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9. Health and restructuring in Europe: National debates and common policy issues

Author

Kieselbach, T., Triomphe, C.E., Andronic, L., Armgarth, E., Bergstrom, O., Bagnara, S., Meyer, S. de, Dodic-Fifak, M., Jankauskus, R., Jefferys, S., Joling, C., Kuhn, K., Nielsen, K.M., Terzyska, I., Pelletier, J., Rodriguez, R., and Thomson, G.

Subjects
Restructuring, European frameworks, Case study reports, Gezondheid, Innovatie, Efficiency, Reorganisatie, Social convoy, Enterprise restructuring, National responses, Health, Collectief ontslag, Healthier change procedures
Abstract

Restructuring has become a daily practice in both private and public sectors in the EU. But often restructuring processes fail to produce the intended effects of secured or increased organizational profitability. On the contrary restructuring puts the physical and psychosocial health of all organizational members at risk. To limit the risks of enterprise restructuring effectively, several groups of actors at the individual, enterprise and societal level have to collaborate towards the implementation of healthier change procedures and to create a “social convoy” in occupational transitions for workers affected by dismissal. The European Expert Group HIRES on Health in Restructuring was coordinated by Prof. Dr. Thomas Kieselbach from the University of Bremen and supported by DG Employment of the European Commission. It presented with its report a concise overview of the effects of enterprise restructuring and the social frameworks and change procedures that should be considered for “healthier restructuring”. With its policy recommendations and the case studies of innovative approaches on a company and regional level the report addresses policy makers, governmental structures like labour inspectorates or federal institutes, unions, managers, occupational health and safety personnel, shareholders and workers alike. The public reception of the HIRES recommendations on Health in Restructuring was impressive all over Europe and across different institutions, stakeholders and professions. They were conceived before the economic crisis started but the development of the economies increased public awareness for the problems addressed in the HIRES report. It was disseminated on an international level within several scientific communities as well. The success of HIRES led to the follow-up project HIRES Plus (co-ordinated by Dr. Claude Emmanuel Triomphe (ASTREES, Paris) and Prof. Dr. Thomas Kieselbach, Bremen), which organized in 13 EU countries national workshops in order to increase awareness of main actors, discuss HIRES conclusions and to test them in the light of the national consultation process, discuss possible ways to include health as an issue when restructuring takes place and to develop networks at national and European levels.

Published
2010

10. Health in restructuring: innovative approaches and policy recommendations

Author

Kieselbach, T., Armgarth, E., Bagnara, S., Elo, A.L., Jefferys, S., Joling, C., Kuhn, K., Nielsen, K., Popma, J., Rogovsky, N., Sahler, B., Thomson, G., Triomphe, C.E., Widerszal-Bazyl, M., and dp14 Herschikking van bevoegdheden en verantwoordelijkheden ten aanzien van de kwaliteit van de arbeidskracht

Subjects
Restructuring, Health, Gezondheid, Innovatie, Collectief ontslag, Efficiency, Reorganisatie
Abstract

The health dimension of enterprise restructuring is a widely neglected area of research, intervention and public concern. Restructuring is taking place in every competing organisation and is therefore affecting all European societies. With restructuring is meant an organizational change that is much more significant than commonplace changes and affecting at least a whole organizational sector or an entire company in the forms of closure, downsizing, outsourcing, off shoring, sub-contracting, merging, delocalisation, internal job mobility or other complex internal reorganizations. Besides or through its effects on employment restructuring also has vast impact on the health of employees, organisations and communities. A concept of enterprise restructuring, that aims at preserving certain features of a European social model of employment relations with the new demands of a globalised competition has to take into account not only economic indicators of the health of a company but also the individual effects of restructuring on the workforce which will show a considerable long-term impact on the competitivity of the economy as well. This new understanding broadens the perspective from a uni-lateral shareholder perspective often pursued in the restructuring efforts to a more balanced view on the interests of all stakeholders involved in the full process of company adaptation and accommodation to the globalised economy with the goal of socially responsible restructuring.

Published
2009

14. Annulate lamellae play only a minor role in the storage of excess nucleoporins in Drosophila embryos

Author

Onischenko, Evgeny A, Gubanova, N V, Kieselbach, T, Kiseleva, E V, Hallberg, Einar, Onischenko, Evgeny A, Gubanova, N V, Kieselbach, T, Kiseleva, E V, and Hallberg, Einar

Abstract

The nuclear pore complexes (NPCs), multiprotein assemblies embedded in the nuclear envelope, conduct nucleo-cytoplasmic traffic of macromolecules. Mimics of NPCs, called annulate lamellae pore complexes (ALPCs), are usually found in cytoplasmic membranous stacks in oocytes and early embryonic cells. They are believed to constitute storage compartments for excess premade nucleoporins. To evaluate the extent to which ALPCs store nucleoporins in early embryonic cells we took advantage of syncytial Drosophila embryos, containing both AL and rapidly proliferating nuclei in the common cytoplasm. Electron microscopic morphometric analysis showed that the number of ALPCs did not decrease to compensate for the growing number of NPCs during syncytial development. We performed Western blot analysis to quantify seven different nucleoporins and analyzed their intraembryonal distribution by confocal microscopy and subcellular fractionation. Syncytial embryos contained a large maternally contributed stockpile of nucleoporins. However, even during interphases, only a small fraction of the excess nucleoporins was assembled into ALPCs, whereas the major fraction was soluble and contained at least one phosphorylated nucleoporin. We conclude that in Drosophila embryos ALPCs play only a minor role in storing the excess maternally contributed nucleoporins. Factors that may prevent nucleoporins from assembly into ALPCs are discussed.

Published
2004
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16. Proteome map of the chloroplast lumen of Arabidopsis thaliana

Author

Schubert, Maria, Petersson, Ulrika A, Haas, B J, Funk, C, Schröder, Wolfgang P, Kieselbach, T, Schubert, Maria, Petersson, Ulrika A, Haas, B J, Funk, C, Schröder, Wolfgang P, and Kieselbach, T

Abstract

The thylakoid membrane of the chloroplast is the center of oxygenic photosynthesis. To better understand the function of the luminal compartment within the thylakoid network, we have carried out a systematic characterization of the luminal thylakoid proteins from the model organism Arabidopsis thaliana. Our data show that the thylakoid lumen has its own specific proteome, of which 36 proteins were identified. Besides a large group of peptidyl-prolyl cis-trans isomerases and pro. teases, a family of novel PsbP domain proteins was found. An analysis of the luminal signal peptides showed that 19 of 36 luminal precursors were marked by a twin-arginine motif for import via the Tat pathway. To compare the model organism Arabidopsis with another typical higher plant, we investigated the proteome from the thylakoid lumen of spinach and found that the luminal proteins from both plants corresponded well. As a complement to our experimental investigation, we made a theoretical prediction of the luminal proteins from the whole Arabidopsis genome and estimated that the thylakoid lumen of the chloroplast contains similar to80 proteins.

