MicL, a new σ <sup>E</sup>-dependent sRNA, combats envelope stress by repressing synthesis of Lpp, the major outer membrane lipoprotein

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Abstract

In enteric bacteria, the transcription factor σ ^E maintains membrane homeostasis by inducing the synthesis of membrane repair proteins as well as two small regulatory RNAs (sRNAs) that down-regulate membrane porin synthesis. Here, Storz and colleagues identify a third σ ^E-dependent sRNA, MicL, transcribed from the cutC gene coding sequence. MicL represses the outer membrane lipoprotein Lpp and is responsible for the copper sensitivity phenotype previously associated with cutC loss. This discovery is critical to understanding the networks that control outer membrane homeostasis in response to stress.

Abstract

In enteric bacteria, the transcription factor σ ^E maintains membrane homeostasis by inducing synthesis of proteins involved in membrane repair and two small regulatory RNAs (sRNAs) that down-regulate synthesis of abundant membrane porins. Here, we describe the discovery of a third σ ^E-dependent sRNA, MicL (mRNA-interfering complementary RNA regulator of Lpp), transcribed from a promoter located within the coding sequence of the cutC gene. MicL is synthesized as a 308-nucleotide (nt) primary transcript that is processed to an 80-nt form. Both forms possess features typical of Hfq-binding sRNAs but surprisingly target only a single mRNA, which encodes the outer membrane lipoprotein Lpp, the most abundant protein of the cell. We show that the copper sensitivity phenotype previously ascribed to inactivation of the cutC gene is actually derived from the loss of MicL and elevated Lpp levels. This observation raises the possibility that other phenotypes currently attributed to protein defects are due to deficiencies in unappreciated regulatory RNAs. We also report that σ ^E activity is sensitive to Lpp abundance and that MicL and Lpp comprise a new σ ^E regulatory loop that opposes membrane stress. Together MicA, RybB, and MicL allow σ ^E to repress the synthesis of all abundant outer membrane proteins in response to stress.

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Nicholas Ingolia, Sina Ghaemmaghami, John R S Newman … (2009)

Techniques for systematically monitoring protein translation have lagged far behind methods for measuring messenger RNA (mRNA) levels. Here, we present a ribosome-profiling strategy that is based on the deep sequencing of ribosome-protected mRNA fragments and enables genome-wide investigation of translation with subcodon resolution. We used this technique to monitor translation in budding yeast under both rich and starvation conditions. These studies defined the protein sequences being translated and found extensive translational control in both determining absolute protein abundance and responding to environmental stress. We also observed distinct phases during translation that involve a large decrease in ribosome density going from early to late peptide elongation as well as widespread regulated initiation at non-adenine-uracil-guanine (AUG) codons. Ribosome profiling is readily adaptable to other organisms, making high-precision investigation of protein translation experimentally accessible.

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Thomas Silhavy, Daniel Kahne, Suzanne Walker (2010)

The bacteria cell envelope is a complex multilayered structure that serves to protect these organisms from their unpredictable and often hostile environment. The cell envelopes of most bacteria fall into one of two major groups. Gram-negative bacteria are surrounded by a thin peptidoglycan cell wall, which itself is surrounded by an outer membrane containing lipopolysaccharide. Gram-positive bacteria lack an outer membrane but are surrounded by layers of peptidoglycan many times thicker than is found in the gram-negatives. Threading through these layers of peptidoglycan are long anionic polymers, called teichoic acids. The composition and organization of these envelope layers and recent insights into the mechanisms of cell envelope assembly are discussed.

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Author and article information

Journal

Journal ID (nlm-ta): Genes Dev

Journal ID (iso-abbrev): Genes Dev

Journal ID (publisher-id): GAD

Title: Genes & Development

Publisher: Cold Spring Harbor Laboratory Press

ISSN (Print): 0890-9369

ISSN (Electronic): 1549-5477

Publication date (Print): 15 July 2014

Volume: 28

Issue: 14

Pages: 1620-1634

Affiliations

[1 ]Department of Microbiology and Immunology, University of California at San Francisco, San Francisco, California 94158, USA;

[2 ]Cell Biology and Metabolism Program, Eunice Kennedy Shriver National Institutes of Health, Bethesda, Maryland 20892, USA;

[3 ]National Center for Biotechnology Information, National Institutes of Health, Bethesda, Maryland 20894, USA

Author notes

[4]

Present address: Genentech, Inc., South San Francisco, CA 94080, USA.

[5]

These authors contributed equally to this work.

[6 ]Corresponding authors E-mail storzg@ 123456mail.nih.gov E-mail cgrossucsf@ 123456gmail.com

Article

Medline ID: 8711660

DOI: 10.1101/gad.243485.114

PMC ID: 4102768

PubMed ID: 25030700

SO-VID: 2a6b6065-9a4a-4819-a828-faff6c7a28da

License:

This article is distributed exclusively by Cold Spring Harbor Laboratory Press for the first six months after the full-issue publication date (see http://genesdev.cshlp.org/site/misc/terms.xhtml). After six months, it is available under a Creative Commons License (Attribution-NonCommercial 4.0 International), as described at http://creativecommons.org/licenses/by-nc/4.0/.

History

Date received : 13 April 2014

Date accepted : 17 June 2014

Page count

Pages: 15

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