Mapping the ATP-Binding Site in the Catalytic Subunit of A denosine-3':5'-monophosphate-Dependent Protein Kinase. Spatial Relationship with the ATP Site of the Undissociated Enzyme

Hoppe, Jürgen; Freist, Wolfgang; Marutzky, R.; Shaltiel, Shmuel

doi:10.1111/j.1432-1033.1978.tb12621.x

Cited by 69 publications

(51 citation statements)

References 12 publications

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“…The present work deals with a detailed analysis of the ATP site of this enzyme using 30 ATP analogues. These data have been compared with previous results on the ATP site of the catalytic subunit of CAMP-dependent protein kinase I from rabbit muscle [25,26]. Furthermore, these studies allow specific inhibitors of the nuclear protein kinase to bc determined.…”

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confidence: 82%

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The ATP Substrate Site of a Cyclic‐Nucleotide‐Independent Protein Kinase from Porcine Liver Nuclei

Baydoun¹,

Hoppe²,

Freist³

et al. 1981

European Journal of Biochemistry

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The ATP substrate site of a second messenger-independent protein kinase of the type NII from porcine liver nuclei was mapped using a series of 30 ATP derivatives with modifications at the base, ribose or triphosphate moiety. Ki values for these derivatives were determined by competition with [1y3'P]ATP; they range from 4 pM to 1.5 mM. For a comparison with data previously reported for the catalytic subunit of CAMP-dependent protein kinase I from rabbit skeletal muscle, the K i values were transformed into 6AC values. These values are related to the Ki value of unsubstituted ATP and indicate the decrease of affinity caused by the different substitutions.With both enzymes the major binding affinity is derived from the interaction of the adenine base. The contributions of the two ribosyl OH groups are marginal and the triphosphate moiety interacts most strongly with its fi-phosphoryl group. Between the two enzymes the most striking differences, however, were observed for the specificity of the nucleobase interaction. While an unmodified N-6 amino group is required in the case of the CAMP-dependent protein kinase, the nuclear enzyme seems to tolerate extensive modification at this position. such as the introduction of a keto group or a bulky benzyl residue. Obviously, thc ATP site of the nuclear kinase has an open cleft next to the N-6 of the adenine and binding of the adenine occurs by hydrophobic interaction without the formation of hydrogen bonds to any of the adenine nitrogens.As protein phosphorylation is the key event in many regulatory processes of the eukaryotic cell, the interest in protein kinases and the number of enzymes described in the literature continuously increases. The protein kinases best characterized are the cyclic-nucleotide-dependent enzymes and in several cases their natural substrates have been identified [I -51. Recently a second group of protein kinases has been investigated more thoroughly, and these consist of cyclic-nucleotideindependent enzymes; many of them prefer acidic proteins as substrates [6-81 in contrast to the first group which phosphorylate basic peptide segments [I]. These protein kinases were purified from the cytosol [9-111, the melnbrane [I21 and the nucleus [I 3-181 of eukaryotic tissues. However, their function and their natural target proteins are largely unknown. The cyclic-nucleotide-independent protein kinases which phosphorylate acidic proteins can be further divided into two subgroups I and 11, according to their elution sequence from DEAE-cellulose columns [13,14]. Determination of the molecular weight revealed that type I1 enzymes are significantly larger proteins than type I enzymes [I 0,13 -IS]. Very reccntly several investigations rurthei-showed that type I1 protein kinases have a rather unspecific ATP site, i.e.

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confidence: 82%

“…they can also use CiTP as phosphoryl donor [7,9,10,17,19 -231. This is in contrast to type I enzymes of this group and also to the cyclic-nucleot ide-dependent enzymes which are highly ATP-specific [25].…”

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confidence: 89%

The ATP Substrate Site of a Cyclic‐Nucleotide‐Independent Protein Kinase from Porcine Liver Nuclei

Baydoun¹,

Hoppe²,

Freist³

et al. 1981

European Journal of Biochemistry

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“…Furthermore no site for ATP in the catalytic subunit other than the active site has been found, as revealed by kinetic studies [23,24] and competition experiments with a variety of different analogues [9]. The idea of two different sites in the catalytic subunit for ATP, one site being completely abolished when the other is created, is fairly unlikely.…”

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confidence: 99%

“…As the nature of the high-affinity site for ATP in the holoenzyme and the catalytic subunit are alm'ost identical with respect to their adenine binding domain [9], it seems reasonable to assume that ATP binds to the same domain in both cases. Furthermore no site for ATP in the catalytic subunit other than the active site has been found, as revealed by kinetic studies [23,24] and competition experiments with a variety of different analogues [9].…”

Section: Conlusionsmentioning

confidence: 99%

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Localization of the High‐Affinity ATP Site in Adenosine‐3′:5′‐monophosphate‐Dependent Protein Kinase Type I

Hoppe

Freist

1979

European Journal of Biochemistry

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8‐Azido‐adenosine 5′‐triphosphate (n38ATP) appeared to be a suitable photoaffinity label for the protein kinase dependent on adenosine 3′:5′‐monophosphate (cAMP). It competes with ATP for the high‐affinity ATP site in the undissociated form of the kinase and in the phosphotransferase reaction catalyzed by the catalytic subunit. Furthermore, it is accepted as a substrate in the phosphotransfer reaction. n38ATP incorporated into the holoenzyme is covalently bound upon irradiation. Protection experiments with ATP indicated that this covalent attachment occurs in the high‐affinity ATP site of the enzyme. Polyacrylamide gel electrophoresis in the presence of sodium dodecylsulfate shows that n38ATP is bound to the catalytic subunit. After irradiation the enzyme was dissociated by cAMP. Proportional to the incorporated [γ‐32P]n38ATP, a loss in phosphotransferase activity was found. These results support our model that both ATP sites coincide with respect to their adenine binding part. Thus binding of the regulatory subunit to the catalytic subunit would then transform the low‐affinity catalytically active ATP site into a high‐affinity inactive site.

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Rational Drug Design of Kinase Inhibitors for Signal Transduction Therapy

Kéri

Őrfi

Németh

2011

Protein Kinases as Drug Targets

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Mapping the ATP-Binding Site in the Catalytic Subunit of A denosine-3':5'-monophosphate-Dependent Protein Kinase. Spatial Relationship with the ATP Site of the Undissociated Enzyme

Cited by 69 publications

References 12 publications

The ATP Substrate Site of a Cyclic‐Nucleotide‐Independent Protein Kinase from Porcine Liver Nuclei

The ATP Substrate Site of a Cyclic‐Nucleotide‐Independent Protein Kinase from Porcine Liver Nuclei

Localization of the High‐Affinity ATP Site in Adenosine‐3′:5′‐monophosphate‐Dependent Protein Kinase Type I

Rational Drug Design of Kinase Inhibitors for Signal Transduction Therapy

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