127 Binding retinoid receptors by specific agonists affects the bovine blastocyst development in vitro.

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dc.contributor Gomez, E
dc.contributor Rodriguez, A
dc.contributor Alonso-Montes, C
dc.contributor Caamano, N
dc.contributor Royo, L J
dc.contributor Goyache, F
dc.contributor Facal, N
dc.contributor Ikeda, S
dc.contributor Alvarez, I
dc.contributor Diez, C
dc.date.accessioned 2012-01-30T22:31:03Z
dc.date.available 2012-01-30T22:31:03Z
dc.date.issued 2006
dc.identifier.citation Rep. Fert. Dev. (2006) 18(1&2): 172-172
dc.identifier.issn 1031-3613
dc.identifier.uri http://livestocklibrary.com.au/handle/1234/17483
dc.description.abstract Production of embryos in vitro with improved inner cell mass (ICM) and high ICM per total cell rate is a major objective in reproductive biotechnology. Exogenous all-trans retinoic acid (ATRA), a vitamin A metabolite, and endogenous retinoid regulate development and differentiation during bovine morula to blastocyst transition in vitro. ATRA binds to retinoic acid-receptor (RAR), and the ATRA isomere 9-cis-retinoic acid (9-cis-RA) binds to both RAR and the retinoid X receptor (RXR). The unspecific binding of 9-cis-RA to receptors makes it difficult to study RXR transactivation. Therefore, in this work we studied blastocyst development and cell counts by using a specific synthetic RXR agonist [LG100268 LG; a gift of Ligand Laboratories] as opossed to the effect exerted by ATRA upon RAR binding. Cumulus-oocyte complexes from slaughterhouse ovaries were matured and fertilized in vitro. Presumptive zygotes were cultured in B2 medium with Vero cells until 139 h post-insemination (Day 6), the time at which embryos [morulae (e90%) + early blastocysts] underwent treatments for 48 h in 400 _L of SOFaaci + 5% FCS. Data (5 replicates per experiment) were analyzed by CATMOD for effects, processed by GLM and Duncan&apos;s test, and expressed as LSM � SE (a,b,c P d 0.05). After a LG dose-response experiment (n = 480 morulae), blastocysts rates from LG 1 _M on Day 7 were higher than LG 10 _M, LG 0.1 _M, and LG 0 _M (Day 7: 42.8 � 4.1 vs. 34.4 � 3.7, 36.8 � 3.7, and 32.4 � 3.7, respectively). On Day 8, LG 1 _M also yielded more blastocysts than LG 0.1 _M (50 � 4.2 vs. 44.4 � 3.7, respectively). By differential cell counting (n = 113 blastocysts), hatched blastocysts with LG 10 _M showed proliferation in the ICM, while trophectoderm (TE) cells decreased conversely to LG concentration. These effects were not obvious in expanded blastocysts. In a subsequent experiment (n = 340 morulae), ATRA led to blastocysts rates on Day 8 that were higher than negative, untreated controls, but not different from LG 1 _M (42.4 � 2.4 vs. 33.1 � 2.0 and 36.0 � 2.4, respectively). ATRA and LG 1 increased TE in expanded blastocysts (n = 42) (102 � 13.2 and 96.23 � 13.2, respectively vs. 72.8 � 10.9 in the untreated group) but not in their hatched counterparts (n = 44). There were no differences in the ICM; but percentages of ICM per total cells were higher in hatched blastocysts cultured with ATRA than in expanded LG 1 _M blastocysts and expanded controls (39.5 � 5.5 vs. 24.2 � 5.7, and 20.9 � 4.7, respectively). Manipulation of retinoid receptor-specific pathways make it possible to control blastocyst development and differentiation, leading to embryos of improved quality and viability. Work is in progress to analyze gene expression in these blastocysts.<fn_group><fn>This work was supported by grant MCYT, project AGL-2005-04479.</fn></fn_group>
dc.publisher CSIRO Publishing
dc.source.uri http://www.publish.csiro.au//nid/44/paper/RDv18n2Ab127.htm
dc.title 127 Binding retinoid receptors by specific agonists affects the bovine blastocyst development in vitro.
dc.type Research
dc.description.version Abstract
dc.identifier.volume 18
dc.identifier.page 172-172
dc.identifier.issue 1&2


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