Published
2002
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17. Human spermatid-specific thioredoxin-1 (Sptrx-1) is a two-domain protein with oxidizing activity

Author

Jimenez, A, Johansson, C, Ljung, J, Sagemark, Johan, Berndt, Kurt D, Ren, B, Tibbelin, G, Ladenstein, R, Kieselbach, T, Holmgren, A, Gustafsson, J A, Miranda-Vizuete, A, Jimenez, A, Johansson, C, Ljung, J, Sagemark, Johan, Berndt, Kurt D, Ren, B, Tibbelin, G, Ladenstein, R, Kieselbach, T, Holmgren, A, Gustafsson, J A, and Miranda-Vizuete, A

Abstract

Spermatid-specific thioredoxin-1 (Sptrx-1) is the first member of the thioredoxin family of proteins with a tissue-specific expression pattern, found exclusively in the tail of elongating spermatids and spermatozoa. We describe here further biochemical characterization of human Sptrx-1 protein structure and enzymatic activity. In gel filtration chromatography human Sptrx-1 eluates as a 400 kDa protein consistent with either an oligomeric form, not maintained by intermolecular disulfide bonding, and/or a highly asymmetrical structure. Analysis of circular dichroism spectra of fragments 1-360 and 361-469 and comparison to spectra of full-length Sptrx-1 supports a two-domain organization with a largely unstructured N-terminal domain and a folded thioredoxin-like C-terminal domain. Functionally, Sptrx-1 behaves as an oxidant in vitro when using selenite, but not oxidized glutathione, as electron acceptor. This oxidizing enzymatic activity suggests that Sptrx-1 might govern the stabilization (by disulfide cross-linking) of the different structures in the developing tail of spermatids and spermatozoa.

Published
2002
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20. Analysis of Schizosaccharomyces pombe mediator reveals a set of essential subunits conserved between yeast and metazoan cells

Author

Spåhr, H, Samuelsen, C O, Baraznenok, V, Ernest, I, Huylebroeck, D, Remacle, J E, Samuelsson, T, Kieselbach, T, Holmberg, S, Gustafsson, C M, Spåhr, H, Samuelsen, C O, Baraznenok, V, Ernest, I, Huylebroeck, D, Remacle, J E, Samuelsson, T, Kieselbach, T, Holmberg, S, and Gustafsson, C M

Abstract

Udgivelsesdato: 2001-Oct-9, With the identification of eight new polypeptides, we here complete the subunit characterization of the Schizosaccharomyces pombe RNA polymerase II holoenzyme. The complex contains homologs to all 10 essential gene products present in the Saccharomyces cerevisiae Mediator, but lacks clear homologs to any of the 10 S. cerevisiae components encoded by nonessential genes. S. pombe Mediator instead contains three unique components (Pmc2, -3, and -6), which lack homologs in other cell types. Presently, pmc2(+) and pmc3(+) have been shown to be nonessential genes. The data suggest that S. pombe and S. cerevisiae share an essential protein module, which associates with nonessential speciesspecific subunits. In support of this view, sequence analysis of the conserved yeast Mediator components Med4 and Med8 reveals sequence homology to the metazoan Mediator components Trap36 and Arc32. Therefore, 8 of 10 essential genes conserved between S. pombe and S. cerevisiae also have a metazoan homolog, indicating that an evolutionary conserved Mediator core is present in all eukaryotic cells. Our data suggest a closer functional relationship between yeast and metazoan Mediator than previously anticipated.

Published
2001

21. A peroxidase homologue and novel plastocyanin located by proteomics to the Arabidopsis chloroplast thylakoid lumen

Author

Kieselbach, T, Bystedt, Maria, Hynds, P, Robinson, C, Schröder, Wolfgang P, Kieselbach, T, Bystedt, Maria, Hynds, P, Robinson, C, and Schröder, Wolfgang P

Abstract

A study by two-dimensional electrophoresis showed that the soluble, lumenal fraction of Arabidopsis thaliana thylakoids can be resolved into 300 protein spots. After subtraction of low-intensity spots and accounting for low-level stromal contamination, the number of more abundant, lumenal proteins was estimated to be between 30 and 60. Two of these proteins have been identified: a novel plastocyanin that also was the predominant component of the total plastocyanin pool, and a putative ascorbate peroxidase. Import studies shamed that these proteins are routed to the thylakoid lumen by the Sec- and delta pH-dependent translocation pathways, respectively, In addition, novel isoforms of PsbO and PsbQ were identified.

Published
2000
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22. Unternehmensverantwortung bei Entlassungen: Berufliche Transitionsberatung zur Sicherung von Beschäftigungsfähigkeit.

Author

Badura, Bernhard, Schellschmidt, Henner, Vetter, Christian, Kieselbach, T., and Beelmann, G.

Abstract

Copyright of Fehlzeiten-Report 2005 is the property of Springer Nature / Books and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published
2006
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26. The thylakoid lumen of chloroplasts. Isolation and characterization.

Author

Kieselbach, T, Hagman, Andersson, B, and Schröder, W P

Abstract

The chloroplast compartment enclosed by the thylakoid membrane, the "lumen," is poorly characterized. The major aims of this work were to design a procedure for the isolation of the thylakoid lumen which could be generally used to characterize lumenal proteins. The preparation was a stepwise procedure in which thylakoid membranes were isolated from intact chloroplasts. Loosely associated thylakoid surface proteins were removed, and following Yeda press fragmentation the lumenal content was recovered in the supernatant following centrifugation. The purity and yield of lumenal proteins were determined using appropriate marker proteins specific for the different chloroplast compartments. Quantitative immunoblot analyses showed that the recovery of soluble lumenal proteins was 60-65% (as judged by the presence of plastocyanin), whereas contamination with stromal enzymes was less than 1% (ribulose-bisphosphate carboxylase) and negligible for thylakoid integral membrane proteins (D1 protein). Approximately 25 polypeptides were recovered in the lumenal fraction, of which several were identified for the first time. Enzymatic measurements and/or amino-terminal sequencing revealed the presence of proteolytic activities, violaxanthin de-epoxidase, polyphenol oxidase, peroxidase, as well as a novel prolyl cis/trans-isomerase.

Published
1998

27. Comparative proteome analysis of Saccharomyces cerevisiae: A global overview of in vivo targets of the yeast activator protein 1

Author

Jun He, Kieselbach Thomas, and Jönsson Leif J

Subjects
Yap1, Saccharomyces cerevisiae, Transcription factor, Stress response, Proteome, Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background The activity of the yeast activator protein 1 (Yap1p) increases under stress conditions, which leads to enhanced transcription of a number of genes encoding protective enzymes or other proteins. To obtain a global overview of changes in expression of Yap1p-targeted proteins, we compared a Yap1p-overexpressing transformant with a control transformant by triplicate analysis of the proteome using two-dimensional gel electrophoresis (2-DE). Proteins of interest were identified using MALDI-MS or LC-MS/MS. Results The relative quantities of 55 proteins were elevated significantly upon overexpression of Yap1p, and most of these proteins were found to have a Yap1p-binding site upstream of their coding sequences. Interestingly, the main metabolic enzymes in the glycolysis and pyruvate-ethanol pathways showed a significant increase in the Yap1p-overexpressing transformant. Moreover, a comparison of our proteome data with transcriptome data from the literature suggested which proteins were regulated at the level of the proteome, and which proteins were regulated at the level of the transcriptome. Eight proteins involved in stress response, including seven heat-shock and chaperone proteins, were significantly more abundant in the Yap1p-overexpressing transformant. Conclusions We have investigated the general protein composition in Yap1p-overexpressing S. cerevisiae using proteomic techniques, and quantified the changes in the expression of the potential Yap1p-targeted proteins. Identification of the potential Yap1p targets and analysis of their role in cellular processes not only give a global overview of the ubiquitous cellular changes elicited by Yap1p, but also provide the framework for understanding the mechanisms behind Yap1p-regulated stress response in yeast.

