Literature DB >> 11098034

A strategy for rapid cooling of mouse embryos within a double straw to eliminate the risk of contamination during storage in liquid nitrogen.

L L Kuleshova1, J M Shaw.   

Abstract

Double packaging, in which an inner straw containing the specimen is inserted into an outer, larger straw (here termed 'straw-in-straw') to prevent the inner straw from coming into direct contact with liquid nitrogen provides a simple strategy for reducing or eliminating the potential contamination risk associated with storage in liquid nitrogen. This approach has in the past been used in conjunction with cryopreservation by slow cooling, but has not previously been tested for use throughout an entire rapid cooling and warming procedure. This study determined whether keeping the straw containing the embryos inside a second protecting container throughout the cryopreservation and storage protocol would compromise embryo viability. We established that a cryoprotectant containing a high polymer concentration (35% dextran or Ficoll) together with 25% ethylene glycol (as the penetrating cryoprotectant) was highly effective for day 2 and day 3 mouse embryos in both single and double straws. The survival and development of all cryopreserved embryos, as assessed both in vitro and in vivo, was not statistically different to their untreated controls. This established that a protein/serum-free cryoprotectant solution supplemented with polymers could provide complete protection of mouse embryos. It also shows, for the first time, that embryos can be cooled by direct immersion in liquid nitrogen and warmed by direct immersion into a waterbath within a double straw arrangement to reduce the likelihood of contamination.

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Year:  2000        PMID: 11098034     DOI: 10.1093/humrep/15.12.2604

Source DB:  PubMed          Journal:  Hum Reprod        ISSN: 0268-1161            Impact factor:   6.918


  12 in total

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Journal:  Reprod Med Biol       Date:  2014-02-05

3.  Closed-system solid surface vitrification versus slow programmable freezing of mouse 2-cell embryos.

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Review 4.  Advanced technologies for the preservation of mammalian biospecimens.

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Journal:  Nat Biomed Eng       Date:  2021-08-23       Impact factor: 29.234

5.  High-Throughput Non-Contact Vitrification of Cell-Laden Droplets Based on Cell Printing.

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6.  Closed vitrification of mouse oocytes using the CryoLogic vitrification method: A modification that improves developmental competence.

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Journal:  Clin Exp Reprod Med       Date:  2013-12-31

7.  From fresh heterologous oocyte donation to autologous oocyte banking.

Authors:  D Stoop
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Review 8.  Oocyte, embryo and blastocyst cryopreservation in ART: systematic review and meta-analysis comparing slow-freezing versus vitrification to produce evidence for the development of global guidance.

Authors:  Laura Rienzi; Clarisa Gracia; Roberta Maggiulli; Andrew R LaBarbera; Daniel J Kaser; Filippo M Ubaldi; Sheryl Vanderpoel; Catherine Racowsky
Journal:  Hum Reprod Update       Date:  2017-03-01       Impact factor: 15.610

9.  Effects of various freezing containers for vitrification freezing on mouse oogenesis.

Authors:  Ji Chul Kim; Jae Myeoung Kim; Byoung Boo Seo
Journal:  J Anim Sci Technol       Date:  2016-03-20

Review 10.  Risk of Contamination of Gametes and Embryos during Cryopreservation and Measures to Prevent Cross-Contamination.

Authors:  Daniel C Joaquim; Eduardo D Borges; Iara G R Viana; Paula A Navarro; Alessandra A Vireque
Journal:  Biomed Res Int       Date:  2017-08-14       Impact factor: 3.411

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