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1. The anti-sigma factor MucA of Pseudomonas aeruginosa: Dramatic differences of a mucA22 vs. a ΔmucA mutant in anaerobic acidified nitrite sensitivity of planktonic and biofilm bacteria in vitro and during chronic murine lung infection

Author

Daniel A. Muruve, Long J. Lu, Dennis E. Ohman, Boo Shan Tseng, Gee W. Lau, Ralph J. Panos, Michael J. Schurr, Shengchang Su, Daniel J. Hassett, Thomas B. Thompson, Hongwei D. Yu, Warunya Panmanee, Cameron T. McDaniel, Xiaoting Zhu, and Zhaowei Ren

Subjects
0301 basic medicine, Pulmonology, Microarrays, Mutant, Gene Expression, ATP-binding cassette transporter, medicine.disease_cause, Sigma factor, Medicine and Health Sciences, Pathogen, Lung, Multidisciplinary, biology, Chemistry, respiratory system, Hydrogen-Ion Concentration, Plankton, 3. Good health, Bioassays and Physiological Analysis, Pseudomonas aeruginosa, Medicine, Research Article, Science, Chronic Obstructive Pulmonary Disease, 030106 microbiology, Anaerobic Bacteria, Research and Analysis Methods, Microbiology, 03 medical and health sciences, Bacterial Proteins, Gene Types, medicine, Genetics, Humans, Pseudomonas Infections, Gene Regulation, Nitrites, Bacteria, Biofilm, Organisms, Biology and Life Sciences, Bacteriology, biology.organism_classification, respiratory tract diseases, Quorum sensing, 030104 developmental biology, Biofilms, Chronic Disease, Mutation, Respiratory Infections, Regulator Genes, Bacterial Biofilms
Abstract

Mucoid mucA22 Pseudomonas aeruginosa (PA) is an opportunistic lung pathogen of cystic fibrosis (CF) and chronic obstructive pulmonary disease (COPD) patients that is highly sensitive to acidified nitrite (A-NO2-). In this study, we first screened PA mutant strains for sensitivity or resistance to 20 mM A-NO2- under anaerobic conditions that represent the chronic stages of the aforementioned diseases. Mutants found to be sensitive to A-NO2- included PA0964 (pmpR, PQS biosynthesis), PA4455 (probable ABC transporter permease), katA (major catalase, KatA) and rhlR (quorum sensing regulator). In contrast, mutants lacking PA0450 (a putative phosphate transporter) and PA1505 (moaA2) were A-NO2- resistant. However, we were puzzled when we discovered that mucA22 mutant bacteria, a frequently isolated mucA allele in CF and to a lesser extent COPD, were more sensitive to A-NO2- than a truncated ΔmucA deletion (Δ157-194) mutant in planktonic and biofilm culture, as well as during a chronic murine lung infection. Subsequent transcriptional profiling of anaerobic, A-NO2--treated bacteria revealed restoration of near wild-type transcript levels of protective NO2- and nitric oxide (NO) reductase (nirS and norCB, respectively) in the ΔmucA mutant in contrast to extremely low levels in the A-NO2--sensitive mucA22 mutant. Proteins that were S-nitrosylated by NO derived from A-NO2- reduction in the sensitive mucA22 strain were those involved in anaerobic respiration (NirQ, NirS), pyruvate fermentation (UspK), global gene regulation (Vfr), the TCA cycle (succinate dehydrogenase, SdhB) and several double mutants were even more sensitive to A-NO2-. Bioinformatic-based data point to future studies designed to elucidate potential cellular binding partners for MucA and MucA22. Given that A-NO2- is a potentially viable treatment strategy to combat PA and other infections, this study offers novel developments as to how clinicians might better treat problematic PA infections in COPD and CF airway diseases.

Published
2018

2. A philosophy for Opening Biotechnology Collaboration for Therapeutics

Author

Jason Barkeloo, Timothy Cripe, Li Guo, Ronald Laymon, Pablo Pomposiello, Heather Ruland-Staines, and Shengchang Su

Abstract

The pharmaceutical industry faces a host of worsening problems: Multibillion-dollar expenses and decade-long development times to bring new drugs to market, high failure rates for new drug candidates, and a patent system that is both expensive and uncertain. Demanding regulatory requirements and governmental pressures on prescription costs add yet more pressure on drug development. Although the situation does not yet constitute a crisis, its current trajectory is becoming increasingly untenable. While the industry itself has been resourceful in introducing technological advances and operating reforms such as increased collaboration through patent pooling, these efforts do not exhaust the possibilities for improvement. In particular, there has been an emerging, more agile and responsive alternative model in pharmaceutical research and development, namely open source synthetic biology – a rapidly developing and highly collaborative effort based on engineering principles involving the design and construction of biological systems using standardized modules of DNA. Synthetic biology began entirely open to those who wished to participate, provided that they agreed to share their results without restrictions. In its current and more mature state, it retains much of its open source character and is consequently less dependent on secrecy and patent protection than the pharmaceutical industry’s largely proprietary approach. The success of open source synthetic biology has inspired us to further develop that approach for research and development in Biotechnology and its pharmaceutical applications. Here, we reviewed the history and progress of open source science and technology.

