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J Thorac Cardiovasc Surg 1994;108:63-67
© 1994 Mosby, Inc.


SURGERY FOR ACQUIRED HEART DISEASE

Biochemical and cellular characterization of cardiac valve tissue after cryopreservation or antibiotic preservation

Samuel J. Lang, DVM, MDa, Marie S. Giordano, RN, MSa, Carlos Cardon-Cardo, MD, PhDb, Barbara D.Summers, BSc, Lisa Staiano-Coico, PhDa, David P. Hajjar, PhDc


New York, N.Y.

Received for publication June 28, 1993. Accepted for publication Nov. 12, 1993. Address for reprints: David P. Hajjar, PhD, Department of Pathology, Cornell University Medical Center, 1300 York Ave., New York, NY 10021.

Abstract

It has been reported that aortic homografts that have been cryopreserved before transplantation remain viable longer as an allograft than tissue stored at 4° C in an antibiotic solution. In the present study, we tested the hypothesis that storage of cardiac valve tissue by cryopreservation or by antibiotic preservation may alter the metabolic status of the tissue. Initially, we collected aortic valves composed of cardiac tissue, aortic root, and valvular tissue from cadaver donors. These specimens were divided into three equal portions, and one portion was analyzed before storage while the other two parts were stored for 3 weeks at either 4° C in an antibiotic solution or at -196° C in liquid nitrogen. All specimens were examined with regard to the following parameters: tissue structure, tissue viability, cell proliferative capacity, metabolic function, and identification of cell-specific antigens. We found no significant alterations in the structure of any of the three tissue components after antibiotic preservation or cryopreservation; however, cell viability and cell number were decreased in all three groups. All tissue samples grew in culture before storage. When we compared activities of the following organellar marker enzymes—lysosomal acid lipase, plasma membrane 5' nucleotidase, mitochondrial cytochrome oxidase, and microsomal neutral {alpha}-glucosidase—we observed no major differences between tissues stored by either technique. In addition, we observed no loss of enzymic activity as a result of storage. Finally, when cell lines isolated from each tissue specimen were incubated with monoclonal antibodies against cell-specific antigens in an immunoperoxidase assay, all the cell cultures proved to be endothelial cells. These results suggest that although cardiac valve tissue stored by cryopreservation or by antibiotic preservation retained its normal structure and metabolic capabilities, both storage techniques produced significant decreases in cell numbers and viability. However, only endothelial cells from tissue stored by cryopreservation retained the capacity to proliferate in vitro. These findings have important implications for the function of aortic homografts transplanted after storage. (J THORACCARDIOVASCSURG1994;108:63-7)




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