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Priprava plazmidnega vektorja in molekulsko kloniranje genov Sox5 in Sox6
ID Mezgec, Klemen (Author), ID Marc, Janja (Mentor) More about this mentor... This link opens in a new window, ID Kodrič, Klemen (Co-mentor)

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Abstract
Bliskovit napredek molekulske biologije nam omogoča enostavno sintezo poljubnih rekombinantnih molekul DNA, ki jih lahko učinkovito izkoriščamo za preučevanje fizioloških in patofizioloških molekulskih mehanizmov v organizmu. Proteini iz družine SOX so izjemno pomembni transkripcijski dejavniki, ki preko ojačevalnih in regulatornih regij uravnavajo izražanje številnih genov, pomembno vpletenih v nadzor celične delitve in sposobnosti diferenciacije v procesu razvoja zarodka. Njihova funkcija v organizmu je tako pomembna, da bi morebitne mutacije v genskem zapisu povzročile razvoj izjemno težkih in kompleksnih bolezenskih stanj. Glavni namen naloge je bil pripraviti ekspresijske plazmide s tehnologijo rekombinantne DNA in tako sklonirati tarčni kodirajoči zaporedji genov SOX5 in SOX6. Sintetizirane rekombinantne plazmidne molekule bodo v transfeciranih celičnih linijah omogočile sintezo označenih fuzijskih proteinov SOX5 in SOX6, ki ju bomo v nadaljnjih študijah uporabili za preučevanje vpletenosti v molekulske mehanizme uravnavanja izražanja tarčnih genov pri razvoju drugih bolezni. Rekombinantne plazmidne molekule smo sintetizirali tako, da smo v poliklonska mesta ekspresijskih vektorjev pFLAG-CMVTM-2 vstavili tarčni kodirajoči zaporedji genov SOX5 in SOX6. V procesu klasičnega molekulskega kloniranja smo za rezanje plazmida in vključkov uporabili restrikcijski endonukleazi NotI ter KpnI, ki sta načrtno ustvarili komplementarne lepljive konce in tako zagotovili pogoje za vstavitev vključkov v rezane molekule vektorja. Po ligaciji smo rekombinantne plazmidne molekule ločili in namnožili na trdnem gojišču z ampicilinom. V zadnjem koraku smo ustreznost molekulskega kloniranja preverili s potrditveno restrikcijsko analizo in elektroforezo na agaroznem gelu ter določitvijo nukleotidnega zaporedja rekombinantnih DNA po Sangerju. Na podlagi rezultatov potrditvenih metod smo ugotovili, da je bilo kloniranje v obeh primerih uspešno. Dokončno potrditev smo dokazali z bioinformacijsko sekvenčno analizo pridobljenih rekombinantnih plazmidov, kjer smo dokazali približno 99 % ujemanje z ustreznima referenčnima različicama tarčnih kodirajočih zaporedij genov SOX5 in SOX6. Transkripcijski dejavniki iz družine SOX so zaradi svoje vsestranskosti in vpletenosti v številne fiziološke ter patofiziološke procese, primerni za nadaljnje raziskave, saj bi nam boljše poznavanje molekulskih mehanizmov lahko omogočilo odkritje novih označevalcev, terapevtskih tarč in inovativnih zdravilnih učinkovin.

Language:Slovenian
Keywords:molekulsko kloniranje, transkripcijski dejavniki, SOX5, SOX6, bioinformacijska sekvenčna analiza
Work type:Master's thesis/paper
Organization:FFA - Faculty of Pharmacy
Year:2019
PID:20.500.12556/RUL-109902 This link opens in a new window
Publication date in RUL:10.09.2019
Views:1348
Downloads:417
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Secondary language

Language:English
Title:Preparation of a plasmid construct and molecular cloning of Sox5 and Sox6 genes
Abstract:
Rapid breakthrough of the molecular biology allows us simple and efficient synthesis of custom designed recombinant DNA molecules, which can be widely used for studying physiological and pathophysiological molecular mechanisms in the organisms. Proteins from the SOX family are remarkably important transcription factors, that play a significant role in regulation of the gene expression, through enhancer and regulatory regions and they are crucial in the control of cell fate decisions and the ability to differentiate during the embryo development process. Their function in the organism is so important, that potential mutations in the SOX genes, could lead to extremely complex and severe diseases. Main purpose of the Master's thesis was to synthesize expression plasmid vectors with recombinant DNA technology and successfully clone target coding regions of SOX5 and SOX6 genes. Synthesized recombinant plasmid molecules will, in transfected cell lines, produce tagged fusion SOX5 and SOX6 proteins, which are going to be used in the following studies for additional investigation of their involvement in the molecular mechanisms of gene expression regulation in connection to other diseases development. We synthesized our recombinant plasmid molecules in the way, that the target coding sequences of the SOX5 and SOX6 genes were precisely inserted into the polyclonal site of pFLAG-CMVTM-2 expression vectors. For cutting plasmids and insert molecules in the process of the convenient molecular cloning, we used NotI and KpnI restriction endonucleases, which generated complementary sticky ends for inserting the target gene coding sequences into cut vector molecules. After ligation, we selected and multiplied recombinant plasmid molecules on the growth medium with ampicillin. At the end, we confirmed molecular cloning with restriction analysis followed by an agarose electrophoresis and Sanger sequencing. Based on results of confirmatory methods we concluded, that molecular cloning was successful in both cases. Final confirmation was conducted by bioinformatic sequence analysis of the recombinant plasmids, where we proved approximately 99 % matching with applicable reference variants of the SOX5 and SOX6 gene coding sequences. Due to their versatility and involvement in many physiological and pathophysiological processes, transcription factors from the SOX family, are suitable for further research, because better understanding of their molecular mechanisms could lead us to discovery of new disease markers, therapeutic targets and innovative drugs.

Keywords:molecular cloning, transcription factors, SOX5, SOX6, bioinformatic sequence analysis

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