2004
DOI: 10.1038/ng1459
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Targeted gene alteration in Caenorhabditis elegans by gene conversion

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Cited by 37 publications
(38 citation statements)
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“…However, semistable, transgenic lines with extrachromosomal arrays containing many copies of injected DNA are relatively simple to generate (Mello et al 1991) and provide templates for DSB repair after excision of the endogenous Tc1 transposon (Plasterk and Groenen 1992). The first examples of endogenous gene editing, including tagging a gene with GFP, were based on Tc1 excision (Barrett et al 2004). This strategy has the disadvantage that Tc1 is active only in mutator strains.…”
mentioning
confidence: 99%
“…However, semistable, transgenic lines with extrachromosomal arrays containing many copies of injected DNA are relatively simple to generate (Mello et al 1991) and provide templates for DSB repair after excision of the endogenous Tc1 transposon (Plasterk and Groenen 1992). The first examples of endogenous gene editing, including tagging a gene with GFP, were based on Tc1 excision (Barrett et al 2004). This strategy has the disadvantage that Tc1 is active only in mutator strains.…”
mentioning
confidence: 99%
“…DNA damage-related neurotic procedures including carcinogenesis [229][230][231][232], maturing [233][234][235][236][237][238][239], and neurodegenerative illnesses are additionally ranges of dynamic research in C. elegans. This exploration has both set up the significance of C. elegans as a model for the investigation of genotoxic specialists (because of protection of the DNA harm reaction) and massively expanded its utility in such reviews by giving an abundance of corresponding and relevant natural data identified with the obsessive reactions to DNA harm in this living being.…”
Section: Pathwaysmentioning
confidence: 99%
“…However, the frequency of recombination between the genome and the homologous transgene was too low to be used as an efficient technique for genome engineering. This strategy was reinvestigated using more efficient mutator backgrounds (Barrett et al 2004). Results indicated that it was possible to generate custom deletions and insert a gfp sequence in a locus.…”
Section: Custom Knockout and Knock In Alleles By Transgene-instructedmentioning
confidence: 99%