Literature DB >> 11906923

Successful piglet production after transfer of blastocysts produced by a modified in vitro system.

Kazuhiro Kikuchi1, Akira Onishi, Naomi Kashiwazaki, Masaki Iwamoto, Junko Noguchi, Hiroyuki Kaneko, Tomiji Akita, Takashi Nagai.   

Abstract

Porcine in vitro production (IVP) systems, including in vitro maturation (IVM) and in vitro fertilization (IVF) of oocytes and their subsequent in vitro culture (IVC), have been modified by many researchers, but are still at a low level because of a low developmental rate of embryos to the blastocyst stage and their poor qualities. Our objectives were to establish reliable IVP procedures for porcine blastocysts and to examine the ability of the blastocysts to develop to term after transfer to recipients. Porcine cumulus-oocyte complexes were matured in vitro under 5% O(2) or 20% O(2), fertilized in vitro under 5% O(2), and subsequently cultured under 5% O(2) in 1) IVC medium supplemented with glucose (IVC-Glu) from Day 0 (the day of IVF) to Day 6; 2) IVC-Glu from Days 0 to 2, then IVC medium supplemented with pyruvate and lactate (IVC-PyrLac) from Days 2 to 6; 3) IVC-PyrLac from Days 0 to 2, then IVC-Glu from Days 2 to 6; and 4) IVC-PyrLac from Days 0 to 6. There were no significant differences in blastocyst formation rates on Day 6 between the 5% O(2) and 20% O(2) conditions (19.9% and 14.0%, respectively). However, the quality of blastocysts, as evaluated by the total cell number, was better after IVM under 5% O(2) than under 20% O(2) (mean cell number, 43.5 and 37.8, respectively). When IVP embryos were cultured in IVC-PyrLac from Days 0 to 2 and subsequently in IVC-Glu from Days 2 to 6, the rate of blastocyst formation (25.3%) and cell number (48.7) were higher than the rates (5.8% to 18.1%) and numbers (35.4 to 37.1) with the IVC-Glu then IVC-Glu, the IVC-Glu then IVC-PyrLac, and the IVC-PyrLac then IVC-PyrLac regimens, respectively. We then prepared conditioned medium (CM) from culture of porcine oviductal epithelial cells for 2 days in IVC-PyrLac and evaluated its effect on development to the blastocyst stage. Cultivation in CM for the first 2 days, followed by IVC-Glu for a further 4 days, had a significantly greater effect in increasing the number of cells in the blastocyst (58.3) than did in IVC-PyrLac (48.4). Finally, we evaluated the ability of blastocysts, generated by IVM under 5% O(2) and IVC in CM, to develop to term. When Day 5 expanding blastocysts (mean cell number, 49.7) were transferred to an estrus-synchronized recipient (50 blastocysts per recipient), the recipient remained pregnant and farrowed eight normal piglets. Furthermore, when Day 6 expanded blastocysts (mean cell number, 80.2) were transferred to two estrus-synchronized recipients, both gilts remained pregnant and farrowed a total of 11 piglets. These results suggest that an excellent piglet production system can be established by using this modified IVP system, which produces high-quality porcine blastocysts. This system has advantages for the generation of cloned and transgenic pigs.

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Year:  2002        PMID: 11906923     DOI: 10.1095/biolreprod66.4.1033

Source DB:  PubMed          Journal:  Biol Reprod        ISSN: 0006-3363            Impact factor:   4.285


  44 in total

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2.  Isolation and characterization of porcine visceral endoderm cell lines derived from in vivo 11-day blastocysts.

Authors:  Neil C Talbot; Le Ann Blomberg; Ayesha Mahmood; Thomas J Caperna; Wesley M Garrett
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3.  Stem Cell-Derived Bioactive Materials Accelerate Development of Porcine In Vitro-Fertilized Embryos.

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Journal:  Cell Reprogram       Date:  2015-06       Impact factor: 1.987

4.  Piglets produced from cloned blastocysts cultured in vitro with GM-CSF.

Authors:  Kiho Lee; Bethany K Redel; Lee Spate; Jennifer Teson; Alana N Brown; Kwang-Wook Park; Eric Walters; Melissa Samuel; Clifton N Murphy; Randall S Prather
Journal:  Mol Reprod Dev       Date:  2013-01-22       Impact factor: 2.609

5.  Production of transgenic-clone pigs by the combination of ICSI-mediated gene transfer with somatic cell nuclear transfer.

Authors:  Mayuko Kurome; Hideto Ueda; Ryo Tomii; Katsutoshi Naruse; Hiroshi Nagashima
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6.  In vitro effects of relaxin on gene expression in porcine cumulus-oocyte complexes and developing embryos.

Authors:  Jean M Feugang; Jonathan M Greene; Scott T Willard; Peter L Ryan
Journal:  Reprod Biol Endocrinol       Date:  2011-01-27       Impact factor: 5.211

7.  Development to the blastocyst stage, the oxidative state, and the quality of early developmental stage of porcine embryos cultured in alteration of glucose concentrations in vitro under different oxygen tensions.

Authors:  Ni Wayan Kurniani Karja; Kazuhiro Kikuchi; Mokhamad Fahrudin; Manabu Ozawa; Tamás Somfai; Katsuhiko Ohnuma; Junko Noguchi; Hiroyuki Kaneko; Takashi Nagai
Journal:  Reprod Biol Endocrinol       Date:  2006-11-06       Impact factor: 5.211

8.  Excess polyspermy reduces the ability of porcine oocytes to promote male pronuclear formation after in vitro fertilization.

Authors:  Hiep Thi Nguyen; Thanh Quang Dang-Nguyen; Tamas Somfai; Nguyen Thi Men; Barbara Beck-Woerner; Nguyen Viet Linh; Bui Xuan Nguyen; Junko Noguchi; Hiroyuki Kaneko; Kazuhiro Kikuchi
Journal:  Anim Sci J       Date:  2021       Impact factor: 1.974

9.  Generation of live piglets for the first time using sperm retrieved from immature testicular tissue cryopreserved and grafted into nude mice.

Authors:  Hiroyuki Kaneko; Kazuhiro Kikuchi; Michiko Nakai; Tamas Somfai; Junko Noguchi; Fuminori Tanihara; Junya Ito; Naomi Kashiwazaki
Journal:  PLoS One       Date:  2013-07-29       Impact factor: 3.240

10.  Selection of in vitro-matured porcine oocytes based on localization patterns of lipid droplets to evaluate developmental competence.

Authors:  Kou Hiraga; Yumi Hoshino; Kentaro Tanemura; Eimei Sato
Journal:  J Reprod Dev       Date:  2013-04-18       Impact factor: 2.214

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