Your search keyword '"Heather M. Brewer"' showing total 42 results

1. Nipah Virus-Like Particle Egress Is Modulated by Cytoskeletal and Vesicular Trafficking Pathways: a Validated Particle Proteomics Analysis

Author

Gunner P. Johnston, Birgit Bradel-Tretheway, Paul D. Piehowski, Heather M. Brewer, Bom Nae Rin Lee, Nicholas T. Usher, J. Lizbeth Reyes Zamora, Victoria Ortega, Erik M. Contreras, Jeremy R. Teuton, Jason P. Wendler, Keesha M. Matz, Joshua N. Adkins, and Hector C. Aguilar

Subjects

Nipah virus, paramyxovirus, proteomics, vesicular trafficking, endocytosis, cytoskeleton, Microbiology, QR1-502

Abstract

ABSTRACT Classified as a biosafety level 4 (BSL4) select agent, Nipah virus (NiV) is a deadly henipavirus in the Paramyxoviridae family, with a nearly 75% mortality rate in humans, underscoring its global and animal health importance. Elucidating the process of viral particle production in host cells is imperative both for targeted drug design and viral particle-based vaccine development. However, little is understood concerning the functions of cellular machinery in paramyxoviral and henipaviral assembly and budding. Recent studies showed evidence for the involvement of multiple NiV proteins in viral particle formation, in contrast to the mechanisms understood for several paramyxoviruses as being reliant on the matrix (M) protein alone. Further, the levels and purposes of cellular factor incorporation into viral particles are largely unexplored for the paramyxoviruses. To better understand the involvement of cellular machinery and the major structural viral fusion (F), attachment (G), and matrix (M) proteins, we performed proteomics analyses on virus-like particles (VLPs) produced from several combinations of these NiV proteins. Our findings indicate that NiV VLPs incorporate vesicular trafficking and actin cytoskeletal factors. The involvement of these biological processes was validated by experiments indicating that the perturbation of key factors in these cellular processes substantially modulated viral particle formation. These effects were most impacted for NiV-F-modulated viral particle formation either autonomously or in combination with other NiV proteins, indicating that NiV-F budding relies heavily on these cellular processes. These findings indicate a significant involvement of the NiV fusion protein, vesicular trafficking, and actin cytoskeletal processes in efficient viral particle formation. IMPORTANCE Nipah virus is a zoonotic biosafety level 4 agent with high mortality rates in humans. The genus to which Nipah virus belongs, Henipavirus, includes five officially recognized pathogens; however, over 20 species have been identified in multiple continents within the last several years. As there are still no vaccines or treatments for NiV infection, elucidating its process of viral particle production is imperative both for targeted drug design as well as for particle-based vaccine development. Developments in high-throughput technologies make proteomic analysis of isolated viral particles a highly insightful approach to understanding the life cycle of pathogens such as Nipah virus.

Published

2019

2. Phloem Exudate Protein Profiles during Drought and Recovery Reveal Abiotic Stress Responses in Tomato Vasculature

Author

Aaron J. Ogden, Jishnu J. Bhatt, Heather M. Brewer, Jack Kintigh, Samwel M. Kariuki, Sairam Rudrabhatla, Joshua N. Adkins, and Wayne R. Curtis

Subjects

phloem exudate, proteomics, drought, abiotic stress, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

Drought is the leading cause of agricultural yield loss among all abiotic stresses, and the link between water deficit and phloem protein contents is relatively unexplored. Here we collected phloem exudates from Solanum lycopersicum leaves during periods of drought stress and recovery. Our analysis identified 2558 proteins, the most abundant of which were previously localized to the phloem. Independent of drought, enrichment analysis of the total phloem exudate protein profiles from all samples suggests that the protein content of phloem sap is complex, and includes proteins that function in chaperone systems, branched-chain amino acid synthesis, trehalose metabolism, and RNA silencing. We observed 169 proteins whose abundance changed significantly within the phloem sap, either during drought or recovery. Proteins that became significantly more abundant during drought include members of lipid metabolism, chaperone-mediated protein folding, carboxylic acid metabolism, abscisic acid signaling, cytokinin biosynthesis, and amino acid metabolism. Conversely, proteins involved in lipid signaling, sphingolipid metabolism, cell wall organization, carbohydrate metabolism, and a mitogen-activated protein kinase are decreased during drought. Our experiment has achieved an in-depth profiling of phloem sap protein contents during drought stress and recovery that supports previous findings and provides new evidence that multiple biological processes are involved in drought adaptation.

Published

2020

3. Correction: Comparative Omics-Driven Genome Annotation Refinement: Application across Yersiniae.

Author

Alexandra C. Schrimpe-Rutledge, Marcus B. Jones, Sadhana Chauhan, Samuel O. Purvine, James A. Sanford, Matthew E. Monroe, Heather M. Brewer, Samuel H. Payne, Charles Ansong, Bryan C. Frank, Richard D. Smith, Scott N. Peterson, Vladimir L. Motin, and Joshua N. Adkins

Subjects

Medicine, Science

Published

2012

4. Temporospatial shifts in the human gut microbiome and metabolome after gastric bypass surgery

Author

Bruce E. Rittmann, David W. Hoyt, Thomas O. Metz, Heather M. Brewer, Dae Wook Kang, Sydney E. Dautel, Rosa Krajmalnik-Brown, Karl K. Weitz, John K. DiBaise, Zehra Esra Ilhan, Michael D. Crowell, Athena A. Schepmoes, Young-Mo Kim, and Nancy G. Isern

Subjects

0301 basic medicine, Male, Physiology, medicine.disease_cause, Applied Microbiology and Biotechnology, Microbial ecology, Feces, 0302 clinical medicine, Weight loss, RNA, Ribosomal, 16S, Longitudinal Studies, Phylogeny, 2. Zero hunger, Bile acid, Fatty Acids, High-Throughput Nucleotide Sequencing, Middle Aged, 3. Good health, Cohort, lcsh:QR100-130, 030211 gastroenterology & hepatology, Female, medicine.symptom, Biotechnology, Adult, DNA, Bacterial, medicine.drug_class, Gastric Bypass, Microbiology, DNA, Ribosomal, Article, lcsh:Microbial ecology, Bile Acids and Salts, 03 medical and health sciences, Spatio-Temporal Analysis, medicine, Metabolome, Humans, Metabolomics, Microbiome, Obesity, Clinical microbiology, Bacteria, business.industry, Gastric bypass surgery, nutritional and metabolic diseases, Sequence Analysis, DNA, medicine.disease, Gastrointestinal Microbiome, 030104 developmental biology, business

Abstract

Although the etiology of obesity is not well-understood, genetic, environmental, and microbiome elements are recognized as contributors to this rising pandemic. It is well documented that Roux-en-Y gastric bypass (RYGB) surgery drastically alters the fecal microbiome, but data are sparse on temporal and spatial microbiome and metabolome changes, especially in human populations. We characterized the structure and function (through metabolites) of the microbial communities in the gut lumen and structure of microbial communities on mucosal surfaces in nine morbidly obese individuals before, 6 months, and 12 months after RYGB surgery. Moreover, using a comprehensive multi-omic approach, we compared this longitudinal cohort to a previously studied cross-sectional cohort (n = 24). In addition to the expected weight reduction and improvement in obesity-related comorbidities after RYGB surgery, we observed that the impact of surgery was much greater on fecal communities in comparison to mucosal ones. The changes in the fecal microbiome were linked to increased concentrations of branched-chain fatty acids and an overall decrease in secondary bile acid concentrations. The microbiome and metabolome data sets for this longitudinal cohort strengthen our understanding of the persistent impact of RYGB on the gut microbiome and its metabolism. Our findings highlight the importance of changes in mucosal and fecal microbiomes after RYGB surgery. The spatial modifications in the microbiome after RYGB surgery corresponded to persistent changes in fecal fermentation and bile acid metabolism, both of which are associated with improved metabolic outcomes.

Published

2020

5. Assessment of the Utility of the Oral Fluid and Plasma Proteomes for Hydrocodone Exposure

Author

Heather M. Brewer, Joshua N. Adkins, Bobbie-Jo M. Webb-Robertson, Jon M. Jacobs, Brooke L. Deatherage Kaiser, Athena A. Schepmoes, Sandra Valtier, and Vikhyat S. Bebarta

Subjects

Adult, Male, Proteomics, Spectrometry, Mass, Electrospray Ionization, Time Factors, Proteome, Health, Toxicology and Mutagenesis, Pharmacology toxicology, Pharmacology, Toxicology, Young Adult, 03 medical and health sciences, 0302 clinical medicine, Predictive Value of Tests, Tandem Mass Spectrometry, Blood plasma, Humans, Medicine, Hydrocodone, 030212 general & internal medicine, Saliva, Chromatography, High Pressure Liquid, Proteomic Profile, business.industry, Opioid use, Solid Phase Extraction, 030208 emergency & critical care medicine, Blood Proteins, Middle Aged, Opioid-Related Disorders, Analgesics, Opioid, Substance Abuse Detection, Opioid, Oral fluid, Female, Original Article, business, medicine.drug

Abstract

INTRODUCTION: Non-medical use and abuse of prescription opioids is a growing problem in both the civilian and military communities, with minimal technologies for detecting hydrocodone use. This study explored the proteomic changes that occur in the oral fluid and blood plasma following controlled hydrocodone administration in 20 subjects. METHODS: The global proteomic profile was determined for samples taken at four time points per subject: pre-exposure and 4, 6, or 168 hours post-exposure. The oral fluid samples analyzed herein provided greater differentiation between baseline and response time points than was observed with blood plasma, at least partially due to significant person-to-person relative variability in the plasma proteome. RESULTS: A total of 399 proteins were identified from oral fluid samples, and the abundance of 118 of those proteins was determined to be significantly different upon metabolism of hydrocodone (4 and 6 hour time points) as compared to baseline levels in the oral fluid (pre-dose and 168 hours). CONCLUSIONS: We present an assessment of the oral fluid and plasma proteome following hydrocodone administration, which demonstrates the potential of oral fluid as a noninvasive sample that may reveal features of hydrocodone in opioid use, and with additional study, may be useful for other opioids and in settings of misuse. ELECTRONIC SUPPLEMENTARY MATERIAL: The online version of this article (10.1007/s13181-019-00731-0) contains supplementary material, which is available to authorized users.

Published

2019

6. Determining the Reliability of Measuring Mercury Cycling Gene Abundance with Correlations with Mercury and Methylmercury Concentrations

Author

Steven D. Brown, Ann M. Wymore, Anthony V. Palumbo, Caitlin M. Gionfriddo, Judy D. Wall, Matthew W. Fields, Heather M. Brewer, Chiachi Hwang, Andrew J. King, Cynthia C. Gilmour, Scott C. Brooks, James G. Moberly, Mircea Podar, Geoff A. Christensen, Stephen J. Callister, Dwayne A. Elias, Anil C. Somenahally, Craig C. Brandt, and Carrie L. Miller

Subjects

Mercury cycling, Reproducibility of Results, chemistry.chemical_element, Mercury, General Chemistry, Methylmercury Compounds, 010501 environmental sciences, 01 natural sciences, Mercury (element), chemistry.chemical_compound, chemistry, RNA, Ribosomal, 16S, Environmental chemistry, Bioaccumulation, Environmental Chemistry, Ecosystem, Methylmercury, Environmental Monitoring, 0105 earth and related environmental sciences

Abstract

Methylmercury (MeHg) is a bioaccumulative toxic contaminant in many ecosystems, but factors governing its production are poorly understood. Recent work has shown that the anaerobic microbial conversion of mercury (Hg) to MeHg requires the Hg-methylation genes

Published

2019

7. Changes of Protein Turnover in Aging Caenorhabditis elegans

Author

Sophie Bauer, Geert Depuydt, Ineke Dhondt, Heather M. Brewer, Richard D. Smith, Bart P. Braeckman, and Vladislav A. Petyuk

Subjects

0301 basic medicine, media_common.quotation_subject, Protein turnover, Longevity, Biology, Bioinformatics, biology.organism_classification, Proteomics, Biochemistry, Analytical Chemistry, Cell biology, 03 medical and health sciences, 030104 developmental biology, Proteostasis, Proteome, Daf-2, Molecular Biology, Vitellogenins, Caenorhabditis elegans, media_common

Abstract

Protein turnover rates severely decline in aging organisms, including C. elegans However, limited information is available on turnover dynamics at the individual protein level during aging. We followed changes in protein turnover at one-day resolution using a multiple-pulse 15N-labeling and accurate mass spectrometry approach. Forty percent of the proteome shows gradual slowdown in turnover with age, whereas only few proteins show increased turnover. Decrease in protein turnover was consistent for only a minority of functionally related protein subsets, including tubulins and vitellogenins, whereas randomly diverging turnover patterns with age were the norm. Our data suggests increased heterogeneity of protein turnover of the translation machinery, whereas protein turnover of ubiquitin-proteasome and antioxidant systems are well-preserved over time. Hence, we presume that maintenance of quality control mechanisms is a protective strategy in aging worms, although the ultimate proteome collapse is inescapable.

