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34 results on '"Andreas Hunziker"'

1. Editorial

Author

Andreas Hunziker and Simon Peng-Keller

Subjects
Philosophy. Psychology. Religion
Published
2014
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3. Editorial

Author

Andreas Hunziker and Benjamin Schliesser

Subjects
Philosophy. Psychology. Religion
Published
2011
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6. Editorial

Author

Simon Peng-Keller and Andreas Hunziker

Subjects
Philosophy. Psychology. Religion
Published
2010
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9. Editorial

Author

Andrea Anker, Andreas Hunziker, Philipp Stoellger, and Hartmut von Sass

Subjects
Philosophy. Psychology. Religion
Published
2008
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19. Loss of Drop1 expression already at early tumor stages in a wide range of human carcinomas

Author

Marina Schorpp-Kistner, Olga Keberlein, Antje Giersch, Herwig Ponstingl, Frederik Marmé, Raffael Kurek, Peter Möller, Andreas Hunziker, Claudia Müller, Jiirgen Kretschmer, Eberhard Spiess, Diethelm Wallwiener, Gerhard Moldenhauer, Uwe Hahn, Alexander Marmé, Hans-Peter Zimmermann, Gunther Bastert, Brigitte Seib, and Faustino Merchán

Subjects
Cancer Research, Pathology, medicine.medical_specialty, Uterus, Breast Neoplasms, Nerve Tissue Proteins, Biology, medicine.disease_cause, Exon, Cell Line, Tumor, Neoplasms, Two-Hybrid System Techniques, Ovarian carcinoma, medicine, Humans, RNA, Messenger, Neoplasm Staging, Oligonucleotide Array Sequence Analysis, Ovarian Neoplasms, Messenger RNA, Nuclear Proteins, Cancer, Exons, medicine.disease, Gene Expression Regulation, Neoplastic, Cytoskeletal Proteins, medicine.anatomical_structure, Oncology, Tumor progression, Immunohistochemistry, Female, Carcinogenesis
Abstract

In a study on gene deregulation in ovarian carcinoma we found a mRNA coding for a 350 kDa protein, Drop1, to be downregulated 20- to 180-fold in the majority of ovarian and mammary carcinomas. The mRNA is encoded by a set of exons in the 5′ region of the SYNE1 gene. Immunohistochemical staining for Drop1 protein by a specific monoclonal antibody corresponds to the pattern seen for the mRNA. cDNA arrays of matched pairs of tumor and normal tissue and in situ hybridizations confirmed the drastic loss of Drop1 mRNA as a common feature in uterus, cervix, kidney, lung, thyroid and pancreas carcinomas, already at early tumor stages and in all metastases. Two-hybrid studies suggest a role of this deficiency in the malignant progression of epithelial tumors. © 2008 Wiley-Liss, Inc.

Published
2008
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20. Characterization of two novel cutaneous human papillomaviruses, HPV93 and HPV96

Author

Andreas Hunziker, Kristina Hazard, Nataša Vasiljević, Linda Eliasson, Hoang Ly, Ethel Michele De Villiers, Joakim Dillner, Bodil Norrild, and Ola Forslund

Subjects
Molecular Sequence Data, Genome, Viral, medicine.disease_cause, Genome, Open Reading Frames, Reference Values, Virology, medicine, Humans, RNA, Messenger, Papillomaviridae, DNA Primers, Skin, biology, Hpv types, Retinoblastoma protein, biology.organism_classification, Open reading frame, Hpv testing, DNA, Viral, biology.protein, RNA, Viral, Carcinogenesis, Viral load
Abstract

Two novel human papillomaviruses (HPVs), HPV93 and HPV96, with genomes of 7450 and 7438 bp, respectively, are described. The L1 open reading frame of HPV93 showed highest identity to HPV24 (79 %) and that of HPV96 had highest identity to HPV92 (71 %). Real-time PCR for HPV92, 93 and 96 on stripped biopsies from tumours and healthy skin from 269 immunocompetent patients found HPV DNA in 2.6 % of tumours and in 0.4 % of healthy skin samples. Double infections were observed in two tumours. HPV92 was detected in four, HPV93 in two and HPV96 in three tumours. The range of viral loads spanned from one copy per 45 cells to one copy per 10 000 cells. The E7 proteins of HPV92, 93 and 96 were found to bind the retinoblastoma protein (pRb). These results suggest a possible role for these HPV types in skin carcinogenesis that deserves further study.

