cDNA cloning and complete primary structure of skeletal muscle phosphorylase kinase (alpha subunit).

Zander, Norbert; Meyer, Helmut E.; Hoffmann-Posorske, Edeltraut; Crabb, John W.; Heilmeyer, Ludwig; Kilimann, Manfred W.

doi:10.1073/pnas.85.9.2929

Cited by 82 publications

(49 citation statements)

References 45 publications

(44 reference statements)

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“…Second, the stretch from 1012 to 1056 is a region of very low homology between the rabbit muscle and liver ␣ subunits (40). Third, at least seven phosphorylation sites occur between residues 972 and 1030 (20). The sum of this evidence strongly suggests that the overlapping region contains regulatory domains, as opposed to an association domain.…”

Section: Discussionmentioning

confidence: 80%

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Self-association of the α Subunit of Phosphorylase Kinase as Determined by Two-hybrid Screening

Ayers¹,

Wilkinson²,

Fitzgerald³

et al. 1999

Journal of Biological Chemistry

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The structural organization of the (␣␤␥␦) 4 phosphorylase kinase complex has been studied using the yeast two-hybrid screen for the purpose of elucidating regions of ␣ subunit interactions. By screening a rabbit skeletal muscle cDNA library with residues 1-1059 of the ␣ subunit of phosphorylase kinase, we have isolated 16 interacting, independent, yet overlapping transcripts of the ␣ subunit containing its C-terminal region. Domain mapping of binary interactions between ␣ constructs revealed two regions involved in the self-association of the ␣ subunit: residues 833-854, a previously unrecognized leucine zipper, and an unspecified region within residues 1015-1237. The cognate binding partner for the latter domain has been inferred to lie within the stretch from residues 864 -1059. Indirect evidence from the literature suggests that the interacting domains contained within the latter two, overlapping regions may be further narrowed to the stretches from 1057 to 1237 and from 864 to 971. Cross-linking of the nonactivated holoenzyme with N-(␥-maleimidobutyroxy)sulfosuccinimide ester produced intramolecularly cross-linked ␣-␣ dimers, consistent with portions of two ␣ subunits in the holoenyzme being in sufficient proximity to associate. This is the first report to identify potential areas of contact between the ␣ subunits of phosphorylase kinase. Additionally, issues regarding the general utility of twohybrid screening as a method for studying homodimeric interactions are discussed.Phosphorylase b kinase (PhK) 1 is among the largest and most complex of the protein kinases, with a mass of 1.3 ϫ 10 6 Da and a subunit stoichiometry of (␣␤␥␦) 4 (reviewed in Refs. 1 and 2). The catalytic ␥ subunit of this complex oligomer is allosterically controlled through alterations in quaternary structure initiated by the regulatory ␣, ␤, and ␦ subunits, the latter being an intrinsic molecule of calmodulin (3). Studies have shown that activation of PhK by multiple effectors occurs concomitantly with common conformational changes in the ␣ and ␤ subunits (4 -6); moreover, the activity of free ␥ subunit is inhibited by the ␣ and ␤ subunits (7,8). It has been proposed that the ␣ and ␤ subunits of PhK impose steric constraint upon ␥ that, when removed, leads to activation of the kinase (7-10).We have chosen to study the largest of the regulatory subunits, ␣, because relatively few studies have been devoted to understanding its role in the structure and function of PhK. Previous studies using electron microscopy and immunoelectron microscopy have suggested that the ␣ subunit is peripherally located in the holoenzyme (11, 12), which is consistent with its high susceptibility to proteolysis by a wide variety of proteases (5). Based upon the probable exposed location of ␣ within the PhK hexadecamer, we hypothesized that this subunit may interact with other muscle proteins and investigated potential PhK ␣ interactions by screening a skeletal muscle cDNA library for potential binding partners of ␣ using the yeast two-hybrid system.The two-hybr...

