. Heterogeneity within Fusobacterium nucleatum, proposal of four subspecies

Author

Haroun N. Shah and Saheer E. Gharbia

Subjects
Genetics, stomatognathic diseases, stomatognathic system, Biology, Fusobacterium nucleatum, Subspecies, biology.organism_classification, Applied Microbiology and Biotechnology, Microbiology
Abstract

Fusobacterium nucleatum strains, isolated from man and animals, were shown to comprise four centres of variation within the species by using a variety of biochemical tests. DNA-DNA hybridization data indicated that they should differences between the groups to warrant their placement into four subspecies for which we propose the following: F. nucleatum subsp. nucleatum (commonly isolated from diseased sites), F. nucleatum subsp. polymorphum (from healthy sites, most frequently isolated), F. nucleatum subsp. fusiforme (from healthy sites, most frequently isolated), F. nucleatum subsp. fusiforme (from healthy sites, rarely isolated) and F. nucleatum subsp. animalis from the colon of animals.

Published
1990
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88. Bacterial examination of endodontic infections by clonal analysis in concert with denaturing high-performance liquid chromatography

Author

Haroun N. Shah, Brenda Paula Figueiredo de Almeida Gomes, D. Rajendram, Rogério de Castilho Jacinto, and M. Desai

Subjects
Microbiology (medical), Staphylococcus aureus, Immunology, medicine.disease_cause, Gram-Positive Bacteria, Nucleic Acid Denaturation, Microbiology, DNA, Ribosomal, Polymerase Chain Reaction, Enterococcus faecalis, law.invention, Denaturing high performance liquid chromatography, Gram-Negative Anaerobic Straight, Curved, and Helical Rods, law, RNA, Ribosomal, 16S, medicine, Tannerella forsythia, Bacteroides, Humans, General Dentistry, Bacillaceae, Polymerase chain reaction, Chromatography, High Pressure Liquid, DNA Primers, biology, Bacteria, Eubacterium, Peptostreptococcus, Dialister pneumosintes, Dental Pulp Diseases, Fusobacterium, biology.organism_classification, Molecular biology, Abscess, Clone Cells, Actinobacteria, Lactobacillus, Streptococcus anginosus, Anaerobic bacteria, Porphyromonas gingivalis
Abstract

Background/aims: The aim of this study was to examine the diversity of bacterial species in the infected root canals of teeth associated with endodontic abscesses by cloning and sequencing techniques in concert with denaturing high-performance liquid chromatography. Methods: Samples collected from five infected root canals were subjected to polymerase chain reaction (PCR) with universal 16S ribosomal DNA primers. Products of these PCRs were cloned and sequenced. Denaturing high-performance liquid chromatography (DHPLC) was used as a screening method to reduce the number of clones necessary for DNA sequencing. Results: All samples were positive for the presence of bacteria and a range of 7–13 different bacteria were found per root canal sample. In total, 48 different oral clones were detected among the five root canal samples. Olsenella profusa was the only species present in all samples. Porphyromonas gingivalis, Dialister pneumosintes, Dialister invisus, Lachnospiraceae oral clone, Staphylococcus aureus, Pseudoramibacter alactolyticus, Peptostreptococcus micros and Enterococcus faecalis were found in two of the five samples. The majority of the taxa were present in only one sample, for example Tannerella forsythia, Shuttleworthia satelles and Filifactor alocis. Some facultative anaerobes that are frequently isolated from endodontic infections such as E. faecalis, Streptococcus anginosus and Lactobacillus spp. were also found in this study. Conclusion: Clonal analysis of the microflora associated with endodontic infections revealed a wide diversity of oral species.

