Your search keyword '"Polyacrylamide-Gels"' showing total 5 results

1. Metabolic Labeling and Protein Linearization Technology Allow the Study of Proteins Secreted by Cultured Cells in Serum-Containing Media

Author

Curzio Rüegg, Faes E, Mara Colzani, Patrice Waridel, Manfredo Quadroni, and Julien Laurent

Subjects

Proteomics, Serum, protein concentration linearization, Statistical-Model, Proteome, medicine.medical_treatment, Quantitative proteomics, Growth-Factor, stable isotope labeling, Biology, Lc-Ms/Ms, Biomarker Discovery, Peptide Mapping, Biochemistry, Mass Spectrometry, Cell Line, Tumor, Stable isotope labeling by amino acids in cell culture, Tumor Microenvironment, medicine, Animals, Humans, Breast-Cancer, Viability assay, Mass-Spectrometry, chemistry.chemical_classification, Quantitative Proteomics, Chromatography, Growth factor, Polyacrylamide-Gels, Proteins, Reproducibility of Results, secretome analysis, Blood Proteins, General Chemistry, Secretomics, Peptide Fragments, Human Plasma Proteome, Amino acid, Secretory protein, chemistry, Cell culture, Culture Media, Conditioned, Isotope Labeling, Cattle

Abstract

Supernatants from cell cultures (also called conditioned media, CMs) are commonly analyzed to study the pool of secreted proteins (secretome). To reduce the exogenous protein background, serum-free media are often used to obtain CMs. Serum deprivation, however, can severely affect cell viability and phenotype, including protein secretion. We present a strategy to analyze the proteins secreted by cells in fetal bovine serum-containing CMs, which combines the advantage of metabolic labeling and protein concentration linearization techniques. Incubation of CMs with a hexapeptide ligand library was used to reduce the dynamic range of the samples and led to the identification of 3 times more proteins than in untreated CM samples. Labeling with a deuterated amino acid was used to distinguish between cellular proteins and homologous bovine proteins contained in the medium. Application of the strategy to two breast cancer cell lines led to the identification of proteins secreted in different amounts and which could correlate with their varying degree of aggressiveness. Selected reaction monitoring (SRM)-based quantitation of three proteins of interest in the crude samples yielded data in good agreement with the results from concentration-equalized samples.

Published

2009

2. Novel alleles of the VERNALIZATION1 genes in wheat are associated with modulation of DNA curvature and flexibility in the promoter region

Author

Alexandr Muterko, Elena A. Salina, Ruslan Kalendar, and Institute of Biotechnology

Subjects

0301 basic medicine, DNA, Plant, Flowering time, REGULATORY ELEMENTS, Mutant, TATA-BOX, Plant Science, Biology, Genes, Plant, 03 medical and health sciences, New alleles, GEOGRAPHICAL VARIATION, Anomalous migration, Genetic variation, POLYACRYLAMIDE-GELS, Cereal, MOLECULAR CHARACTERIZATION, TRITICUM-AESTIVUM L, GENOME-WIDE ANALYSIS, TETRAPLOID WHEAT, Allele, Promoter Regions, Genetic, Gene, 1183 Plant biology, microbiology, virology, Alleles, Triticum, VRN-box, 2. Zero hunger, Genetics, Genetic diversity, Research, Temperature, Promoter, Vernalization, WINTER-WHEAT, VRN1 genes, DNA curvature, 030104 developmental biology, Wheat, Nucleic Acid Conformation, Seasons, Vernalization requirement, SPRING GROWTH HABIT, Sequence motif

Abstract

Background In wheat, the vernalization requirement is mainly controlled by the VRN genes. Different species of hexaploid and tetraploid wheat are widely used as genetic source for new mutant variants and alleles for fundamental investigations and practical breeding programs. In this study, VRN-A1 and VRN-B1 were analysed for 178 accessions representing six tetraploid wheat species (Triticum dicoccoides, T. dicoccum, T. turgidum, T. polonicum, T. carthlicum, T. durum) and five hexaploid species (T. compactum, T. sphaerococcum, T. spelta, T. macha, T. vavilovii). Results Novel allelic variants in the promoter region of VRN-A1 and VRN-B1 were identified based on the change in curvature and flexibility of the DNA molecules. The new variants of VRN-A1 (designated as Vrn-A1a.2, Vrn-A1b.2 – Vrn-A1b.6 and Vrn-A1i) were found to be widely distributed in hexaploid and tetraploid wheat, and in fact were predominant over the known VRN-A1 alleles. The greatest diversity of the new variants of VRN-B1 (designated as VRN-B1.f, VRN-B1.s and VRN-B1.m) was found in the tetraploid and some hexaploid wheat species. For the first time, minor differences within the sequence motif known as the VRN-box of VRN1 were correlated with wheat growth habit. Thus, vrn-A1b.3 and vrn-A1b.4 were revealed in winter wheat in contrast to Vrn-A1b.2, Vrn-A1b.5, Vrn-A1b.6 and Vrn-A1i. It was found that single nucleotide mutation in the VRN-box can influence the vernalization requirement and growth habit of wheat. Our data suggest that both the A-tract and C-rich segment within the VRN-box contribute to its functionality, and provide a new view of the hypothesised role of the VRN-box in regulating transcription of the VRN1 genes. Specifically, it is proposed that combination of mutations in this region can modulate vernalization sensitivity and flowering time of wheat. Conclusions New allelic variants of the VRN-A1 and VRN-B1 genes were identified in hexaploid and tetraploid wheat. Mutations in A-tract and C-rich segments within the VRN-box of VRN-A1 are associated with modulation of the vernalization requirement and flowering time. New allelic variants will be useful in fundamental investigations into the regulation of VRN1 expression, and provide a valuable genetic resource for practical breeding of wheat. Electronic supplementary material The online version of this article (doi:10.1186/s12870-015-0691-2) contains supplementary material, which is available to authorized users.

