Single-molecule imaging of full protein synthesis by immobilized ribosomes

Sotaro Uemura; Ryo Iizuka; Taro Ueno; Yoshihiro Shimizu; Hideki Taguchi; Takuya Ueda; Joseph D. Puglisi; Takashi Funatsu

doi:10.1093/nar/gkn338

Single-molecule imaging of full protein synthesis by immobilized ribosomes

Sotaro Uemura, Ryo Iizuka, Taro Ueno, Yoshihiro Shimizu, Hideki Taguchi, Takuya Ueda, Joseph D. Puglisi, Takashi Funatsu^*

^*Corresponding author for this work

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

34 Citations (Scopus)

Abstract

How folding of proteins is coupled to their synthesis remains poorly understood. Here, we apply single-molecule fluorescence imaging to full protein synthesis in vitro. Ribosomes were specifically immobilized onto glass surfaces and synthesis of green fluorescent protein (GFP) was achieved using modified commercial Protein Synthesis using Recombinant Elements that lacked ribosomes but contained purified factors and enzyme that are required for translation in Escherichia coli. Translation was monitored using a GFP mutant (F64L/S65T/F99S/M153T/V163A) that has a high fluorophore maturation rate and that contained the Secretion Monitor arrest sequence to prevent dissociation from the ribosome. Immobilized ribosomal subunits were labeled with Cy3 and GFP synthesis was measured by colocalization of GFP fluorescence with the ribosome position. The rate of appearance of colocalized ribosome GFP was equivalent to the rates of fluorescence appearance coupled with translation measured in bulk, and the ribosome - polypeptide complexes were stable for hours. The methods presented here are applicable to single-molecule investigation of translational initiation, elongation and cotranslational folding.

Original language	English
Article number	e70
Journal	Nucleic acids research
Volume	36
Issue number	12
DOIs	https://doi.org/10.1093/nar/gkn338
Publication status	Published - 2008 Jul
Externally published	Yes

ASJC Scopus subject areas

Genetics

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title = "Single-molecule imaging of full protein synthesis by immobilized ribosomes",

abstract = "How folding of proteins is coupled to their synthesis remains poorly understood. Here, we apply single-molecule fluorescence imaging to full protein synthesis in vitro. Ribosomes were specifically immobilized onto glass surfaces and synthesis of green fluorescent protein (GFP) was achieved using modified commercial Protein Synthesis using Recombinant Elements that lacked ribosomes but contained purified factors and enzyme that are required for translation in Escherichia coli. Translation was monitored using a GFP mutant (F64L/S65T/F99S/M153T/V163A) that has a high fluorophore maturation rate and that contained the Secretion Monitor arrest sequence to prevent dissociation from the ribosome. Immobilized ribosomal subunits were labeled with Cy3 and GFP synthesis was measured by colocalization of GFP fluorescence with the ribosome position. The rate of appearance of colocalized ribosome GFP was equivalent to the rates of fluorescence appearance coupled with translation measured in bulk, and the ribosome - polypeptide complexes were stable for hours. The methods presented here are applicable to single-molecule investigation of translational initiation, elongation and cotranslational folding.",

author = "Sotaro Uemura and Ryo Iizuka and Taro Ueno and Yoshihiro Shimizu and Hideki Taguchi and Takuya Ueda and Puglisi, {Joseph D.} and Takashi Funatsu",

note = "Funding Information: We are grateful to T. Iwagawa for the vector construction and colleagues in the Funatsu group. This work was supported in part by Takeda Science Foundation, grants-in-aid from the Ministry of Education, Culture, Sports, Science and Technology of Japan and funded by grants to J.D.P. from the NIH and the Packard Foundation. Funding to pay the Open Access publication charges for this article was provided by the Ministry of Education, Culture, Sports, Science and Technology of Japan.",

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AU - Uemura, Sotaro

AU - Iizuka, Ryo

AU - Ueno, Taro

AU - Shimizu, Yoshihiro

AU - Taguchi, Hideki

AU - Ueda, Takuya

AU - Puglisi, Joseph D.

AU - Funatsu, Takashi

N1 - Funding Information: We are grateful to T. Iwagawa for the vector construction and colleagues in the Funatsu group. This work was supported in part by Takeda Science Foundation, grants-in-aid from the Ministry of Education, Culture, Sports, Science and Technology of Japan and funded by grants to J.D.P. from the NIH and the Packard Foundation. Funding to pay the Open Access publication charges for this article was provided by the Ministry of Education, Culture, Sports, Science and Technology of Japan.

PY - 2008/7

Y1 - 2008/7

N2 - How folding of proteins is coupled to their synthesis remains poorly understood. Here, we apply single-molecule fluorescence imaging to full protein synthesis in vitro. Ribosomes were specifically immobilized onto glass surfaces and synthesis of green fluorescent protein (GFP) was achieved using modified commercial Protein Synthesis using Recombinant Elements that lacked ribosomes but contained purified factors and enzyme that are required for translation in Escherichia coli. Translation was monitored using a GFP mutant (F64L/S65T/F99S/M153T/V163A) that has a high fluorophore maturation rate and that contained the Secretion Monitor arrest sequence to prevent dissociation from the ribosome. Immobilized ribosomal subunits were labeled with Cy3 and GFP synthesis was measured by colocalization of GFP fluorescence with the ribosome position. The rate of appearance of colocalized ribosome GFP was equivalent to the rates of fluorescence appearance coupled with translation measured in bulk, and the ribosome - polypeptide complexes were stable for hours. The methods presented here are applicable to single-molecule investigation of translational initiation, elongation and cotranslational folding.

AB - How folding of proteins is coupled to their synthesis remains poorly understood. Here, we apply single-molecule fluorescence imaging to full protein synthesis in vitro. Ribosomes were specifically immobilized onto glass surfaces and synthesis of green fluorescent protein (GFP) was achieved using modified commercial Protein Synthesis using Recombinant Elements that lacked ribosomes but contained purified factors and enzyme that are required for translation in Escherichia coli. Translation was monitored using a GFP mutant (F64L/S65T/F99S/M153T/V163A) that has a high fluorophore maturation rate and that contained the Secretion Monitor arrest sequence to prevent dissociation from the ribosome. Immobilized ribosomal subunits were labeled with Cy3 and GFP synthesis was measured by colocalization of GFP fluorescence with the ribosome position. The rate of appearance of colocalized ribosome GFP was equivalent to the rates of fluorescence appearance coupled with translation measured in bulk, and the ribosome - polypeptide complexes were stable for hours. The methods presented here are applicable to single-molecule investigation of translational initiation, elongation and cotranslational folding.

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Single-molecule imaging of full protein synthesis by immobilized ribosomes

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