Literature DB >> 9538325

Production of normal offspring from mouse oocytes injected with spermatozoa cryopreserved with or without cryoprotection.

T Wakayama1, D G Whittingham, R Yanagimachi.   

Abstract

Epididymal mouse spermatozoa were suspended in various physiological solutions (CZB, PBS or isotonic saline) with or without 18% (w/v) raffinose before cooling to -20 degrees, -50 degrees or -196 degrees C and storage for 1-28 days. After thawing, a few spermatozoa frozen with raffinose were partially motile (about 2%) but in all other treatments they were immotile and diagnosed as 'dead' by staining that differentiates between live and dead spermatozoa. Almost all oocytes injected with sperm heads (nuclei) from spermatozoa frozen with and without raffinose were fertilized normally (95-100%) and developed to the two-cell stage (89-100%). No differences were found between the physiological media. The majority of oocytes fertilized with spermatozoa frozen in CZB medium developed to blastocysts (80-94%) but development was significantly reduced after fertilization with spermatozoa frozen in PBS and isotonic saline especially in the absence of raffinose (69 and 70% versus 51 and 50%). Normal fertile offspring were obtained in all treatments but there were significantly fewer offspring with spermatozoa stored at -196 degrees C in isotonic saline with or without raffinose and CZB with raffinose. Testicular spermatozoa were extremely sensitive to cryodamage: about 50% frozen to -196 degrees C in CZB with or without raffinose disintegrated after thawing. Almost 100% of oocytes injected with sperm heads from intact (at light microscope level) testicular spermatozoa developed to the two-cell stage but development to blastocysts was reduced significantly compared with that of controls especially those without raffinose. The data indicate that cryopreservation of sperm nuclei requires less stringent conditions than those for the retention of normal physiological function of intact spermatozoa. Motility and plasma membrane integrity are not essential for fertilization and the production of live offspring when nuclei of nonviable spermatozoa are injected into oocytes.

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Year:  1998        PMID: 9538325     DOI: 10.1530/jrf.0.1120011

Source DB:  PubMed          Journal:  J Reprod Fertil        ISSN: 0022-4251


  14 in total

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2.  Placental inflammation and oxidative stress in the mouse model of assisted reproduction.

Authors:  J M Raunig; Y Yamauchi; M A Ward; A C Collier
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Review 3.  Male infertility and the genetics of spermatogenesis.

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Review 4.  Simple gamete preservation and artificial reproduction of mammals using micro-insemination techniques.

Authors:  Takehito Kaneko
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5.  Spermatozoa and spermatids retrieved from frozen reproductive organs or frozen whole bodies of male mice can produce normal offspring.

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6.  Improvement in the development of oocytes from C57BL/6 mice after sperm injection.

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Journal:  J Am Assoc Lab Anim Sci       Date:  2011-01       Impact factor: 1.232

7.  Maintenance of genetic integrity in frozen and freeze-dried mouse spermatozoa.

Authors:  H Kusakabe; M A Szczygiel; D G Whittingham; R Yanagimachi
Journal:  Proc Natl Acad Sci U S A       Date:  2001-11-13       Impact factor: 11.205

8.  Production of fertile offspring from genetically infertile male mice.

Authors:  Ryuzo Yanagimachi; Teruhiko Wakayama; Hidefumi Kishikawa; Gian Maria Fimia; Lucia Monaco; Paolo Sassone-Corsi
Journal:  Proc Natl Acad Sci U S A       Date:  2004-02-02       Impact factor: 11.205

Review 9.  Chromosomal integrity and DNA damage in freeze-dried spermatozoa.

Authors:  Hirokazu Kusakabe
Journal:  Reprod Med Biol       Date:  2011-06-01

10.  Production of viable trout offspring derived from frozen whole fish.

Authors:  Seungki Lee; Shinsuke Seki; Naoto Katayama; Goro Yoshizaki
Journal:  Sci Rep       Date:  2015-11-02       Impact factor: 4.379

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