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Izbris daljšega genomskega odseka bakterije Streptomyces rimosus z uporabo CRISPR-Cas9
ID Godec, Tim (Author), ID Petković, Hrvoje (Mentor) More about this mentor... This link opens in a new window

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Abstract
Razvoj celičnih tovarn na osnovi bakterij iz rodu Streptomyces je ključen za proizvodnjo novih in že poznanih biološko aktivnih učinkovin. S postopno delecijo večjih delov genoma lahko razvijemo učinkovito platformo za heterologno izražanje sekundarnih metabolitov. Klasične metode za manipulacije genoma v streptomicetah so zahtevne in časovno potratne. V tem delu, smo z uporabo CRISPR-Cas9 sistema izvedli delecijo genoma bakterije Streptomyces rimosus v velikosti 145 kb. Z bioinformacijsko analizo smo izbrali tarčno regijo genoma, ustrezne homologne regije in vodilne RNA. Z metodama PCR s prekrivanjem in SLiCE kloniranje smo sestavili plazmidni konstrukt za delecijo s CRISPR-Cas9. Konstrukt smo s konjugacijo vnesli v S. rimosus in testirali delecijo v pozitivnih klonih z metodo PCR in sekvenciranjem. Identificirali smo številne seve s pravilno delecijo izbranega fragmenta DNK v velikosti 145 kb.

Language:Slovenian
Keywords:CRISPR, delecija, redukcija genoma, Streptomyces rimosus
Work type:Master's thesis/paper
Typology:2.09 - Master's Thesis
Organization:BF - Biotechnical Faculty
Place of publishing:Ljubljana
Publisher:[T. Godec]
Year:2021
PID:20.500.12556/RUL-130412 This link opens in a new window
UDC:602.3:579.873.7:602.6:579.8(043.2)
COBISS.SI-ID:76574723 This link opens in a new window
Publication date in RUL:15.09.2021
Views:1184
Downloads:2
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Secondary language

Language:English
Title:Large genomic deletion in bacteria Streptomyces rimosus using CRISPR-Cas9
Abstract:
Developing a Streptomyces-based cell factory is key for the production of new or known biologically active compounds. With gradual deletion of large genomic regions one can develop an efficient platform for the heterologous expression of secondary metabolites. Gene manipulations of Streptomyces using classical approaches are demanding and time-consuming. In this work we used CRISPR-Cas9 to achieve a 145 kb genomic deletion in Streptomyces rimosus. With the use of bioinformatics we chose a target region with accompaning homologies and guide RNAs. We then used overlap PCR and SLiCE cloning to construct a plazmid for CRISPR-Cas9 driven deletion. The plasmid was introduced into S. rimosus with conjugation, then positive clones were tested for the deletion using PCR and sequencing. We have identified several isolates with correctly deleted DNA fragment of 145 kb in size.

Keywords:CRISPR, genome reduction, genomic deletion, Streptomyces rimosus

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