i-GONAD: a robust method for in situ germline genome engineering using CRISPR nucleases

Ohtsuka, Masato; Sato, Masahiro; Miura, Hiromi; Takabayashi, Shuji; Matsuyama, Makoto; Koyano, Takayuki; Arifin, Naomi; Nakamura, Shingo; Wada, Kenta; Gurumurthy, Channabasavaiah B.

doi:10.1186/s13059-018-1400-x

Cited by 155 publications

(255 citation statements)

References 30 publications

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“…These results are probably explained by the presence of cumulus cells surrounding the zygotes at Day 0.4; however, by Day 0.7, connections of these cumulus cells become loose, which allows eGFP mRNA solution to reach close to zygotes. Based on this experiment, we conclude that Day 0.7 is the optimal time for GONAD treatment (Ohtsuka et al., ).…”

Section: Development Of I‐gonad and Its Applicationssupporting

confidence: 51%

“…Pregnant females on the day of having copulation plug contain one‐cell stage embryo in the ampulla (in which zygotes exist massively), the dilated area of the oviduct where the fertilization occurs. To assess the optimal time for GONAD, we injected eGFP mRNA into the oviductal lumen of pregnant females on Day 0.4 and Day 0.7, and performed in vivo EP (Ohtsuka et al., ). Observation of embryos from the two‐cell to blastocyst stage showed eGFP fluorescence only in the embryos derived from females subjected to GONAD on Day 0.7 of pregnancy.…”

Section: Development Of I‐gonad and Its Applicationsmentioning

confidence: 99%

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i‐GONAD: A method for generating genome‐edited animals without ex vivo handling of embryos

Ohtsuka

2019

Dev Growth Differ

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The recent development of genome editing technologies has enabled the creation of genome‐edited animals, with alterations at the desired target locus. The clustered regularly interspaced short palindromic repeats (CRISPR) system is widely used for this purpose because it is simpler and more efficient than other genome editing technologies. The conventional methods for creation of genome‐edited animals involve ex vivo handling of embryos (zygotes) for microinjection or in vitro electroporation. However, this process is laborious and time‐consuming, and relatively large numbers of animals are used. Furthermore, these methods require specialized skills for handling embryos. In 2015, we reported a novel method for the creation of genome‐edited animals without ex vivo handling of embryos. The technology known as Genome‐editing via Oviductal Nucleic Acids Delivery (GONAD) involved intraoviductal instillation of genome editing components into a pregnant female and subsequent in vivo electroporation of an entire oviduct. The genome editing components present in the oviductal lumen are transferred to preimplantation embryos in situ for introducing insertion or deletion (indel) mutations at the desired loci. This technology was further improved by optimizing several parameters to develop improved GONAD (i‐GONAD) for the efficient generation of mutant or knock‐in animals. In this review, we discuss the historical background, potential applications, advantages, and future challenges of GONAD/i‐GONAD technology.

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Section: Development Of I‐gonad and Its Applicationssupporting

confidence: 51%

Section: Development Of I‐gonad and Its Applicationsmentioning

confidence: 99%

i‐GONAD: A method for generating genome‐edited animals without ex vivo handling of embryos

Ohtsuka

2019

Dev Growth Differ

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“…The advent of CRISPR/Cas9 technology has opened the door for performing a wide variety of genome editing experiments in both “traditional” and “non‐traditional” model systems, allowing a wide variety of modifications, including gene and enhancer knockouts, transcriptional activation and repression, and insertions of large genomic regions. Furthermore, recent studies in laboratory mice have achieved high genome editing efficiencies by delivering the CRISPR/Cas9 cocktail directly into zygotes inside the female oviduct, using electroporation or adeno‐associated viruses, thereby bypassing some of the hurdles associated with the traditional approach, such as the use of sophisticated micromanipulation equipment for ex vivo zygote microinjection and embryo transfer, usually performed by highly trained personnel. Incorporating these approaches in striped mice holds the promise of achieving precise and efficient genome modification to probe developmental mechanisms underlying pigment pattern formation.…”

Section: Functional Approaches To Studying Pigment Patterns In Rodentsmentioning

confidence: 99%

Periodic patterns in Rodentia: Development and evolution

Johnson

Barsh

Mallarino

2019

Experimental Dermatology

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Mammalian periodic pigment patterns, such as spots and stripes, have long interested mathematicians and biologists because they arise from non-random developmental processes that are programmed to be spatially constrained, and can therefore be used as a model to understand how organized morphological structures develop. Despite such interest, the developmental and molecular processes underlying their formation remain poorly understood. Here, we argue that Arvicanthines, a clade of African rodents that naturally evolved a remarkable array of coat patterns, represent a tractable model system in which to dissect the mechanistic basis of pigment pattern formation. Indeed, we review recent insights into the process of stripe formation that were obtained using an Arvicanthine species, the African striped mouse (Rhabdomys pumilio), and discuss how these rodents can be used to probe deeply into our understanding of the factors that specify and implement positional information in the skin. By combining naturally evolved pigment pattern variation in rodents with classic and novel experimental approaches, we can substantially advance our understanding of the processes by which spatial patterns of cell differentiation are established during embryogenesis, a fundamental question in developmental biology.

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“…Mice C57BL/6 mice were used all in this study. p21 deficient mice were generated by i-GONAD method as previously described (34). In brief, the single strand DNA which contains 3 STOP codons and All animal experiments were approved by the institutional committee.…”

Section: Methodsmentioning

confidence: 99%

“…To investigate the impact of p21 in renal fibrosis, we constructed the novel p21 deficient mice (p21 -/-). To this end, we took the advantages of i-GONAD (improved-Genome-editing via oviductal nucleic acid delivery) method, in which handling the fertilized egg ex vivo is not required (33,34). Tandem STOP codons were integrated into 60 bases after the first ATG (Fig.…”

Section: Impact Of P21 Deficiency In Renal Fibrosis Progressionmentioning

confidence: 99%

The p21 dependent G2 arrest of the cell cycle in epithelial tubular cells links to the early stage of renal fibrosis

Koyano

Namba

Kobayashi

et al. 2019

Preprint

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Renal fibrosis is accompanied with the progression of chronic kidney disease (CKD). Despite a number of past and ongoing studies, our understanding of the underlying mechanisms remains elusive.Here we explored the progression of renal fibrosis by using a mouse model, unilateral ureter obstruction (UUO). We found that in the initial stage of the progression where extracellular matrix did not deposit yet, the proximal tubular cells arrested at the G2 of the cell cycle. This G2 arrest was induced prior to activation of both DNA damage checkpoint and Wnt/β-Catenin pathway. Further analyses in vivo and in vitro indicated the cyclin dependent kinase inhibitor p21 is involved in the G2 arrest after the damage.The newly produced monoclonal antibody against p21 revealed that the p21 levels were sharply upregulated in response to the damage during the initial stage, but dropped down toward the later stage.

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i-GONAD: a robust method for in situ germline genome engineering using CRISPR nucleases

Cited by 155 publications

References 30 publications

i‐GONAD: A method for generating genome‐edited animals without ex vivo handling of embryos

i‐GONAD: A method for generating genome‐edited animals without ex vivo handling of embryos

Periodic patterns in Rodentia: Development and evolution

The p21 dependent G2 arrest of the cell cycle in epithelial tubular cells links to the early stage of renal fibrosis

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