@article{Scheer1982,
  author    = {Scheer, Ulrich},
  title     = {Biologische Objekte im Transmissions-Elektronenmikroskop (Teil 4): Spreitungstechniken},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-39652},
  year      = {1982},
  abstract  = {Visualizing nucleic acids (DNA, RNA), nucleoprotein complexes and chromatin requires the use of special electron microscopicspreading techniques. In part 4 (27 refs.), methods are outlined for spreading DNA and RNA molecules for electron microscopic observation, these methods using modifications of the basic protein film method developed by A. Kleinschmidt and R. K. Zahn (1959). Hybridization techniques that allow the observation of heteroduplexes formed between two DNA molecules or between DNA and RNA molecules are reviewed, with special emphasis being placed on the DNA-RNA hybrids as a tool for elucidating RNA splicing. Techniques for studying DNA-protein interactions without the use of a protein monolayer film are mentioned. Finally, the "Miller spreading technique" for visualizing the nucleosomal organization of eukaryotic chromatin as well as the transcription of genes is discribed and illustrated.},
  language  = {de}
}
@inproceedings{FrankeScheer1975,
  author    = {Franke, Werner W. and Scheer, Ulrich},
  title     = {Biochemical and structural aspects of nucleocytoplasmic transfer of ribonucleoproteins at the nuclear envelope level: facts and theses},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-33766},
  year      = {1975},
  abstract  = {No abstract available},
  language  = {en}
}
@article{ReimerRoseScheeretal.1987,
  author    = {Reimer, Georg and Rose, Kathleen M. and Scheer, Ulrich and Tan, Eng M.},
  title     = {Autoantibody to RNA polymerase I in scleroderma sera},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-34294},
  year      = {1987},
  abstract  = {Autoantibodies to components of the nucleolus are a unique serological feature of patients with scleroderma. There are autoantibodies of several specificities; one type produces a speckled pattern of nucleolar staining in immunofluorescence. In actinomycin D and 5,6-dichloro-{j-D-ribofuranosylbenzimidazoletreated Vero cells, staining was restricted to the fibrillar and not the granular regions. By double immunofluorescence, specific rabbit anti-RNA polymerase I antibodies stained the same fibrillar structures in drug-segregated nucleoli as scleroderma sera. Scleroderma sera immunoprecipitated 13 polypeptides from (35S)methionine-labeled HeLa cell extract with molecular weights ranging from 210,000 to 14,000. Similar polypeptides were precipitated by rabbit anti-RNA polymerase I antibodies, and their common identities were confirmed in immunoabsorption experiments. Microinjection of purified IgG from a patient with speckled nucleolar staining effectively inhibited ribosomal RNA transcription. Autoantibodies to RNA polymerase I were restricted to certain patients with scleroderma and were not found in other autoimmune diseases.},
  language  = {en}
}
@article{RoseSzopaHanetal.1988,
  author    = {Rose, Kathleen M. and Szopa, Jan and Han, Fu-Sheng and Cheng, Yung-Chi and Richter, Arndt and Scheer, Ulrich},
  title     = {Association of DNA topoisomerase I and RNA polymerase I: A possible role for topoisomerase I in ribosomal gene transcription},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-33901},
  year      = {1988},
  abstract  = {RNA polymerase I preparations purified from a rat hepatoma contained DNA topoisomerase activity. The DNA topoisomerase associated with the polymerase had an Mr of 110000, required Mg2+ but not ATP, and was recognized by anti-topoisomerase I antibodies. When added to RNA polymerase I preparations containing topoisomerase activity, anti-topoisomerase I antibodies were able to inhibit the DNA relaxing activity of the preparation as well as RNA synthesis in vitro. RNA polymerase II prepared by analogous procedures did not contain topoisomerase activity and was not recognized by the antibodies. The topoisomerase I: polymerase I complex was reversibly dissociated by column chromatography on Sephacryl S200 in the presence of 0.25 M (NH4hS04. Topoisomerase I was immunolocalized in the transcriptionally active ribosomal gene complex containing RNA polymerase I in situ. These data indicate that topoisomerase I and RNA polymerase I are tightly complexed both in vivo and in vitro, and suggest a role for DNA topoisomerase I in the transcription of ribosomal genes.},
  language  = {en}
}
@misc{FischerWeissenbergerScheer1991,
  author    = {Fischer, Dagmar and Weißenberger, Dieter and Scheer, Ulrich},
  title     = {Assigning functions to nucleolar structures},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-34258},
  year      = {1991},
  abstract  = {Nucleoli provide the fascinating possibility of linking morphologically distinct structures such as those seen in the electron microscope with biochemical f eatures of the formation and step wise maturation of ribosomes. Localization of proteins by immunocytochemistry and of rRNA genes and their transcripts by in situ hybridization has greatly improved our understanding of the structural-functional relationships of the nucleolus. The present review describes some recent results obtained by electron microscopic in situ hybridization and argues that this approach has the potential to correlate each step of the complex pre-rRNA maturation pathway with nucleolar structures. Evidence is accumulating that the nucleolus-specific U3 snRNPs (small nuclear ribonucleoprotein particles) participate in rRNA processing events, similar to the role played by the nucleoplasmic snRNPs in mRNA maturation. The intranucleolar distribution of U3 snRNA is consistent with the view that it is involved in both early and late stages of pre-rRNA processing.},
  language  = {en}
}