Published
2017

3. Construction and characterization of stable, constitutively expressed, chromosomal green and red fluorescent transcriptional fusions in the select agents, Bacillus anthracis , Yersinia pestis , Burkholderia mallei , and Burkholderia pseudomallei

Author

Adin Pemberton, Roland Saldanha, Bruce J. Aronow, Gary E. Dean, Shengchang Su, Thomas J. Lamkin, Hansraj Bangar, and Daniel J. Hassett

Subjects
Burkholderia mallei, Burkholderia, biology, Yersinia pestis, Burkholderia pseudomallei, Virulence, Select agent, biology.organism_classification, Microbiology, Green fluorescent protein, Bacillus anthracis
Abstract

Here, we constructed stable, chromosomal, constitutively expressed, green and red fluorescent protein (GFP and RFP) as reporters in the select agents, Bacillus anthracis, Yersinia pestis, Burkholderia mallei, and Burkholderia pseudomallei. Using bioinformatic approaches and other experimental analyses, we identified P0253 and P1 as potent promoters that drive the optimal expression of fluorescent reporters in single copy in B. anthracis and Burkholderia spp. as well as their surrogate strains, respectively. In comparison, Y. pestis and its surrogate strain need two chromosomal copies of cysZK promoter (P2cysZK) for optimal fluorescence. The P0253-, P2cysZK-, and P1-driven GFP and RFP fusions were first cloned into the vectors pRP1028, pUC18R6KT-mini-Tn7T-Km, pmini-Tn7-gat, or their derivatives. The resultant constructs were delivered into the respective surrogates and subsequently into the select agent strains. The chromosomal GFP- and RFP-tagged strains exhibited bright fluorescence at an exposure time of less than 200 msec and displayed the same virulence traits as their wild-type parental strains. The utility of the tagged strains was proven by the macrophage infection assays and lactate dehydrogenase release analysis. Such strains will be extremely useful in high-throughput screens for novel compounds that could either kill these organisms, or interfere with critical virulence processes in these important bioweapon agents and during infection of alveolar macrophages.

Published
2014

4. A Signaling Pathway Involving the Diguanylate Cyclase CelR and the Response Regulator DivK Controls Cellulose Synthesis in Agrobacterium tumefaciens

Author

Shengchang Su, D. Michael Barnhart, and Stephen K. Farrand

Subjects
Operon, DNA Mutational Analysis, Mutant, Cell morphology, Microbiology, Bacterial Proteins, Two-Hybrid System Techniques, Cellulose synthase complex, Cellulose, Molecular Biology, biology, Cell Cycle, Genetic Complementation Test, Articles, Gene Expression Regulation, Bacterial, Agrobacterium tumefaciens, biology.organism_classification, Repressor Proteins, PilZ domain, Response regulator, Biochemistry, Mutagenesis, Site-Directed, biology.protein, Diguanylate cyclase, Protein Multimerization, Gene Deletion, Signal Transduction, Transcription Factors
Abstract

The production of cellulose fibrils is involved in the attachment of Agrobacterium tumefaciens to its plant host. Consistent with previous studies, we reported recently that a putative diguanylate cyclase, celR , is required for synthesis of this polymer in A. tumefaciens . In this study, the effects of celR and other components of the regulatory pathway of cellulose production were explored. Mutational analysis of celR demonstrated that the cyclase requires the catalytic GGEEF motif, as well as the conserved aspartate residue of a CheY-like receiver domain, for stimulating cellulose production. Moreover, a site-directed mutation within the PilZ domain of CelA, the catalytic subunit of the cellulose synthase complex, greatly reduced cellulose production. In addition, deletion of divK , the first gene of the divK-celR operon, also reduced cellulose production. This requirement for divK was alleviated by expression of a constitutively active form of CelR, suggesting that DivK acts upstream of CelR activation. Based on bacterial two-hybrid assays, CelR homodimerizes but does not interact with DivK. The mutation in divK additionally affected cell morphology, and this effect was complementable by a wild-type copy of the gene, but not by the constitutively active allele of celR . These results support the hypothesis that CelR is a bona fide c-di-GMP synthase and that the nucleotide signal produced by this enzyme activates CelA via the PilZ domain. Our studies also suggest that the DivK/CelR signaling pathway in Agrobacterium regulates cellulose production independent of cell cycle checkpoint systems that are controlled by divK .

Published
2014

5. CelR, an Ortholog of the Diguanylate Cyclase PleD of Caulobacter, Regulates Cellulose Synthesis in Agrobacterium tumefaciens

Author

D. Michael Barnhart, Brenna E. Baccaro, Lois M. Banta, Stephen K. Farrand, and Shengchang Su

Subjects
Protein subunit, Mutant, Gene Expression, Virulence, Applied Microbiology and Biotechnology, Caulobacter, chemistry.chemical_compound, Plant Microbiology, Bacterial Proteins, Cellulose, Phylogeny, Regulation of gene expression, Sequence Homology, Amino Acid, Ecology, biology, Escherichia coli Proteins, Biofilm, Gene Expression Regulation, Bacterial, Agrobacterium tumefaciens, biology.organism_classification, Repressor Proteins, chemistry, Biochemistry, biology.protein, Diguanylate cyclase, Phosphorus-Oxygen Lyases, Gene Deletion, Food Science, Biotechnology
Abstract

Cellulose fibrils play a role in attachment of Agrobacterium tumefaciens to its plant host. While the genes for cellulose biosynthesis in the bacterium have been identified, little is known concerning the regulation of the process. The signal molecule cyclic di-GMP (c-di-GMP) has been linked to the regulation of exopolysaccharide biosynthesis in many bacterial species, including A. tumefaciens . In this study, we identified two putative diguanylate cyclase genes, celR ( atu1297 ) and atu1060 , that influence production of cellulose in A. tumefaciens . Overexpression of either gene resulted in increased cellulose production, while deletion of celR , but not atu1060 , resulted in decreased cellulose biosynthesis. celR overexpression also affected other phenotypes, including biofilm formation, formation of a polar adhesion structure, plant surface attachment, and virulence, suggesting that the gene plays a role in regulating these processes. Analysis of celR and Δ cel mutants allowed differentiation between phenotypes associated with cellulose production, such as biofilm formation, and phenotypes probably resulting from c-di-GMP signaling, which include polar adhesion, attachment to plant tissue, and virulence. Phylogenetic comparisons suggest that species containing both celR and celA , which encodes the catalytic subunit of cellulose synthase, adapted the CelR protein to regulate cellulose production while those that lack celA use CelR, called PleD, to regulate specific processes associated with polar localization and cell division.