Published
2007
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21. Stimme und Gebet

Author

Andreas Hunziker, University of Zurich, and Hunziker, Andreas

Subjects
10236 Institute of Theology, 230 Christianity & Christian theology, General Earth and Planetary Sciences, General Environmental Science
Abstract

There is a long during controversy about the reception of the rhetoric tradition within Christian theology. The essay focuses on the question of the relationship between voice and prayer. Against the tradition of imagining prayer as an essentially mental and inner event, which may be in the background of the grüne Heinrich’s shame about his own voice, the author underlines the essential exteriority of prayer expressed paradigmatically in the voice of prayer. This relation between prayer and voice is shown in a conversation with Martin Luther’s and Jean-Louis Chrétien’s understanding of prayer.

Published
2015

22. Isolation of Multiple TT Virus Genotypes from Spleen Biopsy Tissue from a Hodgkin's Disease Patient: Genome Reorganization and Diversity in the Hypervariable Region

Author

Ethel Michele De Villiers, Ilijas Jelcic, Andreas Hunziker, Agnes Hotz-Wagenblatt, and Harald zur Hausen

Subjects
Genotype, Sequence analysis, Biopsy, Molecular Sequence Data, Immunology, Genome, Viral, Biology, Microbiology, Virus, Virology, Genetic variation, Humans, Anelloviridae, Amino Acid Sequence, ORFS, Torque teno virus, Genetics, Base Sequence, Nucleic acid sequence, Genetic Variation, Sequence Analysis, DNA, biology.organism_classification, Hodgkin Disease, DNA Virus Infections, Hypervariable region, Insect Science, Pathogenesis and Immunity, Spleen
Abstract

We report the isolation of 24 novel genotypes of TT viruses from a surgically removed spleen of a patient with Hodgkin's disease. The sequence analysis of our 24 isolates revealed the remarkable heterogeneity of TT virus isolates not only from the same patient but also from the same biopsy material. These isolates belong to four phylogenetic groups of TT viruses. Nucleotide sequence analyses revealed five distinct genotypes (tth3, tth4, tth5, tth6, and tth7). The limited variation in sequence identity of the other isolates defines the latter as variants of four of these genotypes. A group of 6 isolates (the tth7 group) revealed a reorganization of open reading frame 1 (ORF1) leading to one larger and a varying number of smaller ORFs. The nucleotide difference of the full-length genomes was less than 1%. A variation of 69 to 97% in amino acids of a second group of 8 isolates (the tth3 group) was restricted to the hypervariable region of ORF1, indicating the existence of a quasi-species. These isolates differed by less than 2% in the remainder of their nucleotide sequences. An alignment of these isolates with 79 previously reported TT virus genotypes permits the proposal of TT virus genera and species within the family Anelloviridae in analogy to a previous proposal for the papillomaviruses (family Papillomaviridae ).

Published
2004
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23. Nucleotide sequence and phylogenetic classification of candidate human papilloma virus type 92

Author

Andreas Hunziker, Ethel Michele De Villiers, Annika Antonsson, Ola Forslund, Hajo Delius, Geoff Higgins, and Hoang Ly

Subjects
HPV, Skin Neoplasms, Genes, Viral, Cell, Genome, Viral, Biology, Genome, Complete genome, Open Reading Frames, Quantification, Virology, Carcinoma, medicine, Humans, Basal cell carcinoma, RNA, Messenger, BCC, Papillomaviridae, Gene, Phylogeny, Solar keratosis, Skin, integumentary system, Nucleic acid sequence, medicine.disease, NMSC, SCC, PCR, medicine.anatomical_structure, Carcinoma, Basal Cell, DNA, Viral, RNA, Viral, Viral load
Abstract