Published
2007

89. New approaches to identification of bacterial pathogens by surface enhanced laser desorption/ionization time of flight mass spectrometry in concert with artificial neural networks, with special reference to Neisseria gonorrhoeae

Author

Lee Lancashire, Graham Ball, Renata Culak, Oliver Schmid, and Haroun N Shah

Subjects
Microbiology (medical), Sexually transmitted disease, Back propagation algorithm, medicine.disease_cause, Microbiology, Polymerase Chain Reaction, Ion Channels, RNA, Ribosomal, 16S, medicine, Humans, DNA Primers, Artificial neural network, Bacteria, Base Sequence, Chemistry, General Medicine, equipment and supplies, Neisseria gonorrhoeae, Surface-enhanced laser desorption/ionization, Rapid identification, RNA, Bacterial, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Identification (biology), Neural Networks, Computer, Time-of-flight mass spectrometry, Biological system, Neisseria
Abstract

Surface enhanced laser desorption/ionization-time of flight mass spectrometry (SELDI-TOF MS) has been applied in large numbers of oncological studies but the microbiological field has not been extensively explored to date. This paper describes the application of SELDI-TOF MS in concert with a multi-layer perceptron artificial neural network (ANN) with a back propagation algorithm for the identification of Neisseria gonorrhoeae. N. gonorrhoeae, the aetiological agent of gonorrhoea, is the second most common sexually transmitted disease in the UK and USA. Analysis of over 350 strains of N. gonorrhoeae and closely related species by SELDI-TOF MS facilitated the design of an ANN model and revealed 20 ion peak descriptors of positive, negative and secondary nature that were paramount for the identification of the pathogen. The model performed with over 96 % efficiency when based on these 20 ion peak descriptors and exhibited a sensitivity of 95.7 % and a specificity of 97.1 %, with an area under the curve value of 0.996. The technology has the potential to link several ANN models for a comprehensive rapid identification platform for clinically important pathogens.

Published
2005

90. The distribution of the bft alleles among enterotoxigenic Bacteroides fragilis strains from stool specimens and extraintestinal sites

Author

Nurver Ulger, Güner Söyletir, Tuncay Celenk, Bahadir M. Gulluoglu, Saheer E. Gharbia, Aysegul Yagci, Haroun N. Shah, Levhi Akin, Pakize Demirkalem, and Dunstan Rajendram

Subjects
Gene isoform, Adult, DNA, Bacterial, Colorectal cancer, Bacterial Toxins, Biology, medicine.disease_cause, Microbiology, Polymerase Chain Reaction, Bacteroides fragilis, Feces, Polymorphism (computer science), medicine, Humans, Gene, Alleles, Aged, DNA Primers, Aged, 80 and over, Toxin, Metalloendopeptidases, Middle Aged, Fragilysin, biology.organism_classification, medicine.disease, Bacteroides Infections, Infectious Diseases, Case-Control Studies, Colonic Neoplasms, Restriction fragment length polymorphism, Polymorphism, Restriction Fragment Length
Abstract

Enterotoxigenic Bacteroides fragilis (ETBF) has been implicated in diarrhoeal illness in animals and humans. Recent data suggest that ETBF is associated with flares of inflammatory bowel disease. Toxigenicity is attributed to expression of a toxin referred to as fragilysin, which stimulates fluid accumulation in ligated intestinal segments and alter the morphology of human intestinal cells. Three different isoforms or variants of the enterotoxin gene, designated bft-1, bft-2, and bft-3, have been identified. In this study we investigated the distribution of bft alleles among ETBF strains in stool specimens from patients with colon cancer (n: 31), the control patients (n: 8) and extraintestinal sources (n: 15). We used restriction fragment length polymorphism analysis of the PCR-amplified enterotoxin gene and sequencing the PCR-product to detect the isoforms of bft gene. Among the stool strains, bft-1 was found to be more common than bft-2; as it was detected 27 of 31 strains from colon cancer patients and 7 of 8 control strains. The bft-1 isoform was also found in almost all isolates from extraintestinal sites. No bft-3 subtype was detected among all tested strains.

Published
2005

91. Proteome analysis of serovars Typhimurium and Pullorum of Salmonella enterica subspecies I

Author

Shajna Begum, Vesela Encheva, Saheer E. Gharbia, Haroun N. Shah, and Robin Wait

Subjects
Proteomics, Microbiology (medical), Serotype, Salmonella, Proteome, Population, lcsh:QR1-502, Biology, medicine.disease_cause, Microbiology, lcsh:Microbiology, Bacterial Proteins, Ribosomal protein, medicine, Serotyping, education, Gene, education.field_of_study, Gene Expression Profiling, Salmonella enterica, Gene Expression Regulation, Bacterial, biology.organism_classification, Research Article
Abstract