Published

2017

8. Deep-Dive Targeted Quantification for Ultrasensitive Analysis of Proteins in Nondepleted Human Blood Plasma/Serum and Tissues

Author

Athena A. Schepmoes, Yuqian Gao, Tao Liu, Wei-Jun Qian, Richard D. Smith, Thomas L. Fillmore, Heather M. Brewer, Ehwang Song, Tujin Shi, Song Nie, Karin D. Rodland, and Hui Wang

Subjects

Proteomics, musculoskeletal diseases, 0301 basic medicine, Quantitative proteomics, Target peptide, Mass spectrometry, Sensitivity and Specificity, 01 natural sciences, Article, Antibodies, Mass Spectrometry, Analytical Chemistry, Plasma, 03 medical and health sciences, Blood plasma, Humans, Immunoassay, Chromatography, Reverse-Phase, Chromatography, biology, Human blood, Chemistry, 010401 analytical chemistry, Selected reaction monitoring, Blood Proteins, Prostate-Specific Antigen, Orders of magnitude (mass), 0104 chemical sciences, 030104 developmental biology, biology.protein, Antibody, human activities

Abstract

Mass spectrometry-based targeted proteomics (e.g., selected reaction monitoring, SRM) is emerging as an attractive alternative to immunoassays for protein quantification. Recently we have made significant progress in SRM sensitivity for enabling quantification of low nanograms per milliliter to sub-naograms per milliliter level proteins in nondepleted human blood plasma/serum without affinity enrichment. However, precise quantification of extremely low abundance proteins (e.g., ≤ 100 pg/mL in blood plasma/serum) using targeted proteomics approaches still remains challenging, especially for these samples without available antibodies for enrichment. To address this need, we have developed an antibody-independent deep-dive SRM (DD-SRM) approach that capitalizes on multidimensional high-resolution reversed-phase liquid chromatography (LC) separation for target peptide separation and enrichment combined with precise selection of target peptide fractions of interest, significantly improving SRM sensitivity by ~5 orders of magnitude when compared to conventional LC-SRM. Application of DD-SRM to human serum and tissue provides precise quantification of endogenous proteins at the ~10 pg/mL level in nondepleted serum and at

Published

2017

9. Quantitative cardiac phosphoproteomics profiling during ischemia-reperfusion in an immature swine model

Author

Ljiljana Paša-Tolić, Heather M. Brewer, Dolena R Ledee, Masaki Kajimoto, MinA Kang, Michael A. Portman, and Samuel O. Purvine

Subjects

Male, 0301 basic medicine, Proteome, Swine, Physiology, Myocardium, Ischemia, Phosphoproteomics, Gene Expression Regulation, Developmental, Biology, Phosphoproteins, medicine.disease, 03 medical and health sciences, 030104 developmental biology, Biochemistry, Reperfusion Injury, Physiology (medical), medicine, Animals, Cardiology and Cardiovascular Medicine, Research Article

Abstract

Ischemia-reperfusion (I/R) results in altered metabolic and molecular responses, and phosphorylation is one of the most noted regulatory mechanisms mediating signaling mechanisms during physiological stresses. To expand our knowledge of the potential phosphoproteomic changes in the myocardium during I/R, we used Isobaric Tags for Relative and Absolute Quantitation-based analyses in left ventricular samples obtained from porcine hearts under control or I/R conditions. The data are available via ProteomeXchange with identifier PXD006066. We identified 1,896 phosphopeptides within left ventricular control and I/R porcine samples. Significant differential phosphorylation between control and I/R groups was discovered in 111 phosphopeptides from 86 proteins. Analysis of the phosphopeptides using Motif-x identified five motifs: (..R..S..), (..SP..), (..S.S..), (..S…S..), and (..S.T..). Semiquantitative immunoblots confirmed site location and directional changes in phosphorylation for phospholamban and pyruvate dehydrogenase E1, two proteins known to be altered by I/R and identified by this study. Novel phosphorylation sites associated with I/R were also identified. Functional characterization of the phosphopeptides identified by our methodology could expand our understanding of the signaling mechanisms involved during I/R damage in the heart as well as identify new areas to target therapeutic strategies.NEW & NOTEWORTHY We used Isobaric Tags for Relative and Absolute Quantitation technology to investigate the phosphoproteomic changes that occur in cardiac tissue under ischemia-reperfusion conditions. The results of this study provide an extensive catalog of phosphoproteins, both predicted and novel, associated with ischemia-reperfusion, thereby identifying new pathways for investigation.

Published

2017

10. Phage-specific metabolic reprogramming of virocells

Author

Tijana Glavina del Rio, G Eric Bastien, Ho Bin Jang, Heather M. Brewer, Melissa B. Duhaime, Natalie Solonenko, Joshua N. Adkins, Ahmed A. Zayed, Bill Andreopoulos, Subhadeep Paul, Morgan M Lindback, Matthew B. Sullivan, and Cristina Howard-Varona

Subjects

Genetics, 0303 health sciences, biology, Ecology, 030306 microbiology, biology.organism_classification, Microbiology, Genome, Article, Microbial ecology, 03 medical and health sciences, Pseudoalteromonas, Transcription (biology), Viruses, Environmental Microbiology, Heterochromatin protein 1, Ecosystem, Bacteriophages, Bacterial virus, Ecology, Evolution, Behavior and Systematics, Bacteria, 030304 developmental biology

Abstract

Ocean viruses are abundant and infect 20–40% of surface microbes. Infected cells, termed virocells, are thus a predominant microbial state. Yet, virocells and their ecosystem impacts are understudied, thus precluding their incorporation into ecosystem models. Here we investigated how unrelated bacterial viruses (phages) reprogram one host into contrasting virocells with different potential ecosystem footprints. We independently infected the marine Pseudoalteromonas bacterium with siphovirus PSA-HS2 and podovirus PSA-HP1. Time-resolved multi-omics unveiled drastically different metabolic reprogramming and resource requirements by each virocell, which were related to phage–host genomic complementarity and viral fitness. Namely, HS2 was more complementary to the host in nucleotides and amino acids, and fitter during infection than HP1. Functionally, HS2 virocells hardly differed from uninfected cells, with minimal host metabolism impacts. HS2 virocells repressed energy-consuming metabolisms, including motility and translation. Contrastingly, HP1 virocells substantially differed from uninfected cells. They repressed host transcription, responded to infection continuously, and drastically reprogrammed resource acquisition, central carbon and energy metabolisms. Ecologically, this work suggests that one cell, infected versus uninfected, can have immensely different metabolisms that affect the ecosystem differently. Finally, we relate phage–host genome complementarity, virocell metabolic reprogramming, and viral fitness in a conceptual model to guide incorporating viruses into ecosystem models.

Published

2019

11. Nipah Virus-Like Particle Egress Is Modulated by Cytoskeletal and Vesicular Trafficking Pathways: a Validated Particle Proteomics Analysis

Author

Heather M. Brewer, Paul D. Piehowski, Bom Nae Rin Lee, Victoria Ortega, Jason P. Wendler, Joshua N. Adkins, Hector C. Aguilar, Nicholas Usher, Jeremy Teuton, J Lizbeth Reyes Zamora, Gunner P. Johnston, Erik M Contreras, Birgit Bradel-Tretheway, and Keesha M. Matz

Subjects

0301 basic medicine, Paramyxoviridae, Physiology, Host–pathogen interaction, viruses, lcsh:QR1-502, Nipah virus, host-pathogen interaction, Endocytosis, Proteomics, Biochemistry, Microbiology, lcsh:Microbiology, Host-Microbe Biology, 03 medical and health sciences, paramyxovirus, proteomics, Genetics, endocytosis, Cytoskeleton, Molecular Biology, Ecology, Evolution, Behavior and Systematics, Actin, 030102 biochemistry & molecular biology, biology, cytoskeleton, biology.organism_classification, Virology, Fusion protein, QR1-502, 3. Good health, Computer Science Applications, 030104 developmental biology, Modeling and Simulation, vesicular trafficking, Henipavirus, Research Article

Abstract

Nipah virus is a zoonotic biosafety level 4 agent with high mortality rates in humans. The genus to which Nipah virus belongs, Henipavirus, includes five officially recognized pathogens; however, over 20 species have been identified in multiple continents within the last several years. As there are still no vaccines or treatments for NiV infection, elucidating its process of viral particle production is imperative both for targeted drug design as well as for particle-based vaccine development. Developments in high-throughput technologies make proteomic analysis of isolated viral particles a highly insightful approach to understanding the life cycle of pathogens such as Nipah virus., Classified as a biosafety level 4 (BSL4) select agent, Nipah virus (NiV) is a deadly henipavirus in the Paramyxoviridae family, with a nearly 75% mortality rate in humans, underscoring its global and animal health importance. Elucidating the process of viral particle production in host cells is imperative both for targeted drug design and viral particle-based vaccine development. However, little is understood concerning the functions of cellular machinery in paramyxoviral and henipaviral assembly and budding. Recent studies showed evidence for the involvement of multiple NiV proteins in viral particle formation, in contrast to the mechanisms understood for several paramyxoviruses as being reliant on the matrix (M) protein alone. Further, the levels and purposes of cellular factor incorporation into viral particles are largely unexplored for the paramyxoviruses. To better understand the involvement of cellular machinery and the major structural viral fusion (F), attachment (G), and matrix (M) proteins, we performed proteomics analyses on virus-like particles (VLPs) produced from several combinations of these NiV proteins. Our findings indicate that NiV VLPs incorporate vesicular trafficking and actin cytoskeletal factors. The involvement of these biological processes was validated by experiments indicating that the perturbation of key factors in these cellular processes substantially modulated viral particle formation. These effects were most impacted for NiV-F-modulated viral particle formation either autonomously or in combination with other NiV proteins, indicating that NiV-F budding relies heavily on these cellular processes. These findings indicate a significant involvement of the NiV fusion protein, vesicular trafficking, and actin cytoskeletal processes in efficient viral particle formation. IMPORTANCE Nipah virus is a zoonotic biosafety level 4 agent with high mortality rates in humans. The genus to which Nipah virus belongs, Henipavirus, includes five officially recognized pathogens; however, over 20 species have been identified in multiple continents within the last several years. As there are still no vaccines or treatments for NiV infection, elucidating its process of viral particle production is imperative both for targeted drug design as well as for particle-based vaccine development. Developments in high-throughput technologies make proteomic analysis of isolated viral particles a highly insightful approach to understanding the life cycle of pathogens such as Nipah virus.

Published

2019

12. 'Candidatus Paraporphyromonas polyenzymogenes' encodes multi-modular cellulases linked to the type IX secretion system

Author

Alice C. McHardy, Heather M. Brewer, Live Heldal Hagen, Angela D. Norbeck, Ljiljana Paša-Tolić, Nicole M. Koropatkin, Adrian E. Naas, Kelly C. Wrighton, V.G.H. Eijsink, Magnus Ø. Arntzen, Matthias Hess, I. M. Heggenes, Roderick I. Mackie, Phillip B. Pope, Lindsey M. Solden, and BRICS, Braunschweiger Zentrum für Systembiologie, Rebenring 56, 38106 Braunschweig, Germany.