Published
2012
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28. Enzyme production by filamentous fungi: analysis of the secretome of Trichoderma reesei grown on unconventional carbon source

Author

Kieselbach Thomas, Jun He, and Jönsson Leif J

Subjects
Microbiology, QR1-502
Abstract

Abstract Background Spent hydrolysates from bioethanolic fermentation processes based on agricultural residues have potential as an abundant and inexpensive source of pentose sugars and acids that could serve as nutrients for industrial enzyme-producing microorganisms, especially filamentous fungi. However, the enzyme mixtures produced in such media are poorly defined. In this study, the secretome of Trichoderma reesei Rut C-30 grown either on a spent hydrolysate model medium (SHMM) or on a lactose-based standard medium (LBSM) was explored using proteomics. Results Our results show that both the SHMM and LBSM serve as excellent growth media for T. reesei Rut C-30. In total, 52 protein spots on 2-D gels were identified by using matrix-assisted laser desorption/ionization mass spectrometry (MALDI-MS) and electrospray ionization liquid chromatography tandem mass spectrometry (ESI-LC MS/MS). As expected, a considerable number of the identified proteins were related to the degradation of lignocellulosic biomass. The enzyme production profiles in the two media were similar, but β-glucosidase and β-galactosidase were only produced in LBSM. The main cellobiohydrolases (Cel7A/Cel6A) and endoglucanases (Cel7B/Cel5A) were identified in both media and the cellobiohydrolases, i.e. Cel7A and Cel6A, were the most abundant cellulolytic enzymes. Moreover, both media can also serve as a potent inducer of xylanolytic enzymes. Several key enzymes involved in sugar assimilation and regulation of cellulase formation were identified, and were found to be differentially expressed in the two growth media. Conclusions This study not only provides a catalogue of the prevalent proteins secreted by T. reesei in the two media, but the results also suggest that production of hydrolytic enzymes using unconventional carbon sources, such as components in spent hydrolysates, deserves further attention in the future.

Published
2011
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29. Protein differences between human trapezius and vastus lateralis muscles determined with a proteomic approach

Author

Kieselbach Thomas, Malm Christer, Hellström Fredrik, Hadrévi Jenny, and Pedrosa-Domellöf Fatima

Subjects
Diseases of the musculoskeletal system, RC925-935
Abstract

Abstract Background The trapezius muscle is a neck muscle that is susceptible to chronic pain conditions associated with repetitive tasks, commonly referred to as chronic work-related myalgia, hence making the trapezius a muscle of clinical interest. To provide a basis for further investigations of the proteomic traits of the trapezius muscle in disease, two-dimensional difference gel electrophoresis (2D-DIGE) was performed on the healthy trapezius using vastus lateralis as a reference. To obtain as much information as possible from the vast proteomic data set, both one-way ANOVA, with and without false discovery rate (FDR) correlation, and partial least square projection to latent structures with discriminant analysis (PLS-DA) were combined to compare the outcome of the analysis. Results The trapezius and vastus lateralis showed significant differences in metabolic, contractile and regulatory proteins, with different results depending on choice of statistical approach and pre-processing technique. Using the standard method, FDR correlated one-way ANOVA, 42 protein spots differed significantly in abundance between the two muscles. Complementary analysis using immunohistochemistry and western blot confirmed the results from the 2D-DIGE analysis. Conclusions The proteomic approach used in the present study combining 2D-DIGE and multivariate modelling provided a more comprehensive comparison of the protein profiles of the human trapezius and vastus lateralis muscle, than previously possible to obtain with immunohistochemistry or SDS-PAGE alone. Although 2D-DIGE has inherent limitations it is particularly useful to comprehensively screen for important structural and metabolic proteins, and appears to be a promising tool for future studies of patients suffering from chronic work related myalgia or other muscle diseases.

Published
2011
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30. The submerged economy in Greece, Italy and Spain

Author

Bayetakou D., Espluga J., Lemkow L., Papakostantinu S., Soku K., BORGHI, VANDO, CHICCHI, FEDERICO, LA ROSA, MICHELE, KIESELBACH T. ET AL., Bayetakou D., Borghi V., Chicchi F., Espluga J., La Rosa M., Lemkow L., Papakostantinu S., and Soku K

Subjects
UNEMPLOYMENT, YOUTH, SOCIAL EXCLUSION, SUBMERGED ECONOMY
Abstract

A comparison or the relationships between youth unemployment and submerged economy in different Eu countries.

Published
2008

31. Italy

Author

BORGHI, VANDO, CHICCHI, FEDERICO, LA ROSA, MICHELE, KIESELBACH T. ET AL., Borghi, Vando, Chicchi, Federico, and LA ROSA, Michele

Subjects
UNEMPLOYMENT, VULNERABILITY, YOUTH, SOCIAL EXCLUSION
Abstract

The chapter is part of an international research project about youth unemployment and social exclusion. The Italian case is here specifically addressed.

Published
2008

32. Multi-laboratory experiment PME11 for the standardization of phosphoproteome analysis.

Author

Colomé N, Abian J, Aloria K, Arizmendi JM, Barceló-Batllori S, Braga-Lagache S, Burlet-Schiltz O, Carrascal M, Casal JI, Chicano-Gálvez E, Chiva C, Clemente LF, Elortza F, Estanyol JM, Fernandez-Irigoyen J, Fernández-Puente P, Fidalgo MJ, Froment C, Fuentes M, Fuentes-Almagro C, Gay M, Hainard A, Heller M, Hernández ML, Ibarrola N, Iloro I, Kieselbach T, Lario A, Locard-Paulet M, Marina-Ramírez A, Martín L, Morato-López E, Muñoz J, Navajas R, Odena MA, Odriozola L, de Oliveira E, Paradela A, Pasquarello C, de Los Rios V, Ruiz-Romero C, Sabidó E, Sánchez Del Pino M, Sancho J, Santamaría E, Schaeffer-Reiss C, Schneider J, de la Torre C, Valero ML, Vilaseca M, Wu S, Wu L, Ximénez de Embún P, Canals F, and Corrales FJ

Subjects
Laboratories, Phosphoproteins analysis, Phosphorylation, Reference Standards, Reproducibility of Results, Proteome analysis, Proteomics methods
Abstract

Global analysis of protein phosphorylation by mass spectrometry proteomic techniques has emerged in the last decades as a powerful tool in biological and biomedical research. However, there are several factors that make the global study of the phosphoproteome more challenging than measuring non-modified proteins. The low stoichiometry of the phosphorylated species and the need to retrieve residue specific information require particular attention on sample preparation, data acquisition and processing to ensure reproducibility, qualitative and quantitative robustness and ample phosphoproteome coverage in phosphoproteomic workflows. Aiming to investigate the effect of different variables in the performance of proteome wide phosphoprotein analysis protocols, ProteoRed-ISCIII and EuPA launched the Proteomics Multicentric Experiment 11 (PME11). A reference sample consisting of a yeast protein extract spiked in with different amounts of a phosphomix standard (Sigma/Merck) was distributed to 31 laboratories around the globe. Thirty-six datasets from 23 laboratories were analyzed. Our results indicate the suitability of the PME11 reference sample to benchmark and optimize phosphoproteomics strategies, weighing the influence of different factors, as well as to rank intra and inter laboratory performance., (Copyright © 2021 The Authors. Published by Elsevier B.V. All rights reserved.)