Background Salmonella enterica subspecies I includes several closely related serovars which differ in host ranges and ability to cause disease. The basis for the diversity in host range and pathogenic potential of the serovars is not well understood, and it is not known how host-restricted variants appeared and what factors were lost or acquired during adaptations to a specific environment. Differences apparent from the genomic data do not necessarily correspond to functional proteins and more importantly differential regulation of otherwise identical gene content may play a role in the diverse phenotypes of the serovars of Salmonella. Results In this study a comparative analysis of the cytosolic proteins of serovars Typhimurium and Pullorum was performed using two-dimensional gel electrophoresis and the proteins of interest were identified using mass spectrometry. An annotated reference map was created for serovar Typhimurium containing 233 entries, which included many metabolic enzymes, ribosomal proteins, chaperones and many other proteins characteristic for the growing cell. The comparative analysis of the two serovars revealed a high degree of variation amongst isolates obtained from different sources and, in some cases, the variation was greater between isolates of the same serovar than between isolates with different sero-specificity. However, several serovar-specific proteins, including intermediates in sulphate utilisation and cysteine synthesis, were also found despite the fact that the genes encoding those proteins are present in the genomes of both serovars. Conclusion Current microbial proteomics are generally based on the use of a single reference or type strain of a species. This study has shown the importance of incorporating a large number of strains of a species, as the diversity of the proteome in the microbial population appears to be significantly greater than expected. The characterisation of a diverse selection of strains revealed parts of the proteome of S. enterica that alter their expression while others remain stable and allowed for the identification of serovar-specific factors that have so far remained undetected by other methods.

Published
2005

92. Which species concept for pathogenic bacteria? An E-Debate

Author

Sylvain Godreuil, Michel Tibayrenc, Frederick M. Cohan, and Haroun N. Shah

Subjects
Microbiology (medical), Recombination, Genetic, Bacteria, Concept Formation, Zoology, Library science, Biological evolution, Health protection, Biology, Models, Theoretical, Microbiology, Biological Evolution, Infectious Diseases, Molecular Diagnostic Techniques, Genetics, Molecular diagnostic techniques, Animals, Humans, Molecular Biology, Ecology, Evolution, Behavior and Systematics, Molecular identification
Abstract

Sylvain Godreuil, Frederick Cohan, Haroun Shah, Michel Tibayrenc* Genetique et Evolution des Maladies Infectieuses (GEMI), UMR IRD/CNRS 2724, IRD, BP 64501, 34374 Montpellier Cedex 5, France Department of Biology, Wesleyan University, Middletown, CT 06459-0170, USA Molecular Identification Services, NCTC, Health Protection Agency, Specialist and Reference Microbiology Division (SRMD), 61 Colindale Avenue, London NW9 5HT, UK

Published
2004

93. Reclassification of Bacteroides levii (Holdeman, Cato, and Moore) in the Genus Porphyromonas, as Porphyromonas levii comb. nov

Author

Matthew D. Collins, Haroun N. Shah, Ingar Olsen, Bruce J. Paster, and Floyd E. Dewhirst

Subjects
biology, Porphyromonas levii, Immunology, food and beverages, Zoology, biology.organism_classification, Microbiology, Incertae sedis, Type species, Taxonomy (biology), Bacteroides fragilis, Bacteroides, Ribosomal DNA, Bacteroidaceae
Abstract

The genus Bacteroides was recently redefined to include only the type species Bacteroides fragilis and closely related taxa. Most other species that were previously designated Bacteroides have been reclassified in new genera. The taxonomic position of Bacteroides levii (Holdeman, Cato, and Moore) has remained incertae sedis. On the basis of biochemical, chemical and comparative 16S rRNA sequence analyses, this species shares a high degree of similarity with members of the genus Porphyromonas. We therefore formally propose that Bacteroides levii (Holdeman, Cato, and Moore) be reclassified in the genus Porphyromonas, as Porphyromonas levii comb. nov.

