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THE CHARACTERIZATION OF ANTIZYME IN DEVELOPING Xenopus laevis EMBRYOS Alexandra Silveira and Charles Toth Department of Biology Providence College, Providence, RI Protein Degradation Cell cycle and proliferation Differentiation and development Stress response Genesis of neural networks Modulation of cell surface receptors Regulation of immune response Apoptosis Transcriptional regulation Pathogenesis – Cancer, cystic fibrosis, neurodegenerative diseases Charles Toth, Providence College Protein degradation by the 26S proteasome http://www.rpi.edu/dept/bcbp/molbiochem/MBWeb/mb2/part1/protease.htm Protein degradation by the 26S proteasome ODC degradation – a unique protein degradation pathway John Mitchell, University of Northern Iowa John Mitchell, University of Northern Iowa ODC and Polyamine Biosynthesis http://www.bios.niu.edu/mitchellab/general.html Polyamines Organic compounds found bound to RNA and DNA in cells High levels are toxic Necessary for cell growth and survival – gate currents of ion channels – have effects on chromatin condensation and transcriptional regulation – neutralize negative charges of RNA and DNA – regulate the levels of AZ – provide a necessary postranslational modification to eIF-5a protein http://www.biol.lu.se/zoofysiol/Cellprolif/Research/research_area_1.html AZ Functions ODC degradation Anti-proliferative effect on cells Blocks uptake of additional polyamines when polyamine levels are too high High levels of polyamines in turn regulate AZ through a ribosomal frameshift http://www.bios.niu.edu/mitchellab/general.html Ribosomal Frame-Shifting High levels of polyamines cause a ribosomal frame shift that produces an active form of AZ. Without the ribosomal shift a truncated and inactive AZ is formed. Why study antizyme? Studying the unique ODC degradation pathway can lead to a better understanding of – ubiquitin mediated protein degradation – the many roles of polyamines in the cell AZ is a member of an ancient gene family – AZ1 and AZ2 widely expressed and involved in ODC degradation – AZ3 is testis specific Why study antizyme? AZ has been cloned from various organisms – vertebrate-man, chicken, rat, mouse, zebrafish, Xenopus, electric ray – invertebrate-Drosophila, S. pombe, C. elegans, silk worms, gray mold, etc. AZ knockout in mice (Matsufuji & Noda) – viable and morphologically normal – high rate of prenatal fatality from high levels of ODC – phenotype complicated by additional family members Xenopus As A Developmental Model Ideal model because: – easily cared for in lab – in vitro fertilization – the developing embryos are easily cared for – the embryos develop quickly http://www.xenopus.com/products.htm Xenopus life cycle Wolpert et al., Development 2000 Methods In vitro fertilization Northern Blot Immunohistochemical Staining In Vitro Fertilization Female frogs are injected with HCG to induce ovulation Male frogs are sacrificed in order to obtain internal testicles Eggs are fertilized in vitro http://www.fundamentalbiology.arc.nasa.gov/Image1.jpg Northern blot analysis www.columbia.edu/.../c2005/handouts/ northernforweb.gif Northern blot results AZ is expressed as a maternal and zygotic transcript Size of message increases post-MBT – MBT is the point where zygotic genes are expressed instead of maternal genes and the cell cycle becomes asynchronous indicating the beginning of differentiation Charles Toth, Providence College Conclusions Different sizes of antizyme mRNA are present during different times in embryonic development. A larger mRNA message is present postMBT. Possible Implications The larger messages can indicate a – a closely related familial gene – different post-transcriptional modifications that ensure zygotic gene expression Results are inconclusive because of the ribosomal frame-shift needed to produce an active form of AZ. Immunohistochemical Staining Antibodies against antizyme are used to detect and stain antizyme in the developing embryo. http://www-celanphy.sci.kun.nl/Bruce%20web/Bruce%20Gifs/immunocyto.gif Immunohistochemical Staining Results Stage 10 embryos There is a darkly staining ring around the blastopore from which the mesoderm will develop. The animal cap is almost uniformly stained. Immunohistochemical Staining Results Stage 18/19 Top image: – staining along the neural groove and at both the anterior and posterior ends of the embryo, some staining at the ventral side Bottom image: – dorsal side shows dark staining at the posterior and anterior ends and a ring pattern of staining in the area that will eventually give rise to the mesoderm Immunohistochemical Staining Results Stage 33/34 Staining is primarily focused around the somites and the anterior end of the tadpole These locations are where the muscles and nerves are developing Conclusions There is clearly a differential expression of antizyme during the various stages of embryonic development. – staining of ring around the blastopore and animal cap – staining of the neural groove, anterior and posterior ends, ventral, and dorsal lateral staining – staining of the somites and anterior portion of the tadpole Possible Implications The staining around the blastopore ring, the dorsal-lateral staining of the neurula, and the somite staining of the tadpole implicate a role of antizyme in muscle development. The staining of the animal cap and the anterior end of the developing embryo implicate a role of antizyme in the development of the central nervous system. Future Endeavors In situ Western ablation studies forced expression Acknowledgements Dr. Charles Toth Dr. Senya Matsufuji – Jikei University, Tokyo Tiffany LaFortune My family My roommates