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Kloniranje in optimizacija izražanja rekombinantnih proteinov skupkov Neat1 in G4C2 za in vitro opazovanje njihovega nastanka
ID Nograšek, Teo (Author), ID Rogelj, Boris (Mentor) More about this mentor... This link opens in a new window

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Abstract
Prepisana heksanukleotidna razširitvena mutacija gena C9orf72 predstavlja osnovo za izgradnjo toksičnih nemembranskih skupkov G4C2. Te se pogosto pojavljajo pri družinskih različicah amiotrofične lateralne skleroze in frontotemporalne demence. Mehanizmi nastanka toksičnih skupkov niso dobro poznani in bi lahko bili temelj novega načina zdravljenja bolezni. Za raziskave skupkov so potrebni proteini, ki se kolokalizirajo z mutiranim prepisom in tvorijo skupke G4C2. Zato smo v okviru diplomske naloge pripravili plazmide za in vitro transkripcijo/translacijo in za izražanje proteinov SFPQ, NONO, PABPC1, TDP-43 ter FUS v bakterijah E. coli BL21(DE3). Nemutiranim različicam proteinov smo dodali fuzijski maltoza vezavni protein za povečano topnost konstruktov in fluorescenčni protein NeonGreen. Plazmid je vseboval tudi heksahistidinsko oznako in cepitveno mesto TEV za lažjo izolacijo konstruktov. Proteine SFPQ, PABPC1, TDP-43 in FUS smo izražali pri 37 oC, 1 mM IPTG, tri ure in pri 30 oC, 0,5 mM IPTG, pet ur. Najboljši pogoji za izražanje proteina so bili pri nižji temperaturi in nižji koncentraciji induktorja, ker se je takrat večina proteina nahajala v topni frakciji. V prenizkih količinah za nadaljnjo izolacijo sta se izražala konstrukta SFPQ in SFPQNeonGreen. V nadaljevanju je potrebno preveriti izražanje konstruktov NONO, NONONeonGreen in NeonGreen-PABPC1 ter z uporabo Ni2+ ionov izolirati izražene proteine, da dosežemo naš cilj.

Language:Slovenian
Keywords:ALS, FTD, nemembranski organeli, izražanje proteinov, C9orf72, skupki G4C2, SFPQ, TDP-43, NONO, PABPC1, FUS
Work type:Bachelor thesis/paper
Typology:2.11 - Undergraduate Thesis
Organization:FKKT - Faculty of Chemistry and Chemical Technology
Year:2021
PID:20.500.12556/RUL-130169 This link opens in a new window
COBISS.SI-ID:83269635 This link opens in a new window
Publication date in RUL:10.09.2021
Views:1819
Downloads:181
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Secondary language

Language:English
Title:Cloning and optimization of expression of recombinant proteins of Neat1 and G4C2 clusters for in vitro observation of their formation
Abstract:
C9orf72 hexanucleotide repeat expansion transcript is the foundation on which toxic membraneless G4C2 foci are built. These are common among patients with familial amyotrophic lateral sclerosis and frontotemporal dementia. Mechanisms underlying the formation of toxic G4C2 foci are unknown and could represent the basis for new treatments. To research G4C2 foci proteins that localize and form these structures are needed. For that reason, this work focuses on the production of plasmids for in vitro transcription/translation and expression of SFPQ, NONO, PABPC1, TDP-43 and FUS proteins in E. coli BL21(DE3) bacteria. A fluorescent NeonGreen protein was fused to the wild type proteins along with maltose binding protein for increased construct solubility. The plasmids also contained a hexahistidine tag and a TEV cleavage site to assist with protein purification. SFPQ, PABPC1, TDP-43 and FUS were expressed at 37 oC with 1 mM IPTG for three hours and at 30 oC, with 0,5 mM IPTG for five hours. Lower temperature expression yielded a better result since most of the protein was in the soluble fraction of the cell lysate. Both SFPQ and SFPQ-NeonGreen were expressed in too low a quantity for further protein isolation. Further work needs to check the expression of NONO, NONO-NeonGreen, NeonGreen-PABPC1 and purify all of the constructs to achieve our goal.

Keywords:ALS, FTD, membranelles organelles, protein expression, C9orf72, G4C2 foci, SFPQ, TDP-43, NONO, PABPC1, FUS

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