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Site recognition and substrate screens for PKN family proteins
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The PRKs [protein kinase C-related kinases; also referred to as PKNs (protein kinase Ns)] are a kinase family important in diverse functions including migration and cytokinesis. In the present study, we have re-evaluated and compared the specificity of PKN1 and PKN3 and assessed the predictive value in substrates. We analysed the phosphorylation consensus motif of PKNs using a peptide library approach and demonstrate that both PKN1 and PKN3 phosphorylate serine residues in sequence contexts that have an arginine residue in position −3. In contrast, PKN1 and PKN3 do not tolerate arginine residues in position +1 and −1 respectively. To test the predictive value of this motif, site analysis was performed on the PKN substrate CLIP-170 (cytoplasmic linker protein of 170 kDa); a PKN target site was identified that conformed to the predicted pattern. Using a protein array, we identified 22 further substrates for PKN1, of which 20 were previously undescribed substrates. To evaluate further the recognition signature, the site on one of these hits, EGFR (epidermal growth factor receptor), was identified. This identified Thr654 in EGFR as the PKN1 phosphorylation site and this retains an arginine residue at the −3 position. Finally, the constitutive phosphorylation of EGFR on Thr654 is shown to be modulated by PKN in vivo.
Title: Site recognition and substrate screens for PKN family proteins
Description:
The PRKs [protein kinase C-related kinases; also referred to as PKNs (protein kinase Ns)] are a kinase family important in diverse functions including migration and cytokinesis.
In the present study, we have re-evaluated and compared the specificity of PKN1 and PKN3 and assessed the predictive value in substrates.
We analysed the phosphorylation consensus motif of PKNs using a peptide library approach and demonstrate that both PKN1 and PKN3 phosphorylate serine residues in sequence contexts that have an arginine residue in position −3.
In contrast, PKN1 and PKN3 do not tolerate arginine residues in position +1 and −1 respectively.
To test the predictive value of this motif, site analysis was performed on the PKN substrate CLIP-170 (cytoplasmic linker protein of 170 kDa); a PKN target site was identified that conformed to the predicted pattern.
Using a protein array, we identified 22 further substrates for PKN1, of which 20 were previously undescribed substrates.
To evaluate further the recognition signature, the site on one of these hits, EGFR (epidermal growth factor receptor), was identified.
This identified Thr654 in EGFR as the PKN1 phosphorylation site and this retains an arginine residue at the −3 position.
Finally, the constitutive phosphorylation of EGFR on Thr654 is shown to be modulated by PKN in vivo.
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