| Id |
Subject |
Object |
Predicate |
Lexical cue |
| T1 |
0-92 |
Sentence |
denotes |
Biochemical characterization of the human cyclin-dependent protein kinase activating kinase. |
| T1 |
0-92 |
Sentence |
denotes |
Biochemical characterization of the human cyclin-dependent protein kinase activating kinase. |
| T2 |
93-145 |
Sentence |
denotes |
Identification of p35 as a novel regulatory subunit. |
| T2 |
93-145 |
Sentence |
denotes |
Identification of p35 as a novel regulatory subunit. |
| T3 |
146-338 |
Sentence |
denotes |
The activation of cyclin-dependent protein kinases (Cdks) is dependent upon site-specific phosphorylation and dephosphorylation reactions, as well as positive and negative regulatory subunits. |
| T3 |
146-338 |
Sentence |
denotes |
The activation of cyclin-dependent protein kinases (Cdks) is dependent upon site-specific phosphorylation and dephosphorylation reactions, as well as positive and negative regulatory subunits. |
| T4 |
339-473 |
Sentence |
denotes |
The human Cdk-activating protein kinase (Cak1) is itself a Cdc2-related cyclin-dependent protein kinase that associates with cyclin H. |
| T4 |
339-473 |
Sentence |
denotes |
The human Cdk-activating protein kinase (Cak1) is itself a Cdc2-related cyclin-dependent protein kinase that associates with cyclin H. |
| T5 |
474-645 |
Sentence |
denotes |
The present study utilized specific anti-Cak1 antibodies and immunoaffinity chromatography to identify additional Cak1-associated proteins and potential target substrates. |
| T5 |
474-645 |
Sentence |
denotes |
The present study utilized specific anti-Cak1 antibodies and immunoaffinity chromatography to identify additional Cak1-associated proteins and potential target substrates. |
| T6 |
646-853 |
Sentence |
denotes |
Immunoprecipitation of metabolically labeled human osteosarcoma cells revealed a number of Cak1-associated proteins, including p95, p37 (cyclin H), and a 35-kDa protein that was further characterized herein. |
| T6 |
646-853 |
Sentence |
denotes |
Immunoprecipitation of metabolically labeled human osteosarcoma cells revealed a number of Cak1-associated proteins, including p95, p37 (cyclin H), and a 35-kDa protein that was further characterized herein. |
| T7 |
854-1061 |
Sentence |
denotes |
Microsequence analysis obtained after limited proteolysis revealed peptide fragments that are similar, but not identical to, human and yeast cyclins, thus identifying p35 as a cyclin-like regulatory subunit. |
| T7 |
854-1061 |
Sentence |
denotes |
Microsequence analysis obtained after limited proteolysis revealed peptide fragments that are similar, but not identical to, human and yeast cyclins, thus identifying p35 as a cyclin-like regulatory subunit. |
| T8 |
1062-1182 |
Sentence |
denotes |
The greatest sequence similarity of human p35 is with Mcs2, a yeast cyclin that is essential for cell cycle progression. |
| T8 |
1062-1182 |
Sentence |
denotes |
The greatest sequence similarity of human p35 is with Mcs2, a yeast cyclin that is essential for cell cycle progression. |
| T9 |
1183-1410 |
Sentence |
denotes |
Immunoaffinity chromatography performed under nondenaturing conditions afforded the isolation of enzymatically active Cak1 from cell lysates, enabling studies of kinase autophosphorylation and comparative substrate utilization. |
| T9 |
1183-1410 |
Sentence |
denotes |
Immunoaffinity chromatography performed under nondenaturing conditions afforded the isolation of enzymatically active Cak1 from cell lysates, enabling studies of kinase autophosphorylation and comparative substrate utilization. |
| T10 |
1411-1591 |
Sentence |
denotes |
Immunoaffinity-purified Cak1 phosphorylated monomeric Cdc2 and Cdk2, but not Cdk4; the phosphorylation of both Cdc2 and Cdk2 were increased in the presence of recombinant cyclin A. |
| T10 |
1411-1591 |
Sentence |
denotes |
Immunoaffinity-purified Cak1 phosphorylated monomeric Cdc2 and Cdk2, but not Cdk4; the phosphorylation of both Cdc2 and Cdk2 were increased in the presence of recombinant cyclin A. |
| T11 |
1592-1814 |
Sentence |
denotes |
These studies indicate that the Cak1 catalytic subunit, like Cdc2 and Cdk2, associates with multiple regulatory partners and suggests that subunit composition may be an important determinant of this multifunctional enzyme. |
| T11 |
1592-1814 |
Sentence |
denotes |
These studies indicate that the Cak1 catalytic subunit, like Cdc2 and Cdk2, associates with multiple regulatory partners and suggests that subunit composition may be an important determinant of this multifunctional enzyme. |