From a basal cell carcinoma (BCC) the complete genome of candidate human papillomavirus (HPV) type 92 was characterized. Phylogenetically, the candidate HPV 92 was relatively distantly related to other cutaneous HPV types within the B1 group. By quantitative real time PCR, 94 viral copies were present per cell in the BCC and another BCC contained 1 viral copy per cell. Lower copy numbers were found in two solar keratoses (1 copy per 33 cells and 1 copy per 60 cells) and two squamous cell carcinomas (1 copy per 436 cells and 1 copy per 1143 cells). The high viral load of HPV 92 in two BCCs differs from the low amount of HPV DNA reported from nonmelanoma skin cancers.

Published
2003
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24. Impaired membrane traffic in defective ether lipid biosynthesis

Author

Karin Gorgas, Ann B. Moser, Anna Jauch, Thanh Phuong Thai, Wilhelm W. Just, Andreas Hunziker, and Claus Rodemer

Subjects
Male, Plasmalogen, Plasmalogens, Golgi Apparatus, Transferrin receptor, Biology, Caveolae, Endoplasmic Reticulum, Peroxisomal Disorders, Mice, symbols.namesake, Receptors, Transferrin, Peroxisomal disorder, Genetics, medicine, Animals, Humans, Molecular Biology, Cells, Cultured, Genetics (clinical), Skin, Alkyl and Aryl Transferases, Endoplasmic reticulum, Chromosome Mapping, Phospholipid Ethers, Clathrin-Coated Vesicles, General Medicine, Fibroblasts, Golgi apparatus, Membrane transport, Peroxisome, medicine.disease, Endocytosis, Cell biology, Protein Transport, Phenotype, Biochemistry, Mutation, symbols, Female, Acyltransferases
Abstract

The first steps of ether lipid biosynthesis are exclusively localized to peroxisomes and hence some peroxisomal disorders are characterized by a severe deficiency of plasmalogens, the main ether lipids in humans. Here we report on gene defects of plasmalogen biosynthesis, chromosomal localization of the corresponding genes and, as a consequence of plasmalogen deficiency, on structural alterations of caveolae, clathrin-coated pits, endoplasmic reticulum and Golgi cisternae, as well as on the reduced rate of transferrin receptor cycling. The data suggest that plasmalogens, analogous to cholesterol, are essential for correct membrane functioning and their deficiency results in impaired membrane trafficking.

Published
2001
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25. [Untitled]

Author

Heinz Walter Thielmann, Andreas Hunziker, Peter Bannasch, Eiman Aleem, Thomas Flohr, and Doris Mayer

Subjects
Messenger RNA, Clinical Biochemistry, Phosphatase, Skeletal muscle, Cell Biology, General Medicine, Biology, Molecular biology, Reverse transcription polymerase chain reaction, Open reading frame, medicine.anatomical_structure, Complementary DNA, Gene expression, medicine, Northern blot, Molecular Biology
Abstract

The mRNA expression of protein phosphatase inhibitor-1 (inhibitor-1) in rat liver was demonstrated using highly sensitive semi-quantitative reverse transcription polymerase chain reaction (RT-PCR). Quantification by real-time RT-PCR (LightCycler technology) yielded the same copy number of inhibitor-1 mRNA in total rat liver and isolated hepatocytes (12 copies per cell). This novel finding shows that rat liver expresses indeed inhibitor-1 mRNA, albeit in low amounts. The low copy number explains why the mRNA had not been detected by Northern blotting so far. For comparison, about 425 copies/cell were detected in brain and 2500 copies/cell in skeletal muscle from rat. The full-length coding sequence of rat liver inhibitor-1 was cloned and sequenced, 100% homology with the muscle cDNA was obtained, indicating the expression of the same gene in liver and muscle. In vitro transcription and translation yielded a protein (Mr ~ 30 kDa) which could be detected with a specific antibody by immunoblotting. This indicates an intact open reading frame of inhibitor-1 in rat liver. Immunoblotting of liver extract yielded a very weak band which comigrated with the inhibitor-1 proteins from muscle and brain. It is concluded that mRNA expression of inhibitor-1 may have implications for the regulation of protein phosphatase-1 (PP1) in rat liver.

