DFG Research Group FOR855

    Prof. Dr. Elmar Wahle

    Project Summary:

    Deadenylation is the first and often rate-limiting step in mRNA decay. Deadenylation is also used as a means of translational repression. Translation of the nanos (nos) mRNA of Drosophila is repressed by the protein Smaug. Smaug also induces deadenylation by the CCR4-NOT complex. We have reproduced both deadenylation and translational repression in extracts of Drosophila embryos. The deadenylation activity, which is associated with rapidly sedimenting particles, depends on the Smaug binding sites in the RNA and on an ATP-regenerating system. Micrococcal nuclease inhibits the reaction. The proposal aims to identify the factors responsible for the reaction by an affinity purification approach with the goal of analyzing the mechanism of accelerated deadenylation. Deadenylation contributes to translational repression of nos, but a second, deadenylation-independent mechanism is also operating. We will test the model that repression depends on Smaug-dependent recruitment of the protein Cup, which then displaces the initiation factor eIF4G from the cap-binding protein eIF4E. We will also examine whether the repressed nos mRNA is in fact on polysomes, as previously reported, or whether it forms non-polysomal repressed RNPs. We will examine which role the factors identified by affinity-purification play in translational repression.

    Selected publications (2007-09):

    1. Bönisch, C., Temme, C., Moritz, B, Wahle, E. (2007) Degradation of hsp70 and other mRNAs in Drosophila via the 5'-3' pathway and its regulation by heat shock. J. Biol. Chem., 282, 21818 - 21828.

    2. Fronz, K., Otto, S., Kölbel, K., Kühn, U., Friedrich, H., Schierhorn, A., Beck-Sickinger, A. G., Ostareck-Lederer, A., Wahle, E. (2008) Promiscuous modification of the nuclear poly(A) binding protein by multiple protein arginine methyl transferases does not affect the aggregation behavior. J. Biol. Chem. 283, 20408-20420.

    3. Jeske, M., Wahle, E. (2008) Cell-free deadenylation assays using Drosophila embryo extracts. Methods Enzymol. 448, 107-118.

    4. Weidensdorfer, D., Stöhr, N., Baude, A., Lederer, M., Köhn, M., Schierhorn, A., Buchmeier, S., Wahle, E., Hüttelmaier, S. (2009) Control of c-myc mRNA stability by IGF2BP1 associated cytoplasmic RNPs. RNA 15, 104-115.

    5. Temme, C., Weissbach, R., Lilie, H., Wilson, C., Meinhart, A., Meyer, S., Golbik, R., Schierhorn, A., Wahle, E. (2009) The Drosophila melanogaster gene CG4930 encodes a high affinity inhibitor for endonuclease G. J. Biol. Chem. 284, 8337-8348.

    6. Kölbel, K., Ihling, C., Bellmann-Sickert, K., Neundorf, I., Beck-Sickinger, A. G., Sinz, A., Kühn, U., Wahle, E. (2009) Type I arginine methyl transferases PRMT1 and 3 act distributively. J. Biol. Chem. 284, 8274-8282.

    7. Kühn, U., Gündel, M., Knoth, A., Kerwitz, Y., Rüdel. S., Wahle, E. (2009) Poly(A) tail length is controlled by the nuclear poly(A) binding protein regulating the interaction between poly(A) polymerase and the cleavage and polyadenylation specificity factor. J. Biol. Chem. 284, 22803-22814.

    8. Loll, B., Gebhardt, M., Wahle, E., Meinhart, A. (2009) Crystal structure of the EndoG/EndoGI complex: Mechanism of EndoG inhibition. Nucleic Acids Res., im Druck.

    Kontakt

    Universität Würzburg
    Sanderring 2
    97070 Würzburg

    Tel.: +49 931 31-0
    Fax: +49 931 31-82600

    Suche Ansprechpartner

    Sanderring Röntgenring Hubland Nord Hubland Süd Campus Medizin