Efficient Mitochondrial Genome Editing by CRISPR/Cas9

The Clustered Regularly Interspaced Short Palindromic Repeats (CRISPR)/Cas9 system has been widely used for nuclear DNA editing to generate mutations or correct specific disease alleles. Despite its flexible application, it has not been determined if CRISPR/Cas9, originally identified as a bacterial...

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Published inBioMed research international Vol. 2015; no. 2015; pp. 1 - 10
Main Authors Lee, Yunjong, Lee, Yun-Song, Kim, SangSeong, Lee, Yun-Il, Lee, Gum Hwa, Ham, Sangwoo, Jo, Areum, Shin, Joo-Ho
Format Journal Article
LanguageEnglish
Published Cairo, Egypt Hindawi Publishing Corporation 01.01.2015
John Wiley & Sons, Inc
Hindawi Limited
Subjects
Biomedical research
CRISPR-Cas Systems
Cytochrome
Deoxyribonucleic acid
Design
DNA
DNA, Mitochondrial - genetics
DNA, Mitochondrial - metabolism
Editing
Genome, Mitochondrial
Genomes
Genomics
HEK293 Cells
Humans
Immunoglobulins
Methods
Mitochondria
Mitochondrial DNA
Mitochondrial Proteins - genetics
Mitochondrial Proteins - metabolism
Mutation
Oxidative stress
Parkinson's disease
Phosphorylation
Physiological aspects
Proteins
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Summary:The Clustered Regularly Interspaced Short Palindromic Repeats (CRISPR)/Cas9 system has been widely used for nuclear DNA editing to generate mutations or correct specific disease alleles. Despite its flexible application, it has not been determined if CRISPR/Cas9, originally identified as a bacterial defense system against virus, can be targeted to mitochondria for mtDNA editing. Here, we show that regular FLAG-Cas9 can localize to mitochondria to edit mitochondrial DNA with sgRNAs targeting specific loci of the mitochondrial genome. Expression of FLAG-Cas9 together with gRNA targeting Cox1 and Cox3 leads to cleavage of the specific mtDNA loci. In addition, we observed disruption of mitochondrial protein homeostasis following mtDNA truncation or cleavage by CRISPR/Cas9. To overcome nonspecific distribution of FLAG-Cas9, we also created a mitochondria-targeted Cas9 (mitoCas9). This new version of Cas9 localizes only to mitochondria; together with expression of gRNA targeting mtDNA, there is specific cleavage of mtDNA. MitoCas9-induced reduction of mtDNA and its transcription leads to mitochondrial membrane potential disruption and cell growth inhibition. This mitoCas9 could be applied to edit mtDNA together with gRNA expression vectors without affecting genomic DNA. In this brief study, we demonstrate that mtDNA editing is possible using CRISPR/Cas9. Moreover, our development of mitoCas9 with specific localization to the mitochondria should facilitate its application for mitochondrial genome editing.
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Academic Editor: Janusz Blasiak
ISSN:2314-6133
2314-6141
DOI:10.1155/2015/305716