Published
2001
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27. Human papillomavirus type 16 E6 and E7 genotypes in head-and-neck carcinomas

Author

Claudia Lohrey, Tomas Kahn, Andreas Hunziker, Elisabeth Schwarz, and Markus Hoffmann

Subjects
Oncology, Cancer Research, medicine.medical_specialty, viruses, Papillomavirus E7 Proteins, Biology, medicine.disease_cause, Polymerase Chain Reaction, Metastasis, Internal medicine, Genotype, medicine, Carcinoma, Humans, neoplasms, Papillomaviridae, Oligonucleotide Array Sequence Analysis, Cervical cancer, Oncogene, Base Sequence, DNA, Neoplasm, Oncogene Proteins, Viral, medicine.disease, Repressor Proteins, Epidermoid carcinoma, Head and Neck Neoplasms, Lymphatic Metastasis, DNA, Viral, Mutation, Carcinoma, Squamous Cell, Oral Surgery, Carcinogenesis
Abstract

Human papillomavirus type 16 (HPV16) is associated with squamous cell carcinomas of the head and neck (HNSCC) particularly from the Waldeyer's tonsillar ring. A causal role of HPV16 in carcinogenesis is linked to the activity of the viral oncoproteins E6 and E7 which inactivate the cellular tumor suppressors p53 and pRB, respectively. Lack of E6 expression in HPV16-positive HNSCC has been reported, in some cases caused by disruption of the E6 gene. We have examined the status of the HPV16 E6-E7 gene region in tumor and metastasis samples of 24 HNSCC patients employing genomic PCR. No cases with a disrupted E6-E7 region could be identified. Sequence analysis of the E6-E7 segments revealed three different HPV16 E6-E7 genotypes: the HPV16 prototype (6 of 21 cases), the E6 variant T350G (8 of 21 cases), and the E6-E7 variant A131G/C712A (7 of 21 cases). The E6 variants T350G and A131G have been associated with increased oncogenic potential in cervical cancer patients depending on host genetic factors. Their high prevalence in the HNSCC samples studied indicates that they may be important also in HNSCC development.

Published
2003

28. The evolutionarily conserved single-copy gene for murine Tpr encodes one prevalent isoform in somatic cells and lacks paralogs in higher eukaryotes

Author

Andreas Hunziker, Linda Sandblad, Volker C. Cordes, Nikolai V. Kuznetsov, Manuela E. Hase, and Michaela Hergt

Subjects
Gene isoform, Gene Expression, Evolution, Molecular, Exon, Mice, Proto-Oncogene Proteins, Genetics, Animals, Humans, Protein Isoforms, Tissue Distribution, RNA, Messenger, Nuclear pore, Nuclear protein, Gene, Genetics (clinical), Caenorhabditis elegans, Conserved Sequence, Phylogeny, Expressed sequence tag, biology, Sequence Homology, Amino Acid, Chromosome Mapping, Nuclear Proteins, biology.organism_classification, Cosmids, Nuclear Pore Complex Proteins, genomic DNA, Eukaryotic Cells, Microscopy, Fluorescence, Sequence Alignment
Abstract

