Your search keyword '"Microinjections veterinary"' showing total 7 results

1. Next Generation Transgenic Rat Model Production.

Author

Filipiak WE, Hughes ED, Gavrilina GB, LaForest AK, and Saunders TL

Subjects

Animals, CRISPR-Cas Systems, Gene Expression, Genes, Reporter, Microinjections veterinary, Models, Animal, Rats, Rats, Transgenic genetics, Genetic Engineering methods, Rats, Transgenic growth & development, Zygote growth & development

Abstract

The next generation of new genetically engineered rat models by microinjection is described. Genome editors such as CRISPR/Cas9 have greatly increased the efficiency with which the rat genome can be modified to generate research models for biomedical research. Pronuclear microinjection of transgene DNA into rat zygotes results in random multicopy transgene integration events that use exogenous promoters to drive expression. Best practices in transgenic animal design indicate the use of precise single copy transgene integration in the genome. This ideal can be achieved by repair of CRISPR/Cas9 chromosome breaks by homology directed repair. The most effective way to achieve this type of transgenic rat model is to deliver genome modification reagents to rat zygotes by pronuclear microinjection. The keys to success in this process are to obtain fertilized eggs (zygotes) from the rat strain of choice, to purify the microinjection reagents, to deliver the reagents to the eggs by pronuclear microinjection, to use the surgical transfer of microinjected eggs to pseudopregnant rats to obtain G0 founder animals that carry the novel genetic modification. Ultimately the success of new rat models is measured by changes in gene expression as in the expression of a new reporter protein such as eGFP, Cre recombinase, or other protein of interest.

Published

2019

2. Effects of downregulating GLIS1 transcript on preimplantation development and gene expression of bovine embryos.

Author

Takahashi K, Sakurai N, Emura N, Hashizume T, and Sawai K

Subjects

Animals, Blastocyst cytology, Blastocyst metabolism, Blastomeres cytology, Cattle, DNA-Binding Proteins antagonists & inhibitors, DNA-Binding Proteins genetics, Female, Fertilization in Vitro veterinary, HSC70 Heat-Shock Proteins genetics, HSC70 Heat-Shock Proteins metabolism, In Vitro Oocyte Maturation Techniques veterinary, Microinjections veterinary, Morula cytology, Morula metabolism, Oocytes cytology, Pyruvate Dehydrogenase (Lipoamide) genetics, Pyruvate Dehydrogenase (Lipoamide) metabolism, RNA Interference, RNA, Messenger metabolism, RNA, Small Interfering, Transcription Factors antagonists & inhibitors, Transcription Factors genetics, Zygote cytology, Blastomeres metabolism, DNA-Binding Proteins metabolism, Ectogenesis, Gene Expression Regulation, Developmental, Oocytes metabolism, Transcription Factors metabolism, Zygote metabolism

Abstract

Krüppel-like protein Gli-similar 1 (GLIS1) is known as a direct reprogramming factor for the generation of induced pluripotent stem cells. The objective of this study was to investigate the role of GLIS1 in the preimplantation development of bovine embryos. GLIS1 transcripts in in vitro-matured oocytes and 1-cell to 4-cell stage embryos were detected, but they were either absent or at trace levels at the 8-cell to blastocyst stages. We attempted GLIS1 downregulation of bovine early embryos by RNA interference and evaluated developmental competency and gene transcripts, which are involved in zygotic gene activation (ZGA) in GLIS1-downregulated embryos. Injection of specific siRNA resulted in a distinct decrease in GLIS1 transcript in bovine embryos at the 4-cell stage. Although the bovine embryos injected with GLIS1-siRNA could develop to the 16-cell stage, these embryos had difficulty in developing beyond the 32-cell stage. Gene transcripts of PDHA1 and HSPA8, which are transcribed after ZGA, showed lower level in GLIS1 downregulated embryos. It is possible that GLIS1-downregulated embryos fail to initiate ZGA. Our results indicated that GLIS1 is an important factor for the preimplantation development of bovine embryos.

Published

2015

3. Pronuclear embryo yield in Canindé and Saanen goats for DNA microinjection.

Author

Moura RR, Lopes-Junior ES, Teixeira DI, Serova IA, Andreeva LE, Melo LM, and Freitas VJ

Subjects

Animals, Animals, Genetically Modified, Estrus Synchronization, Female, Fertility Agents, Female administration & dosage, Fertility Agents, Female pharmacology, Superovulation, Zygote drug effects, DNA genetics, Goats embryology, Goats genetics, Microinjections veterinary, Zygote physiology

