A comprehensive library of fluorescent transcriptional reporters for Escherichia coli

Alon Zaslaver; Anat Bren; Michal Ronen; Shalev Itzkovitz; Ilya Kikoin; Seagull Shavit; Wolfram Liebermeister; Michael G. Surette; Uri Alon

doi:10.1038/nmeth895

A comprehensive library of fluorescent transcriptional reporters for Escherichia coli

Alon Zaslaver, Anat Bren, Michal Ronen, Shalev Itzkovitz, Ilya Kikoin, Seagull Shavit, Wolfram Liebermeister, Michael G. Surette, Uri Alon

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

Abstract

E. coli is widely used for systems biology research; there exists a need, however, for tools that can be used to accurately and comprehensively measure expression dynamics in individual living cells. To address this we present a library of transcriptional fusions of gfp to each of about 2,000 different promoters in E. coli K12, covering the great majority of the promoters in the organism. Each promoter fusion is expressed from a low-copy plasmid. We demonstrate that this library can be used to obtain highly accurate dynamic measurements of promoter activity on a genomic scale, in a glucose-lactose diauxic shift experiment. The library allowed detection of about 80 previously uncharacterized transcription units in E. coli, including putative internal promoters within previously known operons, such as the lac operon. This library can serve as a tool for accurate, high-resolution analysis of transcription networks in living E. coli cells.

Original language	English
Pages (from-to)	623-628
Number of pages	6
Journal	Nature Methods
Volume	3
Issue number	8
DOIs	https://doi.org/10.1038/nmeth895
State	Published - Aug 2006
Externally published	Yes

ASJC Scopus subject areas

Biotechnology
Biochemistry
Molecular Biology
Cell Biology

Access to Document

10.1038/nmeth895

Cite this

@article{3c06121f6fc14737a8d11f3a6474d8db,

title = "A comprehensive library of fluorescent transcriptional reporters for Escherichia coli",

abstract = "E. coli is widely used for systems biology research; there exists a need, however, for tools that can be used to accurately and comprehensively measure expression dynamics in individual living cells. To address this we present a library of transcriptional fusions of gfp to each of about 2,000 different promoters in E. coli K12, covering the great majority of the promoters in the organism. Each promoter fusion is expressed from a low-copy plasmid. We demonstrate that this library can be used to obtain highly accurate dynamic measurements of promoter activity on a genomic scale, in a glucose-lactose diauxic shift experiment. The library allowed detection of about 80 previously uncharacterized transcription units in E. coli, including putative internal promoters within previously known operons, such as the lac operon. This library can serve as a tool for accurate, high-resolution analysis of transcription networks in living E. coli cells.",

author = "Alon Zaslaver and Anat Bren and Michal Ronen and Shalev Itzkovitz and Ilya Kikoin and Seagull Shavit and Wolfram Liebermeister and Surette, {Michael G.} and Uri Alon",

year = "2006",

month = aug,

doi = "10.1038/nmeth895",

language = "English",

volume = "3",

pages = "623--628",

journal = "Nature Methods",

issn = "1548-7091",

publisher = "Nature Research",

number = "8",

}

TY - JOUR

T1 - A comprehensive library of fluorescent transcriptional reporters for Escherichia coli

AU - Zaslaver, Alon

AU - Bren, Anat

AU - Ronen, Michal

AU - Itzkovitz, Shalev

AU - Kikoin, Ilya

AU - Shavit, Seagull

AU - Liebermeister, Wolfram

AU - Surette, Michael G.

AU - Alon, Uri

PY - 2006/8

Y1 - 2006/8

N2 - E. coli is widely used for systems biology research; there exists a need, however, for tools that can be used to accurately and comprehensively measure expression dynamics in individual living cells. To address this we present a library of transcriptional fusions of gfp to each of about 2,000 different promoters in E. coli K12, covering the great majority of the promoters in the organism. Each promoter fusion is expressed from a low-copy plasmid. We demonstrate that this library can be used to obtain highly accurate dynamic measurements of promoter activity on a genomic scale, in a glucose-lactose diauxic shift experiment. The library allowed detection of about 80 previously uncharacterized transcription units in E. coli, including putative internal promoters within previously known operons, such as the lac operon. This library can serve as a tool for accurate, high-resolution analysis of transcription networks in living E. coli cells.

AB - E. coli is widely used for systems biology research; there exists a need, however, for tools that can be used to accurately and comprehensively measure expression dynamics in individual living cells. To address this we present a library of transcriptional fusions of gfp to each of about 2,000 different promoters in E. coli K12, covering the great majority of the promoters in the organism. Each promoter fusion is expressed from a low-copy plasmid. We demonstrate that this library can be used to obtain highly accurate dynamic measurements of promoter activity on a genomic scale, in a glucose-lactose diauxic shift experiment. The library allowed detection of about 80 previously uncharacterized transcription units in E. coli, including putative internal promoters within previously known operons, such as the lac operon. This library can serve as a tool for accurate, high-resolution analysis of transcription networks in living E. coli cells.

UR - http://www.scopus.com/inward/record.url?scp=33746415885&partnerID=8YFLogxK

U2 - 10.1038/nmeth895

DO - 10.1038/nmeth895

M3 - Article

C2 - 16862137

AN - SCOPUS:33746415885

SN - 1548-7091

VL - 3

SP - 623

EP - 628

JO - Nature Methods

JF - Nature Methods

IS - 8

ER -

A comprehensive library of fluorescent transcriptional reporters for Escherichia coli

Abstract

ASJC Scopus subject areas

Access to Document

Other files and links

Fingerprint

Cite this