Subjects

0301 basic medicine, Microbiology (medical), Carbohydrate, Rumen, Microorganism, Cellulase, Lignin, Microbiology, lcsh:Microbial ecology, 03 medical and health sciences, Microbial ecology, Affordable and Clean Energy, Orpinomyces, Animals, Cellulases, Bacterial Secretion Systems, Sheep, biology, Ecology, Bacteroidetes, Research, Type IX secretion system, Plants, biology.organism_classification, Gastrointestinal Microbiome, active enzymes, 030104 developmental biology, Biochemistry, Medical Microbiology, Candidatus, biology.protein, Carbohydrate-active enzymes, lcsh:QR100-130, Carbohydrate Metabolism, Cattle, Bacteria

Abstract

Background In nature, obligate herbivorous ruminants have a close symbiotic relationship with their gastrointestinal microbiome, which proficiently deconstructs plant biomass. Despite decades of research, lignocellulose degradation in the rumen has thus far been attributed to a limited number of culturable microorganisms. Here, we combine meta-omics and enzymology to identify and describe a novel Bacteroidetes family (“Candidatus MH11”) composed entirely of uncultivated strains that are predominant in ruminants and only distantly related to previously characterized taxa. Results The first metabolic reconstruction of Ca. MH11-affiliated genome bins, with a particular focus on the provisionally named “Candidatus Paraporphyromonas polyenzymogenes”, illustrated their capacity to degrade various lignocellulosic substrates via comprehensive inventories of singular and multi-modular carbohydrate active enzymes (CAZymes). Closer examination revealed an absence of archetypical polysaccharide utilization loci found in human gut microbiota. Instead, we identified many multi-modular CAZymes putatively secreted via the Bacteroidetes-specific type IX secretion system (T9SS). This included cellulases with two or more catalytic domains, which are modular arrangements that are unique to Bacteroidetes species studied to date. Core metabolic proteins from Ca. P. polyenzymogenes were detected in metaproteomic data and were enriched in rumen-incubated plant biomass, indicating that active saccharification and fermentation of complex carbohydrates could be assigned to members of this novel family. Biochemical analysis of selected Ca. P. polyenzymogenes CAZymes further iterated the cellulolytic activity of this hitherto uncultured bacterium towards linear polymers, such as amorphous and crystalline cellulose as well as mixed linkage β-glucans. Conclusion We propose that Ca. P. polyenzymogene genotypes and other Ca. MH11 members actively degrade plant biomass in the rumen of cows, sheep and most likely other ruminants, utilizing singular and multi-domain catalytic CAZymes secreted through the T9SS. The discovery of a prominent role of multi-modular cellulases in the Gram-negative Bacteroidetes, together with similar findings for Gram-positive cellulosomal bacteria (Ruminococcus flavefaciens) and anaerobic fungi (Orpinomyces sp.), suggests that complex enzymes are essential and have evolved within all major cellulolytic dominions inherent to the rumen. Electronic supplementary material The online version of this article (10.1186/s40168-018-0421-8) contains supplementary material, which is available to authorized users.

Published

2018

13. Diurnal cycling of rhizosphere bacterial communities is associated with shifts in carbon metabolism

Author

Thalita Regina Tuleski, Richard A. Ferrieri, Beverly J. Agtuca, Yaya Cui, Christopher Staley, Malak M. Tfaily, Charles Ansong, Susannah G. Tringe, Fernanda Plucani do Amaral, Michael J. Sadowsky, Angela D. Norbeck, Jared B. Shaw, Ping Wang, Meng Markillie, Tomás Pellizzaro, Abigail P. Ferrieri, Rosalie K. Chu, Gary Stacey, Ljiljana Paša-Tolić, and Heather M. Brewer

Subjects

0106 biological sciences, 0301 basic medicine, Microbiology (medical), 16S, Circadian clock, Arabidopsis, Plant Development, Bacterial Physiological Phenomena, 01 natural sciences, Microbiology, lcsh:Microbial ecology, 03 medical and health sciences, Microbial ecology, RNA, Ribosomal, 16S, Botany, Genetics, Arabidopsis thaliana, Soil Microbiology, Ribosomal, Rhizosphere, Ecology, biology, Bacteria, Arabidopsis Proteins, Research, Microbiota, food and beverages, High-Throughput Nucleotide Sequencing, Biodiversity, biology.organism_classification, Carbon, Circadian Rhythm, 030104 developmental biology, Microbial population biology, Medical Microbiology, Diurnal rhythm, lcsh:QR100-130, RNA, Bacterial community structure, Brachypodium, Brachypodium distachyon, Sleep Research, Soil microbiology, 010606 plant biology & botany, Transcription Factors

Abstract

Background The circadian clock regulates plant metabolic functions and is an important component in plant health and productivity. Rhizosphere bacteria play critical roles in plant growth, health, and development and are shaped primarily by soil communities. Using Illumina next-generation sequencing and high-resolution mass spectrometry, we characterized bacterial communities of wild-type (Col-0) Arabidopsis thaliana and an acyclic line (OX34) ectopically expressing the circadian clock-associated cca1 transcription factor, relative to a soil control, to determine how cycling dynamics affected the microbial community. Microbial communities associated with Brachypodium distachyon (BD21) were also evaluated. Results Significantly different bacterial community structures (P = 0.031) were observed in the rhizosphere of wild-type plants between light and dark cycle samples. Furthermore, 13% of the community showed cycling, with abundances of several families, including Burkholderiaceae, Rhodospirillaceae, Planctomycetaceae, and Gaiellaceae, exhibiting fluctuation in abundances relative to the light cycle. However, limited-to-no cycling was observed in the acyclic CCAox34 line or in soil controls. Significant cycling was also observed, to a lesser extent, in Brachypodium. Functional gene inference revealed that genes involved in carbohydrate metabolism were likely more abundant in near-dawn, dark samples. Additionally, the composition of organic matter in the rhizosphere showed a significant variation between dark and light cycles. Conclusions The results of this study suggest that the rhizosphere bacterial community is regulated, to some extent, by the circadian clock and is likely influenced by, and exerts influences, on plant metabolism and productivity. The timing of bacterial cycling in relation to that of Arabidopsis further suggests that diurnal dynamics influence plant-microbe carbon metabolism and exchange. Equally important, our results suggest that previous studies done without relevance to time of day may need to be reevaluated with regard to the impact of diurnal cycles on the rhizosphere microbial community. Electronic supplementary material The online version of this article (doi:10.1186/s40168-017-0287-1) contains supplementary material, which is available to authorized users.

Published

2017

14. Multiple mechanisms drive phage infection efficiency in nearly identical hosts

Author

Cristina Howard-Varona, Charles Ansong, Heather M. Brewer, Richard A. White, Lye Meng Markillie, Katherine R. Hargreaves, Matthew B. Sullivan, Joshua N. Adkins, Natalie Solonenko, and Galya Orr

Subjects

0301 basic medicine, Proteomics, Proteome, Transcription, Genetic, Mutant, Genomics, Biology, Microbiology, Article, Transcriptome, 03 medical and health sciences, Transcription (biology), Protein biosynthesis, Metabolomics, Bacteriophages, Gene, Ecology, Evolution, Behavior and Systematics, Genetics, Bacteroidetes, Sequence Analysis, RNA, 030104 developmental biology, Protein Biosynthesis, Mutation, Flavobacteriaceae

Abstract

Phage-host interactions are critical to ecology, evolution, and biotechnology. Central to those is infection efficiency, which remains poorly understood, particularly in nature. Here we apply genome-wide transcriptomics and proteomics to investigate infection efficiency in nature's own experiment: two nearly identical (genetically and physiologically) Bacteroidetes bacterial strains (host18 and host38) that are genetically intractable, but environmentally important, where phage infection efficiency varies. On host18, specialist phage phi18:3 infects efficiently, whereas generalist phi38:1 infects inefficiently. On host38, only phi38:1 infects, and efficiently. Overall, phi18:3 globally repressed host18's transcriptome and proteome, expressed genes that likely evaded host restriction/modification (R/M) defenses and controlled its metabolism, and synchronized phage transcription with translation. In contrast, phi38:1 failed to repress host18's transcriptome and proteome, did not evade host R/M defenses or express genes for metabolism control, did not synchronize transcripts with proteins and its protein abundances were likely targeted by host proteases. However, on host38, phi38:1 globally repressed host transcriptome and proteome, synchronized phage transcription with translation, and infected host38 efficiently. Together these findings reveal multiple infection inefficiencies. While this contrasts the single mechanisms often revealed in laboratory mutant studies, it likely better reflects the phage-host interaction dynamics that occur in nature.

Published

2017

15. Changes of Protein Turnover in Aging

Author

Ineke, Dhondt, Vladislav A, Petyuk, Sophie, Bauer, Heather M, Brewer, Richard D, Smith, Geert, Depuydt, and Bart P, Braeckman

Subjects

Aging, Time Factors, Muscles, Research, Proteostasis, Animals, Pharynx, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Energy Metabolism, Half-Life

Abstract

Protein turnover rates severely decline in aging organisms, including C. elegans. However, limited information is available on turnover dynamics at the individual protein level during aging. We followed changes in protein turnover at one-day resolution using a multiple-pulse 15N-labeling and accurate mass spectrometry approach. Forty percent of the proteome shows gradual slowdown in turnover with age, whereas only few proteins show increased turnover. Decrease in protein turnover was consistent for only a minority of functionally related protein subsets, including tubulins and vitellogenins, whereas randomly diverging turnover patterns with age were the norm. Our data suggests increased heterogeneity of protein turnover of the translation machinery, whereas protein turnover of ubiquitin-proteasome and antioxidant systems are well-preserved over time. Hence, we presume that maintenance of quality control mechanisms is a protective strategy in aging worms, although the ultimate proteome collapse is inescapable.

Published

2017

16. Feathermoss and epiphytic Nostoc cooperate differently: expanding the spectrum of plant-cyanobacteria symbiosis

Author

Denis, Warshan, Josh L, Espinoza, Rhona K, Stuart, R Alexander, Richter, Sea-Yong, Kim, Nicole, Shapiro, Tanja, Woyke, Nikos, C Kyrpides, Kerrie, Barry, Vasanth, Singan, Erika, Lindquist, Charles, Ansong, Samuel O, Purvine, Heather, M Brewer, Philip D, Weyman, Christopher L, Dupont, and Ulla, Rasmussen

Subjects

Nitrogen, Chemotaxis, Nitrogen Fixation, Taiga, Original Article, Plants, Cyanobacteria, Nostoc, Symbiosis

Abstract

Dinitrogen (N2)-fixation by cyanobacteria in symbiosis with feathermosses is the primary pathway of biological nitrogen (N) input into boreal forests. Despite its significance, little is known about the cyanobacterial gene repertoire and regulatory rewiring needed for the establishment and maintenance of the symbiosis. To determine gene acquisitions and regulatory changes allowing cyanobacteria to form and maintain this symbiosis, we compared genomically closely related symbiotic-competent and -incompetent Nostoc strains using a proteogenomics approach and an experimental set up allowing for controlled chemical and physical contact between partners. Thirty-two gene families were found only in the genomes of symbiotic strains, including some never before associated with cyanobacterial symbiosis. We identified conserved orthologs that were differentially expressed in symbiotic strains, including protein families involved in chemotaxis and motility, NO regulation, sulfate/phosphate transport, and glycosyl-modifying and oxidative stress-mediating exoenzymes. The physical moss–cyanobacteria epiphytic symbiosis is distinct from other cyanobacteria–plant symbioses, with Nostoc retaining motility, and lacking modulation of N2-fixation, photosynthesis, GS-GOGAT cycle and heterocyst formation. The results expand our knowledge base of plant–cyanobacterial symbioses, provide a model of information and material exchange in this ecologically significant symbiosis, and suggest new currencies, namely nitric oxide and aliphatic sulfonates, may be involved in establishing and maintaining the cyanobacteria–feathermoss symbiosis.