Abstract

The objective of this study was to examine the effect of donor breed on pronuclear-stage embryo yield to be used for DNA microinjection in a transgenesis goat program. Twelve Canindé and twelve Saanen goats were heat synchronized using a progestagen-cloprostenol treatment. Forty-eight hours before the sponge removal, superovulation was induced with a total administration of 4.4 mg/kg bodyweight NIH-FSH-P1, given twice daily in decreasing doses over 3 days. In addition, goats received 100 μg of GnRH and they were hand-mated at 36 and 48 h after progestagen removal. Embryo recovery was performed by oviduct flushing at 72 h after sponge removal. Embryos were microinjected with a DNA construct and noticeable swelling of the nuclei was the criterion for successful microinjection. The total diameter, cytoplasm diameter, zona pellucida thickness and pronuclei diameter were measured for each microinjected embryo. A higher (p < 0.05) percentage of fertilized ova was observed in Canindé (89.9%) than Saanen (36.2%) goats. In addition, Canindé donors produced a higher percentage of pronuclear embryos when compared with Saanen: 72.5% vs 20.6% (p < 0.05), respectively. Successful microinjection was verified in 96.7% and 73.3% of times in Canindé and Saanen embryos, respectively (p < 0.05). Significant differences were observed for all morphometric parameters except for cytoplasm diameter. In conclusion, under our study experimental conditions, Canindé were more efficient than Saanen goats concerning the pronuclear embryo yield and manipulation. The use of Canindé goats in transgenesis programs could be increase the interest in their breeding and could be contribute to saving them from extinction., (© 2009 Blackwell Verlag GmbH.)

Published

2010

4. Production of transgenic goats by pronuclear microinjection of in vitro produced zygotes derived from oocytes recovered by laparoscopy.

Author

Baldassarre H, Wang B, Kafidi N, Gauthier M, Neveu N, Lapointe J, Sneek L, Leduc M, Duguay F, Zhou JF, Lazaris A, and Karatzas CN

Subjects

Animals, Animals, Genetically Modified physiology, DNA administration & dosage, DNA genetics, Embryo Transfer veterinary, Female, Fertilization in Vitro methods, Goats physiology, Laparoscopy veterinary, Microinjections veterinary, Ovarian Follicle cytology, Animals, Genetically Modified genetics, Fertilization in Vitro veterinary, Goats genetics, Oocytes physiology, Zygote physiology

Abstract

Oocytes collected by laparoscopic ovum pick-up (LOPU) were successfully used to produce transgenic goats by pronuclear microinjection of in vitro zygotes. Estrus cycles of 109 donor goats were synchronized using intravaginal sponges impregnated with 60 mg of medroxyprogesterone acetate and treatment with 70 mg NIH-FSH-P1 and 300 IU eCG to stimulate follicular development. Follicles were aspirated under laparoscopic observation. In vitro maturation (IVM) of oocytes was performed in M199 supplemented with hormones, kanamycin and 10% estrus goat serum. Following IVM, oocytes were cocultured with capacitated semen in TALP supplemented with 20% estrus goat serum for 15-20 h. The resulting zygotes were microinjected with a linear DNA fragment. In total, 3293 follicles were aspirated (15.7+/-9 follicles aspirated per donor) and 2823 oocytes were recovered (13.4+/-8 oocytes per donor). A total of 1366 zygotes were microinjected and transferred into 219 recipient goats by midventral laparotomy (average 6.2 embryos per recipient). A total of 150 kids were born, of which 9 (6 M: 3 F) were confirmed to be transgenic by PCR and Southern blotting analyses. These results demonstrate that acceptable transgenesis rates can be obtained in goats by DNA microinjection of in vitro produced zygotes.

Published

2003

5. Production of transgenic rabbits using centrifuged pronuclear zygotes.

Author

Hirabayashi M, Hirao M, Takahashi R, Kimura K, Hirasawa K, Ueda M, and Hochi S

Subjects

Animals, Centrifugation veterinary, DNA administration & dosage, Female, Microinjections veterinary, Polymerase Chain Reaction veterinary, Rabbits genetics, Specific Pathogen-Free Organisms, Superovulation, Zygote Intrafallopian Transfer veterinary, Animals, Genetically Modified embryology, Gene Transfer Techniques veterinary, Rabbits embryology, Zygote growth & development

