Your search keyword '"Reimer, Ulf"' showing total 112 results

101. PATIENTS WITH EARLY INFLAMMATORY ARTHRITIS WHO ARE ANTI-CCP ANTIBODY POSITIVE HAVE ANTIBODIES AGAINST ACETYLATED AND CARBAMYLATED VIMENTIN PEPTIDES

Author

Juarez, Maria, Bang, Holger, Hammar, Friederike, Reimer, Ulf, Dyke, Bernard, Christopher Dominic Buckley, Fisher, Benjamin, Filer, Andrew, and Raza, Karim

102. Biocomputing in a Nutshell

Author

Fuellen, Georg, Reimer, Ulf, Smith, Martin, Fuellen, Georg, Reimer, Ulf, and Smith, Martin

Abstract

This website, written by Ulf Reimer and Georg Fuellen and presented by the University of Bielefeld in Germany, offers a broad introduction to bioinformatics. Beginning with the development of modern molecular biology, and then discussing the huge amount of data and how to analyze it, the article concludes that an interdisciplinary approach to biocomputing is advantageous because it allows research to "transcend the limits of reductionism; from the vast quantities of bytes and pieces, the contours of complex structures and relationships might emerge from the genetic alphabet soup as life itself once emerged from the primordial soup."

103. Peptide libraries for the comprehensive coverage of the tumor mutanome for immune monitoring and immuno therapy

Author

von Hoegen, Paul, Knaute, Tobias, Wenschuh, Holger, and Reimer, Ulf

Subjects

Pharmacology, Cancer Research, Oncology, Poster Presentation, Immunology, Molecular Medicine, Immunology and Allergy

104. Serotyping of Toxoplasma gondii in Cats (Felis domesticus) Reveals Predominance of Type II Infections in Germany.

Author

Maksimov, Pavlo, Zerweck, Johannes, Dubey, Jitender P., Pantchev, Nikola, Frey, Caroline F., Maksimov, Aline, Reimer, Ulf, Schutkowski, Mike, Hosseininejad, Morteza, Ziller, Mario, Conraths, Franz J., and Schares, Gereon

Subjects

TOXOPLASMA gondii, CATS, IMMUNOGLOBULINS, PARASITES, EPIDEMIOLOGY, SEROTYPING

Abstract

Background:Cats are definitive hosts of Toxoplasma gondii and play an essential role in the epidemiology of this parasite. The study aims at clarifying whether cats are able to develop specific antibodies against different clonal types of T. gondii and to determine by serotyping the T. gondii clonal types prevailing in cats as intermediate hosts in Germany. Methodology:To establish a peptide-microarray serotyping test, we identified 24 suitable peptides using serological T. gondii positive (n=21) and negative cat sera (n=52). To determine the clonal type-specific antibody response of cats in Germany, 86 field sera from T. gondii seropositive naturally infected cats were tested. In addition, we analyzed the antibody response in cats experimentally infected with non-canonical T. gondii types (n=7). Findings:Positive cat reference sera reacted predominantly with peptides harbouring amino acid sequences specific for the clonal T. gondii type the cats were infected with. When the array was applied to field sera from Germany, 98.8% (85/86) of naturally-infected cats recognized similar peptide patterns as T. gondii type II reference sera and showed the strongest reaction intensities with clonal type II-specific peptides. In addition, naturally infected cats recognized type II-specific peptides significantly more frequently than peptides of other type-specificities. Cats infected with non-canonical types showed the strongest reactivity with peptides presenting amino-acid sequences specific for both, type I and type III. Conclusions:Cats are able to mount a clonal type-specific antibody response against T. gondii. Serotyping revealed for most seropositive field sera patterns resembling those observed after clonal type II-T. gondii infection. This finding is in accord with our previous results on the occurrence of T. gondii clonal types in oocysts shed by cats in Germany. [ABSTRACT FROM AUTHOR]

Published

2013

105. An Overview of Peptides and Peptide Pools for Antigen-Specific Stimulation in T-Cell Assays.

Author

Schnatbaum K, Holenya P, Pfeil S, Drosch M, Eckey M, Reimer U, Wenschuh H, and Kern F