Published
2022
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33. Extra-plastidial degradation of chlorophyll and photosystem I in tobacco leaves involving 'senescence-associated vacuoles'.

Author

Gomez FM, Carrión CA, Costa ML, Desel C, Kieselbach T, Funk C, Krupinska K, and Guiamet J

Subjects
Aging, Cellular Senescence, Darkness, Plastids metabolism, Proteolysis, Chlorophyll metabolism, Chloroplasts metabolism, Photosystem I Protein Complex metabolism, Plant Leaves metabolism, Plant Proteins metabolism, Nicotiana metabolism, Vacuoles metabolism
Abstract

Chlorophyll (Chl) loss is the main visible symptom of senescence in leaves. The initial steps of Chl degradation operate within the chloroplast, but the observation that 'senescence-associated vacuoles' (SAVs) contain Chl raises the question of whether SAVs might also contribute to Chl breakdown. Previous confocal microscope observations (Martínez et al., 2008) showed many SAVs containing Chl. Isolated SAVs contained Chl a and b (with a Chl a/b ratio close to 5) and lower levels of chlorophyllide a. Pheophytin a and pheophorbide a were formed after the incubation of SAVs at 30°C in darkness, suggesting the presence of Chl-degrading activities in SAVs. Chl in SAVs was bound to a number of 'green bands'. In the most abundant green band of SAVs, Western blot analysis showed the presence of photosystem I (PSI) Chl-binding proteins, including the PsaA protein of the PSI reaction center and the apoproteins of the light-harvesting complexes (Lhca 1-4). This was confirmed by: (i) measurements of 77-K fluorescence emission spectra showing a single emission peak at around 730 nm in SAVs; (ii) mass spectrometry of the most prominent green band with the slowest electrophoretic mobility; and (iii) immunofluorescence detection of PsaA in SAVs observed through confocal microscopy. Incubation of SAVs at 30°C in darkness caused a steady decrease in PsaA levels. Overall, these results indicate that SAVs may be involved in the degradation of PSI proteins and their associated chlorophylls during the senescence of leaves., (© 2019 The Authors The Plant Journal © 2019 John Wiley & Sons Ltd.)

Published
2019
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34. Proteomic analysis of the phycobiliprotein antenna of the cryptophyte alga Guillardia theta cultured under different light intensities.

Author

Kieselbach T, Cheregi O, Green BR, and Funk C

Subjects
Acclimatization radiation effects, Amino Acid Sequence, Cells, Cultured, Cryptophyta growth & development, Light-Harvesting Protein Complexes chemistry, Models, Genetic, Models, Molecular, Photosynthesis radiation effects, Phycobiliproteins chemistry, Plant Proteins chemistry, Protein Subunits chemistry, Protein Subunits metabolism, Spectrometry, Fluorescence, Temperature, Cryptophyta metabolism, Cryptophyta radiation effects, Light, Light-Harvesting Protein Complexes metabolism, Phycobiliproteins metabolism, Plant Proteins metabolism, Proteomics methods
Abstract

Plants and algae have developed various light-harvesting mechanisms for optimal delivery of excitation energy to the photosystems. Cryptophyte algae have evolved a novel soluble light-harvesting antenna utilizing phycobilin pigments to complement the membrane-intrinsic Chl a/c-binding LHC antenna. This new antenna consists of the plastid-encoded β-subunit, a relic of the ancestral phycobilisome, and a novel nuclear-encoded α-subunit unique to cryptophytes. Together, these proteins form the active α 1 β·α 2 β-tetramer. In all cryptophyte algae investigated so far, the α-subunits have duplicated and diversified into a large gene family. Although there is transcriptional evidence for expression of all these genes, the X-ray structures determined to date suggest that only two of the α-subunit genes might be significantly expressed at the protein level. Using proteomics, we show that in phycoerythrin 545 (PE545) of Guillardia theta, the only cryptophyte with a sequenced genome, all 20 α-subunits are expressed when the algae grow under white light. The expression level of each protein depends on the intensity of the growth light, but there is no evidence for a specific light-dependent regulation of individual members of the α-subunit family under the growth conditions applied. GtcpeA10 seems to be a special member of the α-subunit family, because it consists of two similar N- and C-terminal domains, which likely are the result of a partial tandem gene duplication. The proteomics data of this study have been deposited to the ProteomeXchange Consortium and have the dataset identifiers PXD006301 and 10.6019/PXD006301.

Published
2018
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35. Dataset of the proteome of purified outer membrane vesicles from the human pathogen Aggregatibacter actinomycetemcomintans .

Author

Kieselbach T and Oscarsson J

Abstract

The Gram-negative bacterium Aggregatibacter actinomycetemcomitans is an oral and systemic pathogen, which is linked to aggressive forms of periodontitis and can be associated with endocarditis. The outer membrane vesicles (OMVs) of this species contain effector proteins such as cytolethal distending toxin (CDT) and leukotoxin (LtxA), which they can deliver into human host cells. The OMVs can also activate innate immunity through NOD1- and NOD2-active pathogen-associated molecular patterns. This dataset provides a proteome of highly purified OMVs from A. actinomycetemcomitans serotype e strain 173. The experimental data do not only include the raw data of the LC-MS/MS analysis of four independent preparations of purified OMVs but also the mass lists of the processed data and the Mascot.dat files from the database searches. In total 501 proteins are identified, of which 151 are detected in at least three of four independent preparations. In addition, this dataset contains the COG definitions and the predicted subcellular locations (PSORTb 3.0) for the entire genome of A. actinomycetemcomitans serotype e strain SC1083, which is used for the evaluation of the LC-MS/MS data. These data are deposited in ProteomeXchange in the public dataset PXD002509. In addition, a scientific interpretation of this dataset by Kieselbach et al. (2015) [2] is available at http://dx.doi.org/10.1371/journal.pone.0138591.

Published
2016
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36. Proteomics of Aggregatibacter actinomycetemcomitans Outer Membrane Vesicles.