Vertebrate Tpr and its probable homologs in insects and yeast are heptad repeat-dominated nuclear proteins of M(r) 195,000 to M(r) 267,000 the functions of which are still largely unknown. Whereas two homologs exist in Saccharomyces cerevisiae, it has remained uncertain whether metazoans possess different paralogs or isoforms of Tpr that might explain controversial reports on the subcellular localization of this protein. To address these possibilities, we first determined the sequence and structure of the murine tpr gene, revealing a TATA box-less gene of approximately 57 kb and 52 exons. Southern hybridization of genomic DNA and radiation hybrid mapping showed that murine tpr exists as a single-copy gene on chromosome 1; RNA blotting analyses and EST (expressed sequence tag) database mining revealed that its expression results in only one major mRNA in embryonic and most adult tissues. Accordingly, novel antibodies against the N- and C-terminus of Tpr identified the full-length protein as the major translation product in different somatic cell types; reinvestigation of Tpr localization by confocal microscopy corroborated a predominant localization at the nuclear pore complexes in these cells. Antibody specificity and reliability of Tpr localization was demonstrated by post-transcriptional tpr gene silencing using siRNAs that eliminated the Tpr signal at the nuclear periphery but did not affect intranuclear staining of Tpr-unrelated proteins. Finally, we defined several sequence and structural features that characterize Tpr polypeptides in different species and used these as a guideline to search whole-genome sequence databases for putative paralogs of Tpr in higher eukaryotes. This approach resulted in identification of the Tpr orthologs in Arabidopsis thaliana and Caenorhabditis elegans, but also in the realization that no further paralogs of Tpr exist in several metazoan model organisms or in humans. In summary, these results reveal Tpr to be a unique protein localized at the nuclear periphery of the somatic cell in mammals.

Published
2002

29. Danzas: Europäische Distributionsnetzwerke

Author

Andreas Hunziker and Aribert Gerbode

Abstract

Im Zuge der zunehmenden Industrialisierung des „Oberrheins“ grundete Louis Ferdinand Danzas im Jahr 1815 das Familienunternehmen Danzas. Vom anfanglichen Familienbetrieb entwickelte sich das Unternehmen zu einem weltweit agierenden Speditions- und Logistik-Konzern, der bis in das Jahr 1999 selbstandig blieb. Im Marz 1999 ubernahm die Deutsche Post das Unternehmen mit dem Ziel, ihr eigenes Angebot (Paket, Brief und Bank) mit einem starken, international ausgerichteten Logistik-Dienstleister zu erweitern und zu erganzen. Die heutige Organisation der Danzas AG mit Sitz in Basel in der Schweiz besteht aus den Geschaftseinheiten EUCA, INCO sowie SOLS, die einen Profit-Center ahnlichen Charakter aufweisen (vgl. Abbildung 30). Das Gesamtbild der Organisation wird durch die Serviceeinheiten Personal-, Finanz- und EDV-Dienstleistungen abgerundet.

Published
2002
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30. Promoter of the gene encoding the 16 kDa DNA-binding and apoptosis-inducing C1D protein

Author

Karsten Rothbarth, Hermann Stammer, Andreas Hunziker, and Dieter Werner

Subjects
5' flanking region, Green Fluorescent Proteins, Molecular Sequence Data, Biophysics, Apoptosis, Biology, Transfection, Biochemistry, Green fluorescent protein, Cell Line, chemistry.chemical_compound, Mice, Structural Biology, Genetics, Animals, Humans, Promoter Regions, Genetic, Gene, Messenger RNA, Reporter gene, Base Sequence, Molecular biology, DNA-Binding Proteins, Repressor Proteins, Luminescent Proteins, Long Interspersed Nucleotide Elements, chemistry, Gene Expression Regulation, Bioreporter, Co-Repressor Proteins, DNA
Abstract

The 5′ region of the gene encoding the human 16 kDa DNA-binding and apoptosis-inducing C1D protein was analysed for promoter activity. Sections of this region were cloned into a promoterless vector containing the enhanced green fluorescent protein (EGFP) as reporter gene. Expressed EGFP was estimated in transfected cells by quantitative fluorescence microscopy. The sequence between mRNA positions ATG −868 and ATG −12 results in relatively highest EGFP expression in transiently transfected human and murine cells. The upstream segment immediately adjacent to the 5′ end of the most active fragment was identified as an inverted LINE-1 repeat element. Transient transfection experiments point to the presence of cis -acting repressing sequences on this LINE-1 element which reduce the transcriptional activity of the basal C1D promoter in human and murine cells by more than 95%. This result supports previous evidence suggesting that LINE-1 sequences may function as regulatory elements to control the expression of nearby genes.

