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Autor: Ivics, Zoltán

4 záznamů v Medvik Filtry

Článek

Nuclear inclusions of pathogenic ataxin-1 induce oxidative stress and perturb the protein synthesis machinery

Laidou, Stamatia
Autor Laidou, Stamatia Institute of Applied Biosciences/Centre for Research and Technology Hellas, 57001, Thessaloniki, Greece
Alanis-Lobato, Gregorio
Autor Alanis-Lobato, Gregorio Faculty of Biology, Johannes Gutenberg University Mainz, 55122, Mainz, Germany Human Embryo and Stem Cell Laboratory, The Francis Crick Institute, NW1 1AT, London, UK
Pribyl, Jan
Autor Pribyl, Jan Central European Institute of Technology, Masaryk University, 62500, Brno, Czech Republic
Raskó, Tamás
Autor Raskó, Tamás Max-Delbrueck-Center for Molecular Medicine in the Helmholtz Association, Berlin, 13125, Germany
Tichý, Boris
Autor Autorita Central European Institute of Technology, Masaryk University, 62500, Brno, Czech Republic
Mikulasek, Kamil
Autor Mikulasek, Kamil Central European Institute of Technology, Masaryk University, 62500, Brno, Czech Republic National Centre for Biomolecular Research, Faculty of Science, Masaryk University, 62500, Brno, Czech Republic
Tsagiopoulou, Maria
Autor Tsagiopoulou, Maria Institute of Applied Biosciences/Centre for Research and Technology Hellas, 57001, Thessaloniki, Greece
Oppelt, Jan
Autor Oppelt, Jan Central European Institute of Technology, Masaryk University, 62500, Brno, Czech Republic
Kastrinaki, Georgia
Autor Kastrinaki, Georgia Aerosol and Particle Technology Laboratory/Chemical Process & Energy Resources Institute/Centre for Research and Technology Hellas, 57001, Thessaloniki, Greece
Lefaki, Maria
Autor Lefaki, Maria Institute of Biology, Medicinal Chemistry & Biotechnology/National Hellenic Research Foundation, 11365, Athens, Greece

Redox biology. 2020 ; 32 (-) : 101458. [pub] 20200211

Redox Biol
ISSN 2213-2317
Medvik
Zdroj

Spinocerebellar ataxia type-1 (SCA1) is caused by an abnormally expanded polyglutamine (polyQ) tract in ataxin-1. These expansions are responsible for protein misfolding and self-assembly into intranuclear inclusion bodies (IIBs) that are somehow linked to neuronal death. However, owing to lack of a suitable cellular model, the downstream consequences of IIB formation are yet to be resolved. Here, we describe a nuclear protein aggregation model of pathogenic human ataxin-1 and characterize IIB effects. Using an inducible Sleeping Beauty transposon system, we overexpressed the ATXN1(Q82) gene in human mesenchymal stem cells that are resistant to the early cytotoxic effects caused by the expression of the mutant protein. We characterized the structure and the protein composition of insoluble polyQ IIBs which gradually occupy the nuclei and are responsible for the generation of reactive oxygen species. In response to their formation, our transcriptome analysis reveals a cerebellum-specific perturbed protein interaction network, primarily affecting protein synthesis. We propose that insoluble polyQ IIBs cause oxidative and nucleolar stress and affect the assembly of the ribosome by capturing or down-regulating essential components. The inducible cell system can be utilized to decipher the cellular consequences of polyQ protein aggregation. Our strategy provides a broadly applicable methodology for studying polyQ diseases.

MeSH
ataxin-1 genetika metabolismus MeSH
intranukleární inkluzní tělíska * metabolismus MeSH
jaderné proteiny genetika metabolismus MeSH
lidé MeSH
oxidační stres MeSH
proteiny nervové tkáně * genetika metabolismus MeSH
Check Tag
lidé MeSH
Publikační typ
časopisecké články MeSH
práce podpořená grantem MeSH

Článek

Germline transgenesis in pigs by cytoplasmic microinjection of Sleeping Beauty transposons

Nature protocols. 2014 ; 9 (4) : 810-27.

Nat Protoc
ISSN 1750-2799
Medvik
Zdroj

The pig has emerged as an important large animal model in biomedical and pharmaceutical research. We describe a protocol for high-efficiency germline transgenesis and sustained transgene expression in pigs by using the Sleeping Beauty (SB) transposon system. The protocol is based on co-injection of a plasmid encoding the SB100X hyperactive transposase, together with a second plasmid carrying a transgene flanked by binding sites for the transposase, into the cytoplasm of porcine zygotes. The transposase mediates excision of the transgene cassette from the plasmid vector and its permanent insertion into the genome to produce stable transgenic animals. This method compares favorably in terms of both efficiency and reliable transgene expression to classic pronuclear microinjection or somatic cell nuclear transfer (SCNT), and it offers comparable efficacies to lentiviral approaches, without limitations on vector design, issues of transgene silencing and the toxicity and biosafety concerns of working with viral vectors. Microinjection of the vectors into zygotes and transfer of the embryos to recipient animals can be performed in 1 d; generation of germline-transgenic lines by using this protocol takes ∼1 year.

Článek

Germline transgenesis in rabbits by pronuclear microinjection of Sleeping Beauty transposons

Nature protocols. 2014 ; 9 (4) : 794-809.

Nat Protoc
ISSN 1750-2799
Medvik
Zdroj

The laboratory rabbit (Oryctolagus cuniculus) is widely used as a model for a variety of inherited and acquired human diseases. In addition, the rabbit is the smallest livestock animal that is used to transgenically produce pharmaceutical proteins in its milk. Here we describe a protocol for high-efficiency germline transgenesis and sustained transgene expression in rabbits by using the Sleeping Beauty (SB) transposon system. The protocol is based on co-injection into the pronuclei of fertilized oocytes of synthetic mRNA encoding the SB100X hyperactive transposase together with plasmid DNA carrying a transgene construct flanked by binding sites for the transposase. The translation of the transposase mRNA is followed by enzyme-mediated excision of the transgene cassette from the plasmids and its permanent genomic insertion to produce stable transgenic animals. Generation of a germline-transgenic founder animal by using this protocol takes ∼2 months. Transposon-mediated transgenesis compares favorably in terms of both efficiency and reliable transgene expression with classic pronuclear microinjection, and it offers comparable efficacies (numbers of transgenic founders obtained per injected embryo) to lentiviral approaches, without limitations on vector design, issues of transgene silencing, and the toxicity and biosafety concerns of working with viral vectors.

Článek

Germline transgenesis in rodents by pronuclear microinjection of Sleeping Beauty transposons

Nature protocols. 2014 ; 9 (4) : 773-93.

Nat Protoc
ISSN 1750-2799
Medvik
Zdroj

We describe a protocol for high-efficiency germline transgenesis and sustained transgene expression in two important biomedical models, the mouse and the rat, by using the Sleeping Beauty transposon system. The procedure is based on co-injection of synthetic mRNA encoding the SB100X hyperactive transposase, together with circular plasmid DNA carrying a transgene construct flanked by binding sites for the transposase, into the pronuclei of fertilized oocytes. Upon translation of the transposase mRNA, enzyme-mediated excision of the transgene cassettes from the injected plasmids followed by permanent genomic insertion produces stable transgenic animals. Generation of a germline-transgenic founder animal by using this protocol takes ∼3 months. Transposon-mediated transgenesis compares favorably in terms of both efficiency and reliable transgene expression with classic pronuclear microinjection, and it offers comparable efficacies to lentiviral approaches without limitations on vector design, issues of transgene silencing, and the toxicity and biosafety concerns of working with viral vectors.

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