It takes two transducins to activate the cGMP-phosphodiesterase 6 in retinal 
rods

Qureshi, Bilal M.; Behrmann, Elmar; Schöneberg, Johannes; Loerke, Justus; Bürger, Jörg; Mielke, Thorsten; Giesebrecht, Jan; Noé, Frank; Lamb, Trevor D.; Hofmann, Klaus Peter; Spahn, Christian M. T.; Heck, Martin

doi:10.1098/rsob.180075

Item

ITEM ACTIONSEXPORT

Add to Basket

Local TagsRelease HistoryDetailsSummary

Released

Journal Article

It takes two transducins to activate the cGMP-phosphodiesterase 6 in retinal rods

MPS-Authors

Behrmann, Elmar
Max Planck Research Group Structural Dynamics of Proteins, Center of Advanced European Studies and Research (caesar), Max Planck Society;

/persons/resource/persons73855

Bürger, Jörg
Microscopy and Cryo-Electron Microscopy (Head: Thorsten Mielke), Scientific Service (Head: Christoph Krukenkamp), Max Planck Institute for Molecular Genetics, Max Planck Society;

/persons/resource/persons50431

Mielke, Thorsten
Microscopy and Cryo-Electron Microscopy (Head: Thorsten Mielke), Scientific Service (Head: Christoph Krukenkamp), Max Planck Institute for Molecular Genetics, Max Planck Society;

External Resource

No external resources are shared

Fulltext (restricted access)

There are currently no full texts shared for your IP range.

Fulltext (public)

Qureshi.pdf
(Publisher version), 890KB

Supplementary Material (public)

There is no public supplementary material available

Citation

Qureshi, B. M., Behrmann, E., Schöneberg, J., Loerke, J., Bürger, J., Mielke, T., et al. (2018). It takes two transducins to activate the cGMP-phosphodiesterase 6 in retinal rods. Open Biology, 8(8): 180075. doi:10.1098/rsob.180075.

Cite as: https://hdl.handle.net/21.11116/0000-0003-564C-8

Abstract

Among cyclic nucleotide phosphodiesterases (PDEs), PDE6 is unique in serving as an effector enzyme in G protein-coupled signal transduction. In retinal rods and cones, PDE6 is membrane-bound and activated to hydrolyse its substrate, cGMP, by binding of two active G protein α-subunits (Gα*). To investigate the activation mechanism of mammalian rod PDE6, we have collected functional and structural data, and analysed them by reaction-diffusion simulations. Gα* titration of membrane-bound PDE6 reveals a strong functional asymmetry of the enzyme with respect to the affinity of Gα* for its two binding sites on membrane-bound PDE6 and the enzymatic activity of the intermediary 1 : 1 Gα* · PDE6 complex. Employing cGMP and its 8-bromo analogue as substrates, we find that Gα* · PDE6 forms with high affinity but has virtually no cGMP hydrolytic activity. To fully activate PDE6, it takes a second copy of Gα* which binds with lower affinity, forming Gα* · PDE6 · Gα*. Reaction-diffusion simulations show that the functional asymmetry of membrane-bound PDE6 constitutes a coincidence switch and explains the lack of G protein-related noise in visual signal transduction. The high local concentration of Gα* generated by a light-activated rhodopsin molecule efficiently activates PDE6, whereas the low density of spontaneously activated Gα* fails to activate the effector enzyme.