Author

Kieselbach T, Zijnge V, Granström E, and Oscarsson J

Subjects
Humans, Proteomics, Aggregatibacter actinomycetemcomitans metabolism, Bacterial Outer Membrane Proteins metabolism, Periodontitis microbiology, Secretory Vesicles metabolism
Abstract

Aggregatibacter actinomycetemcomitans is an oral and systemic pathogen associated with aggressive forms of periodontitis and with endocarditis. Outer membrane vesicles (OMVs) released by this species have been demonstrated to deliver effector proteins such as cytolethal distending toxin (CDT) and leukotoxin (LtxA) into human host cells and to act as triggers of innate immunity upon carriage of NOD1- and NOD2-active pathogen-associated molecular patterns (PAMPs). To improve our understanding of the pathogenicity-associated functions that A. actinomycetemcomitans exports via OMVs, we studied the proteome of density gradient-purified OMVs from a rough-colony type clinical isolate, strain 173 (serotype e) using liquid chromatography-tandem mass spectrometry (LC-MS/MS). This analysis yielded the identification of 151 proteins, which were found in at least three out of four independent experiments. Data are available via ProteomeXchange with identifier PXD002509. Through this study, we not only confirmed the vesicle-associated release of LtxA, and the presence of proteins, which are known to act as immunoreactive antigens in the human host, but we also identified numerous additional putative virulence-related proteins in the A. actinomycetemcomitans OMV proteome. The known and putative functions of these proteins include immune evasion, drug targeting, and iron/nutrient acquisition. In summary, our findings are consistent with an OMV-associated proteome that exhibits several offensive and defensive functions, and they provide a comprehensive basis to further disclose roles of A. actinomycetemcomitans OMVs in periodontal and systemic disease.

Published
2015
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37. Isolation of monomeric photosystem II that retains the subunit PsbS.

Author

Haniewicz P, De Sanctis D, Büchel C, Schröder WP, Loi MC, Kieselbach T, Bochtler M, and Piano D

Subjects
Chlorophyll metabolism, Electrophoresis, Polyacrylamide Gel, Light-Harvesting Protein Complexes metabolism, Mass Spectrometry, Photosynthesis, Photosystem II Protein Complex metabolism, Plant Proteins metabolism, Protein Subunits, Thylakoids metabolism, Nicotiana metabolism, Light-Harvesting Protein Complexes isolation & purification, Oxygen metabolism, Photosystem II Protein Complex isolation & purification, Nicotiana physiology
Abstract

Photosystem II has been purified from a transplastomic strain of Nicotiana tabacum according to two different protocols. Using the procedure described in Piano et al. (Photosynth Res 106:221-226, 2010) it was possible to isolate highly active PSII composed of monomers and dimers but depleted in their PsbS protein content. A "milder" procedure than the protocol reported by Fey et al. (Biochim Biophys Acta 1777:1501-1509, 2008) led to almost exclusively monomeric PSII complexes which in part still bind the PsbS protein. This finding might support a role for PSII monomers in higher plants.

Published
2013
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38. Oxidative folding in chloroplasts.

Author

Kieselbach T

Subjects
Arabidopsis chemistry, Arabidopsis cytology, Arabidopsis metabolism, Disulfides metabolism, Oxidation-Reduction, Chloroplast Proteins chemistry, Chloroplast Proteins metabolism, Chloroplasts chemistry, Chloroplasts metabolism, Protein Folding
Abstract

Significance: Disulfide-bonded proteins in chloroplasts from green plants exist in the envelope and the thylakoid membrane, and in the stroma and the lumen. The formation of disulfide bonds in proteins is referred to as oxidative folding and is linked to the import and folding of chloroplast proteins as well as the assembly and repair of thylakoid complexes. It is also important in the redox regulation of enzymes and signal transfer., Recent Advances: Green-plant chloroplasts contain enzymes that can form and isomerize disulfide bonds in proteins. In Arabidopsis thaliana, four proteins are identified that are relevant for the catalysis of disulfide bond formation in chloroplast proteins. The proteins' low quantum yield of Photosystem II 1 (LQY1, At1g75690) and snowy cotyledon 2 (SCO2, At3g19220) exhibits protein disulfide isomerase activity and is suggested to function in the assembly and repair of Photosystem II (PSII), and the biogenesis of thylakoids in cotyledons, respectively. The thylakoid-located Lumen thiol oxidoreductase 1 (LTO1, At4g35760) can catalyze the formation of the disulfide bond of the extrinsic PsbO protein of PSII. In addition, the stroma-located protein disulfide isomerase PDIL1-3 (At3g54960) may have a role in oxidative folding., Critical Issues: Research on oxidative folding in chloroplasts plants is in an early stage and little is known about the mechanisms of disulfide bond formation in chloroplast proteins., Future Directions: The close link between the import and folding of chloroplast proteins suggests that Hsp93, a component of the inner envelope's import apparatus, may have co-chaperones that can catalyze disulfide bond formation in newly imported proteins.

Published
2013
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39. Purification, crystallization and preliminary X-ray analysis of PPD6, a PsbP-domain protein from Arabidopsis thaliana.

Author

Hall M, Kieselbach T, Sauer UH, and Schröder WP

Subjects
Crystallization, Crystallography, X-Ray, Arabidopsis enzymology, Arabidopsis Proteins chemistry
Abstract

The PsbP protein is an extrinsic component of photosystem II that together with PsbO and PsbQ forms the thylakoid lumenal part of the oxygen-evolving complex in higher plants. In addition to PsbP, the thylakoid lumen contains two PsbP-like proteins (PPLs) and six PsbP-domain proteins (PPDs). While the functions of the PsbP-like proteins PPL1 and PPL2 are currently under investigation, the function of the PsbP-domain proteins still remains completely unknown. PPD6 is unique among the PsbP family of proteins in that it contains a conserved disulfide bond which can be reduced in vitro by thioredoxin. The crystal structure determination of the PPD6 protein has been initiated in order to elucidate its function and to gain deeper insights into redox-regulation pathways in the thylakoid lumen. PPD6 has been expressed, purified and crystallized and preliminary X-ray diffraction data have been collected. The crystals belonged to space group P2(1), with unit-cell parameters a = 47.0, b = 64.3, c = 62.0 Å, β = 94.2°, and diffracted to a maximum d-spacing of 2.1 Å., (© 2012 International Union of Crystallography)

Published
2012
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40. Boosting the globalization of plant proteomics through INPPO: current developments and future prospects.

Author

Agrawal GK, Sarkar A, Agrawal R, Ndimba BK, Tanou G, Dunn MJ, Kieselbach T, Cramer R, Wienkoop S, Chen S, Rafudeen MS, Deswal R, Barkla BJ, Weckwerth W, Heazlewood JL, Renaut J, Job D, Chakraborty N, and Rakwal R

Subjects
Crops, Agricultural, International Cooperation, Internationality, Organizational Objectives, Organizations, Nonprofit, Plant Proteins, Proteomics trends
Abstract