Published
2013

6. A microliter-scale microbial fuel cell array for bacterial electrogenic screening

Author

Shengchang Su, Daniel J. Hassett, Warunya Panmanee, Sayantika Mukherjee, Seokheun Choi, and Randall T. Irvin

Subjects
Microbial fuel cell, biology, Metals and Alloys, Homoserine, Analytical chemistry, Proton exchange membrane fuel cell, Condensed Matter Physics, biology.organism_classification, Nitrite reductase, Cathode, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, Anode, law.invention, chemistry.chemical_compound, chemistry, law, Biophysics, Electrical and Electronic Engineering, Shewanella oneidensis, Instrumentation, Bacteria
Abstract

We have developed an array of six MEMS (micro-electro-mechanical systems) microbial fuel cells (MFCs), a compact and reliable platform for rapid screening of electrochemically active bacteria. The MFC array contains vertically stacked 1.5 μL anode/cathode chambers separated by a proton exchange membrane (PEM), and represents the smallest MEMS MFC array currently available. Each layer, except for the PEM, was micro-patterned by using laser micromachining and was precisely aligned. Within just 5 h, we successfully determined the electricity generation capacity of two known bacterial electrogens (wild-type S. oneidensis and P. aeruginosa ) and another metabolically more voracious organism with 4 isogenic mutants constructed with the hypothesis that such mutations could alter their electrogenic properties. Genetically engineered genes in P. aeruginosa including nirS (nitrite reductase), lasl ( N -(3-oxododecanoyl)- l -homoserine lactone synthase), bdlA (biofiilm dispersion locus) and pilT (controls the number of Type IV pili on the poles of the bacteria) sensitively showed different efficiencies of extracellular electron transfer to the anode in the significantly reduced micro-chambers. In addition, the percent deviation of all six MFC units was less than 1.4% from their open circuit voltages recorded, which is far less than that of mL-sized MFC arrays (25%) and even MEMS MFC arrays (>8%). This analytical platform would provide the practical tools for fundamental study and characterization of the behavior and physiology of microorganisms and their interaction with MFCs with a greater level of insight and productivity.

Published
2013

7. Cyclic voltammetric, fluorescence and biological analysis of purified aeruginosin A, a secreted red pigment of Pseudomonas aeruginosa PAO1

Author

Larry Sallans, Shengchang Su, William R. Heineman, Eme A. Abu, Daniel J. Hassett, Raymond E. Boissy, and Amanda Greatens

Subjects
Keratinocytes, Staphylococcus aureus, Stereochemistry, medicine.disease_cause, Microbiology, Fluorescence, Mass Spectrometry, chemistry.chemical_compound, Pigment, Betaine, Pyocyanin, In vivo, Electrochemistry, Escherichia coli, medicine, Humans, Organic Chemicals, Cells, Cultured, Pseudomonas aeruginosa, Chemistry, Quorum Sensing, Pigments, Biological, visual_art, Biophysics, visual_art.visual_art_medium, Cyclic voltammetry, Oxidation-Reduction
Abstract

The opportunistic pathogen Pseudomomas aeruginosa produces multiple pigments during in vitro culture and in vivo during colonization of burn wounds and in the airways of cystic fibrosis (CF) patients. One pigment is a deep 'merlot'-coloured compound known as aeruginosin A (AA). However, the red pigment(s) of P. aeruginosa are often collectively called pyorubrin, of which there is no known chemical composition. Here, we purified and confirmed by MS and assessed the physicochemical properties of AA (2-amino-6-carboxy-10-methylphenazinium betaine) by first focusing on its ability to redox-cycle using cyclic voltammetry and its spectroscopic (as well as fluorescent) properties, experiments that were conducted at physiological pH. AA exhibited reversible electrochemistry at a glassy carbon electrode within a potential range of -500 to -200 mV. Electrochemical anodic and cathodic peak currents were observed at -327 and -360 mV, respectively, with a low formal reduction potential of -343.5 mV versus Ag/AgCl. AA absorbed at 516 nm and fluoresced at 606 nm. Results from the spectro-electrochemistry of pyorubrin revealed that its strongest fluorescence was in its parent or oxidized form. Production of AA by P. aeruginosa was found to be controlled by the rhl component of the intercellular signalling system known as quorum sensing and was produced maximally during the stationary growth phase. However, unlike its downstream blue redox-active toxin, pyocyanin, AA had no adverse effects on methicillin-resistant Staphylococcus aureus USA300, Escherichia coli DH5-α or human keratinocytes. We close with some thoughts on the potential commercial use(s) of AA.

