Your search keyword '"Matthias Kübler"' showing total 2 results

1. Identification of a Novel Ran Binding Protein 2 Related Gene (RANBP2L1) and Detection of a Gene Cluster on Human Chromosome 2q11–q12

Author

David M. Kurnit, Birgit Brandl, Dagmar Denich, Matthias Kübler, Mike Stubanus, Hans Gerd Nothwang, Friedhelm Hildebrandt, Cornelia Rensing, and Thomas Haaf

Subjects

DNA, Complementary, Sequence analysis, Molecular Sequence Data, Biology, Homology (biology), Fetus, Gene cluster, Gene duplication, Genetics, Humans, Amino Acid Sequence, Cloning, Molecular, Peptide sequence, Base Sequence, Sequence Homology, Amino Acid, cDNA library, Binding protein, Nucleic acid sequence, Brain, Chromosome Mapping, Nuclear Proteins, Molecular biology, DNA-Binding Proteins, Nuclear Pore Complex Proteins, Chromosomes, Human, Pair 2, Multigene Family, Molecular Chaperones

Abstract

The giant 358-kDa protein Ran binding protein 2 (RanBP2/Nup358) is localized at the cytoplasmic side of the nuclear pore complex and likely constitutes the Ran-GTP binding site at the cytoplasmic face of the complex. RanBP2/Nup358 furthermore acts as a chaperone for red/green opsin molecules. Here, we report on the physical mapping of human RanBP2 between markers D2S340 and D2S1893. A duplication of the 5'-end sequence of RanBP2 occurs within 3 Mb distal to RanBP2. Detailed sequence analysis resulted in primers specific for this distal duplication. Polymerase chain reaction-based screening of cDNA libraries indicates that this transcript, called RanBP2alpha (HGMW-approved symbol RANBP2L1), is expressed in several tissues. Screening of a fetal brain cDNA library yielded a 4057-bp partial cDNA clone for RanBP2alpha. Its 5'-end is almost identical to RanBP2, whereas its 3'-part is distinct from RanBP2. Northern blot analysis using a probe of the 3'-untranslated sequence of RanBP2alpha detected in several tissues an 8-kb transcript representing the full length of the transcript. In pancreas and placenta, an additional transcript of 14 kb was detected. PAC clones containing the bona fide RanBP2 sequences were localized to 2q11-q12 by FISH analysis, and a region of high similarity was detected on 2p11-p12. In summary, we have identified a RanBP2 gene cluster on 2q11-q12 together with a novel gene termed RanBP2alpha, with high sequence similarity to RanBP2.

Published

1998

2. Construction of a Gene Map of the Nephronophthisis Type 1 (NPHP1) Region on Human Chromosome 2q12–q13

Author

Antoaneta Mincheva, Urs Vossmerbäumer, Peter Lichter, Matthias Kübler, Helge Hanusch, Hans Gerd Nothwang, Friedhelm Hildebrandt, Jörn Adolphs, Dagmar Denich, and Mike Stubanus

Subjects

Genetic Markers, government.form_of_government, Molecular Sequence Data, Biology, medicine.disease_cause, Gene mapping, Complementary DNA, Genetics, medicine, Humans, Juvenile nephronophthisis, Cloning, Molecular, Gene, Adaptor Proteins, Signal Transducing, Polycystic Kidney Diseases, Expressed sequence tag, Mutation, Base Sequence, Contig, Homozygote, Chromosome Mapping, Membrane Proteins, Proteins, food and beverages, Cytoskeletal Proteins, Chromosomes, Human, Pair 2, Multigene Family, government, Kidney disorder, Gene Deletion

Abstract

A gene for the autosomal recessive kidney disorder juvenile nephronophthisis (NPH) is located on chromosome 2q between markers D2S1893 and D2S1888. Recently, the presence of large homozygous deletions was described in the majority of NPH patients. We constructed an integrated YAC/PAC contig of 54 markers and 30 PAC clones that encompasses this deletion and the flanking inverted duplication. Thirty-six novel sequence-tagged site markers were generated for this region of 2–3 Mb, 22 of which represent PAC ends. Ten of 18 multiplex NPH families show a homozygous deletion for 8 consecutive markers. BlastN database search and expressed sequence tag (EST) mapping led to the localization of 18 EST clones to the integrated contig, representing 11 putative transcribed sequences. Seven EST clones were localized to the NPHP1 region between D2S1893 and D2S1888. Two EST clones, zc07a11 from a human parathyroid tumor library and yy63e10 from a multiple sclerosis lesion library, are located in the deletion region. PCR amplification experiments indicate that zc07a11 represents a chimeric cDNA. Through FISH analysis the NPHP1 deletion region was localized to 2q12–q13. In summary, our study provides a high-resolution physical map of the NPHP1 region with 7 precisely localized expressed sequences, 2 of which have recently been shown to be part of a gene for NPH. These data will alleviate the identification of further genes of a homozygous gene deletion syndrome in patients with NPH and oculomotor apraxia and will be instrumental in the characterization of the molecular mechanism leading to the large homozygous deletion in this region. The data furthermore provide an important step toward the construction of a sequence-ready PAC contig of this region.

Published

1998