Minimal volume vitrification of epididymal spermatozoa results in successful in vitro fertilization and embryo development in mice

This study compared three cryopreservation protocols on sperm functions, IVF outcomes, and embryo development. Epididymal spermatozoa cryopreserved using slow-cooling (18% w/v raffinose, RS-C) were compared with spermatozoa vitrified using 0.25 M sucrose (SV) or 18% w/v raffinose (RV). The motility,...

Full description

Saved in:
Bibliographic Details
Published in:Asian journal of andrology 2017-01, Vol.19 (1), p.107-112
Main Authors: Horta, Fabrizzio, Alzobi, Hamida, Jitanantawittaya, Sutthipat, Catt, Sally, Chen, Penny, Pangestu, Mulyoto, Temple-Smith, Peter
Format: Article
Language:English
Subjects:
Animals
Blastocyst
Cell Survival
Cooling
Cryopreservation - methods
cryopreservation
epididymal sperm
in vitro fertilization/intracytoplasmic sperm injection
reproductive techniques
sperm DNA damage
vitrification
Deoxyribonucleic acid
Design
DNA
DNA Fragmentation
Embryonic Development
Embryos
Experiments
Female
Fertilization in Vitro - methods
Fish
Glycerol
In vitro fertilization
Infertility
Male
Methods
Mice
Motility
Nitrogen
Observations
Oocytes
Original
Physiological aspects
Reproductive technologies
Rodents
Semen Preservation - methods
Sperm
Sperm Motility
Sperm Retrieval
Spermatozoa - metabolism
Studies
Sucrose
Supervision
Vitrification
Citations: Items that cite this one
Online Access:Get full text
Tags: Add Tag
No Tags, Be the first to tag this record!
Description
Summary:This study compared three cryopreservation protocols on sperm functions, IVF outcomes, and embryo development. Epididymal spermatozoa cryopreserved using slow-cooling (18% w/v raffinose, RS-C) were compared with spermatozoa vitrified using 0.25 M sucrose (SV) or 18% w/v raffinose (RV). The motility, vitality, and DNA damage (TUNEL assay) of fresh control (FC) spermatozoa were compared with post-thawed or warmed RS-C, RV, and SV samples. Mouse oocytes (n = 267) were randomly assigned into three groups for insemination: RV (n = 102), RS-C (n = 86), and FC (n = 79). The number and the proportion of two-cell embryos and blastocysts from each treatment were assessed. Sperm motility (P 〈 0.01) and vitality (P 〈 0.05) were significantly reduced after vitrification compared with slow-cooled spermatozoa. However, DNA fragmentation was significantly reduced in spermatozoa vitrified using sucrose (15 - 1.8% [SV] vs 26 - 2.8% [RV] and 27 - 1.2% [RS-C]; P 〈 0.01). Although the number of two-cell embryos produced by RS-C, RV, and FC spermatozoa was not significantly different, the number of blastocysts produced from two-cell embryos using RV spermatozoa was significantly higher than FC spermatozoa (P = 0.0053). This simple, small volume vitrification protocol and standard insemination method allows successful embryo production from small numbers of epididymal spermatozoa and may be applied clinically to circumvent the need for ICSI, which has the disadvantage of bypassing sperm selection.
ISSN:1008-682X
1745-7262
DOI:10.4103/1008-682X.183378