The biosynthesis of glucagon was studied by using the recirculated, isolated perfused rat pancreas. [3H]Tryptophan was initially incorporated into acid–ethanol-extractable protein, which on gel filtration was eluted with a molecular weight of about 9000 and contained a small amount of glucagon immunoreactivity. With longer incubation [3H]tryptophan incorporation into a second peak was obtained in an identical position with that of the majority of rat glucagon immunoreactivity. This peak of labelled protein exhibited migration characteristics on polyacrylamide-gel electrophoresis identical with those of rat glucagon and was identified as newly synthesized glucagon by demonstration of specific binding and dissociation behaviour with glucagon antibodies. The incorporation of [3H]tryptophan into acid–ethanol-extractable protein was inhibited by cycloheximide. High concentrations of glucose increased [3H]tryptophan incorporation into high-molecular-weight protein but decreased incorporation into proteins smaller than cytochrome c. The pattern of [3H]leucine incorporation into protein was similar to that of [3H]tryptophan.
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June 1973
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Research Article|
June 01 1973
The biosynthesis of glucagon in perfused rat pancreas Available to Purchase
Kevin J. O'Connor;
Kevin J. O'Connor
1Diabetes Research Unit, The Wellcome Foundation, Temple Hill, Dartford, Kent, U.K.
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Adrian Gay;
Adrian Gay
1Diabetes Research Unit, The Wellcome Foundation, Temple Hill, Dartford, Kent, U.K.
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Norman R. Lazarus
Norman R. Lazarus
1Diabetes Research Unit, The Wellcome Foundation, Temple Hill, Dartford, Kent, U.K.
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Publisher: Portland Press Ltd
© 1973 London: The Biochemical Society
1973
Biochem J (1973) 134 (2): 473–480.
Citation
Kevin J. O'Connor, Adrian Gay, Norman R. Lazarus; The biosynthesis of glucagon in perfused rat pancreas. Biochem J 1 June 1973; 134 (2): 473–480. doi: https://doi.org/10.1042/bj1340473
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