AI Article Synopsis

  • The study presents a dynamical Markov state model of CLC-2 "fast" gating based on 600 microseconds of molecular dynamics simulation, starting with both gates closed.
  • The first conformational change involves the rotation of the inner gate backbone, resembling a similar change seen in the cryo-EM structure of CLC-K, but with a more expanded intracellular region in the CLC-2 model.
  • Two additional states are observed with flips of the outer-gate residue GLUex, leading to an open or near-open channel pore in one state and occlusion in another, both linked to the protonation of GLUex and consistent with previous experimental findings.

Article Abstract

This work reports a dynamical Markov state model of CLC-2 "fast" (pore) gating, based on 600 microseconds of molecular dynamics (MD) simulation. In the starting conformation of our CLC-2 model, both outer and inner channel gates are closed. The first conformational change in our dataset involves rotation of the inner-gate backbone along residues S168-G169-I170. This change is strikingly similar to that observed in the cryo-EM structure of the bovine CLC-K channel, though the volume of the intracellular (inner) region of the ion conduction pathway is further expanded in our model. From this state (inner gate open and outer gate closed), two additional states are observed, each involving a unique rotameric flip of the outer-gate residue GLUex. Both additional states involve conformational changes that orient GLUex away from the extracellular (outer) region of the ion conduction pathway. In the first additional state, the rotameric flip of GLUex results in an open, or near-open, channel pore. The equilibrium population of this state is low (∼1%), consistent with the low open probability of CLC-2 observed experimentally in the absence of a membrane potential stimulus (0 mV). In the second additional state, GLUex rotates to occlude the channel pore. This state, which has a low equilibrium population (∼1%), is only accessible when GLUex is protonated. Together, these pathways model the opening of both an inner and outer gate within the CLC-2 selectivity filter, as a function of GLUex protonation. Collectively, our findings are consistent with published experimental analyses of CLC-2 gating and provide a high-resolution structural model to guide future investigations.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7145265PMC
http://dx.doi.org/10.1371/journal.pcbi.1007530DOI Listing

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