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Literature DB >> 27842062

Tuning membrane protein mobility by confinement into nanodomains.

Andreas Karner¹, Benedikt Nimmervoll¹, Birgit Plochberger², Enrico Klotzsch³, Andreas Horner⁴, Denis G Knyazev⁴, Roland Kuttner⁴, Klemens Winkler⁴, Lukas Winter⁴, Christine Siligan⁴, Nicole Ollinger⁴, Peter Pohl⁴, Johannes Preiner¹.

Abstract

High-speed atomic force microscopy (HS-AFM) can be used to visualize function-related conformational changes of single soluble proteins. Similar studies of single membrane proteins are, however, hampered by a lack of suitable flat, non-interacting membrane supports and by high protein mobility. Here we show that streptavidin crystals grown on mica-supported lipid bilayers can be used as porous supports for membranes containing biotinylated lipids. Using SecYEG (protein translocation channel) and GlpF (aquaglyceroporin), we demonstrate that the platform can be used to tune the lateral mobility of transmembrane proteins to any value within the dynamic range accessible to HS-AFM imaging through glutaraldehyde-cross-linking of the streptavidin. This allows HS-AFM to study the conformation or docking of spatially confined proteins, which we illustrate by imaging GlpF at sub-molecular resolution and by observing the motor protein SecA binding to SecYEG.

Entities: Chemical

Mesh：

Substances：

Year: 2016 PMID： 27842062 PMCID： PMC5734611 DOI： 10.1038/nnano.2016.236

Source DB: PubMed Journal: Nat Nanotechnol ISSN： 1748-3387 Impact factor: 39.213

46 in total

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