Published
2013

8. Characterization of stable, constitutively expressed, chromosomal green and red fluorescent transcriptional fusions in the select agent bacterium, Francisella tularensis Schu S4 and the surrogate type B live vaccine strain (LVS)

Author

Adin Pemberton, Thomas J. Lamkin, Steven A. Kawamoto, Bruce J. Aronow, Hansraj Bangar, Roland Saldanha, Daniel J. Hassett, and Shengchang Su

Subjects
Green Fluorescent Proteins, Mutant, Gene Expression, Virulence, Applied Microbiology and Biotechnology, Microbiology, Green fluorescent protein, Genes, Reporter, Humans, Replicon, Francisella tularensis, Tularemia, Gene, Reporter gene, biology, Macrophages, General Medicine, Chromosomes, Bacterial, biology.organism_classification, Virology, Luminescent Proteins, Bacterial Vaccines, Francisella, Genetic Engineering, Biotechnology
Abstract

Here, we constructed stable, constitutively expressed, chromosomal green (GFP) and red fluorescent (RFP) reporters in the genome of the surrogate strain, Francisella tularensis spp. holarctica LVS (herein LVS), and the select agent, F. tularensis Schu S4. A bioinformatic approach was used to identify constitutively expressed genes. Two promoter regions upstream of the FTT1794 and rpsF(FTT1062) genes were selected and fused with GFP and RFP reporter genes in pMP815, respectively. While the LVS strains with chromosomally integrated reporter fusions exhibited fluorescence, we were unable to deliver the same fusions into Schu S4. Neither a temperature-sensitive Francisella replicon nor a pBBR replicon in the modified pMP815 derivatives facilitated integration. However, a mini-Tn7 integration system was successful at integrating the reporter fusions into the Schu S4 genome. Finally, fluorescent F. tularensis LVS and a mutant lacking MglA were assessed for growth in monocyte-derived macrophages (MDMs). As expected, when compared to wild-type bacteria, replication of an mglA mutant was significantly diminished, and the overall level of fluorescence dramatically decreased with infection time. The utility of the fluorescent Schu S4 strain was also examined within infected MDMs treated with clarithromycin and enrofloxacin. Taken together, this study describes the development of an important reagent for F. tularensis research, especially since the likelihood of engineered antibiotic resistant strains will emerge with time. Such strains will be extremely useful in high-throughput screens for novel compounds that could interfere with critical virulence processes in this important bioweapons agent and during infection of alveolar macrophages.

Published
2013

9. AnaerobicPseudomonas aeruginosaand other obligately anaerobic bacterial biofilms growing in the thick airway mucus of chronically infected cystic fibrosis patients: an emerging paradigm or 'Old Hat'?

Author

Daniel J. Hassett and Shengchang Su

Subjects
Cystic Fibrosis, Clinical Biochemistry, Biology, medicine.disease_cause, Cystic fibrosis, Microbiology, Drug Discovery, medicine, Prevotella, Humans, Pseudomonas Infections, Pharmacology, Pseudomonas aeruginosa, Obligate anaerobe, biology.organism_classification, medicine.disease, Mucus, Biofilms, Immunology, Molecular Medicine, Sputum, Anaerobic bacteria, medicine.symptom, Bacteria
Abstract

The cystic fibrosis (CF) airway mucus is an ideal niche in which many bacteria can develop antibiotic- and phagocyte-resistance in unique structures known as "mode II biofilms" where bacteria are embedded within the mucus, yet unattached to airway epithelial cells. Pseudomonas aeruginosa is the dominant CF pathogen, yet herein the authors provide burgeoning evidence that obligate anaerobic bacteria (e.g., Prevotella) actually thrive within the CF mucus, a paradigmatic shift that chronic CF is an "aerobic" disease. Interestingly, CF organisms repress virulence factor production (e.g., P. aeruginosa) while others (e.g., S. aureus) increase them under anaerobic conditions.The authors shed additional light on (i) the anoxic nature of the CF airway mucus, (ii) the relative commonality of anaerobic bacteria isolated from CF sputum, (iii) virulence factor production and cross-talk between obligate anaerobes and P. aeruginosa relative to disease progression/remission, (iv) the role of mucoidy in CF, and (v) the role of nitrosative stress in activation of bacteriophage and pyocins within biofilms.The authors conclude with insight as to how we might treat some CF bacteria during mode II biofilm infections that utilizes a metabolite of bacterial anaerobic respiration and an aerobic oxidation product of airway-generated NO, acidified NO(2)(-).

Published
2012

10. Induction and Loss of Ti Plasmid Conjugative Competence in Response to the Acyl-Homoserine Lactone Quorum-Sensing Signal

Author

Shengchang Su, Stephen K. Farrand, and Sharik R. Khan

Subjects
Blotting, Western, Mutant, Homoserine, Biology, Microbiology, chemistry.chemical_compound, Ti plasmid, Plasmid, 4-Butyrolactone, Plant Tumor-Inducing Plasmids, Molecular Biology, Models, Genetic, Quorum Sensing, Meeting Presentations, Gene Expression Regulation, Bacterial, Agrobacterium tumefaciens, biology.organism_classification, Cell biology, Kinetics, Quorum sensing, Biochemistry, chemistry, Conjugation, Genetic, Mutation, Signal transduction, Signal Transduction
Abstract

