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J Thorac Cardiovasc Surg 1998;115:638-643
© 1998 Mosby, Inc.
CARDIAC AND PULMONARY REPLACEMENT |
This work was supported by the Mayo Clinic and Foundation, Rochester, Minnesota, and the Bruce and Ruth Rappaport Program in Vascular Biology. Dr Anders Jeppsson is a visiting scientist supported by grants from University of Gothenburg, Assar Gabrielsson Foundation, Swedish Medical Society, Swedish Medical Research Council and Gothenburg Medical Society.
Received for publication May 22, 1997; revisions requested July 15, 1997; revisions received August 13, 1997; accepted for publication Sept. 22, 1997. Address for reprints: C. G. A. McGregor, MB, FRCS, 6-716 Mary Brigh D, Saint Marys Hospital, Mayo Clinic, Rochester, MN 55905.
Abstract
Objectives: Gene therapy may provide a means of modifying factors that contribute to the development of pathologic processes in transplanted lungs. Experiments were designed to study the feasibility of adenovirus-mediated gene transfer by way of the airways to the transplanted lung.
Methods: Orthotopic left lung transplantation (Lewis to Lewis rats) was performed on four groups of animals. 300 µl of adenovirus solution encoding for ß-galactosidase was infused into the left bronchus of donor rats at viral concentrations of 108 pfu/ml (n = 5), 109 pfu/ml (n = 6), and 1010 pfu/ml (n = 6), and the lung was ventilated for 5 minutes. Controls (n = 6) received medium only. Seven days after transplantation, native and transduced, transplanted lungs were harvested. Sections of lung were fixed and stained with a solution of X-Gal (5-bromo-4-chloro-3-indolyl-ß-D-galactopyranoside) and staining was evaluated for distribution by cell type and intensity.
Results: ß-Galactosidase expression was absent in the control group and in the native lungs. Two of five lungs in the 108 group expressed ß-galactosidase, but in a limited distribution and intensity. All six lungs in the 109 group and five of six lungs in the 1010 group expressed ß-galactosidase. The distribution and intensity of ß-galactosidase expression ranged from only a few cells staining per slide to up to 75%. Pneumocytes were the most frequently stained cell type followed by alveolar macrophages.
Conclusions: Gene transfer to the transplanted lung via the bronchial route is feasible and offers a novel technique to modify pathologic processes in the transplanted lung.
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