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AbstractAbstract
[en] Rat skeletal muscle contains a glycogen synthase kinase (GSK-M) which is not stimulated by Ca2+ or cAMP. This kinase has an apparent Mr of 62,000 and uses ATP but not GTP as a phosphoryl donor. GSK-M phosphorylated glycogen synthase at sites 2 and 3. It phosphorylated ATP-citrate lyase and activated MgATP-dependent phosphatase in the presence of ATP but not GTP. As expected, the kinase also phosphorylated phosphatase inhibitor 2 (I-2). Phosphatase incorporation reached approximately 0.3 mol/mol of I-2. Phosphopeptide maps were obtained by digesting 32P-labeled I-2 with trypsin and separating the peptides by reversed phase HPLC. Two partially separated 32P-labeled peaks were obtained when I-2 was phosphorylated with either GSK-M or glycogen synthase kinase 3 (GSK-3) and these peptides were different from those obtained when I-2 was phosphorylated with the catalytic subunit of cAMP-dependent protein kinase (CSU) or casein kinase II (CK-II). When I-2 was phosphorylated with GSK-M or GSK-3 and cleaved by CNBr, a single radioactive peak was obtained. Phosphoamino acid analysis showed that I-2 was phosphorylated by GSK-M or GSK-3 predominately in Thr whereas CSU and CK-II phosphorylated I-2 exclusively in Ser. These results indicate that GSK-M is similar to GSK-3 and to ATP-citrate lyase kinase. However, it appears to differ in Mr from ATP-citrate lyase kinase and it differs from GSK-3 in that it phosphorylates glycogen synthase at site 2 and it does not use GTP as a phosphoryl donor
Primary Subject
Source
76. annual meeting of the Federation of American Society for Experimental Biology; Washington, DC (USA); 8-12 Jun 1986; CONF-8606151--
Record Type
Journal Article
Literature Type
Conference
Journal
Federation Proceedings. Federation of American Societies for Experimental Biology; ISSN 0014-9446;
; CODEN FEPRA; v. 45(6); p. 1802

Country of publication
ANIMALS, BETA DECAY RADIOISOTOPES, BETA-MINUS DECAY RADIOISOTOPES, CARBOHYDRATES, CHEMICAL REACTIONS, CHROMATOGRAPHY, DAYS LIVING RADIOISOTOPES, ENZYMES, ESTERASES, HYDROLASES, ISOTOPE APPLICATIONS, ISOTOPES, KINETICS, LIGHT NUCLEI, MAMMALS, NUCLEI, NUCLEOTIDES, ODD-ODD NUCLEI, ORGANIC COMPOUNDS, PEPTIDE HYDROLASES, PHOSPHORUS ISOTOPES, PHOSPHORUS-GROUP TRANSFERASES, POLYSACCHARIDES, RADIOISOTOPES, REACTION KINETICS, RODENTS, SACCHARIDES, SEPARATION PROCESSES, SERINE PROTEINASES, TRANSFERASES, VERTEBRATES
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