Literature DB >> 9089067

Continuous assessment of human spermatozoa viability during cryopreservation.

S N Mohammad1, C L Barratt, I D Cooke, H D Moore.   

Abstract

Cryomicroscopy has enabled direct observation of freezing and thawing of human spermatozoa. When used with a fluorescent viability kit, sperm membrane damage was not apparent down to temperatures of -5 degrees C, but significant damage occurred after thawing (55% of spermatozoa had damaged membranes). Semen samples were cooled or frozen to temperatures (at decrements of 10 degrees C) from 0 degree C to -110 degrees C. At all these temperatures the proportion of live to membrane-damaged cells remained constant. Samples held at temperatures above -30 degrees C were not adversely affected. Below -30 degrees C there was a gradual increase in the proportion of membrane-damaged cells on thaw and a decrease in the number of live cells recovering motility. At temperatures between -50 degrees C and -60 degrees C there was an equal proportion of live motile, immotile, and membrane-damaged cells. It is concluded that some irreversible damage to spermatozoa was a result of freezing processes in cells frozen to -30 degrees C or less, but most of the cryodamage was incurred during thawing, possibly due to recrystallization.

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Year:  1997        PMID: 9089067

Source DB:  PubMed          Journal:  J Androl        ISSN: 0196-3635


  3 in total

1.  Vitality of oligozoospermic semen samples is improved by both swim-up and density gradient centrifugation before cryopreservation.

Authors:  Madeleine Counsel; Rhys Bellinge; Peter Burton
Journal:  J Assist Reprod Genet       Date:  2004-05       Impact factor: 3.412

2.  The effect of pH and viscosity on bovine spermatozoa motility under controlled conditions.

Authors:  Avez A Rizvi; Mohammed I Quraishi; Vikren Sarkar; Chris DuBois; Sinan Biro; John Mulhall
Journal:  Int Urol Nephrol       Date:  2008-11-11       Impact factor: 2.370

3.  No evidence for killer sperm or other selective interactions between human spermatozoa in ejaculates of different males in vitro.

Authors:  H D Moore; M Martin; T R Birkhead
Journal:  Proc Biol Sci       Date:  1999-12-07       Impact factor: 5.349

  3 in total

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