@misc{DabauvalleScheer1991,
  author    = {Dabauvalle, Marie-Christine and Scheer, Ulrich},
  title     = {Assembly of nuclear pore complexes in Xenopus egg extract},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-41194},
  year      = {1991},
  abstract  = {No abstract available},
  language  = {en}
}
@article{BonaScheerBautz1981,
  author    = {Bona, Marion and Scheer, Ulrich and Bautz, Ekkehard K. F.},
  title     = {Antibodies to RNA polymerase II (B) inhibit transcription in lampbrush chromosomes after microinjection into living amphibian oocytes},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-33128},
  year      = {1981},
  abstract  = {Antibodies directed against RNA polymerase II (B) from Drosophila melanogaster were obtained from rabbit sera and, as monoclonal immunoglobulins, from mouse hybridomas and shown to cross-react with the amphibian enzyme protein. Localization by indirect immunofluorescence microscopy revealed the association of this enzyme with chromatin of interphase nuclei of amphibian cells and its absence in nucleoli. Purified immunoglobulins were microinjected in to nuclei ofliving vitellogenic oocytes of Ple1lrodeles waltlii and X enopus laevis and their effects on transcriptional processes were monitored by biochemical and light and electron microscopic stud ies. RNA polymerase II antibodies from rabbit sera caused a rapid and almost complete release of nascent transcripts from the chromatin axis of the loops of lampbrush chromosomes, followed by collapse of the loops and their retraction on the main chromosome axis. Monoclonal murine antibodies to the Iarge RNA polymerase II subunits also inhibited transcription in chromosome Ioops but appeared to inhibit initiation rather than elongation events. Activities of class land III RNA polymerases were not significantly affected by injection of antibodies to polymerase II, indicating immunological differences between the three RNA polymerases. The potential value of the in vitro test system described , as a very sensitive assay for detecting proteins involved in transcription in living cells, is discussed. 1},
  language  = {en}
}
@article{ScheerFranke1972,
  author    = {Scheer, Ulrich and Franke, Werner W.},
  title     = {Annulate lamellae in plant cells: formation during microsporogenesis and pollen development in Canna generalis Bailey},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-32160},
  year      = {1972},
  abstract  = {The occurrence of stacked annulate tamellae is documented for a plant cell system, namely for pollen mother cells and developing pollen grains of Canna generalis. Their structural subarchiteeture and relationship to endoplasmie reticulum (ER) and nuclear envelope cisternae is described in detail. The results demonstrate structural homology between plant and animal annulate lamellae and are compatible with, though do not prove, the view that annulate lamcllar cisternae may originate as a degenerative form of endoplasmic retieulum.},
  language  = {en}
}
@article{EckertFrankeScheer1972,
  author    = {Eckert, W. A. and Franke, Werner W. and Scheer, Ulrich},
  title     = {Actinomycin D and the central granules in the nuclear pore complex: thin sectioning versus negative staining},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-40636},
  year      = {1972},
  abstract  = {Thin section electron microscopy of Actinomycin D treated Tetrahymena cells and amphibian oocytes (Xenopus laevis, Triturus aZpestris) reveal no reduction in the central granules in the nuclear pore complexes. Possible reasons for the diversity between these results and earlier observations using negatively stained isolated nuclear envelopes from the same objects are discussed. The results clearly show that the presence of central granules within the nuclear pores does neither depend on nuclear RNA synthesis nor does indicate nucleocytoplasmic RNA transport. This conclusion leads to a reconsideration of the nature of the central granule. The functioning of the central granule of the nuclear pore complexes is further discussed in connection with recent studies on the ultrastructure of various types of cisternal pores.},
  language  = {en}
}
@article{HockMoormannFischeretal.1993,
  author    = {Hock, Robert and Moormann, Antoon and Fischer, Dagmar and Scheer, Ulrich},
  title     = {Absence of somatic histone H1 in oocytes and preblastula embryos of Xenopus laevis},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-41350},
  year      = {1993},
  abstract  = {Available data on the occurrence and expression of somatic histone HI during oogenesis and early embryogenesis of Xenopus laevis are contradictory. In particular the reported presence of a large storage pool of histone HIA in oocytes is difficult to reconcile with the high transcriptional activity of all gene classes in this specific cell type. In the present study we have used polyclonal antibodies raised against somatic Xenopus histone HI (HIA and HIA/B) for combined immunoblotting experiments to quantitate HI pools and immunolocalization studies to visualize chromosome- bound HI. Both approaches failed to detect soluble or chromosomal histone HI in vitellogenic oocytes, eggs, and cleavage-stage embryos up to early blastula. In addition, chromatin assembled in Xenopus egg extract was also negative for histone HI as revealed by immunofluorescence microscopy. Lampbrush chromosomes not only lacked histone HI but also the previously identified histone HI-like B4 protein (Smith et al., 1988, Genes Dev. 2,1284-1295). In contrast, chromosomes of eggs and early embryos fluoresced brightly with anti-B4 antibodies. Our results lend further support to the view that histone HI expression is developmentally regulated during Xenopus oogenesis and embryogenesis similar to what is known from other species.},
  language  = {en}
}