Your search keyword '"Frank Wippich"' showing total 4 results

1. Transcript specific mRNP capture from Drosophila egg-chambers for proteomic analysis

Author

Frank Wippich and Anne Ephrussi

Subjects

Proteomics, Messenger RNA, Oligonucleotide, Quantitative proteomics, RNA-binding protein, Biology, General Biochemistry, Genetics and Molecular Biology, Cell biology, Gene Expression Regulation, Ribonucleoproteins, Biotinylation, Gene expression, Animals, Drosophila, Molecular Biology, Post-transcriptional regulation, Protein Binding, Ribonucleoprotein

Abstract

mRNA binding proteins (RBPs) play a major role in post-transcriptional control of gene expression. To understand the complex regulatory processes regulating a specific mRNA during its life-time, a comprehensive view of the bound RBPs is essential. Here, we describe a method for transcript-specific isolation of endogenous ribonucleoprotein complexes (RNPs) from Drosophila egg-chambers. The method, which is based on in-solution hybridization of short biotinylated antisense DNA oligonucleotide probes to multiple segments of a transcript of interest allows unbiased identification of associated proteins by quantitative proteomics.

Published

2020

2. Trafficking of the microdomain scaffolding protein reggie-1/flotillin-2

Author

Frank Wippich, Claudia A. O. Stuermer, Friederike A. Jaeger, Helmut Plattner, Georg Luxenhofer, Alexander Reuter, and Matthias F. Langhorst

Subjects

Scaffold protein, Histology, Prions, Golgi Apparatus, Nerve Tissue Proteins, Membrane trafficking, Biology, Endocytosis, Microtubules, PC12 Cells, Clathrin, Exocytosis, Pathology and Forensic Medicine, Jurkat Cells, symbols.namesake, Membrane Microdomains, Epidermal growth factor, ddc:570, Animals, Humans, Vesicle, Reggie/flotillin, Lipid microdomain, Membrane Proteins, Cell Biology, General Medicine, Golgi apparatus, Protein Structure, Tertiary, Rats, Cell biology, Endocytic cycling, Protein Transport, Cholesterol, Microscopy, Fluorescence, Mutation, biology.protein, symbols, HeLa Cells, TIRF microscopy

Abstract

The reggie/flotillin proteins oligomerize and associate into clusters which form scaffolds for membrane microdomains. Besides their localization at the plasma membrane, the reggies/flotillins reside at various intracellular compartments; however, the trafficking pathways used by reggie-1/flotillin-2 remain unclear. Here, we show that trafficking of reggie-1/flotillin-2 is BFA sensitive and that deletion mutants of reggie-1/flotillin-2 accumulate in the Golgi complex in HeLa, Jurkat and PC12 cells, suggesting Golgi-dependent trafficking of reggie-1/flotillin-2. Using total internal reflection fluorescence microscopy, we observed fast cycling of reggie-1/flotillin-2-positive vesicles at the plasma membrane, which engaged in transient interactions with the plasma membrane only. Reggie-1/flotillin-2 cycling was independent of clathrin, but was inhibited by cholesterol depletion and microtubule disruption. Cycling of reggie-1/flotillin-2 was negatively correlated with cell-cell contact formation but was stimulated by serum, epidermal growth factor and by cholesterol loading mediated by low density lipoproteins. However, reggie-1/flotillin-2 was neither involved in endocytosis of the epidermal growth factor itself nor in endocytosis of GPI-GFPs or the GPI-anchored cellular prion protein (PrP(c)). Reggie-2/flotillin-1 and stomatin-1 also exhibited cycling at the plasma membrane similar to reggie-1/flotillin-2, but these vesicles and microdomains only partially co-localized with reggie-2/flotillin-1. Thus, regulated vesicular cycling might be a general feature of SPFH protein-dependent trafficking.

Published

2008

3. TRICK

Author

Johannes H Wilbertz, Frank Wippich, Anne Ephrussi, James M. Halstead, Timothée Lionnet, and Jeffrey A. Chao

Subjects

0301 basic medicine, Messenger RNA, biology, Cell, RNA, Translation (biology), biology.organism_classification, Cell biology, 03 medical and health sciences, 030104 developmental biology, medicine.anatomical_structure, Live cell imaging, Mammalian cell, medicine, Fluorescence microscope, Drosophila melanogaster

Abstract

The life of an mRNA is dynamic within a cell. The development of quantitative fluorescent microscopy techniques to image single molecules of RNA has allowed many aspects of the mRNA lifecycle to be directly observed in living cells. Recent advances in live-cell multicolor RNA imaging, however, have now made it possible to investigate RNA metabolism in greater detail. In this chapter, we present an overview of the design and implementation of the translating RNA imaging by coat protein knockoff RNA biosensor, which allows untranslated mRNAs to be distinguished from ones that have undergone a round of translation. The methods required for establishing this system in mammalian cell lines and Drosophila melanogaster oocytes are described here, but the principles may be applied to any experimental system.

Published

2016

4. An RNA biosensor for imaging the first round of translation from single cells to living animals

Author

James M. Halstead, Anne Ephrussi, Robert H. Singer, Johannes H Wilbertz, Jeffrey A. Chao, Timothée Lionnet, and Frank Wippich

Subjects

Biosensing Techniques, Biology, oskar, Article, Cytosol, medicine, Protein biosynthesis, Drosophila Proteins, Animals, RNA, Messenger, Peptide Chain Initiation, Translational, Cell Nucleus, Messenger RNA, Multidisciplinary, RNA, Biological Transport, Translation (biology), Oocyte, Cell biology, Molecular Imaging, Cell nucleus, Drosophila melanogaster, medicine.anatomical_structure, Microscopy, Fluorescence, Oocytes, Drosophila Protein

Abstract

Measuring translation in space and time The ribosome translates the information contained within messenger RNAs (mRNAs) into proteins. When and where ribosomes encounter mRNAs can regulate gene expression. Halstead et al. developed an RNA biosensor that allows single molecules of mRNAs that have never been translated to be distinguished from ones that have undergone translation by the ribosome in living cells (see the Perspective by Popp and Maquat). The authors demonstrated the utility of their technique by examining the spatial and temporal regulation of translation in single cells and in Drosophila oocytes during development. Science , this issue p. 1367 ; see also p. 1316

Published

2015