Schenkel | RNP Particles, Splicing and Autoimmune Diseases | Buch | 978-3-642-48975-4 | sack.de

Buch, Englisch, 225 Seiten, Format (B × H): 155 mm x 235 mm, Gewicht: 365 g

Reihe: Springer Lab Manuals

Schenkel

RNP Particles, Splicing and Autoimmune Diseases


1998
ISBN: 978-3-642-48975-4
Verlag: Springer

Buch, Englisch, 225 Seiten, Format (B × H): 155 mm x 235 mm, Gewicht: 365 g

Reihe: Springer Lab Manuals

ISBN: 978-3-642-48975-4
Verlag: Springer


The first insights into the site and mechanisms of RNA process­ ing to functional mRNA in eukaryotic cells came from the group of Georgiev (Lukanidin et al. 1972) who demonstrated the association of rapidly labelled, heterogeneous nuclear RNA (hnRNA) with a limited number of specific proteins in the cell nucleus. These "informofers", i. e. packaged precursors of mRNA (pre-mRNA or hnRNA), are in a form presumably amenable to the action of nucleases. With the availability of better analytical techniques, the considerable heterogeneity of hnRNA associated proteins was revealed (Niessing and Sekeris 1970), suggesting a role that was more composite, rather than solely structural, for these proteins. Later studies investigated the RNA binding behavior of these proteins (Schenkel et al. 1988, 1989; Wilk et al. 1983). For a long time, the small nuclear RNAs, well characterized with respect to primary structure (reviewed by Reddy and Busch 1983), were naively ignored regarding their function. Several events then set the stage for a detailed study of the intricate mechanisms of the splicing process and other steps involved in hnRNA processing: (1) The demonstration of a second class of nuclear ribonucleoproteins (RNPs), composed of small nuclear RNAs (snRNAs) and another characteristic group ofheterogene­ ous proteins (Lerner et al. 1980; Guialis et al. 1983); (2) the detec­ tion of the association of snRNPs with hnRNPs by virtue of base pairing between hnRNA and snRNA (Flytzanis et al.

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Weitere Infos & Material


1 Isolation and Immunochemical Characterization of hnRNP Particles.- 2 The lnRNP Particle — A Naturally Assembled Complex of Pre-mRNA and Splicing Factors.- 3 Intrinsic Fluorescence Techniques for Studies on Protein-Protein and Protein-RNA Interactions in RNP Particles.- 4 Procedures for Three-Dimensional Reconstruction from Thin Sections with Electron Tomography.- 5 Purification and Electron Microscopy of Spliceosomal snRNPs.- 6 Detection of Autoantibodies to Extractable Cellular Antigens.- 7 Methods in Immunolocalization of Autoantigens.- 8 In vitro Splicing of Pre-mRNA in HeLa Extracts.- Abbreviations.



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