The chick oviduct in tissue culture. I. Initial characterization of growing primary oviduct tissue cultures |
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Authors: | S S Seaver J van der Bosch G Sato |
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Institution: | 1. Department of Molecular Biology, Vanderbilt University, Nashville, TN 37235, USA;2. Department of Biology, University of California, San Diego, USA;3. Cancer Center, University of California at San Diego, La Jolla, CA 92093, USA |
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Abstract: | A simple three-enzyme treatment of collagenase, dispase and hyaluronidase on finely minced chick oviduct yields clumps of 50-150 cells. These cells attach to collagen-treated dishes and survive in culture for at least 2 weeks without subculturing. Oviduct cell cultures can also be induced to grow. Estradiol or epidermal growth factor (EGF) induce a 40% increase in cells in 4 days when cultures are grown in serum levels that do not support growth. Serum from estrogen-stimulated chicks promotes rapid cellular proliferation (doubling times of 1-2 days). Sera from estrogen withdrawn chicks, laying hen or horse do not support as rapid proliferation. The oviduct growth-promoting factors in serum from estrogen-stimulated chicks are not steroids or fibroblast growth factors (FGF). Removal of steroids from these sera by charcoal treatment or delipidization does not decrease the rate of growth. The addition of 1-100 nM estradiol does not increase a serum's ability to promote growth. Purified FGF or platelet-derived growth factor (PDGF) do not induce oviduct proliferation. These results were reproduced in oviduct cell cultures started from estrogen-stimulated and withdrawn chicks as well as laying hens. Thus the factors in serum from estrogen-stimulated chicks that promote rapid oviduct growth are induced by estrogen treatments in vivo, but do not seem to be only steroids. |
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Keywords: | To whom offprint requests should be sent Please request reprint number RP085 Current address: Millipore Corporation 80 Ashby Road Bedford MA 01730 USA |
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