Reading the primary structure of a protein with 0.07 nm 3 resolution using a subnanometre-diameter pore

Reading the primary structure of a protein with 0.07 nm 3 resolution using a subnanometre-diameter pore

The primary structure of a protein consists of a sequence of amino acids and is a key factor in determining how a protein folds and functions. However, conventional methods for sequencing proteins, such as mass spectrometry and Edman degradation, suffer from short reads and lack sensitivity, so alte...

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Veröffentlicht in:Nature nanotechnology 2016-11, Vol.11 (11), p.968
Hauptverfasser: Kennedy, Eamonn, Dong, Zhuxin, Tennant, Clare, Timp, Gregory
Format: Artikel
Sprache:eng
Schlagworte:
Amino Acid Sequence
Image Processing, Computer-Assisted
Lab-On-A-Chip Devices
Lysine - chemistry
Membranes, Artificial
Mercaptoethanol - chemistry
Microscopy, Electron, Scanning Transmission - instrumentation
Nanotechnology - instrumentation
Nanotechnology - methods
Protein Denaturation
Proteins - analysis
Proteins - chemistry
Silicon Compounds
Sodium Dodecyl Sulfate - chemistry
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container_title Nature nanotechnology
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creator Kennedy, Eamonn
Dong, Zhuxin
Tennant, Clare
Timp, Gregory
description The primary structure of a protein consists of a sequence of amino acids and is a key factor in determining how a protein folds and functions. However, conventional methods for sequencing proteins, such as mass spectrometry and Edman degradation, suffer from short reads and lack sensitivity, so alternative approaches are sought. Here, we show that a subnanometre-diameter pore, sputtered through a thin silicon nitride membrane, can be used to detect the primary structure of a denatured protein molecule. When a denatured protein immersed in electrolyte is driven through the pore by an electric field, measurements of a blockade in the current reveal nearly regular fluctuations, the number of which coincides with the number of residues in the protein. Furthermore, the amplitudes of the fluctuations are highly correlated with the volumes that are occluded by quadromers (four residues) in the primary structure. Each fluctuation, therefore, represents a read of a quadromer. Scrutiny of the fluctuations reveals that the subnanometre pore is sensitive enough to read the occluded volume that is related to post-translational modifications of a single residue, measuring volume differences of ∼0.07 nm , but it is not sensitive enough to discriminate between the volumes of all twenty amino acids.
doi_str_mv 10.1038/nnano.2016.120
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subjects Amino Acid Sequence
Image Processing, Computer-Assisted
Lab-On-A-Chip Devices
Lysine - chemistry
Membranes, Artificial
Mercaptoethanol - chemistry
Microscopy, Electron, Scanning Transmission - instrumentation
Nanotechnology - instrumentation
Nanotechnology - methods
Protein Denaturation
Proteins - analysis
Proteins - chemistry
Silicon Compounds
Sodium Dodecyl Sulfate - chemistry
title Reading the primary structure of a protein with 0.07 nm 3 resolution using a subnanometre-diameter pore
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