Cryopreservation of isolated blood vessels.

Canine saphenous veins were immersed in fetal calf serum (FCS) containing various cryoprotective agents, slowly frozen and stored for several weeks at subzero temperatures. Pharmacological investigations of frozen/thawed tissues revealed considerable attenuation of the contractile force of frozen stored veins as compared to unfrozen veins. The best recovery after thawing of frozen stored canine veins was obtained on tissues which had been frozen slowly to -70 degrees C and stored in liquid nitrogen while being immersed in FCS containing 1.8 mol/l dimethyl sulfoxide (DMSO). Though the maximum response to noradranline of helical strips prepared from these veins was diminished to about 60% the evidence suggests that there may be a very good preservation of the main biochemical properties, such as monoamine oxidase activity, endogenous prostaglandin synthesis and neuronal uptake mechanism in veins stored under these conditions. The same method of cryopreservation was applied to store samples of human veins. Comparison of the pD2 values for various agonists and of the blocking activities of various antagonists of both 5-HT receptors and alpha-adrenoceptors yielded an excellent correlation between the parameters determined on frozen/thawed and unfrozen human veins. It is concluded that freezing isolated blood vessels may be considered an effective means of preserving and storing vascular tissues for pharmacological investigations.