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JBC, Vol. 251, Issue 5, 1258-1263, Mar, 1976
D. A. Thomas and B. E. Wright
A purified preparation of glycogen phosphorylase from Dictyostelium
discoideum was used to elicit specific antisera in rabbits. The antisera
were used to quantitate the amount of precipitable phosphorylase protein
from cell extracts prepared at various stages of the developmental cycle.
Following isotope incorporation studies in differentiating cells, the
specific radioactivity of enzyme isolated by antibody precipitation was
compared to that of acid-insoluble protein. Prior to 5 hours of
development, glycogen phosphorylase could not be detected enzymatically or
immunologically. Between aggregation and culmination, the rate of enzyme
synthesis increased about 6-fold, then decreased to an insignificant value
in young sorocarps. The rate of enzyme degradation was negligible during
the period of maximal enzyme accumulation, then increased to a peak value
of 40% after culmination, coincident with a rapid drop in phosphorylase
activity. The data indicated that the increase in glycogen phosphorylase
activity during development results from an increase in the rate of enzyme
synthesis.
Glycogen phosphorylase in Dictyostelium discoideum. II. Synthesis and degradation during differentiation
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