Conjugative transfer of the Ti plasmids of Agrobacterium tumefaciens is controlled by a quorum-sensing system composed of TraR and its signal N -(3-oxo-octanoyl)- l -homoserine lactone. This system is, in turn, controlled by the conjugative opines produced by crown gall tumors induced on plants by the bacteria. Using nonpolar traI mutants, we examined the kinetics of induction of conjugative transfer in response to exogenous acyl-homoserine lactone. In the absence of the antiactivator TraM, onset of induction of transfer requires about 30 min, 15 to 20 min of which is needed for expression and construction of the conjugative apparatus. TraM delays the onset of conjugation by 30 min. While the rate of development of conjugative competence was not significantly affected by levels of TraR, maximum efficiencies of transfer were correlated with amounts of the activator in the donors. Donors harboring Ti plasmids lacking TraM were fully induced by the quormone at concentrations as low as 100 pM. TraM raised the concentration of signal required for maximum activity to 1 nM. Donors grown in batch culture retained conjugative competence following signal removal, even when in stationary phase. However, donors kept in balanced growth rapidly lost transfer ability following signal removal. Loss of transfer was mirrored by a decrease in levels of active TraR. Decreases in TraR activity and conjugative competence could be accounted for by dilution associated with cell division, suggesting that while induction of Ti plasmid conjugation is an active process, the cells lack a mechanism for disassembling the conjugative apparatus when signals become limiting.

Published
2008

11. Molecular Basis of Transcriptional Antiactivation

Author

Stephen K. Farrand, Shengchang Su, and Yinping Qin

Subjects
biology, Agrobacterium, Activator (genetics), Dimer, Cell Biology, biology.organism_classification, Biochemistry, Nucleoprotein, chemistry.chemical_compound, Plasmid, chemistry, Biophysics, Autoinducer, Dna complex, Molecular Biology, DNA
Abstract

Conjugative transfer of Agrobacterium Ti plasmids is regulated by TraR, a quorum-sensing activator. Quorum dependence requires TraM, which binds to and inactivates TraR. In this study, we showed that TraR and TraM form a 151-kDa stable complex composed of two TraR and two TraM dimers both in vitro and in vivo. When interacted with TraR bound to tra box DNA, wild-type TraM formed a nucleoprotein complex of 77 kDa composed of one dimer of each protein and DNA. The complex converted to the 151-kDa species with concomitant release of DNA with a half-life of 1.6 h. TraR in the complex still retained tightly bound autoinducer. From these results, we conclude that TraM interacts in a two-step process with DNA-TraR to form a large, stable antiactivation complex. Mutagenesis identified residues of TraR important for interacting with TraM. These residues form two patches, possibly defining the binding interfaces. Consistent with this interpretation, comparison of the trypsin-digested polypeptides of TraR and of TraM with that of the TraR-TraM complex revealed that a tryptic site at position 177 of TraR around these patches is accessible on free TraR but is blocked by TraM in the complex. From these genetic and structural considerations, we constructed three-dimensional models of the complex that shed light on the mechanism of TraM-mediated inhibition of TraR and on TraM-mediated destabilization of the TraR-DNA complex.

Published
2007

12. Dimerization properties of TraM, the antiactivator that modulates TraR-mediated quorum-dependent expression of the Ti plasmid tra genes

Author

Stephen K. Farrand, Audra J. Smyth, Shengchang Su, and Yinping Qin

Subjects
Serine, Ti plasmid, Biochemistry, Mutant protein, DNA-binding domain, Biology, Molecular Biology, Microbiology, Gene, In vitro, Function (biology), Cysteine
Abstract

Summary TraM, an 11.2 kDa antiactivator, modulates the acyl-homoserine lactone-mediated autoinduction of Ti plasmid conjugative transfer by interacting directly with TraR, the quorum-sensing transcriptional activator. Most antiactivators and antisigma factors examined to date act in dimer form. However, whether, and if so, how TraM dimerizes is unknown. Analyses based on a genetic assay using fusions of TraM to the λ cI DNA binding domain, and biochemical assays using chemical crosslinking and gel filtration chromatography showed that TraM forms homodimers. Although SDS-PAGE studies suggested that the lone cysteine residue at position 71 was involved in interprotomer disulfide-bridging in TraM, altering Cys-71 to a serine did not significantly affect dimerization or the antiactivator activity of this mutant protein when expressed at wild-type levels in vivo. Analysis of N-terminal, C-terminal, and internal deletion mutants of TraM identified two regions of the protein involved in dimerization; one located within a segment between residues 20 and 50, and the other located to a segment between residues 67 and 96. Both regions are required for formation of fully stable dimers. Analysis of the activity of these deletion mutants in vivo, and their ability to bind TraR and to disrupt TraR-DNA complexes in vitro, suggests that while the internal segment of the protein is required for dimerization, determinants located at the far C-terminus and beginning at between residues 10 and 20 at the N-terminus play a role in TraR binding and antiactivator function. When co-expressed with λ cI′::TraR fusions, wild-type TraM mediated quormone-independent dimerization of the transcriptional activator, suggesting that dimers of TraM can multimerize TraR.