Published

2016

3. A glycomic approach reveals a new mycobacterial polysaccharide

Author

Henrieta Škovierová, Germain Puzo, Jérôme Nigou, Gerald Larrouy-Maumus, Martine Gilleron, Patrick J. Brennan, Mary Jackson, Sophie Zuberogoitia, Imperial College London, Institut de pharmacologie et de biologie structurale (IPBS), Centre National de la Recherche Scientifique (CNRS)-Université Toulouse III - Paul Sabatier (UT3), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées, Juola and Associates, and Colorado State University [Fort Collins] (CSU)

Subjects

Lipopolysaccharides, Glycan, Biochemistry & Molecular Biology, BACTERIAL LIPOPOLYSACCHARIDES, MOLECULAR-PATTERNS, GEL-ELECTROPHORESIS, TUBERCULOSIS, 01 natural sciences, Biochemistry, Bacterial cell structure, Mycobacterium, Glycomics, 03 medical and health sciences, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, POLYACRYLAMIDE-GELS, ComputingMilieux_MISCELLANEOUS, CELL-ENVELOPE, 030304 developmental biology, Gel electrophoresis, 0303 health sciences, Lipoarabinomannan, Science & Technology, biology, Mycobacterium smegmatis, 010401 analytical chemistry, Polysaccharides, Bacterial, MASS-SPECTROMETRY, SMEGMATIS, Mycobacterium tuberculosis, 11 Medical And Health Sciences, 06 Biological Sciences, biology.organism_classification, 0104 chemical sciences, BOVIS BCG, polysaccharide, biology.protein, LIPOARABINOMANNAN, ORIGINAL ARTICLES, Cell envelope, glycomic, Life Sciences & Biomedicine

Abstract

Mycobacterium tuberculosis lipoarabinomannan (LAM) and biosynthetically related lipoglycans and glycans play an important role in host–pathogen interactions. Therefore, the elucidation of the complete biosynthetic pathways of these important molecules is expected to afford novel therapeutic targets. The characterization of biosynthetic enzymes and transporters involved in the formation and localization of these complex macromolecules in the bacterial cell envelope largely relies on genetic manipulation of mycobacteria and subsequent analyses of lipoglycan structural alterations. However, lipoglycans are present in relatively low amounts. Their purification to homogeneity remains tedious and time-consuming. To overcome these issues and to reduce the biomass and time required for lipoglycan purification, we report here the development of a methodology to efficiently purify lipoglycans by sodium deoxycholate–polyacrylamide gel electrophoresis. This faster purification method can be applied on a small amount of mycobacterial cells biomass (10–50 mg), resulting in tens of micrograms of purified lipoglycans. This amount of purified products was found to be sufficient to undertake structural analyses of lipoglycans and glycans carbohydrate domains by a combination of highly sensitive analytical procedures, involving cryoprobe NMR analysis of intact macromolecules and chemical degradations monitored by gas chromatography and capillary electrophoresis. This glycomic approach was successfully applied to the purification and structural characterization of a newly identified polysaccharide, structurally related to LAM, in the model fast-growing species Mycobacterium smegmatis.

Published

2015

4. Liver mitochondrial membrane crosslinking and destruction in a rat model of Wilson disease

Author

Karl H. Summer, Nathan L. Bandow, Christian Rust, Martin Goettlicher, Daniela Wartini, Sabine Schulz, Nora Jägemann, Luise Jennen, Josef Lichtmannegger, Sabine Schmitt, Alan A. DiSpirito, Lorenzo Galluzzi, Veronique Chajes, Guido Kroemer, Nathanael Larochette, Hans Zischka, Valerie S. Gilles, and Irene Esposito

Subjects

ATPase, Mitochondria, Liver, Oxidative phosphorylation, In Vitro Techniques, Mitochondrion, medicine.disease_cause, Mitochondrial Proteins, Gene Knockout Techniques, Hepatolenticular Degeneration, Microscopy, Electron, Transmission, In vivo, medicine, Animals, Humans, Copper transporting atpase, Evans cinnamon rats, Cell-death, Oxidative stress, permeability transition, Superoxide-dismutase, Catalyzed oxidation, Polyacrylamide-gels, Oxidant injury, Oral therapy, Sulfhydryl Compounds, Inner mitochondrial membrane, Cation Transport Proteins, Chelating Agents, Adenosine Triphosphatases, Cell-Free System, biology, General Medicine, Rats, Transport protein, Disease Models, Animal, Cross-Linking Reagents, Biochemistry, Copper-Transporting ATPases, Copper-transporting ATPases, biology.protein, Copper