Subjects

Amino Acid Sequence, Reproducibility of Results, Peptides, T-Lymphocytes

Abstract

The analysis of antigen-specific T-cell responses has become routine in many laboratories. Functional T-cell assays like enzyme-linked-immuno-spot (ELISPOT), which depend on antigen-specific stimulation, increasingly use peptides to represent the antigen of interest. Besides single peptides, mixtures of peptides (peptide pools) are very frequently applied. Such peptide pools may, for example, represent entire proteins (with overlapping peptides covering a protein sequence) or include noncontiguous peptides such as a collection of T-cell-stimulating peptides. The optimum specification of single peptides or peptide pools for T-cell stimulation assays will depend on the purpose of the test, the target T-cell population, the availability of sample, requirements regarding reproducibility, and, last but not least, the available budget, to mention only the most important factors. Because of the way peptides are produced, they will always contain certain amounts of impurities such as peptides with deletions or truncated peptides, and there may be additional by-products of peptide synthesis. Optimized synthesis protocols as well as purification help reduce impurities that might otherwise cause false-positive assay results. However, specific requirements with respect to purity will vary depending on the purpose of an assay. Finally, storage conditions significantly affect the shelf life of peptides, which is relevant especially for longitudinal studies. The present book chapter addresses all of these aspects in detail. It should provide the researcher with all necessary background knowledge for making the right decisions when it comes to choosing, using, and storing peptides for ELISPOT and other T-cell stimulation assays., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

106. PRISMA and BioID disclose a motifs-based interactome of the intrinsically disordered transcription factor C/EBPα.

Author

Ramberger E, Sapozhnikova V, Kowenz-Leutz E, Zimmermann K, Nicot N, Nazarov PV, Perez-Hernandez D, Reimer U, Mertins P, Dittmar G, and Leutz A

Abstract

C/EBPα represents a paradigm intrinsically disordered transcription factor containing short linear motifs and post-translational modifications (PTM). Unraveling C/EBPα protein interaction networks is a prerequisite for understanding the multi-modal functions of C/EBPα in hematopoiesis and leukemia. Here, we combined arrayed peptide matrix screening (PRISMA) with BioID to generate an in vivo validated and isoform specific interaction map of C/EBPα. The myeloid C/EBPα interactome comprises promiscuous and PTM-regulated interactions with protein machineries involved in gene expression, epigenetics, genome organization, DNA replication, RNA processing, and nuclear transport. C/EBPα interaction hotspots coincide with homologous conserved regions of the C/EBP family that also score as molecular recognition features. PTMs alter the interaction spectrum of C/EBP-motifs to configure a multi-valent transcription factor hub that interacts with multiple co-regulatory components, including BAF/SWI-SNF or Mediator complexes. Combining PRISMA and BioID is a powerful strategy to systematically explore the PTM-regulated interactomes of intrinsically disordered transcription factors., Competing Interests: The authors declare no conflicts of interest., (© 2021 The Authors.)

Published

2021

107. A Universal Peptide Matrix Interactomics Approach to Disclose Motif-Dependent Protein Binding.

Author

Ramberger E, Suarez-Artiles L, Perez-Hernandez D, Haji M, Popp O, Reimer U, Leutz A, Dittmar G, and Mertins P

Subjects

Amino Acid Motifs, HeLa Cells, Humans, Peptides chemistry, Point Mutation, Protein Binding, Protein Interaction Domains and Motifs, Protein Processing, Post-Translational, Proteomics methods

Abstract

Protein-protein interactions mediated by intrinsically disordered regions are often based on short linear motifs (SLiMs). SLiMs are implicated in signal transduction and gene regulation yet remain technically laborious and notoriously challenging to study. Here, we present an optimized method for a protein interaction screen on a peptide matrix (PRISMA) in combination with quantitative MS. The protocol was benchmarked with previously described SLiM-based protein-protein interactions using peptides derived from EGFR, SOS1, GLUT1, and CEBPB and extended to map binding partners of kinase activation loops. The detailed protocol provides practical considerations for setting up a PRISMA screen and subsequently implementing PRISMA on a liquid-handling robotic platform as a cost-effective high-throughput method. Optimized PRISMA can be universally applied to systematically study SLiM-based interactions and associated post-translational modifications or mutations to advance our understanding of the largely uncharacterized interactomes of intrinsically disordered protein regions., Competing Interests: Conflict of interest The authors declare no competing interests., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2021

108. The Choice of Search Engine Affects Sequencing Depth and HLA Class I Allele-Specific Peptide Repertoires.

Author

Parker R, Tailor A, Peng X, Nicastri A, Zerweck J, Reimer U, Wenschuh H, Schnatbaum K, and Ternette N

Subjects

Alleles, Amino Acid Sequence, Histocompatibility Antigens Class I genetics, Humans, Mass Spectrometry, Peptide Library, Peptides genetics, Proteomics methods, Histocompatibility Antigens Class I chemistry, Peptides chemistry, Search Engine

