Optimized orthogonal translation of unnatural amino acids enables spontaneous protein double-labelling and FRET

Kaihang Wang; Amit Sachdeva; Daniel J. Cox; Nabil W. Wilf; Kathrin Lang; Stephen Wallace; Ryan A. Mehl; Jason W. Chin

doi:10.1038/nchem.1919

Optimized orthogonal translation of unnatural amino acids enables spontaneous protein double-labelling and FRET

Kaihang Wang
, Amit Sachdeva
, Daniel J. Cox
, Nabil W. Wilf
, Kathrin Lang
, Stephen Wallace
, Ryan A. Mehl
, Jason W. Chin

Cambridge Biomedical Campus
Oregon State University

Research output: Contribution to journal › Article › peer-review

234 Scopus citations

Abstract

The ability to introduce different biophysical probes into defined positions in target proteins will provide powerful approaches for interrogating protein structure, function and dynamics. However, methods for site-specifically incorporating multiple distinct unnatural amino acids are hampered by their low efficiency. Here we provide a general solution to this challenge by developing an optimized orthogonal translation system that uses amber and evolved quadruplet-decoding transfer RNAs to encode numerous pairs of distinct unnatural amino acids into a single protein expressed in Escherichia coli with a substantial increase in efficiency over previous methods. We also provide a general strategy for labelling pairs of encoded unnatural amino acids with different probes via rapid and spontaneous reactions under physiological conditions. We demonstrate the utility of our approach by genetically directing the labelling of several pairs of sites in calmodulin with fluorophores and probing protein structure and dynamics by Förster resonance energy transfer.

Original language	English
Pages (from-to)	393-403
Number of pages	11
Journal	Nature Chemistry
Volume	6
Issue number	5
DOIs	https://doi.org/10.1038/nchem.1919
State	Published - May 2014
Externally published	Yes

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title = "Optimized orthogonal translation of unnatural amino acids enables spontaneous protein double-labelling and FRET",

abstract = "The ability to introduce different biophysical probes into defined positions in target proteins will provide powerful approaches for interrogating protein structure, function and dynamics. However, methods for site-specifically incorporating multiple distinct unnatural amino acids are hampered by their low efficiency. Here we provide a general solution to this challenge by developing an optimized orthogonal translation system that uses amber and evolved quadruplet-decoding transfer RNAs to encode numerous pairs of distinct unnatural amino acids into a single protein expressed in Escherichia coli with a substantial increase in efficiency over previous methods. We also provide a general strategy for labelling pairs of encoded unnatural amino acids with different probes via rapid and spontaneous reactions under physiological conditions. We demonstrate the utility of our approach by genetically directing the labelling of several pairs of sites in calmodulin with fluorophores and probing protein structure and dynamics by F{\"o}rster resonance energy transfer.",

author = "Kaihang Wang and Amit Sachdeva and Cox, \{Daniel J.\} and Wilf, \{Nabil W.\} and Kathrin Lang and Stephen Wallace and Mehl, \{Ryan A.\} and Chin, \{Jason W.\}",

note = "Funding Information: We thank the Medical Research Council (U105181009, UD99999908) and the European Research Council (MC-A024-5PG0A) for financial support. We thank S-P. Chew (MRC-LMB Mass Spectrometry) for obtaining MALDI data. Funding Information: In the version of this Article originally published, the middle initial of the co-author Nabil M. Wilf was incorrect, and the Acknowledgements section was missing a reference to the European Research Council; the statement should have read: “We thank the Medical Research Council (U105181009, UD99999908) and the European Research Council (MC-A024-PG0A) for financial support. We thank S-P. Chew (MRC-LMB Mass Spectrometry) for obtaining MALDI data.” These errors have now been corrected in the online versions of the Article.",

year = "2014",

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doi = "10.1038/nchem.1919",

language = "English",

volume = "6",

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journal = "Nature Chemistry",

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AU - Wang, Kaihang

AU - Sachdeva, Amit

AU - Cox, Daniel J.

AU - Wilf, Nabil W.

AU - Lang, Kathrin

AU - Wallace, Stephen

AU - Mehl, Ryan A.

AU - Chin, Jason W.

N1 - Funding Information: We thank the Medical Research Council (U105181009, UD99999908) and the European Research Council (MC-A024-5PG0A) for financial support. We thank S-P. Chew (MRC-LMB Mass Spectrometry) for obtaining MALDI data. Funding Information: In the version of this Article originally published, the middle initial of the co-author Nabil M. Wilf was incorrect, and the Acknowledgements section was missing a reference to the European Research Council; the statement should have read: “We thank the Medical Research Council (U105181009, UD99999908) and the European Research Council (MC-A024-PG0A) for financial support. We thank S-P. Chew (MRC-LMB Mass Spectrometry) for obtaining MALDI data.” These errors have now been corrected in the online versions of the Article.

PY - 2014/5

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N2 - The ability to introduce different biophysical probes into defined positions in target proteins will provide powerful approaches for interrogating protein structure, function and dynamics. However, methods for site-specifically incorporating multiple distinct unnatural amino acids are hampered by their low efficiency. Here we provide a general solution to this challenge by developing an optimized orthogonal translation system that uses amber and evolved quadruplet-decoding transfer RNAs to encode numerous pairs of distinct unnatural amino acids into a single protein expressed in Escherichia coli with a substantial increase in efficiency over previous methods. We also provide a general strategy for labelling pairs of encoded unnatural amino acids with different probes via rapid and spontaneous reactions under physiological conditions. We demonstrate the utility of our approach by genetically directing the labelling of several pairs of sites in calmodulin with fluorophores and probing protein structure and dynamics by Förster resonance energy transfer.

AB - The ability to introduce different biophysical probes into defined positions in target proteins will provide powerful approaches for interrogating protein structure, function and dynamics. However, methods for site-specifically incorporating multiple distinct unnatural amino acids are hampered by their low efficiency. Here we provide a general solution to this challenge by developing an optimized orthogonal translation system that uses amber and evolved quadruplet-decoding transfer RNAs to encode numerous pairs of distinct unnatural amino acids into a single protein expressed in Escherichia coli with a substantial increase in efficiency over previous methods. We also provide a general strategy for labelling pairs of encoded unnatural amino acids with different probes via rapid and spontaneous reactions under physiological conditions. We demonstrate the utility of our approach by genetically directing the labelling of several pairs of sites in calmodulin with fluorophores and probing protein structure and dynamics by Förster resonance energy transfer.

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JO - Nature Chemistry

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Optimized orthogonal translation of unnatural amino acids enables spontaneous protein double-labelling and FRET

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