Published

2017

17. A parts list for fungal cellulosomes revealed by comparative genomics

Author

Alan Kuo, Theo A. van Alen, Charles H. Haitjema, John K. Henske, Johannes H. P. Hackstein, Jennifer Chiniquy, Igor V. Grigoriev, Samuel O. Purvine, Randall de Groot, Kevin V. Solomon, Zhiying Zhao, Stephen J. Mondo, Kurt LaButti, Aaron T. Wright, Heather M. Brewer, Sean P. Gilmore, Kerrie Barry, Brigitte Boxma, Matthieu Hainaut, Bernard Henrissat, Scott E. Baker, Michelle A. O’Malley, Asaf Salamov, Department of Chemical Engineering, Department of chemical engineering, US Department of Energy, Joint Genome Institute (JGI), Environmental Molecular Sciences Laboratory, Earth and Biological Sciences Directorate, Pacific Northwest National Laboratory (PNNL), Biological Sciences Division, Earth and Biological Sciences Directorate, Architecture et fonction des macromolécules biologiques (AFMB), Institut National de la Recherche Agronomique (INRA)-Aix Marseille Université (AMU)-Centre National de la Recherche Scientifique (CNRS), Aix Marseille Université (AMU), Institut National de la Recherche Agronomique (INRA), Department of Evolutionary Microbiology, Radboud University Nijmegen, Department of Biological Sciences, The Open University [Milton Keynes] (OU), Department of Plant and Microbial Biology, US Department of Energy (DE-SC0010352), the US Department of Agriculture (award no. 2011-67017-20459), the National Science Foundation (DGE 1144085), W911NF-09-0001 (FICUS), DE-AC02-05CH11231 (JGI)DE-AC05-76RL01830 (EMSL).IDEX Aix-Marseille (Grant Microbio-E) (grant no. ANR-14-CE06-0020), and Centre National de la Recherche Scientifique (CNRS)-Aix Marseille Université (AMU)-Institut National de la Recherche Agronomique (INRA)

Subjects

0301 basic medicine, Proteomics, [SDV]Life Sciences [q-bio], Neocallimastigales, microbiome, Dockerin, approche protéomique, Applied Microbiology and Biotechnology, Cellulosome assembly, Cellulosome, Fungal genetics, neocallimastix, 2.2 Factors relating to the physical environment, Aetiology, biology, Genomics, Cellulosomes, Infectious Diseases, Medical Microbiology, fungal genome, anaeromyces, Piromyces, Anaerobic bacteria, génome fongique, Infection, Biotechnology, Protein Binding, Microbiology (medical), 030106 microbiology, Immunology, Multienzyme complexes, Computational biology, Microbiology, Fungal Proteins, 03 medical and health sciences, Genetics, analyse génomique, biomasse végétale, Comparative genomics, Cell Biology, biology.organism_classification, piromyces, 030104 developmental biology, Neocallimastigomycota, cellulosome, Ecological Microbiology, génie génétique, Protein Multimerization

Abstract

© 2017 Macmillan Publishers Limited, part of Springer Nature. All rights reserved. Cellulosomes are large, multiprotein complexes that tether plant biomass-degrading enzymes together for improved hydrolysis1. These complexes were first described in anaerobic bacteria, where species-specific dockerin domains mediate the assembly of enzymes onto cohesin motifs interspersed within protein scaffolds 1. The versatile protein assembly mechanism conferred by the bacterial cohesin-dockerin interaction is now a standard design principle for synthetic biology2,3. For decades, analogous structures have been reported in anaerobic fungi, which are known to assemble by sequence-divergent non-catalytic dockerin domains (NCDDs)4. However, the components, modular assembly mechanism and functional role of fungal cellulosomes remain unknown5,6. Here, we describe a comprehensive set of proteins critical to fungal cellulosome assembly, including conserved scaffolding proteins unique to the Neocallimastigomycota. High-quality genomes of the anaerobic fungi Anaeromyces robustus, Neocallimastix californiae and Piromyces finnis were assembled with long-read, single-molecule technology. Genomic analysis coupled with proteomic validation revealed an average of 312 NCDD-containing proteins per fungal strain, which were overwhelmingly carbohydrate active enzymes (CAZymes), with 95 large fungal scaffoldins identified across four genera that bind to NCDDs. Fungal dockerin and scaffoldin domains have no similarity to their bacterial counterparts, yet several catalytic domains originated via horizontal gene transfer with gut bacteria. However, the biocatalytic activity of anaerobic fungal cellulosomes is expanded by the inclusion of GH3, GH6 and GH45 enzymes. These findings suggest that the fungal cellulosome is an evolutionarily chimaeric structure - an independently evolved fungal complex that co-opted useful activities from bacterial neighbours within the gut microbiome.

Published

2017

18. Automated Genome Mining of Ribosomal Peptide Natural Products

Author

Nuno Bandeira, Pavel A. Pevzner, Roland D. Kersten, Mingxun Wang, Wei-Ting Liu, Bradley S. Moore, Si Wu, Samuel O. Purvine, Hosein Mohimani, Ljiljana Paša-Tolić, Heather M. Brewer, and Pieter C. Dorrestein

Subjects

Proteomics, Molecular Sequence Data, Genomics, Computational biology, Biology, Mass spectrometry, Tandem mass spectrometry, 01 natural sciences, Biochemistry, Genome, 03 medical and health sciences, Metabolomics, Tandem Mass Spectrometry, Databases, Genetic, Drug Discovery, Database search engine, Amino Acid Sequence, 030304 developmental biology, Genetics, 0303 health sciences, Biological Products, 010405 organic chemistry, Drug discovery, General Medicine, Articles, Streptomyces, 0104 chemical sciences, Multigene Family, Molecular Medicine, Peptides, Protein Processing, Post-Translational, Ribosomes, Genome, Bacterial

Abstract

Ribosomally synthesized and posttranslationally modified peptides (RiPPs), especially from microbial sources, are a large group of bioactive natural products that are a promising source of new (bio)chemistry and bioactivity.1 In light of exponentially increasing microbial genome databases and improved mass spectrometry (MS)-based metabolomic platforms, there is a need for computational tools that connect natural product genotypes predicted from microbial genome sequences with their corresponding chemotypes from metabolomic data sets. Here, we introduce RiPPquest, a tandem mass spectrometry database search tool for identification of microbial RiPPs, and apply it to lanthipeptide discovery. RiPPquest uses genomics to limit search space to the vicinity of RiPP biosynthetic genes and proteomics to analyze extensive peptide modifications and compute p-values of peptide-spectrum matches (PSMs). We highlight RiPPquest by connecting multiple RiPPs from extracts of Streptomyces to their gene clusters and by the discovery of a new class III lanthipeptide, informatipeptin, from Streptomyces viridochromogenes DSM 40736 to reflect that it is a natural product that was discovered by mass spectrometry based genome mining using algorithmic tools rather than manual inspection of mass spectrometry data and genetic information. The presented tool is available at cyclo.ucsd.edu.

Published

2014

19. Top-down proteomics reveals a unique protein S-thiolation switch in Salmonella Typhimurium in response to infection-like conditions

Author

Heather M. Brewer, Pavel A. Pevzner, Ernesto S. Nakayasu, Ljiljana Paša-Tolić, John R. Cort, Brooke L. Deatherage Kaiser, Fred Heffron, Charles Ansong, Joshua N. Adkins, Richard D. Smith, Xiaowen Liu, Da Meng, and Si Wu

Subjects

Proteomics, Salmonella typhimurium, Cell signaling, Salmonella, Computational biology, Top-down proteomics, medicine.disease_cause, Mass Spectrometry, Protein Structure, Secondary, Protein structure, Bacterial Proteins, medicine, Humans, Cysteine, Pathogen, Multidisciplinary, biology, Biological Sciences, biology.organism_classification, Protein Structure, Tertiary, Biochemistry, Salmonella Infections, Proteome, Dimerization, Protein Processing, Post-Translational, Sulfur, Bacteria, Chromatography, Liquid

Abstract

Characterization of the mature protein complement in cells is crucial for a better understanding of cellular processes on a systems-wide scale. Toward this end, we used single-dimension ultra–high-pressure liquid chromatography mass spectrometry to investigate the comprehensive “intact” proteome of the Gram-negative bacterial pathogen Salmonella Typhimurium. Top-down proteomics analysis revealed 563 unique proteins including 1,665 proteoforms generated by posttranslational modifications (PTMs), representing the largest microbial top-down dataset reported to date. We confirmed many previously recognized aspects of Salmonella biology and bacterial PTMs, and our analysis also revealed several additional biological insights. Of particular interest was differential utilization of the protein S-thiolation forms S-glutathionylation and S-cysteinylation in response to infection-like conditions versus basal conditions. This finding of a S-glutathionylation-to-S-cysteinylation switch in a condition-specific manner was corroborated by bottom-up proteomics data and further by changes in corresponding biosynthetic pathways under infection-like conditions and during actual infection of host cells. This differential utilization highlights underlying metabolic mechanisms that modulate changes in cellular signaling, and represents a report of S-cysteinylation in Gram-negative bacteria. Additionally, the functional relevance of these PTMs was supported by protein structure and gene deletion analyses. The demonstrated utility of our simple proteome-wide intact protein level measurement strategy for gaining biological insight should promote broader adoption and applications of top-down proteomics approaches.

Published

2013

20. Haloferax volcaniiarchaeosortase is required for motility, mating, and C-terminal processing of the S-layer glycoprotein

Author

Friedhelm Pfeiffer, Si Wu, Heather M. Brewer, Samuel H. Payne, Ljiljana Paša-Tolić, Mechthild Pohlschroder, Mohd Farid Abdul Halim, Nikola Tolić, James Zou, Andrew Frisch, and Daniel H. Haft

Subjects

chemistry.chemical_classification, biology, Haloferax volcanii, Exosortase, biology.organism_classification, Microbiology, Cell membrane, Transmembrane domain, medicine.anatomical_structure, Biochemistry, chemistry, Sortase, medicine, Lipid modification, Glycoprotein, Molecular Biology, S-layer

Abstract

Cell surfaces are decorated by a variety of proteins that facilitate interactions with their environments and support cell stability. These secreted proteins are anchored to the cell by mechanisms that are diverse, and, in archaea, poorly understood. Recently published in silico data suggest that in some species a subset of secreted euryarchaeal proteins, which includes the S-layer glycoprotein, is processed and covalently linked to the cell membrane by enzymes referred to as archaeosortases. In silico work led to the proposal that an independent, sortase-like system for proteolysis-coupled, carboxy-terminal lipid modification exists in bacteria (exosortase) and archaea (archaeosortase). Here, we provide the first in vivo characterization of an archaeosortase in the haloarchaeal model organism Haloferax volcanii. Deletion of the artA gene (HVO_0915) resulted in multiple biological phenotypes: (a) poor growth, especially under low-salt conditions, (b) alterations in cell shape and the S-layer, (c) impaired motility, suppressors of which still exhibit poor growth, and (d) impaired conjugation. We studied one of the ArtA substrates, the S-layer glycoprotein, using detailed proteomic analysis. While the carboxy-terminal region of S-layer glycoproteins, consisting of a putative threonine-rich O-glycosylated region followed by a hydrophobic transmembrane helix, has been notoriously resistant to any proteomic peptide identification, we were able to identify two overlapping peptides from the transmembrane domain present in the ΔartA strain but not in the wild-type strain. This clearly shows that ArtA is involved in carboxy-terminal post-translational processing of the S-layer glycoprotein. As it is known from previous studies that a lipid is covalently attached to the carboxy-terminal region of the S-layer glycoprotein, our data strongly support the conclusion that archaeosortase functions analogously to sortase, mediating proteolysis-coupled, covalent cell surface attachment.

Published

2013

21. A multi-omic systems approach to elucidating Yersinia virulence mechanisms

Author

Richard D. Smith, Marcus B. Jones, Brooke L. Deatherage Kaiser, Alexandra C. Schrimpe-Rutledge, Hugh D. Mitchell, Heather M. Brewer, Bryan C. Frank, Thomas O. Metz, Kathleen McAteer, Young-Mo Kim, Scott N. Peterson, Jennifer L. DuBois, Sadhana Chauhan, Joshua N. Adkins, Charles Ansong, Jason E. McDermott, and Vladimir L. Motin

Subjects

Proteomics, Glutamic Acid, Virulence, Yersinia, Models, Biological, Article, Body Temperature, Transcriptome, Animals, Cluster Analysis, Yersinia pseudotuberculosis, Molecular Biology, Pathogen, Mammals, Genetics, biology, Gene Expression Profiling, biology.organism_classification, Gene expression profiling, Yersinia pestis, Host-Pathogen Interactions, Proteome, Siphonaptera, Biotechnology

Abstract

The underlying mechanisms that lead to dramatic differences between closely related pathogens are not always readily apparent. For example, the genomes of Yersinia pestis (YP) the causative agent of plague with a high mortality rate and Yersinia pseudotuberculosis (YPT) an enteric pathogen with a modest mortality rate are highly similar with some species specific differences; however the molecular causes of their distinct clinical outcomes remain poorly understood. In this study, a temporal multi-omic analysis of YP and YPT at physiologically relevant temperatures was performed to gain insights into how an acute and highly lethal bacterial pathogen, YP, differs from its less virulent progenitor, YPT. This analysis revealed higher gene and protein expression levels of conserved major virulence factors in YP relative to YPT, including the Yop virulon and the pH6 antigen. This suggests that adaptation in the regulatory architecture, in addition to the presence of unique genetic material, may contribute to the increased pathogenenicity of YP relative to YPT. Additionally, global transcriptome and proteome responses of YP and YPT revealed conserved post-transcriptional control of metabolism and the translational machinery including the modulation of glutamate levels in Yersiniae. Finally, the omics data was coupled with a computational network analysis, allowing an efficient prediction of novel Yersinia virulence factors based on gene and protein expression patterns.