Abstract

Standardization of immunopeptidomics experiments across laboratories is a pressing issue within the field, and currently a variety of different methods for sample preparation and data analysis tools are applied. Here, we compared different software packages to interrogate immunopeptidomics datasets and found that Peaks reproducibly reports substantially more peptide sequences (~30-70%) compared with Maxquant, Comet, and MS-GF+ at a global false discovery rate (FDR) of <1%. We noted that these differences are driven by search space and spectral ranking. Furthermore, we observed differences in the proportion of peptides binding the human leukocyte antigen (HLA) alleles present in the samples, indicating that sequence-related differences affected the performance of each tested engine. Utilizing data from single HLA allele expressing cell lines, we observed significant differences in amino acid frequency among the peptides reported, with a broadly higher representation of hydrophobic amino acids L, I, P, and V reported by Peaks. We validated these results using data generated with a synthetic library of 2000 HLA-associated peptides from four common HLA alleles with distinct anchor residues. Our investigation highlights that search engines create a bias in peptide sequence depth and peptide amino acid composition, and resulting data should be interpreted with caution., Competing Interests: Conflict of interest N. T. is directing immunopeptidomics research at Enara Bio part-time and serves on the Scientific Advisory Boards of Enara Bio and T-Cypher Bio. N. T. is consultant to Hoffman-La Roche and Grey Wolf Therapeutics. All other authors declare no conflict of interest., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2021

109. High-Throughput Microarray Incubations Using Multi-Well Chambers.

Author

Zerweck J, Reimer U, Jansong J, Pawlowski N, Tersch C, Eckey M, and Knaute T

Subjects

Amino Acid Sequence, Analytic Sample Preparation Methods, Humans, Molecular Sequence Data, Peptides chemistry, Peptides metabolism, Protein Array Analysis methods

Abstract

Peptide microarrays are ideal tools for a variety of applications ranging from epitope mapping to immune monitoring. Here we present a method for high-throughput screening of biological samples using only standard microtiter plate equipment. Parallel incubation of a large number of samples with a small library of peptides is enabled by printing multiple identical mini-arrays on one microarray slide and further combining four slides to yield an incubation frame possessing the dimensions of a 96-well microtiter plate. Applying conventional lab equipment such as ELISA washers, hundreds of samples can be processed in 1 day yielding approx. 200 data points in triplicates per sample.

Published

2016

110. Antibody signatures defined by high-content peptide microarray analysis.

Author

Masch A, Zerweck J, Reimer U, Wenschuh H, and Schutkowski M

Subjects

Animals, Antibodies blood, False Positive Reactions, Humans, Immunoglobulins immunology, Peptides immunology, Antibodies immunology, Immunoassay methods, Peptides analysis, Protein Array Analysis methods

Abstract

Circulating antibodies are highly selective binding reagents directed to a vast repertoire of antigens. Candidate antigens displayed as overlapping peptides on microarrays can be used to screen for recognition by serum antibodies from clinically well-defined patient populations. The methodology is robust and enables unbiased visualization of antigen-specific B-cell responses. Additionally, autoantibody signatures of diagnostic value could be detected using microarrays displaying thousands of human peptides.

Published

2010

111. Design and synthesis of a new class of selective integrin alpha5beta1 antagonists.

Author

Stragies R, Osterkamp F, Zischinsky G, Vossmeyer D, Kalkhof H, Reimer U, and Zahn G

Subjects

Drug Design, Esters, Integrin alphaVbeta3 chemistry, Ligands, Models, Molecular, Peptides, Cyclic chemistry, Protein Conformation, Pyridines chemistry, Pyrrolidines chemistry, Stereoisomerism, Structure-Activity Relationship, Sulfonamides chemical synthesis, Sulfonamides chemistry, Integrin alpha5beta1 antagonists & inhibitors, Integrin alpha5beta1 chemistry, Pyridines chemical synthesis, Pyrrolidines chemical synthesis

Abstract

Starting from the structure of integrin alphavbeta3 in a complex with a peptidic ligand plus SAR data on nonpeptidic ligands, we derived a new class of integrin alpha5beta1 antagonists (1). Several synthesis strategies were applied to evaluate the chemical space around the essential pharmacophore groups R1 to R3 to obtain highly active and selective pyrrolidine derivatives as integrin alpha5beta1 antagonists. Integrin selectivity was controlled by switching from a sulfonamide moiety to a mesitylene amide moiety for R3. This finding represents a general feature for modulating selectivity toward other related integrin receptors. On the basis of the encouraging results from various in vitro studies, the most active compounds were selected for further in vivo studies in animal models and preclinical development.

Published

2007

112. High-content peptide microarrays for deciphering kinase specificity and biology.

Author

Schutkowski M, Reimer U, Panse S, Dong L, Lizcano JM, Alessi DR, and Schneider-Mergener J

Subjects

Automation, Binding Sites, Electrophoresis, Polyacrylamide Gel, Peptides analysis, Phosphotransferases analysis, Substrate Specificity, Peptides metabolism, Phosphotransferases metabolism, Protein Array Analysis methods

Published

2004