ライフサイエンスコーパス: phosphorylase B

1 of phosphorylase that lacked the N-terminus (phosphorylase b').

2 ) have been determined for the rabbit muscle phosphorylase b.

3 inimal binding requirements of rabbit muscle phosphorylase b.

4 N-oxide on the self-association behaviour of phosphorylase b.

5 e mutants are more like phosphorylase a than phosphorylase b.

6 sphorylase a, and unlike the dephospho-form, phosphorylase b.

7 accommodates the phosphorylatable serine in phosphorylase b.

8 lation by gamma(1-300) compared to wild-type phosphorylase b.

9 iency for gamma(1-300), compared to that for phosphorylase b.

10 time the full thermodynamic effect of AMP on phosphorylase b.

11 ing the allosteric effect of AMP on glycogen phosphorylase b.

12 of glycerol, sucrose and ethylene glycol on phosphorylase b activity, phenomena that have been attri

13 6A and R16E, four other mutants behaved like phosphorylase b after phosphorylation.

14 digests, using a standard dilution series of phosphorylase B and carbonic anhydrase, separated by SDS

15 lamide gel electrophoresis with cross-linked phosphorylase B as standard is a suitable gel system for

16 determinants employed in the recognition of phosphorylase b as substrate are utilized in the recogni

17 utant enzymes were generated, using glycogen phosphorylase b as the structural template.

18 ing studies to 2.4 A resolution with T state phosphorylase b crystals showed that nojirimycin tetrazo

19 The original report on phosphorylase b' examined the allosteric characteristics

20 o enzyme-catalyzed reaction using the enzyme phosphorylase b from rabbit muscle and Deinococcus geoth

21 x that phosphorylates and activates glycogen phosphorylase b (GP b) in a Ca (2+)-dependent reaction t

22 to the analysis of the kinetics of glycogen phosphorylase b (GPb).

23 The receptor geometry of glycogen phosphorylase b, GPb, is available for structure-based d

24 zing the self-association of muscle glycogen phosphorylase b has been reappraised.

25 strates and allosteric effectors to glycogen phosphorylase b has provided evidence that the device is

26 inants for protein phosphatase-1, mutants of phosphorylase b have been converted to phosphorylase a a

27 sedimentation equilibrium distributions for phosphorylase b in 40 mM Hepes buffer (pH 6.8) supplemen

28 Phosphorylase b kinase (PbK) from skeletal muscle is a h

29 The activity of phosphorylase b kinase (PbK) is stimulated by Ca2+ ions,

30 16 subunits of the (alphabetagammadelta)(4) phosphorylase b kinase (PhK) complex can only be achieve

31 the glycogen branching enzyme (GBE) and the phosphorylase b kinase alpha subunit (PhKalpha) protein,

32 to be discovered for some glycogenoses (e.g. phosphorylase-b-kinase deficiency or branching enzyme de

33 Crosslinked phosphorylase B oligomers served as molecular weight sta

34 t interact with the amino terminus in either phosphorylase b or a, showed little difference in phosph

35 ion opposite the regulatory face of glycogen phosphorylase b (P-b), providing a probe for detecting a

36 nd the physical interaction between glycogen phosphorylase-b (P-b) and its only known kinase, phospho

37 atured rTromp1 eluted at the position of the phosphorylase b protein standard (97 kDa), suggesting a

38 hose terms the marginally enhanced extent of phosphorylase b self-association observed in the presenc

39 It has been reported that phosphorylase b' shows no allostery, neither homotropic

40 to 'open-loop' Ca2+-dependent conversion of phosphorylase b to a, and partly to the 'closed loop' in

41 25 fmol, and the lowest gel loading in which phosphorylase B was identified using electroextraction w

42 The lowest gel loading in which phosphorylase B was identified using the standard extrac

43 the presence of the inhibitor glucose, while phosphorylase b was phosphorylated normally with this in

44 hK is the only kinase that can phosphorylate phosphorylase b, which in turn is the only physiological

45 phosphorylase is found in resting muscle as phosphorylase b, which is inactive without AMP.

46 o be a competitive inhibitor with respect to phosphorylase b with a K(i) of 6.0 microm.

47 ) is a competitive inhibitor with respect to phosphorylase b, with a K(i) of 1.8 microm.