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Glycogen metabolism in cultured chick hepatocytes: A morphological study
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AbstractUltrastructural and autoradiographic observations of cultured chick hepatocytes under the following conditins are described: Induction of glycogen synthesis with glucose alone and glucose plus insulin, and glucagon‐induced glucogen glucogen breakdown. Profiles of hepatocytes cultured in medium containig 10 mM glucose showed typical cellular organelles and occasionally a few glycogen granules. After incubation of hepatocytes with 3H‐glucose, silver grains were found over these sparse glycogen granules, indicating a low level of glycogen synthesis by a few cells. After addition of 75 mM glucose for 1 hr about 3% of the profiles of cells showed glycogen, and by 24 hr half of the hepatocytes had glycogen. Addition ofinsulin plus glucose induced glycogen synthesis in 82% of the cells after 6 hr. and by 24 hr almost every cellular profile showed glyocgen particles. Morphologically, glycogen accumulation was similar whether the cells were stimulated by high glucose or by glucose plus insulin: glycogen granules appeared in restricted regions of the cytoplasm, which were rich in smooth endoplasmic reticulum (SER), and peroxisomes were found close to the newly deposited glycogen particles. At maximum glycogen accumulation the association of SER and peroxisomes with glycogen was less obvious. Glycogenolysis induced by incubation of glycogen‐rich hepatocytes with glucagon resulted in proliferation of SER in the glycogen regions of the cells. These observations are compatible with the concept of regions in the hepatocyte cytoplasm specialized for glycogen metabolism. Possible roles for SER and peroxisomes found near glycogen particles and other organelles in hepatic glycogen metabolism are discussed.
Title: Glycogen metabolism in cultured chick hepatocytes: A morphological study
Description:
AbstractUltrastructural and autoradiographic observations of cultured chick hepatocytes under the following conditins are described: Induction of glycogen synthesis with glucose alone and glucose plus insulin, and glucagon‐induced glucogen glucogen breakdown.
Profiles of hepatocytes cultured in medium containig 10 mM glucose showed typical cellular organelles and occasionally a few glycogen granules.
After incubation of hepatocytes with 3H‐glucose, silver grains were found over these sparse glycogen granules, indicating a low level of glycogen synthesis by a few cells.
After addition of 75 mM glucose for 1 hr about 3% of the profiles of cells showed glycogen, and by 24 hr half of the hepatocytes had glycogen.
Addition ofinsulin plus glucose induced glycogen synthesis in 82% of the cells after 6 hr.
and by 24 hr almost every cellular profile showed glyocgen particles.
Morphologically, glycogen accumulation was similar whether the cells were stimulated by high glucose or by glucose plus insulin: glycogen granules appeared in restricted regions of the cytoplasm, which were rich in smooth endoplasmic reticulum (SER), and peroxisomes were found close to the newly deposited glycogen particles.
At maximum glycogen accumulation the association of SER and peroxisomes with glycogen was less obvious.
Glycogenolysis induced by incubation of glycogen‐rich hepatocytes with glucagon resulted in proliferation of SER in the glycogen regions of the cells.
These observations are compatible with the concept of regions in the hepatocyte cytoplasm specialized for glycogen metabolism.
Possible roles for SER and peroxisomes found near glycogen particles and other organelles in hepatic glycogen metabolism are discussed.
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