Published
2004

13. Construction and characterization of stable, constitutively expressed, chromosomal green and red fluorescent transcriptional fusions in the select agents, Bacillus anthracis, Yersinia pestis, Burkholderia mallei, and Burkholderia pseudomallei

Author

Shengchang, Su, Hansraj, Bangar, Roland, Saldanha, Adin, Pemberton, Bruce, Aronow, Gary E, Dean, Thomas J, Lamkin, and Daniel J, Hassett

Subjects
Burkholderia pseudomallei, Virulence, Yersinia pestis, select agents, Green Fluorescent Proteins, Gene Expression, Bacterial Infections, Chromosomes, Bacterial, GFP, Burkholderia mallei, fluorescent tagging, Cell Line, Luminescent Proteins, Genes, Reporter, Bacillus anthracis, Macrophages, Alveolar, RFP, Humans, Original Research
Abstract

Here, we constructed stable, chromosomal, constitutively expressed, green and red fluorescent protein (GFP and RFP) as reporters in the select agents, Bacillus anthracis, Yersinia pestis, Burkholderia mallei, and Burkholderia pseudomallei. Using bioinformatic approaches and other experimental analyses, we identified P0253 and P1 as potent promoters that drive the optimal expression of fluorescent reporters in single copy in B. anthracis and Burkholderia spp. as well as their surrogate strains, respectively. In comparison, Y. pestis and its surrogate strain need two chromosomal copies of cysZK promoter (P2cysZK) for optimal fluorescence. The P0253-, P2cysZK-, and P1-driven GFP and RFP fusions were first cloned into the vectors pRP1028, pUC18R6KT-mini-Tn7T-Km, pmini-Tn7-gat, or their derivatives. The resultant constructs were delivered into the respective surrogates and subsequently into the select agent strains. The chromosomal GFP- and RFP-tagged strains exhibited bright fluorescence at an exposure time of less than 200 msec and displayed the same virulence traits as their wild-type parental strains. The utility of the tagged strains was proven by the macrophage infection assays and lactate dehydrogenase release analysis. Such strains will be extremely useful in high-throughput screens for novel compounds that could either kill these organisms, or interfere with critical virulence processes in these important bioweapon agents and during infection of alveolar macrophages.

Published
2014

14. Gallium disrupts iron uptake by intracellular and extracellular Francisella strains and exhibits therapeutic efficacy in a murine pulmonary infection model

Author

John S. Gunn, Bradley E. Britigan, Oyebode Olakanmi, Daniel J. Hassett, Shengchang Su, and Shilpa Soni

Subjects
Adult, Lung Diseases, Iron, Gallium, medicine.disease_cause, Antioxidants, Microbiology, Superoxide dismutase, Tularemia, Mice, Drug Resistance, Bacterial, medicine, Extracellular, Animals, Humans, Pharmacology (medical), Experimental Therapeutics, Francisella novicida, Francisella, Francisella tularensis, Pharmacology, chemistry.chemical_classification, Mice, Inbred BALB C, biology, Lactoferrin, Superoxide Dismutase, Macrophages, Hydrogen Peroxide, biology.organism_classification, medicine.disease, bacterial infections and mycoses, Catalase, Infectious Diseases, chemistry, Transferrin, biology.protein, Female, Gram-Negative Bacterial Infections
Abstract

Francisella tularensisrequires iron (Fe) for growth, but the biologic sources of Fe for this organism are largely unknown. We found thatFrancisellasp. growing in broth culture or within human macrophages can acquire Fe from the two major host Fe-binding proteins, lactoferrin (Lf) and transferrin (Tf). Fe acquisition is a potential target for novel therapies. Gallium (Ga) is a transition metal that interferes with cellular Fe metabolism by competing with Fe for uptake/utilization. Growth of eitherF. tularensislive vaccine strain (LVS) orFrancisella novicidawas inhibited by ≥2 μM Ga chelated to Tf or Lf, with GaLf being somewhat more potent.Francisellaspp. express two Fe-containing antioxidant enzymes, catalase (KatG) and Fe cofactored superoxide dismutase (FeSOD). Growth of LVS with 10 μM GaTf or GaLf led to a dramatic decrease in bacterial catalase activity and in FeSOD activity that was associated with an increased susceptibility to H2O2. Ga also protected mice from intranasal challenge withF. novicida. Whereas 100% of theF. novicida-infected mice died by day 9, 75% of the mice receiving Ga continued to survive to at least day 15. Thus, a single intranasal dose of Ga followed by daily intraperitoneal Ga at a dose tolerated by the animals resulted in prolonged survival. These data support the potential utility of Ga as a therapy forF. tularensisinfection of the lung.

Published
2009

15. Molecular basis of transcriptional antiactivation. TraM disrupts the TraR-DNA complex through stepwise interactions

Author

Yinping, Qin, Shengchang, Su, and Stephen K, Farrand

Subjects
DNA, Bacterial, DNA-Binding Proteins, Models, Molecular, Bacterial Proteins, Transcription, Genetic, Agrobacterium tumefaciens, Multiprotein Complexes, Plant Tumor-Inducing Plasmids, Carrier Proteins, Dimerization, Protein Binding
Abstract

Conjugative transfer of Agrobacterium Ti plasmids is regulated by TraR, a quorum-sensing activator. Quorum dependence requires TraM, which binds to and inactivates TraR. In this study, we showed that TraR and TraM form a 151-kDa stable complex composed of two TraR and two TraM dimers both in vitro and in vivo. When interacted with TraR bound to tra box DNA, wild-type TraM formed a nucleoprotein complex of 77 kDa composed of one dimer of each protein and DNA. The complex converted to the 151-kDa species with concomitant release of DNA with a half-life of 1.6 h. TraR in the complex still retained tightly bound autoinducer. From these results, we conclude that TraM interacts in a two-step process with DNA-TraR to form a large, stable antiactivation complex. Mutagenesis identified residues of TraR important for interacting with TraM. These residues form two patches, possibly defining the binding interfaces. Consistent with this interpretation, comparison of the trypsin-digested polypeptides of TraR and of TraM with that of the TraR-TraM complex revealed that a tryptic site at position 177 of TraR around these patches is accessible on free TraR but is blocked by TraM in the complex. From these genetic and structural considerations, we constructed three-dimensional models of the complex that shed light on the mechanism of TraM-mediated inhibition of TraR and on TraM-mediated destabilization of the TraR-DNA complex.

