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Vpliv mesta integracije gena za zeleni fluorescenčni protein na njegovo izražanje v kvasovki Yarrowia lipolytica
ID Rupar, Ana (Author), ID Petrovič, Uroš (Mentor) More about this mentor... This link opens in a new window

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Abstract
Yarrowia lipolytica je vrsta kvasovke, ki kot glavni mehanizem popravljanja dvojnih prelomov DNA uporablja povezovanje nehomolognih koncev. S tem se po vnosu v celico fragmenti DNA integrirajo v netarčne lokuse, kar ima lahko neželjen učinek na dobljen rekombinantni sev. Sicer običajno načrtujemo integracijo v izbrane genomske lokacije zato, da dobimo seve, ki imajo stabilno vstavljen fragment DNA v lokus. Bioinformatsko smo določili 12 genomskih lokacij za tarčno integracijo in jih primerjali z naključno integracijo v mesto zeta, ki se na genomu pojavi večkrat. Za ovrednotenje integracijskih mest smo uporabili poročevalski gen za zeleni fluorescenčni protein (GFP), ki ga enostavno merimo s spektrofotometrom. Z metodo kloniranja Golden Gate in metodo kloniranja po Gibsonu smo sestavili rekombinantne plazmidne molekule DNA, ki so vsebovale ekspresijsko kaseto z genom za heterologni protein GFP. Plazmidi so se razlikovali po zaporedju homologne DNA za vsako izmed integracijskih mest. Pri delu smo uporabljali sva različna seva Y. lipolytica: CH-164 in PO1f. Uspešno smo dobili transformante z integracijo v vsa tarčna mesta. Produkcija GFP se je med transformantami razlikovala, najvišja je bila pri integraciji v integracijsko mesto B1. To se nahaja na kromosomu B, na lokusu med dvema genoma, za katera funkcija še ni znana. S spektrofotometričnim merjenjem fluorescence, poliakrilamidno elektroforezo v prisotnosti SDS in imunodetekcijo proteina s prenosom western smo uspešno detektirali izražen GFP.

Language:Slovenian
Keywords:kvasovke, Yarrowia lipolytica, GFP, tarčna integracija, homologna rekombinacija, metoda Gibson, metoda Golden Gate
Work type:Master's thesis/paper
Typology:2.09 - Master's Thesis
Organization:BF - Biotechnical Faculty
Year:2024
PID:20.500.12556/RUL-161197 This link opens in a new window
COBISS.SI-ID:207426051 This link opens in a new window
Publication date in RUL:08.09.2024
Views:190
Downloads:54
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Secondary language

Language:English
Title:Effect of the integration site of the gene encoding green fluorescent protein on its expression in the yeast Yarrowia lipolytica
Abstract:
Yarrowia lipolytica is a yeast species that utilizes non-homologous end joining as the main mechanism for repairing double-strand DNA breaks. During this process, DNA fragments integrate into non-target loci, which can have unexpected effects on the resulting recombinant strain. By designing integration into the selected genomic loci, we can obtain strains with stably inserted DNA fragments at the desired locus. Bioinformatically, we identified 12 genomic loci for targeted integration and compared them with random integration at zeta locus, which appears multiple times in the genome. To evaluate integration sites, we used a reporter gene for green fluorescent protein (GFP), which can be easily measured with a spectrophotometer. Using Golden Gate assembly and Gibson cloning methods we assembled recombinant plasmid DNA molecules containing an expression cassette with the gene for the heterologous GFP. Plasmids differed in the homologous DNA sequence for each integration site. We used two different strains of Y. lipolytica: CH-164 and PO1f. We obtained transformants with integration at all target sites. Production of GFP protein varied among the transformants, with the highest observed at the integration site B1, which is located on the B chromosome, at a locus between two genes whose function is unknown. Through spectrophotometric measurement of fluorescence, SDS-polyacrylamide gel electrophoresis and Western blot protein detection, we successfully detected expressed GFP.

Keywords:yeast, Yarrowia lipolytica, GFP, targeted integation, homologous recombination, Gibson assembly, Golden Gate assembly

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