Published

2013

22. Characterization of Macaque Pulmonary Fluid Proteome during Monkeypox Infection

Author

Richard D. Smith, Nathan P. Manes, Ryan D. Estep, Theresa R. Clauss, Joshua N. Adkins, Megan A. O'Connor, Heather M. Brewer, Daniel Lopez-Ferrer, Joseph N. Brown, Scott W. Wong, and Helen Li

Subjects

biology, medicine.diagnostic_test, Viral pathogenesis, Respiratory infection, biology.organism_classification, medicine.disease, Biochemistry, Virology, Virus, Analytical Chemistry, chemistry.chemical_compound, Monkeypox, Bronchoalveolar lavage, chemistry, Extracellular fluid, Immunology, medicine, Monkeypox virus, Vaccinia, Molecular Biology

Abstract

Understanding viral pathogenesis is challenging because of confounding factors, including nonabrasive access to infected tissues and high abundance of inflammatory mediators that may mask mechanistic details. In diseases such as influenza and smallpox where the primary cause of mortality results from complications in the lung, the characterization of lung fluid offers a unique opportunity to study host-pathogen interactions with minimal effect on infected animals. This investigation characterizes the global proteome response in the pulmonary fluid, bronchoalveolar lavage fluid, of macaques during upper respiratory infection by monkeypox virus (MPXV), a close relative of the causative agent of smallpox, variola virus. These results are compared and contrasted against infections by vaccinia virus (VV), a low pathogenic relative of MPXV, and with extracellular fluid from MPXV-infected HeLa cells. To identify changes in the pulmonary protein compartment, macaque lung fluid was sampled twice prior to infection, serving as base line, and up to six times following intrabronchial infection with either MPXV or VV. Increased expression of inflammatory proteins was observed in response to both viruses. Although the increased expression resolved for a subset of proteins, such as C-reactive protein, S100A8, and S100A9, high expression levels persisted for other proteins, including vitamin D-binding protein and fibrinogen γ. Structural and metabolic proteins were substantially decreased in lung fluid exclusively during MPXV and not VV infection. Decreases in structural and metabolic proteins were similarly observed in the extracellular fluid of MPXV-infected HeLa cells. Results from this study suggest that the host inflammatory response may not be the only facilitator of viral pathogenesis, but rather maintaining pulmonary structural integrity could be a key factor influencing disease progression and mortality.

Published

2010

23. Proteome of Salmonella Enterica Serotype Typhimurium Grown in a Low Mg2+/pH Medium

Author

Jason E. McDermott, Fred Heffron, Joshua N. Adkins, Heather M. Brewer, Richard D. Smith, Angela D. Norbeck, Ronald C. Taylor, Liang Shi, Jean K. Gustin, Leah M. Rommereim, Heather S. Smallwood, and Charles Ansong

Subjects

Growth medium, Salmonella, medicine.diagnostic_test, biology, Cell Biology, medicine.disease_cause, biology.organism_classification, Biochemistry, Pathogenicity island, Computer Science Applications, Type three secretion system, Microbiology, chemistry.chemical_compound, chemistry, Biotin, Western blot, Salmonella enterica, Proteome, medicine, bacteria, Molecular Biology

Abstract

To determine the impact of a low Mg2+/pH defined growth medium (MgM) on the proteome of Salmonella enterica serotype Typhimurium, we cultured S. Typhimurium cells in the medium under two different conditions termed MgM Shock and MgM Dilution and then comparatively analyzed the bacterial cells harvested from these conditions by a global proteomic approach. Proteomic results showed that MgM Shock and MgM Dilution differentially affected the S. Typhimurium proteome. MgM Shock induced a group of proteins whose induction usually occurred at low O2 level, while MgM Dilution induced those related to the type III secretion system (T3SS) of Salmonella Pathogenicity Island 2 (SPI2) and those involved in thiamine or biotin biosynthesis. The metabolic state of the S. Typhimurium cells grown under MgM Shock condition also differed significantly from that under MgM Dilution condition. Western blot analysis not only confirmed the proteomic results, but also showed that the abundances of SPI2- T3SS proteins SsaQ and SseE and biotin biosynthesis proteins BioB and BioD increased after S. Typhimurium infection of RAW 264.7 macrophages. Deletion of the gene encoding BioB reduced the bacterial ability to replicate inside the macrophages, suggesting a biotin-limited environment encountered by S. Typhimurium within RAW 264.7 macrophages.

Published

2009

24. Multicopy Single-Stranded DNA Directs Intestinal Colonization of Enteric Pathogens

Author

Joshua N. Adkins, Helene Andrews-Polymenis, Lydia M. Bogomolnaya, Michael McClelland, L. Garry Adams, Johanna R. Elfenbein, Leigh A. Knodler, Heather M. Brewer, Charles Ansong, Ernesto S. Nakayasu, and Fang, Ferric C

Subjects

Salmonella typhimurium, Cancer Research, lcsh:QH426-470, Mutant, DNA, Single-Stranded, medicine.disease_cause, RetroN, Microbiology, Vaccine Related, chemistry.chemical_compound, Mice, Single-Stranded, Biodefense, medicine, Genetics, Escherichia coli, Animals, Anaerobiosis, Molecular Biology, Genetics (clinical), Ecology, Evolution, Behavior and Systematics, biology, Prevention, DNA, biology.organism_classification, Foodborne Illness, Reverse transcriptase, 3. Good health, Intestines, lcsh:Genetics, Infectious Diseases, Emerging Infectious Diseases, chemistry, Multicopy single-stranded DNA, Anaerobic bacteria, Digestive Diseases, Bacteria, Developmental Biology, Research Article

Abstract

Multicopy single-stranded DNAs (msDNAs) are hybrid RNA-DNA molecules encoded on retroelements called retrons and produced by the action of retron reverse transcriptases. Retrons are widespread in bacteria but the natural function of msDNA has remained elusive despite 30 years of study. The major roadblock to elucidation of the function of these unique molecules has been the lack of any identifiable phenotypes for mutants unable to make msDNA. We report that msDNA of the zoonotic pathogen Salmonella Typhimurium is necessary for colonization of the intestine. Similarly, we observed a defect in intestinal persistence in an enteropathogenic E. coli mutant lacking its retron reverse transcriptase. Under anaerobic conditions in the absence of msDNA, proteins of central anaerobic metabolism needed for Salmonella colonization of the intestine are dysregulated. We show that the msDNA-deficient mutant can utilize nitrate, but not other alternate electron acceptors in anaerobic conditions. Consistent with the availability of nitrate in the inflamed gut, a neutrophilic inflammatory response partially rescued the ability of a mutant lacking msDNA to colonize the intestine. These findings together indicate that the mechanistic basis of msDNA function during Salmonella colonization of the intestine is proper production of proteins needed for anaerobic metabolism. We further conclude that a natural function of msDNA is to regulate protein abundance, the first attributable function for any msDNA. Our data provide novel insight into the function of this mysterious molecule that likely represents a new class of regulatory molecules., Author Summary Multicopy single-stranded DNA (msDNA) is a unique molecule consisting of both an RNA and DNA portion. This molecule is produced by a reverse transcriptase and has no known natural function despite more than 30 years of study. We report that msDNA is important for both Salmonella Typhimurium and an enteropathogenic E. coli, two pathogens that cause diarrhea in susceptible hosts, to survive in the intestine. Using mutant strains incapable of producing msDNA, we show that msDNA is needed for Salmonella to grow in the absence of oxygen. Mutants grown in oxygen-deficient conditions have substantial changes in overall protein composition, including numerous proteins known to be important for anaerobic metabolism and growth in the intestine. Our findings link msDNA to the ability of Salmonella to thrive in an oxygen-deficient environment similar to the conditions inside the gut. We report that msDNA regulates the quantity of proteins, the first natural function attributed to this molecule. msDNA may represent a new class of regulatory molecules.

Published

2015

25. Microscale depletion of high abundance proteins in human biofluids using IgY14 immunoaffinity resin: analysis of human plasma and cerebrospinal fluid

Author

Heather M. Brewer, Tao Liu, Paul D. Piehowski, Athena A. Schepmoes, Daniel J. Orton, Rui Zhao, Rosalie K. Chu, Seok Won Hyung, Richard D. Smith, Therese R. W. Clauss, Ronald J. Moore, and Thomas L. Fillmore

Subjects

Proteomics, Chromatography, Multiple Sclerosis, Proteome, Abundance (chemistry), Chemistry, Blood Proteins, Tandem mass spectrometry, Mass spectrometry, Biochemistry, Blood proteins, Article, Chromatography, Affinity, Analytical Chemistry, Volumetric flow rate, Column chromatography, Volume (thermodynamics), Tandem Mass Spectrometry, Albumins, Humans, Microscale chemistry, Biomarkers, Chromatography, Liquid

Abstract

Removal of highly abundant proteins in plasma is often carried out using immunoaffinity depletion to extend the dynamic range of measurements to lower abundance species. While commercial depletion columns are available for this purpose, they generally are not applicable to limited sample quantities (

Published

2014

26. Metaproteomics reveals differential modes of metabolic coupling among ubiquitous oxygen minimum zone microbes

Author

Alyse K. Hawley, Heather M. Brewer, Steven J. Hallam, Ljiljana Paša-Tolić, and Angela D. Norbeck

Subjects

Proteomics, Thaumarchaeota, Denitrification, Proteome, Nitrogen, Oxygen minimum zone, Models, Biological, Genes, Archaeal, Total inorganic carbon, Cluster Analysis, Ecosystem, Multidisciplinary, biology, Bacteria, Ecology, Gene Expression Profiling, Water, Gene Expression Regulation, Bacterial, Biological Sciences, biology.organism_classification, Anoxic waters, Archaea, Oxygen, Anammox, Genes, Bacterial, Nitrification, Gene Expression Regulation, Archaeal, Energy Metabolism, Nitrospira, Oxidation-Reduction, Sulfur

Abstract

Marine oxygen minimum zones (OMZs) are intrinsic water column features arising from respiratory oxygen demand during organic matter degradation in stratified waters. Currently OMZs are expanding due to global climate change with resulting feedback on marine ecosystem function. Here we use metaproteomics to chart spatial and temporal patterns of gene expression along defined redox gradients in a seasonally stratified fjord to better understand microbial community responses to OMZ expansion. The expression of metabolic pathway components for nitrification, anaerobic ammonium oxidation (anammox), denitrification, and inorganic carbon fixation were differentially expressed across the redoxcline and covaried with distribution patterns of ubiquitous OMZ microbes including Thaumarchaeota, Nitrospina, Nitrospira, Planctomycetes, and SUP05/ARCTIC96BD-19 Gammaproteobacteria. Nitrification and inorganic carbon fixation pathways affiliated with Thaumarchaeota dominated dysoxic waters, and denitrification, sulfur oxidation, and inorganic carbon fixation pathways affiliated with the SUP05 group of nitrate-reducing sulfur oxidizers dominated suboxic and anoxic waters. Nitrifier nitrite oxidation and anammox pathways affiliated with Nirospina, Nitrospira, and Planctomycetes, respectively, also exhibited redox partitioning between dysoxic and suboxic waters. The numerical abundance of SUP05 proteins mediating inorganic carbon fixation under anoxic conditions suggests that SUP05 will become increasingly important in global ocean carbon and nutrient cycling as OMZs expand.