The International Plant Proteomics Organization (INPPO) is a non-profit-organization consisting of people who are involved or interested in plant proteomics. INPPO is constantly growing in volume and activity, which is mostly due to the realization among plant proteomics researchers worldwide for the need of such a global platform. Their active participation resulted in the rapid growth within the first year of INPPO's official launch in 2011 via its website (www.inppo.com) and publication of the 'Viewpoint paper' in a special issue of PROTEOMICS (May 2011). Here, we will be highlighting the progress achieved in the year 2011 and the future targets for the year 2012 and onwards. INPPO has achieved a successful administrative structure, the Core Committee (CC; composed of President, Vice-President, and General Secretaries), Executive Council (EC), and General Body (GB) to achieve INPPO objectives. Various committees and subcommittees are in the process of being functionalized via discussion amongst scientists around the globe. INPPO's primary aim to popularize the plant proteomics research in biological sciences has also been recognized by PROTEOMICS where a section dedicated to plant proteomics has been introduced starting January 2012, following the very first issue of this journal devoted to plant proteomics in May 2011. To disseminate organizational activities to the scientific community, INPPO has launched a biannual (in January and July) newsletter entitled 'INPPO Express: News & Views' with the first issue published in January 2012. INPPO is also planning to have several activities in 2012, including programs within the Education Outreach committee in different countries, and the development of research ideas and proposals with priority on crop and horticultural plants, while keeping tight interactions with proteomics programs on model plants such as Arabidopsis thaliana, rice, and Medicago truncatula. Altogether, the INPPO progress and upcoming activities are because of immense support, dedication, and hard work of all members of the INPPO community, and also due to the wide encouragement and support from the communities (scientific and non-scientific)., (Copyright © 2012 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published
2012
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41. Proteomics of protein secretion by Aggregatibacter actinomycetemcomitans.

Author

Zijnge V, Kieselbach T, and Oscarsson J

Subjects
Humans, Intracellular Space metabolism, Pasteurellaceae cytology, Pasteurellaceae pathogenicity, Protein Transport, Bacterial Proteins metabolism, Pasteurellaceae metabolism, Proteomics
Abstract

The extracellular proteome (secretome) of periodontitis-associated bacteria may constitute a major link between periodontitis and systemic diseases. To obtain an overview of the virulence potential of Aggregatibacter actinomycetemcomitans, an oral and systemic human pathogen implicated in aggressive periodontitis, we used a combined LC-MS/MS and bioinformatics approach to characterize the secretome and protein secretion pathways of the rough-colony serotype a strain D7S. LC-MS/MS revealed 179 proteins secreted during biofilm growth. Further to confirming the release of established virulence factors (e.g. cytolethal distending toxin [CDT], and leukotoxin [LtxA]), we identified additional putative virulence determinants in the secretome. These included DegQ, fHbp, LppC, Macrophage infectivity protein (MIP), NlpB, Pcp, PotD, TolB, and TolC. This finding indicates that the number of extracellular virulence-related proteins is much larger than previously demonstrated, which was also supported by in silico analysis of the strain D7S genome. Moreover, our LC-MS/MS and in silico data revealed that at least Type I, II, and V secretion are actively used to excrete proteins directly into the extracellular space, or via two-step pathways involving the Sec/Tat systems for transport across the inner membrane, and outer membrane factors, secretins and auto-transporters, respectively for delivery across the outer membrane. Taken together, our results provide a molecular basis for further elucidating the role of A. actinomycetemcomitans in periodontal and systemic diseases.

Published
2012
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42. Degradation of PsbO by the Deg protease HhoA Is thioredoxin dependent.

Author

Roberts IN, Lam XT, Miranda H, Kieselbach T, and Funk C

Subjects
Amino Acid Sequence, Bacterial Proteins chemistry, Base Sequence, Blotting, Western, DNA Primers, Electrophoresis, Polyacrylamide Gel, Kinetics, Mass Spectrometry, Molecular Sequence Data, Proteolysis, Recombinant Proteins metabolism, Subcellular Fractions enzymology, Substrate Specificity, Bacterial Proteins metabolism, Synechocystis metabolism, Thioredoxins metabolism
Abstract

The widely distributed members of the Deg/HtrA protease family play an important role in the proteolysis of misfolded and damaged proteins. Here we show that the Deg protease rHhoA is able to degrade PsbO, the extrinsic protein of the Photosystem II (PSII) oxygen-evolving complex in Synechocystis sp. PCC 6803 and in spinach. PsbO is known to be stable in its oxidized form, but after reduction by thioredoxin it became a substrate for recombinant HhoA (rHhoA). rHhoA cleaved reduced eukaryotic (specifically, spinach) PsbO at defined sites and created distinct PsbO fragments that were not further degraded. As for the corresponding prokaryotic substrate (reduced PsbO of Synechocystis sp. PCC 6803), no PsbO fragments were observed. Assembly to PSII protected PsbO from degradation. For Synechocystis sp. PCC 6803, our results show that HhoA, HhoB, and HtrA are localized in the periplasma and/or at the thylakoid membrane. In agreement with the idea that PsbO could be a physiological substrate for Deg proteases, part of the cellular fraction of the three Deg proteases of Synechocystis sp. PCC 6803 (HhoA, HhoB, and HtrA) was detected in the PSII-enriched membrane fraction.

Published
2012
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43. Drosophila Nora virus capsid proteins differ from those of other picorna-like viruses.

Author

Ekström JO, Habayeb MS, Srivastava V, Kieselbach T, Wingsle G, and Hultmark D

Subjects
Animals, Capsid Proteins isolation & purification, Genes, Viral, Mass Spectrometry, Molecular Sequence Data, Open Reading Frames, Picornaviridae isolation & purification, RNA, Viral genetics, Sequence Analysis, DNA, Capsid Proteins chemistry, Capsid Proteins genetics, Drosophila melanogaster virology, Picornaviridae chemistry, Picornaviridae genetics
Abstract

The recently discovered Nora virus from Drosophila melanogaster is a single-stranded RNA virus. Its published genomic sequence encodes a typical picorna-like cassette of replicative enzymes, but no capsid proteins similar to those in other picorna-like viruses. We have now done additional sequencing at the termini of the viral genome, extending it by 455 nucleotides at the 5' end, but no more coding sequence was found. The completeness of the final 12,333-nucleotide sequence was verified by the production of infectious virus from the cloned genome. To identify the capsid proteins, we purified Nora virus particles and analyzed their proteins by mass spectrometry. Our results show that the capsid is built from three major proteins, VP4A, B and C, encoded in the fourth open reading frame of the viral genome. The viral particles also contain traces of a protein from the third open reading frame, VP3. VP4A and B are not closely related to other picorna-like virus capsid proteins in sequence, but may form similar jelly roll folds. VP4C differs from the others and is predicted to have an essentially α-helical conformation. In a related virus, identified from EST database sequences from Nasonia parasitoid wasps, VP4C is encoded in a separate open reading frame, separated from VP4A and B by a frame-shift. This opens a possibility that VP4C is produced in non-equimolar quantities. Altogether, our results suggest that the Nora virus capsid has a different protein organization compared to the order Picornavirales., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published
2011
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44. Enzyme production by filamentous fungi: analysis of the secretome of Trichoderma reesei grown on unconventional carbon source.