Abstract

Wilson disease (WD) is a rare hereditary condition that is caused by a genetic defect in the copper-transporting ATPase ATP7B that results in hepatic copper accumulation and lethal liver failure. The present study focuses on the structural mitochondrial alterations that precede clinical symptoms in the livers of rats lacking Atp7b, an animal model for WD. Liver mitochondria from these Atp7b–/– rats contained enlarged cristae and widened intermembrane spaces, which coincided with a massive mitochondrial accumulation of copper. These changes, however, preceded detectable deficits in oxidative phosphorylation and biochemical signs of oxidative damage, suggesting that the ultrastructural modifications were not the result of oxidative stress imposed by copper- dependent Fenton chemistry. In a cell-free system containing a reducing dithiol agent, isolated mitochondria exposed to copper underwent modifications that were closely related to those observed in vivo. In this cell-free system, copper induced thiol modifications of three abundant mitochondrial membrane proteins, and this correlated with reversible intramitochondrial membrane crosslinking, which was also observed in liver mitochondria from Atp7b–/– rats. In vivo, copper-chelating agents reversed mitochondrial accumulation of copper, as well as signs of intra-mitochondrial membrane crosslinking, thereby preserving the functional and structural integrity of mitochondria. Together, these findings suggest that the mitochondrion constitutes a pivotal target of copper in WD.

Published

2011

5. Protein fingerprints of cultured CA3-CA1 hippocampal neurons: comparative analysis of the distribution of synaptosomal and cytosolic proteins

Author

Valeria Corti, Giovanni Piccoli, Massimo Alessio, Andrea Bergamaschi, Carlo Vittorio Cannistraci, Linda Pattini, Sergio Cerutti, Angela Bachi, Yovan Sanchez-Ruiz, Antonio Malgaroli, Corti, V, SANCHEZ RUIZ, Y, Piccoli, G, Bergamaschi, A, Cannistraci, Cv, Pattini, L, Cerutti, S, Bachi, A, Alessio, M, and Malgaroli, Antonio

Subjects

LONG-TERM POTENTIATION, MASS-SPECTROMETRY, SYNAPTIC PLASTICITY, POLYACRYLAMIDE-GELS, PROTEOMIC ANALYSIS, LATE MAINTENANCE, IDENTIFICATION, SYNAPSES, ENHANCEMENT, PROBABILITY, Proteomics, Population, Blotting, Western, Hippocampal formation, Biology, Hippocampus, Peptide Mapping, lcsh:RC321-571, Cellular and Molecular Neuroscience, Immunolabeling, Cytosol, Animals, Electrophoresis, Gel, Two-Dimensional, education, lcsh:Neurosciences. Biological psychiatry. Neuropsychiatry, Cells, Cultured, Neurons, education.field_of_study, General Neuroscience, lcsh:QP351-495, Long-term potentiation, Protein subcellular localization prediction, Cell biology, Rats, lcsh:Neurophysiology and neuropsychology, nervous system, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Synaptic plasticity, Proteome, Neuroscience, Synaptosomes, Research Article

Abstract

Background All studies aimed at understanding complex molecular changes occurring at synapses face the problem of how a complete view of the synaptic proteome and of its changes can be efficiently met. This is highly desirable when synaptic plasticity processes are analyzed since the structure and the biochemistry of neurons and synapses get completely reshaped. Because most molecular studies of synapses are nowadays mainly or at least in part based on protein extracts from neuronal cultures, this is not a feasible option: these simplified versions of the brain tissue on one hand provide an homogeneous pure population of neurons but on the other yield only tiny amounts of proteins, many orders of magnitude smaller than conventional brain tissue. As a way to overcome this limitation and to find a simple way to screen for protein changes at cultured synapses, we have produced and characterized two dimensional electrophoresis (2DE) maps of the synaptic proteome of CA3-CA1 hippocampal neurons in culture. Results To obtain 2D maps, hippocampal cultures were mass produced and after synaptic maturation, proteins were extracted following subfractionation procedures and separated by 2D gel electrophoresis. Similar maps were obtained for the crude cytosol of cultured neurons and for synaptosomes purified from CA3-CA1 hippocampal tissue. To efficiently compare these different maps some clearly identifiable reference points were molecularly identified by mass spectrometry and immunolabeling methods. This information was used to run a differential analysis and establish homologies and dissimilarities in these 2D protein profiles. Conclusion Because reproducible fingerprints of cultured synapses were clearly obtained, we believe that our mapping effort could represent a simple tool to screen for protein expression and/or protein localization changes in CA3-CA1 hippocampal neurons following plasticity.

Published

2008