Published

2014

27. LC-MS proteomics analysis of the iInsulin/IGF-1-deficient Caenorhabditis elegans daf-2(e1370) mutant reveals extensive restructuring of intermediary metabolism

Author

Richard D. Smith, Bart P. Braeckman, Arne Smolders, Vladislav A. Petyuk, Geert Depuydt, David G. Camp, Fang Xie, and Heather M. Brewer

Subjects

Proteomics, LARGE GENE LISTS, Proteome, medicine.medical_treatment, Mutant, METHYLMALONYL-COA EPIMERASE, Dauer larva, Biology, LIVED DAF-2 MUTANTS, Biochemistry, Article, Insulin resistance, medicine, Animals, Insulin, ATP-CITRATE LYASE, PYRUVATE-KINASE ACTIVITY, Insulin-Like Growth Factor I, Caenorhabditis elegans Proteins, Caenorhabditis elegans, Transcription factor, mass spectrometry, LIFE-SPAN, NEMATODE CAENORHABDITIS-ELEGANS, INSULIN-RESISTANCE, fungi, aging, Biology and Life Sciences, Forkhead Transcription Factors, DAUER LARVA, General Chemistry, medicine.disease, biology.organism_classification, Receptor, Insulin, Gene Knockdown Techniques, Mutation, physiology, gene expression, C-ELEGANS, Daf-2, metabolism, Metabolic Networks and Pathways, Transcription Factors

Abstract

The insulin/IGF-1 receptor is a major known determinant of dauer formation, stress resistance, longevity, and metabolism in Caenorhabditis elegans. In the past, whole-genome transcript profiling was used extensively to study differential gene expression in response to reduced insulin/IGF-1 signaling, including the expression levels of metabolism-associated genes. Taking advantage of the recent developments in quantitative liquid chromatography mass spectrometry (LC-MS)-based proteomics, we profiled the proteomic changes that occur in response to activation of the DAF-16 transcription factor in the germline-less glp-4(bn2);daf-2(e1370) receptor mutant. Strikingly, the daf-2 profile suggests extensive reorganization of intermediary metabolism, characterized by the upregulation of many core intermediary metabolic pathways. These include glycolysis/gluconeogenesis, glycogenesis, pentose phosphate cycle, citric acid cycle, glyoxylate shunt, fatty acid beta-oxidation, one-carbon metabolism, propionate and tyrosine catabolism, and complexes I, II, III, and V of the electron transport chain. Interestingly, we found simultaneous activation of reciprocally regulated metabolic pathways, which is indicative of spatiotemporal coordination of energy metabolism and/or extensive post-translational regulation of these enzymes. This restructuring of daf-2 metabolism is reminiscent to that of hypometabolic dauers, allowing the efficient and economical utilization of internal nutrient reserves and possibly also shunting metabolites through alternative energy-generating pathways to sustain longevity.

Published

2014

28. Salmonella modulates metabolism during growth under conditions that induce expression of virulence genes

Author

Marcus B. Jones, Fred Heffron, Brooke L. Deatherage Kaiser, Joshua N. Adkins, Young-Mo Kim, Brian J. Schmidt, Hugh D. Mitchell, Afshan S. Kidwai, Charles Ansong, Heather M. Brewer, Bernhard O. Palsson, Daniel R. Hyduke, Thomas O. Metz, Richard D. Smith, Scott N. Peterson, and Jason E. McDermott

Subjects

Salmonella typhimurium, Virulence Factors, Systems biology, Metabolic network, Virulence, Context (language use), Gene Expression Regulation, Bacterial, Biology, biology.organism_classification, Article, Metabolomics, Biochemistry, Bacterial Proteins, Salmonella enterica, Metabolome, Polyamines, Amino Acids, Molecular Biology, Pathogen, Metabolic Networks and Pathways, Biotechnology

Abstract

Salmonella enterica serovar Typhimurium (S. Typhimurium) is a facultative pathogen that uses complex mechanisms to invade and proliferate within mammalian host cells. To investigate possible contributions of metabolic processes to virulence in S. Typhimurium grown under conditions known to induce expression of virulence genes, we used a metabolomics-driven systems biology approach coupled with genome-scale modeling. First, we identified distinct metabolite profiles associated with bacteria grown in either rich or virulence-inducing media and report the most comprehensive coverage of the S. Typhimurium metabolome to date. Second, we applied an omics-informed genome-scale modeling analysis of the functional consequences of adaptive alterations in S. Typhimurium metabolism during growth under our conditions. Modeling efforts highlighted a decreased cellular capability to both produce and utilize intracellular amino acids during stationary phase culture in virulence conditions, despite significant abundance increases for these molecules as observed by our metabolomics measurements. Furthermore, analyses of omics data in the context of the metabolic model indicated rewiring of the metabolic network to support pathways associated with virulence. For example, cellular concentrations of polyamines were perturbed, as well as the predicted capacity for secretion and uptake.

Published

2013

29. Comparative Omics-Driven Genome Annotation Refinement: Application across Yersiniae

Author

Heather M. Brewer, Samuel H. Payne, Scott N. Peterson, Sadhana Chauhan, Matthew E. Monroe, Samuel O. Purvine, Joshua N. Adkins, Vladimir L. Motin, James A. Sanford, Marcus B. Jones, Alexandra C. Schrimpe-Rutledge, Charles Ansong, Bryan C. Frank, and Richard D. Smith

Subjects

Multidisciplinary, Data collection, business.industry, Science, lcsh:R, lcsh:Medicine, Library science, Environmental research, Correction, Genome project, Bioinformatics, Medicine, lcsh:Q, User Facility, lcsh:Science, business, National laboratory

Abstract

There were errors in the Funding section. The correct funding information is as follows: This research was supported by the National Institute of Allergy and Infectious Diseases NIH/DHHS through Interagency agreement Y1-AI-8401. Proteomics capabilities were developed under support from the U.S. Department of Energy (DOE) Office of Biological and Environmental Research and the NIH National Center for Research Resources (RR018522) and work was performed in the Environmental Molecular Sciences Laboratory, a DOE-BER national scientific user facility at Pacific Northwest National Laboratory (PNNL). PNNL is a multi-program national laboratory operated by Battelle Memorial Institute for the DOE under contract DE-AC05-76RLO 1830. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

Published

2012

30. Label-free quantitative LC-MS proteomics of Alzheimer's disease and normally aged human brains

Author

Victor P. Andreev, Fang Xie, Jennifer Clarke, Heather M. Brewer, Richard D. Smith, Zafar Nawaz, Amanda J. Myers, Vladislav A. Petyuk, David G. Camp, Jimmy El Hokayem, Andrew P. Lieberman, Roger L. Albin, and Yuliya V. Karpievitch

Subjects

Male, Proteomics, Cytoskeleton organization, Proteome, Quantitative proteomics, Computational biology, Biology, Tandem mass spectrometry, Orbitrap, Bioinformatics, Biochemistry, Article, law.invention, law, Alzheimer Disease, Tandem Mass Spectrometry, medicine, Humans, Protein phosphorylation, Gene Regulatory Networks, Aged, Aged, 80 and over, Brain, Reproducibility of Results, General Chemistry, medicine.disease, Case-Control Studies, Alzheimer's disease, Chromatography, Liquid, Transcription Factors

Abstract

Quantitative proteomics analysis of cortical samples of ten Alzheimer’s disease (AD) brains versus ten normally aged brains was performed by following the accurate mass and time tag (AMT) approach with the high resolution LTQ Orbitrap mass spectrometer. More than 1400 proteins were identified and quantitated. A conservative approach of selecting only the consensus results of four normalization methods was suggested and used. A total of 197 proteins were shown to be significantly differentially abundant (p-values

Published

2012

31. Comparative Omics-Driven Genome Annotation Refinement: Application across Yersiniae

Author

James A. Sanford, Richard D. Smith, Matthew E. Monroe, Charles Ansong, Samuel O. Purvine, Alexandra C. Schrimpe-Rutledge, Bryan C. Frank, Vladimir L. Motin, Heather M. Brewer, Samuel H. Payne, Joshua N. Adkins, Marcus B. Jones, Sadhana Chauhan, and Scott N. Peterson

Subjects

Proteomics, Bacterial Diseases, Pseudogene, Gene prediction, Molecular Sequence Data, lcsh:Medicine, Genomics, Computational biology, Biology, Vertebrate and Genome Annotation Project, Genome, Open Reading Frames, Genome Analysis Tools, Amino Acid Sequence, lcsh:Science, Frameshift Mutation, Genetics, Multidisciplinary, Base Sequence, Systems Biology, lcsh:R, Computational Biology, Molecular Sequence Annotation, Genome project, Yersinia, Infectious Diseases, Proteome, Medicine, lcsh:Q, Transcription Initiation Site, Peptides, Sequence Alignment, Genome, Bacterial, Pseudogenes, Research Article

Abstract

Genome sequencing continues to be a rapidly evolving technology, yet most downstream aspects of genome annotation pipelines remain relatively stable or are even being abandoned. The annotation process is now performed almost exclusively in an automated fashion to balance the large number of sequences generated. One possible way of reducing errors inherent to automated computational annotations is to apply data from omics measurements (i.e. transcriptional and proteomic) to the un-annotated genome with a proteogenomic-based approach. Here, the concept of annotation refinement has been extended to include a comparative assessment of genomes across closely related species. Transcriptomic and proteomic data derived from highly similar pathogenic Yersiniae (Y. pestis CO92, Y. pestis Pestoides F, and Y. pseudotuberculosis PB1/+) was used to demonstrate a comprehensive comparative omic-based annotation methodology. Peptide and oligo measurements experimentally validated the expression of nearly 40% of each strain's predicted proteome and revealed the identification of 28 novel and 68 incorrect (i.e., observed frameshifts, extended start sites, and translated pseudogenes) protein-coding sequences within the three current genome annotations. Gene loss is presumed to play a major role in Y. pestis acquiring its niche as a virulent pathogen, thus the discovery of many translated pseudogenes, including the insertion-ablated argD, underscores a need for functional analyses to investigate hypotheses related to divergence. Refinements included the discovery of a seemingly essential ribosomal protein, several virulence-associated factors, a transcriptional regulator, and many hypothetical proteins that were missed during annotation.

Published

2012

32. Genes for the major structural components of Thermotogales species' togas revealed by proteomic and evolutionary analyses of OmpA and OmpB homologs

Author

Kristen S. Swithers, Ljiljana Paša-Tolić, Si Wu, J. Peter Gogarten, Heather M. Brewer, Amanda K. Petrus, Chaman Ranjit, and Kenneth M. Noll

Subjects

Proteomics, Genome, Microbial Physiology, Peptide sequence, Phylogeny, Genetics, Chromatography, Likelihood Functions, Spectrometric Identification of Proteins, Multidisciplinary, Ecology, biology, Phylogenetic tree, Circular Dichroism, Microbial Growth and Development, Bacterial Biochemistry, Porin, Medicine, Research Article, Bacterial Outer Membrane Proteins, Science, Molecular Sequence Data, Porins, Microbiology, Synteny, Microbial Ecology, Evolution, Molecular, Extremophiles, Species Specificity, Phylogenetics, Sequence Homology, Nucleic Acid, Centrifugation, Density Gradient, Thermotoga maritima, Amino Acid Sequence, Biology, Gene, Whole genome sequencing, Evolutionary Biology, Bacterial Evolution, Base Sequence, Cell Membrane, Bacteriology, Astrobiology, biology.organism_classification, Organismal Evolution, Durapatite, Genes, Bacterial, Microbial Evolution, bacteria, Protein Multimerization, Developmental Biology

Abstract

The unifying structural characteristic of members of the bacterial order Thermotogales is their toga, an unusual cell envelope that includes a loose-fitting sheath around each cell. Only two toga-associated structural proteins have been purified and characterized in Thermotoga maritima: the anchor protein OmpA1 (or Ompa) and the porin OmpB (or Ompb). The gene encoding OmpA1 (ompA1) was cloned and sequenced and later assigned to TM0477 in the genome sequence, but because no peptide sequence was available for OmpB, its gene (ompB) was not annotated. We identified six porin candidates in the genome sequence of T. maritima. Of these candidates, only one, encoded by TM0476, has all the characteristics reported for OmpB and characteristics expected of a porin including predominant b-sheet structure, a carboxy terminus porin anchoring motif, and a porin-specific amino acid composition. We highly enriched a toga fraction of cells for OmpB by sucrose gradient centrifugation and hydroxyapatite chromatography and analyzed it by LC/MS/MS. We found that the only porin candidate that it contained was the TM0476 product. This cell fraction also had b-sheet character as determined by circular dichroism, consistent with its enrichment for OmpB. We conclude that TM0476 encodes OmpB. A phylogenetic analysis of OmpB found orthologsmore » encoded in syntenic locations in the genomes of all but two Thermotogales species. Those without orthologs have putative isofunctional genes in their place. Phylogenetic analyses of OmpA1 revealed that each species of the Thermotogales has one or two OmpA homologs. T. maritima has two OmpA homologs, encoded by ompA1 (TM0477) and ompA2 (TM1729), both of which were found in the toga protein-enriched cell extracts. These annotations of the genes encoding toga structural proteins will guide future examinations of the structure and function of this unusual lineage-defining cell sheath.« less

