4.4 Article

The effects of vitrification on gene expression in mature mouse oocytes by nested quantitative PCR

Journal

JOURNAL OF ASSISTED REPRODUCTION AND GENETICS
Volume 27, Issue 11, Pages 599-604

Publisher

SPRINGER/PLENUM PUBLISHERS
DOI: 10.1007/s10815-010-9453-0

Keywords

Cryotop; Gene expression; Nested quantitative; PCR (nqPCR); Vitrified oocyte (MII)

Funding

  1. CITA-A, University of the Azores, Angra do Hero ismo, Portugal
  2. Medical School of Shaheed Beheshti University of Medical Sciences and Health Services, Tehran, Iran
  3. Cellular and Molecular Biology Researcher Center (CMBRC)

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This study was conducted on the effects of vitrification cryotop method on gene expression of mature oocytes in Mus musculus. Transcript analyses of three mouse genes, namely Mater, Hook1 and Sod1, were performed upon non-vitrified and vitrified oocytes with different concentrations of dimethyl sulfoxide (DMSO) and ethylene glycol (EG),15%: 7.5% DMSO + 7.5% EG, and 30%: 15% DMSO + 15% EG, using cryotop following normalization of transcripts with Hprt1 by nested quantitative PCR. Vitrification caused down-regulation of Mater and Hook1 and up-regulation of Sod1 when lower concentrations of cryoprotectants were used as opposed to the control group. The relative expression of Sod1 in vit(2) (30% v/v) was significantly higher than vit(1) (15% v/v)(.) Quantitative transcript analysis of Mater and Hook1 for the vit(2) condition failed to produce any data. Survival rates were the same for both vitrification treatments and significantly lower than control group. Although vit(1) treatment had lower survival rate compared to control group, it demonstrated better stability comparing to vit(2) based on the transcript analysis.

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