Published
2007

16. Lon protease of the alpha-proteobacterium Agrobacterium tumefaciens is required for normal growth, cellular morphology and full virulence

Author

Stephen K. Farrand, Gladys Alexandre, Bonnie B. Stephens, and Shengchang Su

Subjects
Kalanchoe, Hot Temperature, Protease La, Ultraviolet Rays, medicine.medical_treatment, Movement, Mutant, Blotting, Western, Virulence, Mutagenesis (molecular biology technique), medicine.disease_cause, Microbiology, medicine, Escherichia coli, Promoter Regions, Genetic, Plant Diseases, Sinorhizobium meliloti, Protease, Binding Sites, biology, Sequence Homology, Amino Acid, Chemotaxis, Genetic Complementation Test, Polysaccharides, Bacterial, Agrobacterium tumefaciens, Gene Expression Regulation, Bacterial, biology.organism_classification, Blotting, Northern, Molecular biology, Complementation, Plant Leaves, Mutagenesis, Insertional, RNA, Bacterial, bacteria, Gene Deletion
Abstract

The ATP-dependent Lon (La) protease is ubiquitous in nature and regulates a diverse set of physiological responses in bacteria. In this paper alonmutant of theα-proteobacteriumAgrobacterium tumefaciensC58 has been characterized. Unlikelonmutants ofEscherichia coli, thelonmutant ofA. tumefaciensgrows very slowly, is not filamentous and exhibits normal resistance to UV irradiation. The mutant retains motility and chemotaxis, produces apparently normal amounts of exopolysacchride, but displays severe defects in cell morphology, with 80 % of the mutant cells appearing Y-shaped. Lon protease ofA. tumefaciensshares high homology with its counterparts inE. coliand inSinorhizobium meliloti, and functionally complements anE. coli lonmutant for defects in morphology and RcsA-mediated regulation of capsular polysaccharide production. Mutations at sites of LonAtcorresponding to the ATP-binding site and the active site serine of theE. coliLon protease abolish complementation of phenotypes of theA. tumefaciensandE. coli lonmutants. The nucleotide sequence upstream ofA. tumefaciens loncontains an element similar to the consensusσ32heat-shock promoter ofE. coli. Northern and Western blot analyses indicated that expression oflonis induced by elevated temperature, albeit to a much lower level than that ofgroEL. Thelonmutant is highly attenuated for virulence, suggesting that Lon may be required for the proper expression, assembly or function of the VirB/D4-mediated T-DNA transfer system.

Published
2006

17. Dimerization properties of TraM, the antiactivator that modulates TraR-mediated quorum-dependent expression of the Ti plasmid tra genes

Author

Yinping, Qin, Audra J, Smyth, Shengchang, Su, and Stephen K, Farrand

Subjects
DNA, Bacterial, DNA-Binding Proteins, Dithiothreitol, 4-Butyrolactone, Bacterial Proteins, Agrobacterium tumefaciens, Conjugation, Genetic, Recombinant Fusion Proteins, Disulfides, Gene Expression Regulation, Bacterial, Plant Tumor-Inducing Plasmids, Protein Structure, Quaternary, Dimerization
Abstract

TraM, an 11.2 kDa antiactivator, modulates the acyl-homoserine lactone-mediated autoinduction of Ti plasmid conjugative transfer by interacting directly with TraR, the quorum-sensing transcriptional activator. Most antiactivators and antisigma factors examined to date act in dimer form. However, whether, and if so, how TraM dimerizes is unknown. Analyses based on a genetic assay using fusions of TraM to the lambda cI DNA binding domain, and biochemical assays using chemical crosslinking and gel filtration chromatography showed that TraM forms homodimers. Although SDS-PAGE studies suggested that the lone cysteine residue at position 71 was involved in interprotomer disulfide-bridging in TraM, altering Cys-71 to a serine did not significantly affect dimerization or the antiactivator activity of this mutant protein when expressed at wild-type levels in vivo. Analysis of N-terminal, C-terminal, and internal deletion mutants of TraM identified two regions of the protein involved in dimerization; one located within a segment between residues 20 and 50, and the other located to a segment between residues 67 and 96. Both regions are required for formation of fully stable dimers. Analysis of the activity of these deletion mutants in vivo, and their ability to bind TraR and to disrupt TraR-DNA complexes in vitro, suggests that while the internal segment of the protein is required for dimerization, determinants located at the far C-terminus and beginning at between residues 10 and 20 at the N-terminus play a role in TraR binding and antiactivator function. When co-expressed with lambda cI'::TraR fusions, wild-type TraM mediated quormone-independent dimerization of the transcriptional activator, suggesting that dimers of TraM can multimerize TraR.