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Section: Discussionmentioning

confidence: 80%

“…Of the 7.8 ϫ 10 6 independent clones obtained, 73% contained inserts averaging 1.6 kilobases in size. Rabbit PhK ␣ cDNA (␣D1) was kindly provided by Dr. Manfred W. Kilimann (Ruhr-Universitä t Bochum, Bochum, Germany) (20) and used as the template for the preparation of all ␣ truncations shown in Fig. 2.…”

Section: Methodsmentioning

confidence: 99%

Self-association of the α Subunit of Phosphorylase Kinase as Determined by Two-hybrid Screening

Ayers¹,

Wilkinson²,

Fitzgerald³

et al. 1999

Journal of Biological Chemistry

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“…Predictions of 2°structure for both subunits suggest them to be predominantly ␣-helical, and our CD measurements of the ␣␥␦ and (␣␤␥␦) 4 complexes are in agreement, showing ␣ and ␤ to have similar 2°structure content. Some minor differences in 2°structure were observed between ␣ and ␤, however, and these likely reflect the presence of several nonhomologous stretches, some of which include phosphorylatable regulatory domains specific to each subunit (20,21). The ␣ subunit has a large phosphorylatable C-terminal regulatory domain with multiple phosphorylation sites (1), whereas the ␤ subunit contains two known phosphorylatable regions, Ser-700 plus Ser-11/Ser-26 in the N-terminal phosphorylatable domain (NB1, residues 1-40) (7,28).…”

Section: Discussionmentioning

confidence: 99%

“…Although the primary structures are known for both ␣ and ␤ (20,21), essentially all higher order secondary (2°) and tertiary (3°) structures reported for these subunits are based on predicted rather than experimental data (22)(23)(24). In contrast, high resolution structural information is available for the catalytic core of the ␥ subunit and for the ␦ subunit (3,25); on the other hand, the small size and location of these subunits in the complex make them unlikely candidates for bridging the two (␣␤␥␦) 2 lobes (14,16).…”

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confidence: 99%

Structure and Location of the Regulatory β Subunits in the (αβγδ)4 Phosphorylase Kinase Complex

Nadeau

Lane

et al. 2012

Journal of Biological Chemistry

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Background: Structural information concerning the phosphorylatable regulatory ␤ subunit of phosphorylase kinase was lacking. Results: Chemical, biochemical, biophysical, and computational approaches revealed secondary, tertiary, and quaternary structures for this subunit. Conclusion: The ␤ subunit is helical and forms the ␤ 4 -bridged core in the (␣␤␥␦) 4 kinase complex. Significance: These findings reveal the architecture of the complex, which provides an explanation for the conformational changes in its bridged core associated with activating ␤-phosphorylation.

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“…Size-fractionated cDNA (larger than 1800 nucleotides (nt)) was synthesized as described [5] and inserted into &tlO with EcoRl linkers. A primary library of 700 000 plaques from rabbit liver was screened under reduced stringency with the phosphorylase kinase y subunit cDNA (complete coding sequence plus 228 nt of 3 '-noncoding sequence) from mouse muscle (donated by J. Chamberlain [2]).…”

Section: Methodsmentioning

confidence: 99%

cDNA encoding a 59 kDa homolog of ribosomal protein S6 kinase from rabbit liver

Harmann

Kilimann

1990

FEBS Letters

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We have isolated cDNA molecules encoding a protein with the characteristic sequence elements that are conserved between the catalytic domains of protein kinases. This protein is apparently a serine/threonine kinase and is most closely related to the amino-terminal half of the ribosomal protein S6 kinase II first characterized in Xenopus eggs (42% overall identity and 56% identity in the predicted catalytic domain). However, it clearly differs from S6 kinase II in that it has only one, rather than two predicted catalytic domains and a deduced molecular mass of 59 109 Da. We propose that is may be more related to, or identical with, the mitogen-inducible S6 kinase of molecular mass 65-70 kDa described in mammalian liver, mouse 3T3 cells and chicken embryos. Remarkable structural features of the cDNA-encoded polypeptide are a section rich in proline, serine and threonine residues that resemble the multiphosphorylation domains of glycogen synthase and phosphorylase kinase a subunit, and a characteristic tyrosine residue in the putative nucleotide-binding glycine cluster which, by analogy to cdc2 kinase, is a potential tyrosine phosphorylation site.

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cDNA cloning and complete primary structure of skeletal muscle phosphorylase kinase (alpha subunit).

Cited by 82 publications

References 45 publications

Self-association of the α Subunit of Phosphorylase Kinase as Determined by Two-hybrid Screening

Self-association of the α Subunit of Phosphorylase Kinase as Determined by Two-hybrid Screening

Structure and Location of the Regulatory β Subunits in the (αβγδ)4 Phosphorylase Kinase Complex

cDNA encoding a 59 kDa homolog of ribosomal protein S6 kinase from rabbit liver

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