Published

2012

33. Comparative Analysis of Proteome and Transcriptome Variation in Mouse

Author

Aldons J. Lusis, Imran N. Mungrue, Richard D. Smith, Nicholas A. Furlotte, Brian J. Bennett, Heather M. Brewer, Karl K. Weitz, Charles Tilford, Hyun Min Kang, Vladislav A. Petyuk, Desmond J. Smith, Janet S. Sinsheimer, Nathan O. Siemers, Christopher C. Park, Isaac M. Neuhaus, Calvin Pan, Raffi Hagopian, David G. Camp, Roumyana Yordanova, Charles R. Farber, Todd G. Kirchgessner, Peter S. Gargalovic, Eleazar Eskin, Ping Zi Wen, Luz D. Orozco, and Anatole Ghazalpour

Subjects

Proteomics, Cancer Research, Proteome, lcsh:QH426-470, Genetics and Genomics/Animal Genetics, Biology, Genetics and Genomics/Complex Traits, Transcriptome, Mice, 03 medical and health sciences, 0302 clinical medicine, Inbred strain, Genetics, Animals, RNA, Messenger, Genetics and Genomics/Genomics, Molecular Biology, Gene, Genetics (clinical), Ecology, Evolution, Behavior and Systematics, Genetics and Genomics/Genetics of Disease, 030304 developmental biology, 0303 health sciences, Gene Expression Profiling, Alternative splicing, Genetic Variation, Genetics and Genomics, Genetics and Genomics/Gene Expression, Genetics and Genomics/Physiogenomics, Gene expression profiling, Alternative Splicing, lcsh:Genetics, DNA microarray, Genetics and Genomics/Comparative Genomics, 030217 neurology & neurosurgery, Genome-Wide Association Study, Research Article

Abstract

The relationships between the levels of transcripts and the levels of the proteins they encode have not been examined comprehensively in mammals, although previous work in plants and yeast suggest a surprisingly modest correlation. We have examined this issue using a genetic approach in which natural variations were used to perturb both transcript levels and protein levels among inbred strains of mice. We quantified over 5,000 peptides and over 22,000 transcripts in livers of 97 inbred and recombinant inbred strains and focused on the 7,185 most heritable transcripts and 486 most reliable proteins. The transcript levels were quantified by microarray analysis in three replicates and the proteins were quantified by Liquid Chromatography–Mass Spectrometry using O(18)-reference-based isotope labeling approach. We show that the levels of transcripts and proteins correlate significantly for only about half of the genes tested, with an average correlation of 0.27, and the correlations of transcripts and proteins varied depending on the cellular location and biological function of the gene. We examined technical and biological factors that could contribute to the modest correlation. For example, differential splicing clearly affects the analyses for certain genes; but, based on deep sequencing, this does not substantially contribute to the overall estimate of the correlation. We also employed genome-wide association analyses to map loci controlling both transcript and protein levels. Surprisingly, little overlap was observed between the protein- and transcript-mapped loci. We have typed numerous clinically relevant traits among the strains, including adiposity, lipoprotein levels, and tissue parameters. Using correlation analysis, we found that a low number of clinical trait relationships are preserved between the protein and mRNA gene products and that the majority of such relationships are specific to either the protein levels or transcript levels. Surprisingly, transcript levels were more strongly correlated with clinical traits than protein levels. In light of the widespread use of high-throughput technologies in both clinical and basic research, the results presented have practical as well as basic implications., Author Summary An old dogma in biology states that, in every cell, the flow of biological information is from DNA to RNA to proteins and that the latter act as a working force to determine the organism's phenotype. This model predicts that changes in DNA that affect the clinical phenotype should also similarly change the cellular levels of RNA and protein levels. In this report, we test this prediction by looking at the concordance between DNA variation in population of mouse inbred strains, the RNA and protein variation in the liver tissue of these mice, and variation in metabolic phenotypes. We show that the relationship between various biological traits is not simple and that there is relatively little concordance of RNA levels and the corresponding protein levels in response to DNA perturbations. In addition, we also find that, surprisingly, metabolic traits correlate better to RNA levels than to protein levels. In light of current efforts in searching for the molecular bases of disease susceptibility in humans, our findings highlight the complexity of information flow that underlies clinical outcomes.

Published

2011

34. Global proteomic analysis of two tick-borne emerging zoonotic agents: anaplasma phagocytophilum and ehrlichia chaffeensis

Author

Yasuko Rikihisa, Angela D. Norbeck, Takane Kikuchi, Mingqun Lin, and Heather M. Brewer

Subjects

Microbiology (medical), Human granulocytic anaplasmosis, lcsh:QR1-502, human granulocytic anaplasmosis, Biology, Proteomics, Microbiology, lcsh:Microbiology, 03 medical and health sciences, medicine, Ehrlichia chaffeensis, human leukocytes, 030304 developmental biology, Original Research, 0303 health sciences, Innate immune system, 030306 microbiology, Intracellular parasite, medicine.disease, biology.organism_classification, bacterial infections and mycoses, proteomic analysis, Anaplasma phagocytophilum, human monocytic ehrlichiosis, Membrane protein, Proteome

Abstract

Anaplasma phagocytophilum and Ehrlichia chaffeensis are obligatory intracellular alpha-proteobacteria that infect human leukocytes and cause potentially fatal emerging zoonoses. In the present study, we determined global protein expression profiles of these bacteria cultured in the human promyelocytic leukemia cell line, HL-60. Mass spectrometric (MS) analyses identified a total of 1,212 A. phagocytophilum and 1,021 E. chaffeensis proteins, representing 89.3% and 92.3% of the predicted bacterial proteomes, respectively. Nearly all bacterial proteins (≥ 99%) with known functions were expressed, whereas only approximately 80% of “hypothetical” proteins were detected in infected human cells. Quantitative MS/MS analyses indicated that highly-expressed proteins in both bacteria included chaperones, enzymes involved in biosynthesis and metabolism, and outer membrane proteins, such as A. phagocytophilum P44 and E. chaffeensis P28/OMP-1. Among 113 A. phagocytophilum p44 paralogous genes, 110 of them were expressed and 88 of them were encoded by pseudogenes. In addition, bacterial infection of HL-60 cells up-regulated the expression of human proteins involved mostly in cytoskeleton components, vesicular trafficking, cell signaling, and energy metabolism, but down-regulated some pattern recognition receptors involved in innate immunity. Our proteomics data represent a comprehensive analysis of A. phagocytophilum and E. chaffeensis proteomes, and provide a quantitative view of human host protein expression profiles regulated by bacterial infection. The availability of these proteomic data will provide new insights into biology and pathogenesis of these obligatory intracellular pathogens.

Published

2010

35. Discovery of Novel Secreted Virulence Factors from Salmonella enterica Serovar Typhimurium by Proteomic Analysis of Culture Supernatants ▿ #

Author

Afke Stufkens, Fred Heffron, Joshua N. Adkins, Athena A. Schepmoes, Jean K. Gustin, Heather M. Brewer, George S. Niemann, Jason E. McDermott, Roslyn N. Brown, Afshan S. Shaikh-Kidwai, Jie Li, and Richard D. Smith

Subjects

Salmonella typhimurium, Salmonella, Mice, 129 Strain, Virulence Factors, Immunology, Virulence, Biology, medicine.disease_cause, Microbiology, Mice, Bacterial Proteins, Artificial Intelligence, medicine, Animals, Secretion, Pathogen, Salmonella Infections, Animal, Cellular Microbiology: Pathogen-Host Cell Molecular Interactions, Effector, Gene Expression Regulation, Bacterial, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, Pathogenicity island, Infectious Diseases, Salmonella enterica, Host cell cytoplasm, Mutation, Parasitology, Algorithms

Abstract

Salmonella enterica serovar Typhimurium is a leading cause of acute gastroenteritis throughout the world. This pathogen has two type III secretion systems (TTSS) encoded in Salmonella pathogenicity islands 1 and 2 (SPI-1 and SPI-2) that deliver virulence factors (effectors) to the host cell cytoplasm and are required for virulence. While many effectors have been identified and at least partially characterized, the full repertoire of effectors has not been catalogued. In this proteomic study, we identified effector proteins secreted into defined minimal medium designed to induce expression of the SPI-2 TTSS and its effectors. We compared the secretomes of the parent strain to those of strains missing essential ( ssaK :: cat ) or regulatory (Δ ssaL ) components of the SPI-2 TTSS. We identified 20 known SPI-2 effectors. Excluding the translocon components SseBCD, all SPI-2 effectors were biased for identification in the Δ ssaL mutant, substantiating the regulatory role of SsaL in TTS. To identify novel effector proteins, we coupled our secretome data with a machine learning algorithm (SIEVE, S VM-based i dentification and e valuation of v irulence e ffectors) and selected 12 candidate proteins for further characterization. Using CyaA′ reporter fusions, we identified six novel type III effectors and two additional proteins that were secreted into J774 macrophages independently of a TTSS. To assess their roles in virulence, we constructed nonpolar deletions and performed a competitive index analysis from intraperitoneally infected 129/SvJ mice. Six mutants were significantly attenuated for spleen colonization. Our results also suggest that non-type III secretion mechanisms are required for full Salmonella virulence.

Published

2010

36. Characterization of macaque pulmonary fluid proteome during monkeypox infection: dynamics of host response

Author

Joseph N, Brown, Ryan D, Estep, Daniel, Lopez-Ferrer, Heather M, Brewer, Theresa R, Clauss, Nathan P, Manes, Megan, O'Connor, Helen, Li, Joshua N, Adkins, Scott W, Wong, and Richard D, Smith

Subjects

Proteome, Research, Molecular Sequence Data, Monkeypox, Polymerase Chain Reaction, Body Fluids, Viral Proteins, Tandem Mass Spectrometry, Animals, Humans, Macaca, Amino Acid Sequence, Lung, HeLa Cells

Abstract

Understanding viral pathogenesis is challenging because of confounding factors, including nonabrasive access to infected tissues and high abundance of inflammatory mediators that may mask mechanistic details. In diseases such as influenza and smallpox where the primary cause of mortality results from complications in the lung, the characterization of lung fluid offers a unique opportunity to study host-pathogen interactions with minimal effect on infected animals. This investigation characterizes the global proteome response in the pulmonary fluid, bronchoalveolar lavage fluid, of macaques during upper respiratory infection by monkeypox virus (MPXV), a close relative of the causative agent of smallpox, variola virus. These results are compared and contrasted against infections by vaccinia virus (VV), a low pathogenic relative of MPXV, and with extracellular fluid from MPXV-infected HeLa cells. To identify changes in the pulmonary protein compartment, macaque lung fluid was sampled twice prior to infection, serving as base line, and up to six times following intrabronchial infection with either MPXV or VV. Increased expression of inflammatory proteins was observed in response to both viruses. Although the increased expression resolved for a subset of proteins, such as C-reactive protein, S100A8, and S100A9, high expression levels persisted for other proteins, including vitamin D-binding protein and fibrinogen γ. Structural and metabolic proteins were substantially decreased in lung fluid exclusively during MPXV and not VV infection. Decreases in structural and metabolic proteins were similarly observed in the extracellular fluid of MPXV-infected HeLa cells. Results from this study suggest that the host inflammatory response may not be the only facilitator of viral pathogenesis, but rather maintaining pulmonary structural integrity could be a key factor influencing disease progression and mortality.

