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Please use this identifier to cite or link to this item: https://biore.bio.bg.ac.rs/handle/123456789/2946
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dc.contributor.authorUddin, Borhanen_US
dc.contributor.authorChen, Nan Pengen_US
dc.contributor.authorPanić, Markoen_US
dc.contributor.authorSchiebel, Elmaren_US
dc.date.accessioned2019-10-29T16:44:24Z-
dc.date.available2019-10-29T16:44:24Z-
dc.date.issued2015-12-21-
dc.identifier.urihttps://biore.bio.bg.ac.rs/handle/123456789/2946-
dc.description.abstract© 2015 Uddin et al. Background: Highly efficient genome editing can be achieved through targeting an endonuclease to specific locus of interest. Engineered zinc-finger nuclease (ZFN) and CRISPR-associated protein-9 nuclease (Cas9) offer such an elegant approach for genome editing in vertebrate cells. In this study, we have utilized ZFN and Cas9-catalyzed double strand break followed by homologous recombination-mediated incorporation of premature stop codon and selection marker to target human cell division cycle 14A (hCDC14A) and cell division cycle 14B (hCDC14B) genes. Results: Targeting of the hCDC14A and hCDC14B loci in telomerase immortalized human retinal pigment epithelium (hTERT-RPE1) and human colon cancer (HCT116) cells were confirmed by Southern blot hybridization. Nevertheless, DNA sequence analysis of reverse transcription polymerase chain reaction (RT-PCR) products confirmed that in all the single/double allele ablations, the targeted exon was spliced out. The phenomenon of exon skipping was independent of the genome editing approaches exploited, Cas9 or ZFN. Because the exons had a nucleotide number that could be divided by 3, the reading frame of the exon deletion was maintained. This indicates an exon-skipping event possibly due to the insertion of large DNA fragment (1.7 to 2.5 Kb) within the targeted exons. As a proof-of-principle, we have used gene disruption followed by non-homologous end joining (NHEJ) approach. Small alterations in the exon (one to fifteen bases) were transcribed to mRNA without exon skipping. Furthermore, loxP site-mediated removal of selection markers left a 45 bp scar within the targeted exon that can be traced in mRNA without exon skipping. Conclusion: From this study, we conclude that insertion of a large DNA fragment into an exon by genome editing can lead to its skipping from the final transcript. Hence, more cautious approach needs to be taken while designing target sites in such that the possible skipping of targeted exon causes a frame-shift mediated incorporation of pre-mature stop codon. On the other hand, exon skipping may be a useful strategy for the introduction of protein deletions.en_US
dc.language.isoenen_US
dc.relation.ispartofBMC Genomicsen_US
dc.subjectCRISPR-Cas9en_US
dc.subjectExon-skippingen_US
dc.subjectGenome engineeringen_US
dc.subjectHCDC14Aen_US
dc.subjectHCDC14Ben_US
dc.subjectZinc-finger nucleasesen_US
dc.titleGenome editing through large insertion leads to the skipping of targeted exonen_US
dc.typeArticleen_US
dc.identifier.doi10.1186/s12864-015-2284-8-
dc.identifier.pmid26691863-
dc.identifier.scopus2-s2.0-84953708487-
dc.identifier.urlhttps://api.elsevier.com/content/abstract/scopus_id/84953708487-
item.fulltextWith Fulltext-
item.openairecristypehttp://purl.org/coar/resource_type/c_18cf-
item.grantfulltextrestricted-
item.languageiso639-1en-
item.openairetypeArticle-
item.cerifentitytypePublications-
crisitem.author.deptChair of Biochemistry and Molecular Biology-
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