Author

Jun H, Kieselbach T, and Jönsson LJ

Subjects
Electrophoresis, Gel, Two-Dimensional, Extracellular Space chemistry, Extracellular Space genetics, Fungal Proteins chemistry, Fungal Proteins genetics, Protein Transport, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Trichoderma chemistry, Trichoderma growth & development, Trichoderma metabolism, Carbon metabolism, Extracellular Space enzymology, Fungal Proteins metabolism, Trichoderma enzymology
Abstract

Background: Spent hydrolysates from bioethanolic fermentation processes based on agricultural residues have potential as an abundant and inexpensive source of pentose sugars and acids that could serve as nutrients for industrial enzyme-producing microorganisms, especially filamentous fungi. However, the enzyme mixtures produced in such media are poorly defined. In this study, the secretome of Trichoderma reesei Rut C-30 grown either on a spent hydrolysate model medium (SHMM) or on a lactose-based standard medium (LBSM) was explored using proteomics., Results: Our results show that both the SHMM and LBSM serve as excellent growth media for T. reesei Rut C-30. In total, 52 protein spots on 2-D gels were identified by using matrix-assisted laser desorption/ionization mass spectrometry (MALDI-MS) and electrospray ionization liquid chromatography tandem mass spectrometry (ESI-LC MS/MS). As expected, a considerable number of the identified proteins were related to the degradation of lignocellulosic biomass. The enzyme production profiles in the two media were similar, but β-glucosidase and β-galactosidase were only produced in LBSM. The main cellobiohydrolases (Cel7A/Cel6A) and endoglucanases (Cel7B/Cel5A) were identified in both media and the cellobiohydrolases, i.e. Cel7A and Cel6A, were the most abundant cellulolytic enzymes. Moreover, both media can also serve as a potent inducer of xylanolytic enzymes. Several key enzymes involved in sugar assimilation and regulation of cellulase formation were identified, and were found to be differentially expressed in the two growth media., Conclusions: This study not only provides a catalogue of the prevalent proteins secreted by T. reesei in the two media, but the results also suggest that production of hydrolytic enzymes using unconventional carbon sources, such as components in spent hydrolysates, deserves further attention in the future.

Published
2011
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45. Clustering of MS spectra for improved protein identification rate and screening for protein variants and modifications by MALDI-MS/MS.

Author

Granlund I, Kieselbach T, Alm R, Schröder WP, and Emanuelsson C

Subjects
Arabidopsis Proteins chemistry, Arabidopsis Proteins isolation & purification, Chloroplasts chemistry, Plant Proteins genetics, Protein Processing, Post-Translational, Spinacia oleracea chemistry, Tandem Mass Spectrometry methods, Plant Proteins isolation & purification, Protein Isoforms isolation & purification, Proteomics methods, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods
Abstract

It is an established fact that allelic variation and post-translational modifications create different variants of proteins, which are observed as isoelectric and size subspecies in two-dimensional gel based proteomics. Here we explore the stromal proteome of spinach and Arabidopsis chloroplast and show that clustering of mass spectra is a useful tool for investigating such variants and detecting modified peptides with amino acid substitutions or post-translational modifications. This study employs data mining by hierarchical clustering of MALDI-MS spectra, using the web version of the SPECLUST program (http://bioinfo.thep.lu.se/speclust.html). The tool can also be used to remove peaks of contaminating proteins and to improve protein identification, especially for species without a fully sequenced genome. Mutually exclusive peptide peaks within a cluster provide a good starting point for MS/MS investigation of modified peptides, here exemplified by the identification of an A to E substitution that accounts for the isoelectric heterogeneity in protein isoforms., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published
2011
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46. Protein differences between human trapezius and vastus lateralis muscles determined with a proteomic approach.

Author

Hadrévi J, Hellström F, Kieselbach T, Malm C, and Pedrosa-Domellöf F

Subjects
Adult, Blotting, Western methods, Humans, Immunohistochemistry methods, Male, Metabolic Networks and Pathways physiology, Models, Molecular, Multivariate Analysis, Muscle Contraction physiology, Muscle Fibers, Skeletal chemistry, Muscle Fibers, Skeletal metabolism, Proteomics standards, Two-Dimensional Difference Gel Electrophoresis methods, Two-Dimensional Difference Gel Electrophoresis standards, Muscle Proteins metabolism, Neck Muscles chemistry, Neck Muscles metabolism, Proteomics methods, Quadriceps Muscle chemistry, Quadriceps Muscle metabolism
Abstract

Background: The trapezius muscle is a neck muscle that is susceptible to chronic pain conditions associated with repetitive tasks, commonly referred to as chronic work-related myalgia, hence making the trapezius a muscle of clinical interest. To provide a basis for further investigations of the proteomic traits of the trapezius muscle in disease, two-dimensional difference gel electrophoresis (2D-DIGE) was performed on the healthy trapezius using vastus lateralis as a reference. To obtain as much information as possible from the vast proteomic data set, both one-way ANOVA, with and without false discovery rate (FDR) correlation, and partial least square projection to latent structures with discriminant analysis (PLS-DA) were combined to compare the outcome of the analysis., Results: The trapezius and vastus lateralis showed significant differences in metabolic, contractile and regulatory proteins, with different results depending on choice of statistical approach and pre-processing technique. Using the standard method, FDR correlated one-way ANOVA, 42 protein spots differed significantly in abundance between the two muscles. Complementary analysis using immunohistochemistry and western blot confirmed the results from the 2D-DIGE analysis., Conclusions: The proteomic approach used in the present study combining 2D-DIGE and multivariate modelling provided a more comprehensive comparison of the protein profiles of the human trapezius and vastus lateralis muscle, than previously possible to obtain with immunohistochemistry or SDS-PAGE alone. Although 2D-DIGE has inherent limitations it is particularly useful to comprehensively screen for important structural and metabolic proteins, and appears to be a promising tool for future studies of patients suffering from chronic work related myalgia or other muscle diseases.

Published
2011
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47. The disulfide proteome and other reactive cysteine proteomes: analysis and functional significance.

Author

Lindahl M, Mata-Cabana A, and Kieselbach T

Subjects
Amino Acid Sequence, Animals, Citric Acid Cycle, Cysteine metabolism, Glycolysis, Humans, Mass Spectrometry methods, Models, Molecular, Molecular Sequence Data, Molecular Structure, Oxidation-Reduction, Photosynthesis, Protein Conformation, Sequence Alignment, Signal Transduction physiology, Sulfhydryl Compounds chemistry, Sulfhydryl Compounds metabolism, Thioredoxins metabolism, Cysteine chemistry, Disulfides chemistry, Proteome analysis
Abstract

Ten years ago, proteomics techniques designed for large-scale investigations of redox-sensitive proteins started to emerge. The proteomes, defined as sets of proteins containing reactive cysteines that undergo oxidative post-translational modifications, have had a particular impact on research concerning the redox regulation of cellular processes. These proteomes, which are hereafter termed "disulfide proteomes," have been studied in nearly all kingdoms of life, including animals, plants, fungi, and bacteria. Disulfide proteomics has been applied to the identification of proteins modified by reactive oxygen and nitrogen species under stress conditions. Other studies involving disulfide proteomics have addressed the functions of thioredoxins and glutaredoxins. Hence, there is a steadily growing number of proteins containing reactive cysteines, which are probable targets for redox regulation. The disulfide proteomes have provided evidence that entire pathways, such as glycolysis, the tricarboxylic acid cycle, and the Calvin-Benson cycle, are controlled by mechanisms involving changes in the cysteine redox state of each enzyme implicated. Synthesis and degradation of proteins are processes highly represented in disulfide proteomes and additional biochemical data have established some mechanisms for their redox regulation. Thus, combined with biochemistry and genetics, disulfide proteomics has a significant potential to contribute to new discoveries on redox regulation and signaling.