Published
1995
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94. Matrix-assisted laser desorption/ionization time-of-flight mass spectrometry and proteomics: a new era in anaerobic microbiology

Author

Oliver Schmid, Carrina J. Keys, Saheer E. Gharbia, and Haroun N. Shah

Subjects
Microbiology (medical), Fusobacterium nucleatum, Proteome, business.industry, Matrix assisted laser desorption ionization time of flight, Proteomics, Diagnostic system, Mass spectrometry, Prevotella intermedia, Microbiology, Matrix-assisted laser desorption/ionization, Bacteria, Anaerobic, Infectious Diseases, Ionization, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Medicine, Porphyromonas, Time-of-flight mass spectrometry, business
Abstract

Genome sequence data provide a framework for predicting potential microbial activities; however, the proteome content of the cell dictates its response to its environment. Microbiology is witnessing a major initiative to elucidate the nature of the proteome of large numbers of species. The tool driving the proteomic revolution is matrix-assisted laser desorption/ionization time-of-flight mass spectrometry. During the analysis process, proteins are ionized and separated on the basis of their mass-to-charge ratios, which results in a characteristic mass-spectral profile. Because of the dynamic nature of the cell and the large number of external parameters that could influence its mass-spectral profile, considerable work was needed initially to optimize sample analysis and obtain consistent and reproducible results. For many anaerobes that grow poorly or are nonreactive in most diagnostic systems, proteome analysis is likely to have a major impact on microbial diagnosis and the delineation of centers of diversity associated with infections.

Published
2002

95. Gastrointestinal microflora studies in late-onset autism

Author

Elizabeth M. Marlowe, Erik K. Read, Marja Liisa Vaisanen, Paul A. Lawson, Mehmet Baysallar, Chengxu Liu, Palwasha Nasir, Paula Summanen, Matthew D. Collins, Patricia Manning, Richard H. Sandler, Thomas J. Tomzynski, Ellen R. Bolte, David A. Haake, Haroun N. Shah, Hannah M. Wexler, Maureen McTeague, Eric A. Johnson, Denise Molitoris, Rial D. Rolfe, Yuli Song, Ajay Kaul, and Sydney M. Finegold

Subjects
Microbiology (medical), Clostridium, Flora, business.industry, Regressive autism, Clostridium difficile, medicine.disease, Developmental disorder, Infectious Diseases, El Niño, Child, Preschool, mental disorders, Immunology, medicine, Autism, Humans, Age of onset, Age of Onset, Autistic Disorder, business, Child, Digestive System, Feces
Abstract

Some cases of late-onset (regressive) autism may involve abnormal flora because oral vancomycin, which is poorly absorbed, may lead to significant improvement in these children. Fecal flora of children with regressive autism was compared with that of control children, and clostridial counts were higher. The number of clostridial species found in the stools of children with autism was greater than in the stools of control children. Children with autism had 9 species of Clostridium not found in controls, whereas controls yielded only 3 species not found in children with autism. In all, there were 25 different clostridial species found. In gastric and duodenal specimens, the most striking finding was total absence of non-spore-forming anaerobes and microaerophilic bacteria from control children and significant numbers of such bacteria from children with autism. These studies demonstrate significant alterations in the upper and lower intestinal flora of children with late-onset autism and may provide insights into the nature of this disorder.

Published
2002

96. Biochemical properties of Fusobacterium naviforme and phenotypically similar isolates

Author

Haroun N. Shah and Saheer E. Gharbia

Subjects
chemistry.chemical_classification, Glutamate dehydrogenase, Reductase, Biology, biology.organism_classification, Applied Microbiology and Biotechnology, Homology (biology), Microbiology, Amino acid, chemistry.chemical_compound, Fusobacterium naviforme, chemistry, Peptidoglycan, Bacteroidaceae, Bacteria
Abstract

Three strains which resemble the type strain of Fusobacterium naviforme (ATCC 25832) by morphological and physiological criteria were isolated from human clinical specimens. All were non-fermentative, produced indole and, in common with other members of the genus Fusobacterium, butyrate was a major end-product of metabolism. Glutamate dehydrogenase and 2-oxoglutarate reductase were present in both taxa, but the enzymes of the test strains migrated to only about half the distance of that of strain ATCC 25832. The latter contained meso-diaminopimelic acid as its peptidoglycan dibasic amino acid whereas the test strains possessed meso-lanthionine. The wide divergence in DNA base composition between strain ATCC 25832 (49 mol% G + C) and the clinical isolates (ca 30–31 mol% G + C) was reflected in their low DNA-DNA homology (ca 5–15%). The present study therefore revealed major differences between F. naviforme (ATCC 25832) and the new isolates and indicate that the latter may belong to a hitherto undescribed taxon within the genus Fusobacterium.

