CRYOPRESERVATION OF SEA URCHIN EMBRYOS AND SPERM. 1979

Eizo Asahina, and Tsuneo Takahashi
Minami 5, Nishi 24, Sapporo, 060 Japan and The American National Red Cross, Blood Research Laboratory, 9312 Old Georgetown Road, Bethesda. MD. 20014 USA.

A simple method for preserving live sea urchin embryos and sperm in liquid nitrogen (LN) wasdeveloped through the use of DMSO as a cryoprotective additive. Samples of late embryos in double test tubes were cooled to- I96°C by two-step freezing, first to - 76°C and then by plunging in LN. In the case of fertilized eggs, samples were previously frozen to - 40°C, at which temperature the samples were kept for 15 min; they were then transferred into LN. After preservation in LN for various lengths of time, samples in the double test tubes were thawed in water at 15°C. The post-thaw survival was more than 90% for late embryos, and about 10% for fertilized eggs. Difference in the length of the cryopreservation period did not affect survival. Post-thaw development in cryopreserved embryos often showed abnormalities in structure. Sperm with 1.5 M DMSO was successfully preserved in LN by a similar method to the one used for cryopreservation of late embryos. Fertilizability in cryopreserved sperm was complete, regardless of the length of the preservation period. Nearly all the eggs fertilized by cryopreserved sperm developed to normal plutei.

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