Published
2011
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48. A novel proteomic approach reveals a role for Mg-protoporphyrin IX in response to oxidative stress.

Author

Kindgren P, Eriksson MJ, Benedict C, Mohapatra A, Gough SP, Hansson M, Kieselbach T, and Strand A

Subjects
Amino Acid Motifs, Arabidopsis enzymology, Arabidopsis genetics, Arabidopsis Proteins genetics, Arabidopsis Proteins metabolism, Blotting, Western, Computational Biology, Gene Expression Regulation, Plant, Light-Harvesting Protein Complexes metabolism, Lyases metabolism, Protein Binding, Protein Subunits metabolism, Reproducibility of Results, Signal Transduction, Spectrometry, Fluorescence, Stress, Physiological, Tetrapyrroles metabolism, Oxidative Stress, Proteomics methods, Protoporphyrins metabolism
Abstract

The presence of genes encoding organellar proteins in different cellular compartments necessitates a tight coordination of expression by the different genomes of the eukaryotic cell. This coordination of gene expression is achieved by organelle-to-nucleus communication. Stress-induced perturbations of the tetrapyrrole pathway trigger large changes in nuclear gene expression. In order to investigate whether the tetrapyrrole Mg-ProtoIX itself is an important part of plastid-to-nucleus communication, we used an affinity column containing Mg-ProtoIX covalently linked to an Affi-Gel matrix. The proteins that bound to Mg-ProtoIX were analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis combined with nano liquid chromatography-mass spectrometry (MS)/MS. Thus, we present a novel proteomic approach to address the mechanisms involved in cellular signaling and we identified interactions between Mg-ProtoIX and a large number of proteins associated with oxidative stress responses. Our approach revealed an interaction between Mg-ProtoIX and the heat shock protein 90-type protein, HSP81-2 suggesting that a regulatory complex including HSP90 proteins and tetrapyrroles controlling gene expression is evolutionarily conserved between yeast and plants. In addition, our list of putative Mg-ProtoIX-binding proteins demonstrated that binding of tetrapyrroles does not depend on a specific amino acid motif but possibly on a specific fold of the protein., (Copyright © Physiologia Plantarum 2011.)

Published
2011
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49. Phosphorylated CpxR restricts production of the RovA global regulator in Yersinia pseudotuberculosis.

Author

Liu J, Obi IR, Thanikkal EJ, Kieselbach T, and Francis MS

Subjects
Acetylation, Adhesins, Bacterial metabolism, Alleles, Amino Acid Sequence, Aspartic Acid metabolism, Bacterial Outer Membrane Proteins chemistry, Bacterial Outer Membrane Proteins metabolism, Bacterial Proteins genetics, Base Sequence, Binding Sites, Cytoplasm metabolism, DNA Footprinting, DNA, Bacterial metabolism, Escherichia coli Proteins chemistry, Escherichia coli Proteins metabolism, Genes, Bacterial genetics, Lipoproteins chemistry, Lipoproteins metabolism, Molecular Sequence Data, Molecular Weight, Mutagenesis, Site-Directed, Phosphorylation, Promoter Regions, Genetic genetics, Protein Binding genetics, Spectrometry, Mass, Electrospray Ionization, Transcription Factors genetics, Virulence genetics, Yersinia pseudotuberculosis genetics, Yersinia pseudotuberculosis pathogenicity, Bacterial Proteins biosynthesis, Bacterial Proteins metabolism, Transcription Factors biosynthesis, Yersinia pseudotuberculosis metabolism
Abstract

Background: RovA is a global transcriptional regulator of gene expression in pathogenic Yersinia. RovA levels are kept in check by a sophisticated layering of distinct transcriptional and post-transcriptional regulatory mechanisms. In the enteropathogen Y. pseudotuberculosis, we have previously reported that the extracytoplasmic stress sensing CpxA-CpxR two-component regulatory system modulates rovA expression., Methodology/principal Findings: In this study, we characterized CpxR phosphorylation (CpxR∼P) in vitro, and determined that phosphorylation was necessary for CpxR to efficiently bind to the PCR-amplified upstream regulatory region of rovA. The precise CpxR∼P binding site was mapped by a nuclease protection assay and directed mutagenesis confirmed that in vivo binding to the rovA promoter inhibits transcription. Reduced RovA production was most pronounced following CpxR∼P accumulation in the Yersinia cytoplasm during chronic Cpx pathway activation and by the indiscriminate phosphodonor action of acetyl phosphate., Conclusions/significance: Cpx pathway activation restricts levels of the RovA global regulator. The regulatory influence of CpxR∼P must therefore extend well beyond periplasmic quality control in the Yersinia envelope, to include genes involved in environmental survival and pathogenicity.

Published
2011
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50. Thioredoxin targets of the plant chloroplast lumen and their implications for plastid function.

Author

Hall M, Mata-Cabana A, Akerlund HE, Florencio FJ, Schröder WP, Lindahl M, and Kieselbach T

Subjects
Alkylation drug effects, Arabidopsis drug effects, Arabidopsis enzymology, Arabidopsis Proteins isolation & purification, Arabidopsis Proteins metabolism, Biocatalysis drug effects, Bridged Bicyclo Compounds metabolism, Chloroplasts drug effects, Chromatography, Affinity, Electrophoresis, Polyacrylamide Gel, Enzyme Activation drug effects, Oxidation-Reduction drug effects, Oxidoreductases antagonists & inhibitors, Oxidoreductases metabolism, Protein Binding drug effects, Protein Processing, Post-Translational drug effects, Proteome metabolism, Staining and Labeling, Sulfhydryl Compounds metabolism, Synechocystis metabolism, Thioredoxins pharmacology, Arabidopsis metabolism, Chloroplasts metabolism, Thioredoxins metabolism
Abstract

The light-dependent regulation of stromal enzymes by thioredoxin (Trx)-catalysed disulphide/dithiol exchange is known as a classical mechanism for control of chloroplast metabolism. Recent proteome studies show that Trx targets are present not only in the stroma but in all chloroplast compartments, from the envelope to the thylakoid lumen. Trx-mediated redox control appears to be a common feature of important pathways, such as the Calvin cycle, starch synthesis and tetrapyrrole biosynthesis. However, the extent of thiol-dependent redox regulation in the thylakoid lumen has not been previously systematically explored. In this study, we addressed Trx-linked redox control in the chloroplast lumen of Arabidopsis thaliana. Using complementary proteomics approaches, we identified 19 Trx target proteins, thus covering more than 40% of the currently known lumenal chloroplast proteome. We show that the redox state of thiols is decisive for degradation of the extrinsic PsbO1 and PsbO2 subunits of photosystem II. Moreover, disulphide reduction inhibits activity of the xanthophyll cycle enzyme violaxanthin de-epoxidase, which participates in thermal dissipation of excess absorbed light. Our results indicate that redox-controlled reactions in the chloroplast lumen play essential roles in the function of photosystem II and the regulation of adaptation to light intensity.

Published
2010
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