Published

2010

37. Proteome of Salmonella Enterica Serotype Typhimurium Grown in a Low Mg/pH Medium

Author

Liang, Shi, Charles, Ansong, Heather, Smallwood, Leah, Rommereim, Jason E, McDermott, Heather M, Brewer, Angela D, Norbeck, Ronald C, Taylor, Jean K, Gustin, Fred, Heffron, Richard D, Smith, and Joshua N, Adkins

Subjects

bacteria, Article

Abstract

To determine the impact of a low Mg(2+)/pH defined growth medium (MgM) on the proteome of Salmonella enterica serotype Typhimurium, we cultured S. Typhimurium cells in the medium under two different conditions termed MgM Shock and MgM Dilution and then comparatively analyzed the bacterial cells harvested from these conditions by a global proteomic approach. Proteomic results showed that MgM Shock and MgM Dilution differentially affected the S. Typhimurium proteome. MgM Shock induced a group of proteins whose induction usually occurred at low O(2) level, while MgM Dilution induced those related to the type III secretion system (T3SS) of Salmonella Pathogenicity Island 2 (SPI2) and those involved in thiamine or biotin biosynthesis. The metabolic state of the S. Typhimurium cells grown under MgM Shock condition also differed significantly from that under MgM Dilution condition. Western blot analysis not only confirmed the proteomic results, but also showed that the abundances of SPI2-T3SS proteins SsaQ and SseE and biotin biosynthesis proteins BioB and BioD increased after S. Typhimurium infection of RAW 264.7 macrophages. Deletion of the gene encoding BioB reduced the bacterial ability to replicate inside the macrophages, suggesting a biotin-limited environment encountered by S. Typhimurium within RAW 264.7 macrophages.

Published

2009

38. Protein and microRNA biomarkers from lavage, urine, and serum in military personnel evaluated for dyspnea

Author

Joshua N. Adkins, Carrie D. Nicora, Richard D. Smith, Karl K. Weitz, Andrew J Skabelund, Ji-Hoon Cho, Joseph N. Brown, Heather M. Brewer, Richard Gelinas, and Michael J. Morris

Subjects

Serum, Proteomics, Vital capacity, medicine.medical_specialty, Lavage fluid, Urine, Lung Disorder, 03 medical and health sciences, 0302 clinical medicine, Internal medicine, medicine, Genetics, Humans, Genetics(clinical), Respiratory system, Precision Medicine, Lung, Genetics (clinical), 030304 developmental biology, Asthma, 0303 health sciences, Bronchoscopy with Bronchoalveolar Lavage, business.industry, medicine.disease, 3. Good health, respiratory tract diseases, MicroRNAs, medicine.anatomical_structure, Dyspnea, 030220 oncology & carcinogenesis, Immunology, Disease Progression, business, Transcriptome, Bronchoalveolar Lavage Fluid, Biomarkers, Research Article

Abstract

Background We have identified candidate protein and microRNA (miRNA) biomarkers for dyspnea by studying serum, lavage fluid, and urine from military personnel who reported serious respiratory symptoms after they were deployed to Iraq or Afghanistan. Methods Forty-seven soldiers with the complaint of dyspnea who enrolled in the STudy of Active Duty Military Personnel for Environmental Dust Exposure (STAMPEDE) underwent comprehensive pulmonary evaluations at the San Antonio Military Medical Center. The evaluation included fiber-optic bronchoscopy with bronchoalveolar lavage. The clinical findings from the STAMPEDE subjects pointed to seven general underlying diagnoses or findings including airway hyperreactivity, asthma, low diffusivity of carbon monoxide, and abnormal cell counts. The largest category was undiagnosed. As an exploratory study, not a classification study, we profiled proteins or miRNAs in lavage fluid, serum, or urine in this group to look for any underlying molecular patterns that might lead to biomarkers. Proteins in lavage fluid and urine were identified by accurate mass tag (database-driven) proteomics methods while miRNAs were profiled by a hybridization assay applied to serum, urine, and lavage fluid. Results Over seventy differentially expressed proteins were reliably identified both from lavage and from urine in forty-eight dyspnea subjects compared to fifteen controls with no known lung disorder. Six of these proteins were detected both in urine and lavage. One group of subjects was distinguished from controls by expressing a characteristic group of proteins. A related group of dyspnea subjects expressed a unique group of miRNAs that included one miRNA that was differentially overexpressed in all three fluids studied. The levels of several miRNAs also showed modest but direct associations with several standard clinical measures of lung health such as forced vital capacity or gas exchange efficiency. Conclusions Candidate proteins and miRNAs associated with the general diagnosis of dyspnea have been identified in subjects with differing medical diagnoses. Since these markers can be measured in readily obtained clinical samples, further studies are possible that test the value of these findings in more formal classification or case–control studies in much larger cohorts of subjects with specific lung diseases such as asthma, emphysema, or some other well-defined lung disease.

39. Multicopy Single-Stranded DNA Directs Intestinal Colonization of Enteric Pathogens.

Author

Johanna R Elfenbein, Leigh A Knodler, Ernesto S Nakayasu, Charles Ansong, Heather M Brewer, Lydia Bogomolnaya, L Garry Adams, Michael McClelland, Joshua N Adkins, and Helene L Andrews-Polymenis

Subjects

Genetics, QH426-470

Abstract

Multicopy single-stranded DNAs (msDNAs) are hybrid RNA-DNA molecules encoded on retroelements called retrons and produced by the action of retron reverse transcriptases. Retrons are widespread in bacteria but the natural function of msDNA has remained elusive despite 30 years of study. The major roadblock to elucidation of the function of these unique molecules has been the lack of any identifiable phenotypes for mutants unable to make msDNA. We report that msDNA of the zoonotic pathogen Salmonella Typhimurium is necessary for colonization of the intestine. Similarly, we observed a defect in intestinal persistence in an enteropathogenic E. coli mutant lacking its retron reverse transcriptase. Under anaerobic conditions in the absence of msDNA, proteins of central anaerobic metabolism needed for Salmonella colonization of the intestine are dysregulated. We show that the msDNA-deficient mutant can utilize nitrate, but not other alternate electron acceptors in anaerobic conditions. Consistent with the availability of nitrate in the inflamed gut, a neutrophilic inflammatory response partially rescued the ability of a mutant lacking msDNA to colonize the intestine. These findings together indicate that the mechanistic basis of msDNA function during Salmonella colonization of the intestine is proper production of proteins needed for anaerobic metabolism. We further conclude that a natural function of msDNA is to regulate protein abundance, the first attributable function for any msDNA. Our data provide novel insight into the function of this mysterious molecule that likely represents a new class of regulatory molecules.

Published

2015

40. Genes for the major structural components of Thermotogales species' togas revealed by proteomic and evolutionary analyses of OmpA and OmpB homologs.

Author

Amanda K Petrus, Kristen S Swithers, Chaman Ranjit, Si Wu, Heather M Brewer, J Peter Gogarten, Ljiljana Pasa-Tolic, and Kenneth M Noll

Subjects

Medicine, Science

Abstract

The unifying structural characteristic of members of the bacterial order Thermotogales is their toga, an unusual cell envelope that includes a loose-fitting sheath around each cell. Only two toga-associated structural proteins have been purified and characterized in Thermotoga maritima: the anchor protein OmpA1 (or Ompα) and the porin OmpB (or Ompβ). The gene encoding OmpA1 (ompA1) was cloned and sequenced and later assigned to TM0477 in the genome sequence, but because no peptide sequence was available for OmpB, its gene (ompB) was not annotated. We identified six porin candidates in the genome sequence of T. maritima. Of these candidates, only one, encoded by TM0476, has all the characteristics reported for OmpB and characteristics expected of a porin including predominant β-sheet structure, a carboxy terminus porin anchoring motif, and a porin-specific amino acid composition. We highly enriched a toga fraction of cells for OmpB by sucrose gradient centrifugation and hydroxyapatite chromatography and analyzed it by LC/MS/MS. We found that the only porin candidate that it contained was the TM0476 product. This cell fraction also had β-sheet character as determined by circular dichroism, consistent with its enrichment for OmpB. We conclude that TM0476 encodes OmpB. A phylogenetic analysis of OmpB found orthologs encoded in syntenic locations in the genomes of all but two Thermotogales species. Those without orthologs have putative isofunctional genes in their place. Phylogenetic analyses of OmpA1 revealed that each species of the Thermotogales has one or two OmpA homologs. T. maritima has two OmpA homologs, encoded by ompA1 (TM0477) and ompA2 (TM1729), both of which were found in the toga protein-enriched cell extracts. These annotations of the genes encoding toga structural proteins will guide future examinations of the structure and function of this unusual lineage-defining cell sheath.

Published

2012

41. Comparative omics-driven genome annotation refinement: application across Yersiniae.

Author

Alexandra C Schrimpe-Rutledge, Marcus B Jones, Sadhana Chauhan, Samuel O Purvine, James A Sanford, Matthew E Monroe, Heather M Brewer, Samuel H Payne, Charles Ansong, Bryan C Frank, Richard D Smith, Scott N Peterson, Vladimir L Motin, and Joshua N Adkins

Subjects

Medicine, Science

Abstract

Genome sequencing continues to be a rapidly evolving technology, yet most downstream aspects of genome annotation pipelines remain relatively stable or are even being abandoned. The annotation process is now performed almost exclusively in an automated fashion to balance the large number of sequences generated. One possible way of reducing errors inherent to automated computational annotations is to apply data from omics measurements (i.e. transcriptional and proteomic) to the un-annotated genome with a proteogenomic-based approach. Here, the concept of annotation refinement has been extended to include a comparative assessment of genomes across closely related species. Transcriptomic and proteomic data derived from highly similar pathogenic Yersiniae (Y. pestis CO92, Y. pestis Pestoides F, and Y. pseudotuberculosis PB1/+) was used to demonstrate a comprehensive comparative omic-based annotation methodology. Peptide and oligo measurements experimentally validated the expression of nearly 40% of each strain's predicted proteome and revealed the identification of 28 novel and 68 incorrect (i.e., observed frameshifts, extended start sites, and translated pseudogenes) protein-coding sequences within the three current genome annotations. Gene loss is presumed to play a major role in Y. pestis acquiring its niche as a virulent pathogen, thus the discovery of many translated pseudogenes, including the insertion-ablated argD, underscores a need for functional analyses to investigate hypotheses related to divergence. Refinements included the discovery of a seemingly essential ribosomal protein, several virulence-associated factors, a transcriptional regulator, and many hypothetical proteins that were missed during annotation.

Published

2012

42. Global Proteomic Analysis of Two Tick-borne Emerging Zoonotic Agents: Anaplasma phagocytophilum and Ehrlichia chaffeensis

Author

Mingqun eLin, Takane eKikuchi, Heather M Brewer, Angela D Norbeck, and Yasuko eRikihisa

Subjects

Anaplasma phagocytophilum, Ehrlichia chaffeensis, Human Granulocytic Anaplasmosis, Human Leukocytes, Human Monocytic Ehrlichiosis, Proteomic analysis, Microbiology, QR1-502

Abstract

Anaplasma phagocytophilum and Ehrlichia chaffeensis are obligatory intracellular alpha-proteobacteria that infect human leukocytes and cause potentially fatal emerging zoonoses. In the present study, we determined global protein expression profiles of these bacteria cultured in the human promyelocytic leukemia cell line, HL-60. Mass spectrometric (MS) analyses identified a total of 1,212 A. phagocytophilum and 1,021 E. chaffeensis proteins, representing 89.3% and 92.3% of the predicted bacterial proteomes, respectively. Nearly all bacterial proteins (≥ 99%) with known functions were expressed, whereas only approximately 80% of hypothetical proteins were detected in infected human cells. Quantitative MS/MS analyses indicated that highly-expressed proteins in both bacteria included chaperones, enzymes involved in biosynthesis and metabolism, and outer membrane proteins, such as A. phagocytophilum P44 and E. chaffeensis P28/OMP-1. Among 113 A. phagocytophilum p44 paralogous genes, 110 of them were expressed and 88 of them were encoded by pseudogenes. In addition, bacterial infection of HL-60 cells up-regulated the expression of human proteins involved mostly in cytoskeleton components, vesicular trafficking, cell signaling, and energy metabolism, but down-regulated some pattern recognition receptors involved in innate immunity. Our proteomics data represent a comprehensive analysis of A. phagocytophilum and E. chaffeensis proteomes, and provide a quantitative view of human host protein expression profiles regulated by bacterial infection. The availability of these proteomic data will provide new insights into biology and pathogenesis of these obligatory intracellular pathogens.

Published

2011