Published
2004

18. Catalase (KatA) Plays a Role in Protection against Anaerobic Nitric Oxide in Pseudomonas aeruginosa

Author

Daniel J. Hassett, Melanie S. Rogers, Jeffrey J. Wilson, Thomas M. Makris, Harry K. Mahtani, Bradley D. VanderWielen, Cameron T. McDaniel, John D. Lipscomb, Shengchang Su, Michael J. Schurr, Qian Li, Warunya Panmanee, Rhett A. Kovall, Jack R. Lancaster, and Randall T. Irvin

Subjects
Bacterial Diseases, Transcription, Genetic, Mutant, lcsh:Medicine, Biochemistry, chemistry.chemical_compound, Medicine and Health Sciences, Anaerobiosis, lcsh:Science, Heme, 0303 health sciences, Multidisciplinary, Ecology, biology, Catalase, Enzymes, Bacterial Pathogens, Bacterial Biochemistry, Anti-Bacterial Agents, Infectious Diseases, Medical Microbiology, Pseudomonas aeruginosa, Nitrogen Oxides, Anaerobic bacteria, Anaerobic exercise, Research Article, Anaerobic respiration, Cellular respiration, Iron, Biophysics, Nitric Oxide, Microbiology, Microbial Ecology, 03 medical and health sciences, Pseudomonas Infections, Microbial Pathogens, Nitrites, 030304 developmental biology, Enzyme Kinetics, 030306 microbiology, lcsh:R, Biology and Life Sciences, Bacteriology, Gene Expression Regulation, Bacterial, Nitrite reductase, chemistry, Biofilms, Enzymology, biology.protein, lcsh:Q, Bacterial Biofilms
Abstract

Pseudomonas aeruginosa (PA) is a common bacterial pathogen, responsible for a high incidence of nosocomial and respiratory infections. KatA is the major catalase of PA that detoxifies hydrogen peroxide (H2O2), a reactive oxygen intermediate generated during aerobic respiration. Paradoxically, PA displays elevated KatA activity under anaerobic growth conditions where the substrate of KatA, H2O2, is not produced. The aim of the present study is to elucidate the mechanism underlying this phenomenon and define the role of KatA in PA during anaerobiosis using genetic, biochemical and biophysical approaches. We demonstrated that anaerobic wild-type PAO1 cells yielded higher levels of katA transcription and expression than aerobic cells, whereas a nitrite reductase mutant ΔnirS produced ∼50% the KatA activity of PAO1, suggesting that a basal NO level was required for the increased KatA activity. We also found that transcription of the katA gene was controlled, in part, by the master anaerobic regulator, ANR. A ΔkatA mutant and a mucoid mucA22 ΔkatA bacteria demonstrated increased sensitivity to acidified nitrite (an NO generator) in anaerobic planktonic and biofilm cultures. EPR spectra of anaerobic bacteria showed that levels of dinitrosyl iron complexes (DNIC), indicators of NO stress, were increased significantly in the ΔkatA mutant, and dramatically in a ΔnorCB mutant compared to basal levels of DNIC in PAO1 and ΔnirS mutant. Expression of KatA dramatically reduced the DNIC levels in ΔnorCB mutant. We further revealed direct NO-KatA interactions in vitro using EPR, optical spectroscopy and X-ray crystallography. KatA has a 5-coordinate high spin ferric heme that binds NO without prior reduction of the heme iron (K d ∼6 μM). Collectively, we conclude that KatA is expressed to protect PA against NO generated during anaerobic respiration. We proposed that such protective effects of KatA may involve buffering of free NO when potentially toxic concentrations of NO are approached.

Published
2014

19. A Statistical Framework for Improving Genomic Annotations of Prokaryotic Essential Genes

Author

Xiaodong Lin, Daniel J. Hassett, Long J. Lu, Shengchang Su, and Jingyuan Deng

Subjects
Transposable element, Gene Transposition, Clinical Research Design, Science, Gene prediction, Mutagenesis (molecular biology technique), Computational biology, Biostatistics, Biology, Computer Applications, Gene mapping, Genome Analysis Tools, Databases, Genetic, Molecular Cell Biology, Escherichia coli, Statistical Methods, Francisella tularensis, Gene, Genetics, Multidisciplinary, Statistics, Computational Biology, Molecular Sequence Annotation, Genomics, Mutagenesis, Essential gene, Computer Science, Web-Based Applications, DNA Transposable Elements, Medicine, Transposon mutagenesis, Transposons, Mathematics, Research Article
Abstract

Large-scale systematic analysis of gene essentiality is an important step closer toward unraveling the complex relationship between genotypes and phenotypes. Such analysis cannot be accomplished without unbiased and accurate annotations of essential genes. In current genomic databases, most of the essential gene annotations are derived from whole-genome transposon mutagenesis (TM), the most frequently used experimental approach for determining essential genes in microorganisms under defined conditions. However, there are substantial systematic biases associated with TM experiments. In this study, we developed a novel Poisson model-based statistical framework to simulate the TM insertion process and subsequently correct the experimental biases. We first quantitatively assessed the effects of major factors that potentially influence the accuracy of TM and subsequently incorporated relevant factors into the framework. Through iteratively optimizing parameters, we inferred the actual insertion events occurred and described each gene's essentiality on probability measure. Evaluated by the definite mapping of essential gene profile in Escherichia coli, our model significantly improved the accuracy of original TM datasets, resulting in more accurate annotations of essential genes. Our method also showed encouraging results in improving subsaturation level TM datasets. To test our model's broad applicability to other bacteria, we applied it to Pseudomonas aeruginosa PAO1 and Francisella tularensis novicida TM datasets. We validated our predictions by literature as well as allelic exchange experiments in PAO1. Our model was correct on six of the seven tested genes. Remarkably, among all three cases that our predictions contradicted the TM assignments, experimental validations supported our predictions. In summary, our method will be a promising tool in improving genomic annotations of essential genes and enabling large-scale explorations of gene essentiality. Our contribution is timely considering the rapidly increasing essential gene sets. A Webserver has been set up to provide convenient access to this tool. All results and source codes are available for download upon publication at http://research.cchmc.org/essentialgene/.

Published
2013

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