Abstract

Superovulation of female rabbits was induced by subcutaneous injection(s) of porcine FSH. Zygotes were recovered 17 to 19 hr after hCG injection and were classified into two categories under a microscope equipped with Nomarski interference-contrast optics at x 200 magnification: (A) zygotes with clearly visible pronuclei, or (B) zygotes with visualized pronuclei after 10 min centrifugation at 12,000 x g. No significant difference between strains was found in the proportion of category-A zygotes (JW 72.6% vs NZW 79.3%). Pronuclei of category-A zygotes were located in the center of the cytoplasm, and the pronuclei of category-B zygotes were slightly moved by centrifugation toward the mass of cytoplasmic lipid droplets. Exogenous DNA solution (5 microg/ml of fusion gene composed of bovine alphaS1-casein promoter and human growth hormone structural gene) was microinjected into the pronucleus of the JW zygotes. The pronucleus of category-A zygotes with a mean volume of 7.4 pl swelled up to 16.6 pl (132% increase), while that of category-B zygotes with a mean volume of 6.1 pl swelled up to 15.9 pl (148% increase). Nevertheless, similar proportions of category-A and category-B zygotes developed into offspring after transfer to recipient females (11.1 and 11.2%, respectively). The efficiency to produce hGH-carrying transgenic rabbits was 0.9% (2/235) from category-A zygotes and 0.5% (1/215) from category-B zygotes (P>0.05). To date, transgenic rabbits have been produced without centrifugation of pronuclear zygotes. However approximately 25% of fertilized rabbit zygotes can be used for DNA microinjection after they have been centrifuged to visualize their pronuclei.

Published

2000

6. Effect of culture conditions, donor age, and injection site on in vitro development of DNA microinjected porcine zygotes.

Author

Hajdu MA, Knight JW, Canseco RS, Krisher RL, Velander WH, Pearson RE, and Gwazdauskas FC

Subjects

Animals, Animals, Genetically Modified, Blastocyst, Culture Media, Female, Microinjections veterinary, Sexual Maturation, Superovulation, Temperature, DNA administration & dosage, Genetic Engineering methods, Swine embryology, Zygote growth & development

Abstract

A series of experiments evaluated development of porcine zygotes microinjected with DNA in three culture media and two incubation temperatures, from postpubertal and prepubertal donors, and between zygotes injected with DNA into the pronucleus and the cytoplasm. Zygotes recovered from 36 postpubertal gilts in Exp. 1 were injected and cultured in modified NCSU-23, modified NCSU-37, and CZB media at 37 degrees C or 39 degrees C for 7 d. In Exp. 2, zygotes were collected from postpubertal or prepubertal gilts, microinjected with DNA, and cultured in modified NCSU-23. In Exp. 3 superovulated prepubertal gilts had DNA injected into the cytoplasm or pronucleus of zygotes. Mean percentages developing to the expanded or hatched blastocyst stage in modified NCSU-23 (42.9) and modified NCSU-37 (40.1) did not differ, but development was greater than that for zygotes cultured in CZB (8.8; P < .05). Development was greater at 39 degrees C (P < .05) than at 37 degrees C (36.5 vs 24.6%). Microinjection of DNA decreased development (P < .05) from that of noninjected controls (18.1 vs 43.1%). Zygotes from postpubertal gilts had a higher percentage (68.0) of expanded and hatched blastocysts than zygotes from prepubertal donors (29.0; P < .05). No development difference was found between DNA injection into the pronucleus (23.1%) or cytoplasm (17.4%), but development was less than for control embryos (64.9%; P < .05). DNA microinjected porcine zygotes can be successfully cultured to the expanded blastocyst stage in modified NCSU-23 and modified NCSU-37 media at 39 degrees C.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1994

7. Effects of cumulus cells on culture of bovine embryos derived from oocytes matured and fertilized in vitro.

Author

Thomas WK and Seidel GE Jr

Subjects

Animals, Culture Media, Conditioned, Culture Techniques, Female, Microinjections veterinary, Ovarian Follicle cytology, Cattle embryology, Embryonic and Fetal Development, Fertilization in Vitro, Ovarian Follicle physiology, Zygote growth & development

Abstract

Bovine zygotes derived from oocytes matured and fertilized in vitro were cultured in vitro. In Exp. 1, zygotes were vortexed to remove cumulus cells and then cultured in oviduct epithelial cell-conditioned TCM-199 medium with or without added cumulus cells. Embryos cultured without cumulus cells developed to blastocysts significantly less often than those cultured with added cumulus cells, 3 vs 38% of cleaved ova (P < .05). Co-culture of embryos with cumulus cells during the first 48 h only, or for the duration of the culture period, resulted in development rates similar to those of controls that were not vortexed. In Exp. 2, denuded zygotes were centrifuged (15,850 x g, 3 min) at room temperature to facilitate visualization of pronuclei. Centrifuged zygotes were either placed directly into conditioned medium for culture (with or without added cumulus cells) or DNA was first microinjected into their cytoplasm or a pronucleus. All microinjected embryos were co-cultured with added cumulus cells. Centrifugation and microinjection did not reduce viability significantly when embryos were co-cultured with cumulus cells. Development was reduced significantly when embryos were cultured without cumulus cells. Thus, when oviduct epithelial cell-conditioned medium was used, cumulus cell co-culture was beneficial during the early cleavage stages of in vitro-derived zygotes, including those that received DNA microinjection.

Published

1993