Published
1991
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98. Characterization of a novel bacteriophage in Fusobacterium varium

Author

Haroun N. Shah, David M.A. Andrews, and SE Gharbia

Subjects
Microbiology (medical), biology, Fusobacterium varium, Fusobacterium, biology.organism_classification, Virology, Virus, Microbiology, Bacteriophage, Infectious Diseases, Bacteriophages, Bacteroidaceae, Bacteria
Published
1997

99. Oral pathogens as contributors to systemic infections

Author

JC Williams, Haroun N. Shah, SE Gharbia, Kishor Gulabivala, David M.A. Andrews, and Nina Mehta

Subjects
Microbiology (medical), medicine.medical_specialty, Mouth, Candidiasis, Stomach Diseases, Drug Resistance, Microbial, Bacterial Infections, Biology, Microbiology, stomatognathic diseases, Infectious Diseases, Virology, Family medicine, medicine, Humans, Dental Pulp Cavity, Periodontal Diseases
Abstract

Overview of a conference held at the Eastman Dental Institute and Hospital for Royal College of Surgeons of England, London, UK, 7–8 March 1996.

Published
1996

100. Demonstration that 1-trans-epoxysuccinyl-L-leucylamido-(4-guanidino) butane (E-64) is one of the most effective low Mr inhibitors of trypsin-catalysed hydrolysis. Characterization by kinetic analysis and by energy minimization and molecular dynamics simulation of the E-64-beta-trypsin complex

Author

Suneal K. Sreedharan, Keith Brocklehurst, SE Gharbia, Simon M. Brocklehurst, Haroun N. Shah, Chandra S. Verma, and Leo S. D. Caves

Subjects
Tris, Models, Molecular, Stereochemistry, Protein Conformation, Molecular Sequence Data, Molecular Conformation, Guanidinium Cation, E-64, Crystallography, X-Ray, Biochemistry, Binding, Competitive, Benzamidine, Catalysis, chemistry.chemical_compound, Structure-Activity Relationship, Leucine, medicine, Animals, Computer Simulation, Trypsin, Carboxylate, Amino Acid Sequence, Molecular Biology, Clostripain, Molecular Structure, Cell Biology, Ligand (biochemistry), Kinetics, chemistry, Cattle, Trypsin Inhibitors, Software, medicine.drug, Research Article
Abstract

1-trans-Epoxysuccinyl-L-leucylamido(4-guanidino)butane (E-64) was shown to inhibit beta-trypsin by a reversible competitive mechanism; this contrasts with the widely held view that E-64 is a class-specific inhibitor of the cysteine proteinases and reports in the literature that it does not inhibit a number of other enzymes including, notably, trypsin. The K1, value (3 x 10(-5) M) determined by kinetic analysis of the hydrolysis of N alpha-benzoyl-L-arginine 4-nitroanilide in Tris/HCl buffer, pH 7.4, at 25 degrees C, I = 0.1, catalysed by beta-trypsin is comparable with those for the inhibition of trypsin by benzamidine and 4-aminobenzamidine, which are widely regarded as the most effective low Mr inhibitors of this enzyme. Computer modelling of the beta-trypsin-E64 adsorptive complex, by energy minimization, molecular dynamics simulation and Poisson-Boltzmann electrostatic-potential calculations, was used to define the probable binding mode of E-64; the ligand lies parallel to the active-centre cleft, anchored principally by the dominant electrostatic interaction of the guanidinium cation at one end of the E-64 molecule with the carboxylate anion of Asp-171 (beta-trypsin numbering from Ile-1) in the S1-subsite, and by the interaction of the carboxylate substituent on C-2 of the epoxide ring at the other end of the molecule with Lys-43; the epoxide ring of E-64 is remote from the catalytic site serine hydroxy group. The possibility that E-64 might bind to the cysteine proteinases clostripain (from Clostridium histolyticum) and alpha-gingivain (one of the extracellular enzymes from phyromonas gingivalis) in a manner analogous to that deduced for the beta-trypsin-E-64 complex is discussed.

Published
1996

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