Published
2001

31. Synthesis of plasmalogens in eye lens epithelial cells

Author

Andreas Hunziker, Thanh-Phuong Thai, Jutta Worsch, Claus Rodemer, Karin Gorgas, and Wilhelm W. Just

Subjects
DNA, Complementary, Plasmalogen, Electrospray ionization, Molecular Sequence Data, Plasmalogens, Biophysics, Peroxisome, Biochemistry, Microbodies, Cataract, chemistry.chemical_compound, Mice, Ethanolamine, Biosynthesis, Species Specificity, Structural Biology, Dihydroxyacetonephosphate acyltransferase, Complementary DNA, Peroxisomal disorder, Electrospray ionization mass spectrometry, Lens, Crystalline, Genetics, medicine, Animals, Humans, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, Alkyl and Aryl Transferases, ATP synthase, biology, Base Sequence, Sequence Homology, Amino Acid, Chemistry, Epithelial Cells, Cell Biology, Lens epithelial cell, medicine.disease, Microscopy, Electron, Eye lens, biology.protein, Acyltransferases
Abstract

The present paper describes cloning and sequencing of the mouse cDNA encoding dihydroxyacetonephosphate acyltransferase (DAPAT), the peroxisomal key enzyme of plasmalogen (PM) biosynthesis. Using monospecific antibodies, we localized DAPAT and alkyl dihydroxyacetonephosphate synthase to peroxisomes of mouse lens epithelial cells (LECs) and determined their enzymatic activity. By electrospray ionization mass spectrometry of mouse lens lipid extracts, we identified phosphatidyl ethanolamine including plasmenyl ethanolamine species as major constituents. Our data demonstrate the capacity of LECs to synthesize PMs and the high coincidence between deficiency of PM and early manifestation of cataract in patients with peroxisomal disorders suggests that ether-bonded lipids may play an important role in maintaining lens transparency.

Published
1999

32. Differential display PCR reveals induction of immediate early genes by vasoactive intestinal peptide in PC12 cells

Author

Andreas Hunziker, Lars Klimaschewski, and Andreas Eschelbach

Subjects
DNA, Complementary, Transcription, Genetic, Vasoactive intestinal peptide, Molecular Sequence Data, Biology, PC12 Cells, General Biochemistry, Genetics and Molecular Biology, Immediate-Early Proteins, History and Philosophy of Science, Sequence Homology, Nucleic Acid, Animals, Genes, Tumor Suppressor, RNA, Messenger, Cloning, Molecular, Gene, Genes, Immediate-Early, Southern blot, Differential display, Messenger RNA, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, General Neuroscience, RNA, Membrane Proteins, Proteins, Molecular biology, Rats, Gene Expression Regulation, Neoplastic, Nucleic acid, Primer (molecular biology), Sequence Alignment, Vasoactive Intestinal Peptide
Abstract

In order to identify genes regulated by vasoactive intestinal peptide, we performed differential display PCR as originally described by Liang and Pardee. Messenger RNA of PC12 cells treated with vasoactive intestinal peptide or nerve growth factor for one hour was reverse transcribed and amplified using different sets of oligo-dT and random primers. Radioactively labeled PCR products were displayed on polyacrylamide gels and candidate cDNAs extracted from the gel, re-amplified by PCR, cloned, and sequenced. Differential expression was verified by RT-PCR applying sets of specific primers obtained from the sequence. The specificity of the PCR product was confirmed by Southern blotting using a radioactively labeled internal primer and semi-quantitative densitometric analysis. This rapid and sensitive protocol led to the isolation of two immediate early genes, pip92 and PC4, known to be increased on mRNA level by nerve growth factor in PC 12 cells.

