Your search keyword '"Joachim Füllekrug"' showing total 3 results

1. VIP36 localisation to the early secretory pathway

Author

Joachim Füllekrug, Peter Scheiffele, and Kai Simons

Subjects

1-Deoxynojirimycin, Glycosylation, Endosome, Recombinant Fusion Proteins, Detergents, Golgi Apparatus, Biology, Kidney, N-Acetylglucosaminyltransferases, Transfection, Coatomer Protein, Vesicular stomatitis Indiana virus, Cell Line, chemistry.chemical_compound, symbols.namesake, Dogs, Viral Envelope Proteins, Chlorocebus aethiops, Animals, Humans, Vero Cells, Integral membrane protein, Secretory pathway, Glycoproteins, Brefeldin A, Hybridomas, Membrane Glycoproteins, Membrane Proteins, Membrane Transport Proteins, Biological Transport, Cell Biology, Endoplasmic Reticulum, Smooth, Golgi apparatus, Cell biology, Mannose-Binding Lectins, Solubility, chemistry, Coatomer, symbols, Medial Golgi, Glycolipids, Carrier Proteins, Protein Processing, Post-Translational, Biomarkers, HeLa Cells

Abstract

VIP36, an integral membrane protein previously isolated from epithelial MDCK cells, is an intracellular lectin of the secretory pathway. Overexpressed VIP36 had been localised to the Golgi complex, plasma membrane and endocytic structures suggesting post-Golgi trafficking of this molecule (Fiedler et al., 1994). Here we provide evidence that endogenous VIP36 is localised to the Golgi apparatus and the early secretory pathway of MDCK and Vero cells and propose that retention is easily saturated. High resolution confocal microscopy shows partial overlap of VIP36 with Golgi marker proteins. Punctate cytoplasmic structures colocalise with coatomer and ERGIC-53, labeling ER-Golgi intermediate membrane structures. Cycling of VIP36 is suggested by colocalisation with anterograde cargo trapped in pre-Golgi structures and modification of its N-linked carbohydrate by glycosylation enzymes of medial Golgi cisternae. Furthermore, after brefeldin A treatment VIP36 is segregated from resident Golgi proteins and codistributes with ER-Golgi recycling proteins.

Published

1999

2. Cellular uptake of fatty acids driven by the ER-localized acyl-CoA synthetase FATP4

Author

Thomas Herrmann, Katrin Milger, Joachim Füllekrug, Wolfgang Stremmel, Jelena Zickwolf, Robert Ehehalt, Daniel Gotthardt, Paul A. Watkins, and Christiane Becker

Subjects

Recombinant Fusion Proteins, Biological Transport, Active, Endoplasmic Reticulum, Cell Line, Mitochondrial Proteins, Mice, Free fatty acid receptor 1, Coenzyme A Ligases, Basic Helix-Loop-Helix Transcription Factors, Animals, Humans, Coenzyme A, adipocyte protein 2, Beta oxidation, chemistry.chemical_classification, biology, Fatty Acid Transport Proteins, Cell Membrane, Fatty Acids, Fatty acid, Cell Biology, Rats, Fatty acid synthase, chemistry, Biochemistry, Mutation, biology.protein, Free fatty acid receptor, Beta-ketoacyl-ACP synthase

Abstract

Long-chain fatty acids are important metabolites for the generation of energy and the biosynthesis of lipids. The molecular mechanism of their cellular uptake has remained controversial. The fatty acid transport protein (FATP) family has been named according to its proposed function in mediating this process at the plasma membrane. Here, we show that FATP4 is in fact localized to the endoplasmic reticulum and not the plasma membrane as reported previously. Quantitative analysis confirms the positive correlation between expression of FATP4 and uptake of fatty acids. However, this is dependent on the enzymatic activity of FATP4, catalyzing the esterification of fatty acids with CoA. Monitoring fatty acid uptake at the single-cell level demonstrates that the ER localization of FATP4 is sufficient to drive transport of fatty acids. Expression of a mitochondrial acyl-CoA synthetase also enhances fatty acid uptake, suggesting a general relevance for this mechanism. Our results imply that cellular uptake of fatty acids can be regulated by intracellular acyl-CoA synthetases. We propose that the enzyme FATP4 drives fatty acid uptake indirectly by esterification. It is not a transporter protein involved in fatty acid translocation at the plasma membrane.

Published

2006

3. Identification and characterization of a novel human plant pathogenesis-related protein that localizes to lipid-enriched microdomains in the Golgi complex

Author

Dora V. Kaloyanova, Andreas Schlosser, Friedrich Lottspeich, Ramon L Serrano, Joachim Füllekrug, J. Bernd Helms, Felix T. Wieland, Wolf D. Lehmann, and Heike B. Eberle

Subjects

Male, Immunoprecipitation, Caveolin 1, Molecular Sequence Data, Golgi Apparatus, CHO Cells, Biology, Caveolins, symbols.namesake, Cytosol, Membrane Microdomains, Cricetinae, Caveolin, Animals, Humans, Endomembrane system, Tissue Distribution, Amino Acid Sequence, Golgi localization, Pathogenesis-related protein, Plant Proteins, Protein Synthesis Inhibitors, Brefeldin A, Base Sequence, Sequence Homology, Amino Acid, Endoplasmic reticulum, Lipid microdomain, Membrane Proteins, Cell Biology, Sequence Analysis, DNA, Golgi apparatus, Cell biology, Rats, Molecular Weight, Biochemistry, symbols, Female

Abstract

Group 1 of plant pathogenesis-related proteins (PR-1) and a variety of related mammalian proteins constitute a superfamily of proteins that share structural similarities. Little is known about their function, but all the family members identified to date are co-translationally translocated to the lumen of the endoplasmic reticulum and are secreted as soluble proteins or are targeted to vacuoles. Here we report the identification of a novel family member that localizes to the cytosolic site of the endomembrane system in mammalian cells. After detergent solubilization of isolated Golgi membranes, a 17 kDa protein was found associated with a low-density detergent-insoluble fraction. The amino-acid sequence, determined by microsequencing and molecular cloning, revealed a significant homology with the superfamily of PR-1 proteins. Golgi-associated PR-1 protein (GAPR-1) showed a brefeldin-A-sensitive Golgi localization in immunofluorescence. Interestingly,the protein remained associated with the microdomain fraction in the presence of Brefeldin A. By mass spectrometry, GAPR-1 was shown to be myristoylated. Immunoprecipitation of GAPR- 1 from Golgi membranes resulted in the coimmunoprecipitation of caveolin-1, indicating a direct interaction between these two proteins. Myristoylation, together with protein-protein or electrostatic interactions at physiological pH owing to the highly basic pI of GAPR-1 (pI 9.4) could explain the strong membrane association of GAPR-1. Tissue screening revealed that GAPR-1 is not detectably expressed in liver,heart or adrenal glands. High expression was found in monocytes, leukocytes,lung, spleen and embryonic tissue. Consistent with the involvement of PR-1 proteins in the plant immune system, these data could indicate that GAPR-1 is involved in the immune system.

Published

2002