共 65 条
CRISPR/Cas9-induced double-strand breaks in the huntingtin locus lead to CAG repeat contraction through DNA end resection and homology-mediated repair
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作者:

Sledzinski, Pawel
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Polish Acad Sci, Inst Bioorgan Chem, Dept Genome Engn, PL-61704 Poznan, Poland Polish Acad Sci, Inst Bioorgan Chem, Dept Genome Engn, PL-61704 Poznan, Poland

Nowaczyk, Mateusz
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Polish Acad Sci, Inst Bioorgan Chem, Dept Genome Engn, PL-61704 Poznan, Poland Polish Acad Sci, Inst Bioorgan Chem, Dept Genome Engn, PL-61704 Poznan, Poland

Smielowska, Marianna Iga
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Polish Acad Sci, Inst Bioorgan Chem, Dept Genome Engn, PL-61704 Poznan, Poland Polish Acad Sci, Inst Bioorgan Chem, Dept Genome Engn, PL-61704 Poznan, Poland

Olejniczak, Marta
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Polish Acad Sci, Inst Bioorgan Chem, Dept Genome Engn, PL-61704 Poznan, Poland Polish Acad Sci, Inst Bioorgan Chem, Dept Genome Engn, PL-61704 Poznan, Poland
机构:
[1] Polish Acad Sci, Inst Bioorgan Chem, Dept Genome Engn, PL-61704 Poznan, Poland
来源:
关键词:
DNA repair;
Genome editing;
Short tandem repeats;
TMEJ;
BASE EXCISION-REPAIR;
TRIPLET REPEATS;
IN-VITRO;
GENOME;
PROTEIN;
REPLICATION;
POLYMERASES;
INSTABILITY;
EXPANSION;
SEQUENCE;
D O I:
10.1186/s12915-024-02079-6
中图分类号:
Q [生物科学];
学科分类号:
07 ;
0710 ;
09 ;
摘要:
Background The expansion of CAG/CTG repeats in functionally unrelated genes is a causative factor in many inherited neurodegenerative disorders, including Huntington's disease (HD), spinocerebellar ataxias (SCAs), and myotonic dystrophy type 1 (DM1). Despite many years of research, the mechanism responsible for repeat instability is unknown, and recent findings indicate the key role of DNA repair in this process. The repair of DSBs induced by genome editing tools results in the shortening of long CAG/CTG repeats in yeast models. Understanding this mechanism is the first step in developing a therapeutic strategy based on the controlled shortening of repeats. The aim of this study was to characterize Cas9-induced DSB repair products at the endogenous HTT locus in human cells and to identify factors affecting the formation of specific types of sequences. Results The location of the cleavage site and the surrounding sequence influence the outcome of DNA repair. DSBs within CAG repeats result in shortening of the repeats in frame in similar to 90% of products. The mechanism of this contraction involves MRE11-CTIP and RAD51 activity and DNA end resection. We demonstrated that a DSB located upstream of CAG repeats induces polymerase theta-mediated end joining, resulting in deletion of the entire CAG tract. Furthermore, using proteomic analysis, we identified novel factors that may be involved in CAG sequence repair. Conclusions Our study provides new insights into the complex mechanisms of CRISPR/Cas9-induced shortening of CAG repeats in human cells.
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