Published
1999

33. Ether lipid biosynthesis: isolation and molecular characterization of human dihydroxyacetonephosphate acyltransferase

Author

Karin Gorgas, Andreas Hunziker, Hans-Richard Rackwitz, Hans Heid, Wilhelm W. Just, and Thanh-Phuong Thai

Subjects
Sequence analysis, Molecular Sequence Data, Biophysics, Peptide, Protein Sorting Signals, Biology, Microbodies, Biochemistry, Plasmalogen, Structural Biology, Dihydroxyacetonephosphate acyltransferase, Complementary DNA, Centrifugation, Density Gradient, Genetics, Animals, Humans, Ether lipid biosynthesis, Amino Acid Sequence, Cloning, Molecular, Microscopy, Immunoelectron, Molecular Biology, Peptide sequence, Peroxisomal targeting signal, chemistry.chemical_classification, Base Sequence, Molecular mass, Harderian Gland, cDNA library, Brain, Phospholipid Ethers, Sequence Analysis, DNA, Cell Biology, Peroxisome, Precipitin Tests, Molecular biology, Peptide Fragments, chemistry, Alkyldihydroxyacetonephosphate synthase, Electrophoresis, Polyacrylamide Gel, Rabbits, Acyltransferases
Abstract

In this paper we describe isolation and molecular characterization of human dihydroxyacetonephosphate acyltransferase (DAP-AT). The enzyme was extracted from rabbit Harderian gland peroxisomes and isolated as a trimeric complex by sucrose density gradient centrifugation. From peptide sequences matching EST-clones were obtained which allowed cloning and sequencing of the cDNA from a human cDNA library. The nucleotide-derived amino acid sequence revealed a protein consisting of 680 amino acid residues of molecular mass 77 187 containing a C-terminal type 1 peroxisomal targeting signal. Monospecific antibodies raised against this polypeptide efficiently immunoprecipitated DAP-AT activity from solubilized peroxisomal preparations, thus demonstrating that the cloned cDNA codes for DAP-AT.

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34. Targeting of the 22 kDa integral peroxisomal membrane protein

Author

Rainer Saffrich, Andreas Hunziker, Wilhelm Ansorge, Birgit Pause, and Wilhelm W. Just

Subjects
Peroxisomal membrane, Recombinant Fusion Proteins, Amino Acid Motifs, Green Fluorescent Proteins, Molecular Sequence Data, Biophysics, CHO Cells, Biology, Peroxisome, medicine.disease_cause, Transfection, Biochemistry, Structural Biology, Cricetinae, Protein targeting, Genetics, medicine, Peroxisomes, Animals, Amino Acid Sequence, Molecular Biology, Peroxisomal targeting signal, Peroxisomal membrane protein, Sequence Homology, Amino Acid, Conserved motif, Membrane Proteins, Pmp22p, Biological Transport, Cell Biology, Intracellular Membranes, Membrane targeting signal, Transmembrane protein, Peroxisomal membrane targeting, Molecular Weight, Luminescent Proteins, Membrane, Cytoplasm, Signal Transduction
Abstract

Investigating targeting of the 22 kDa peroxisomal membrane protein (Pmp22p) to the peroxisomal membrane we have confined the targeting signal to amino acid residues 16–37 located in the N-terminal cytoplasmic tail. Comparison of Pmp22p orthologous sequences revealed a conserved motif Y3xL3xP3x(KQN) which might represent the core of this targeting signal not found so far in other Pmps. Fusion of the Pmp22p N-terminal tail to the C-terminal portion of Pmp22p which per se is not targeted to peroxisomes, conveys peroxisomal targeting. These data suggest that Pmp22p is targeted to peroxisomes by a new membrane targeting signal which is necessary and sufficient to target a polypeptide containing two transmembrane spans to peroxisomes.

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