1. Cryopreservation of fish gametes

2. What is cryopreservation?
Cryopreservation is the long term preservation of biological material at ultra-low temperatures, usually at C, the temperature of liquid nitrogen.
At this temperature, the cellular viability can be stored in a genetically stable form and is affected only by background radiation.

3. Why cryopreservation?
Cryopreservation has several practical applications in fisheries and aquaculture. They are :
Wider distribution of gametes from one location to another location
Reduces number of male broodfish to be maintained
Facilitates extension of period of seed availability
Selective breeding programmes wherein a large number of families have to be maintained
Production of androgenetic fish
Conservation of genetic resources

4. Cryopreservation of fish spermatozoa:
The spermatozoa of several species of finfish and shellfish have been cryopreserved and `Sperm banks’ established for some species.
This is because of :
-Smaller size (4-6 um)
-Larger number per unit volume (several million spermatozoa/ml milt)
-Repeatability and ease of collection and handling
-Simple membrane (easy to dehydrate or cryoprotect spermatozoa)
Figure: Minute spermatozoa found within Figure: A mature egg (oocyte)
seminiferous lobule

5. Handling of spermatozoa prior to freezing
Collection of spermatozoa from mature male, avoiding contamination with urine, mucus, water, faeces, etc.
Collection of spermatozoa
Males may be injected with spawning agent to ensure higher milt volume
Motility test to be carried out to ensure milt quality
Spermatozoa showing 70% or more motility should be selected for cryopreservation

6. EXTENDER
Extender is a solution of inorganic and organic chemicals, resembling that of blood or seminal plasma
An extender is slightly hypertonic and prevents spermatozoa dehydration/exhaustion
Chemical formulations of extenders used for cryopreservation vary widely depending upon the physiological and chemical characteristics of spermatozoa
Extenders inhibit motility, but initiate motility when diluted with water or activating solution
Figure: Determination of pH of extender Figure: Checking motilityof spermatzoa

7. CRYOPROTECTANT :
Cryoprotectant is added to extender – milt mixture to minimize freeze-damage to cells during cooling/ freezing.
Common cryoprotectants recommended are – dimethyl sulfoxide (DMSO), methanol, glycerol, DMA, etc.
The optimum concentration of cryoprotectant is 5-15% of the total volume of the diluent (extender + milt + cryoprotectant).
Cryoprotectants are of two types- intracellular (penetrating) and extracellular (non-penetrating)
Equilibration period : It is the time allowed for cryoprotectant to penetrate into the sperm cells. It may vary from a few minutes to several minutes.

8. Storage containers: 
Diluted spermatozoa are normally stored in polypropylene vials (1-2 ml), as pellets ( µl) and in 0.25 or 0.50 ml plastic and then it forms a seal when comes in contact with a fluid.
Figure: Filling plastic straw with diluted spermatozoa

9. Dilution ratio:
The spz : diluent ratio varies between 1:1 and 1:10, depending upon species.
The dilution ratio should be such that the spz need not be diluted further at the time of fertilization.

10. Cooling/freezing rate:
Cooling/freezing is considered the most critical variable of cryopreservation.
The optimum rate is between 10 and 450C per minute.
Liquid nitrogen (-1960C) is the most commonly used cryogen for freezing and storing spz.
Frozen spermatozoa samples are stored in vapor phase or immersed under liquid nitrogen.
Figure: Straws being frozen over LN Figure: Frozen straws being immersed in LN2

11. Warming/thawing rate:
Thawing is also considered an important variable in cryopreservation.
Very rapid thawing rates are used to avoid recrystallization.
Slow warming rate may result in recrystallization.
Thawing of preserved spz is accomplished by agitating them in hot-water bath at 370C for seconds
Thawing rates of C are recommended, although higher rates of C have also been used.
Figure: Straws being thawed at 370C

12. Viability of cryopreserved spermatozoa :
Spermatozoa stored under LN2 remain fertile indefinite.
They should be thawed only when required for checking motility.
Motility, fertilization and hatching rates, fry survival, etc. are the common criteria for judging the post-thaw viability/fertility of cryopreserved spermatozoa

13. Cryopreservation of eggs/embryos:
No success
The fundamental problems are – insufficient dehydration during cooling/freezing due to relatively large size (1-6 mm) of fish eggs, the presence of membranes of different water permeability.
Also permeation of cryoprotectant even into smaller eggs and embryos is low.
However, success has been achieved with invertebrate eggs and embryos.
Sea urchin embryos, oyster larvae (trochophore) and penaied shrimp naupli have been successfully cryopreserved and revived.

14. Embryonic cell cryopreservation:
Studies show that the cells from blastula can be removed and successfully cryopreserved
This involves dechorionization of unfertilized water-hardened egg, removal of nucleus from the egg, micro-injection of thawed dissociated cells from mid-blastula into the enucleated egg and its subsequent development into a viable embryo