The properties of phosphodiesterase 11A4 GAF domains are regulated by modifications in its N‐terminal domain

Gross-Langenhoff, Marco; Stenzl, Arnulf; Altenberend, Florian; Schultz, Anita; Schultz, Joachim E.

doi:10.1111/j.1742-4658.2008.06319.x

Cited by 24 publications

(21 citation statements)

References 33 publications

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“…As reported previously (7,16,30,31), we note that the basal activities of different constructs vary considerably. Thus, one may argue that the expression of the chimeras may result in polypeptides that are different, both structurally and functionally, from the wild-type constructs due to, for example, aberrant folding or domain assembly.…”

Section: Discussionsupporting

confidence: 82%

Functional Chimeras of the Phosphodiesterase 5 and 10 Tandem GAF Domains

Hofbauer

Schultz

2008

Journal of Biological Chemistry

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The tandem GAF domain of hPDE10A uses cAMP as an allosteric ligand (Gross-Langenhoff, M., Hofbauer, K., Weber, J., Schultz, A., and Schultz, J. E. (2006) J. Biol. Chem. 281, 2841-2846). We used a two-pronged approach to study how discrimination of ligand is achieved in human (h)PDE10A and how domain selection in the phosphodiesterase GAF tandems is determined. First, we examined which functional groups of cAMP are responsible for purine ring discrimination. Changes at the C-6 ring position (removal of the amino group; chloride substitution) and at the N-1 ring position reduced stimulation efficacy by 80%, i.e. marking those positions as decisive for nucleotide discrimination. Second, we generated a GAF tandem chimera that consisted of the cGMP-binding GAF-A unit from hPDE5A1, which signals through cGMP in PDE5, and the GAF-B from hPDE10A1, which signals through cAMP in PDE10. Stimulation of the reporter enzyme exclusively was through the GAF-B domain of hPDE10A1 (EC 50 ‫؍‬ 7 M cAMP) as shown by respective point mutations. The PDE5 GAF-A domain in the chimera did not signal, and its function was reduced to a strictly structural role. Signaling was independent of the origin of the N terminus. Generating 10 additional PDE5/10 tandem GAF chimeras surprisingly demonstrated that the length-conserved linker in GAF tandems between GAF-A and GAF-B played an unforeseen decisive role in intramolecular signaling. Swapping the linker sections between PDE5 and PDE10 GAF tandem domains abrogated signaling completely pointing to specific domain interactions within GAF tandems, which are not visible in the available crystal structures with bound ligands.

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Section: Discussionsupporting

confidence: 82%

Functional Chimeras of the Phosphodiesterase 5 and 10 Tandem GAF Domains

Hofbauer

Schultz

2008

Journal of Biological Chemistry

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“…In chimeric proteins composed of the N-terminal part of PDE11A4 including the GAF domains and the catalytic domain of Anabaena adenylyl cyclases, the N-terminal part preceding the GAF domains had a tremendous effect on the ability of cGMP to stimulate the chimera. Truncation of 196 N-terminal amino acids increased the cGMP affinity 20-fold (39). However, deletion of these 196 amino acids in the PDE11A4 holoenzyme abolished stimulation by the cGMP analogue but did not enable cGMP stimulation (data not shown).…”

Section: Discussionmentioning

confidence: 95%

Activation of PDE10 and PDE11 Phosphodiesterases

Jäger

Russwurm

Schwede

et al. 2012

Journal of Biological Chemistry

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Background:The cyclic nucleotide phosphodiesterases PDE10 and PDE11 contain putatively regulatory GAF domains with unknown function. Results: Synthetic GAF domain ligands can activate both PDEs. Conclusion: PDE10 is activated by cAMP, whereas the physiological ligand of the PDE11 GAF domains remains unknown. Significance: This is the first demonstration of a functional role of the PDE10 and PDE11 GAF domains.

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“…small kinases will have better efficacy than large kinases. It is also interesting to note that the N terminus of PDE11A4 and the phosphorylation of its 2 serine residues impact the activities of PDE11-cyclase hybrids (36).…”

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confidence: 99%