4.8 Article

Main-chain mutagenesis reveals intrahelical coupling in an ion channel voltage-sensor

Journal

NATURE COMMUNICATIONS
Volume 9, Issue -, Pages -

Publisher

NATURE PUBLISHING GROUP
DOI: 10.1038/s41467-018-07477-3

Keywords

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Funding

  1. NIH/NIGMS [GM087546, GM122420, P41-GM104601]
  2. NIH [GM087519]
  3. XSEDE [MCA06N060]
  4. Blue Waters [ACI-1713784]
  5. [5EIA22180002]
  6. NATIONAL INSTITUTE OF GENERAL MEDICAL SCIENCES [R01GM122420, R01GM087546, R01GM106569, P41GM104601, U54GM087519] Funding Source: NIH RePORTER
  7. NATIONAL INSTITUTE OF NEUROLOGICAL DISORDERS AND STROKE [R24NS104617] Funding Source: NIH RePORTER

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Membrane proteins are universal signal decoders. The helical transmembrane segments of these proteins play central roles in sensory transduction, yet the mechanistic contributions of secondary structure remain unresolved. To investigate the role of main-chain hydrogen bonding on transmembrane function, we encoded amide-to-ester substitutions at sites throughout the S4 voltage-sensing segment of Shaker potassium channels, a region that undergoes rapid, voltage-driven movement during channel gating. Functional measurements of ester-harboring channels highlight a transitional region between alpha-helical and 3(10) segments where hydrogen bond removal is particularly disruptive to voltage-gating. Simulations of an active voltage sensor reveal that this region features a dynamic hydrogen bonding pattern and that its helical structure is reliant upon amide support. Overall, the data highlight the specialized role of main-chain chemistry in the mechanism of voltage-sensing; other catalytic transmembrane segments may enlist similar strategies in signal transduction mechanisms.

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