Cell lysis directed by σ E in early stationary phase and effect of induction of the rpoE gene on global gene expression in Escherichia coli

Kabir, Md. Shahinur; Yamashita, Daisuke; Koyama, Satoshi; Oshima, Taku; Kurokawa, Ken; Maeda, Maki; Tsunedomi, Ryouichi; Murata, Masayuki; Wada, Chieko; Mori, Hirotada; Yamada, Mamoru

doi:10.1099/mic.0.28004-0

Cited by 67 publications

(96 citation statements)

References 45 publications

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“…In previous studies of E -directed cell lysis with a ΔrseA mutant in early stationary phase, the optical densities, CFU per milliliter, and release of protein into culture supernatants were examined, but E activity was not investigated (25)(26)(27). Because we had observed that mutants with reduced E activity occasionally appeared when overnight cultures of a ΔrseA strain were plated, we decided to monitor E activity using the E -dependent rpoHp3-lacZ fusion, in addition to measuring the optical density and CFU per milliliter.…”

Section: Resultsmentioning

confidence: 99%

“…This proposal is based on observations that cultures with elevated E activity due to E overexpression or deletion of the rseA gene have lower optical densities (ODs) in early stationary phase than do isogenic wild-type cells, although the CFU per milliliter for the two strains are comparable. Cultures with elevated E activity also have higher levels of proteins released into the growth medium than wild-type cultures, suggesting that cells that are not able to form colonies have lysed (25)(26)(27).…”

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Appropriate Regulation of the σ ^E -Dependent Envelope Stress Response Is Necessary To Maintain Cell Envelope Integrity and Stationary-Phase Survival in Escherichia coli

2017

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The alternative sigma factor E is a key component of the Escherichia coli response to cell envelope stress and is required for viability even in the absence of stress. The activity of E increases during entry into stationary phase, suggesting an important role for E when nutrients are limiting. Elevated E activity has been proposed to activate a pathway leading to the lysis of nonculturable cells that accumulate during early stationary phase. To better understand E -directed cell lysis and the role of E in stationary phase, we investigated the effects of elevated E activity in cultures grown for 10 days. We demonstrate that high E activity is lethal for all cells in stationary phase, not only those that are nonculturable. Spontaneous mutants with reduced E activity, due primarily to point mutations in the region of E that binds the Ϫ35 promoter motif, arise and take over cultures within 5 to 6 days after entry into stationary phase. High E activity leads to large reductions in the levels of outer membrane porins and increased membrane permeability, indicating membrane defects. These defects can be counteracted and stationary-phase lethality delayed significantly by stabilizing membranes with Mg 2ϩ and buffering the growth medium or by deleting the E -dependent small RNAs (sRNAs) MicA, RybB, and MicL, which inhibit the expression of porins and Lpp. Expression of these sRNAs also reverses the loss of viability following depletion of E activity. Our results demonstrate that appropriate regulation of E activity, ensuring that it is neither too high nor too low, is critical for envelope integrity and cell viability.IMPORTANCE The Gram-negative cell envelope and cytoplasm differ significantly, and separate responses have evolved to combat stress in each compartment. An array of cell envelope stress responses exist, each of which is focused on different parts of the envelope. The E response is conserved in many enterobacteria and is tuned to monitor pathways for the maturation and delivery of outer membrane porins, lipoproteins, and lipopolysaccharide to the outer membrane. The activity of E is tightly regulated to match the production of E regulon members to the needs of the cell. In E. coli, loss of E results in lethality. Here we demonstrate that excessive E activity is also lethal and results in decreased membrane integrity, the very phenotype the system is designed to prevent.KEYWORDS cell envelope, stress response, transcriptional regulation S tress responses allow cells to rapidly adapt their gene expression to cope with changing conditions. Signal transduction pathways sense an inducing stress and transduce that information to a transcription factor, which, in turn, regulates the expression of specialized sets of genes required to combat the stress. Once the stress Citation Nicoloff H, Gopalkrishnan S, Ades SE. 2017. Appropriate regulation of the σ Edependent envelope stress response is necessary to maintain cell envelope integrity and stationary-phase survival in Escherichia coli.

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Section: Resultsmentioning

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Appropriate Regulation of the σ ^E -Dependent Envelope Stress Response Is Necessary To Maintain Cell Envelope Integrity and Stationary-Phase Survival in Escherichia coli

2017

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“…The lipoproteins of the E. coli BAM complex are transcriptionally regulated by s E (Dartigalongue et al, 2001;Kabir et al, 2005;Lewis et al, 2008;Rezuchova et al, 2003), an extracytoplasmic function (ECF) sigma factor that directs the transcription of chaperones, assembly factors and proteases to restore homeostasis after envelope stress . The Caulobacter genome encodes 13 ECF sigma factors (Nierman et al, 2001), and it is currently unclear which of them perform functions analogous to E. coli s E (Alvarez-Martinez et al, 2006.…”

Section: Discussionmentioning

confidence: 99%

The BAM complex subunit BamE (SmpA) is required for membrane integrity, stalk growth and normal levels of outer membrane β-barrel proteins in Caulobacter crescentus

2010

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The outer membrane of Gram-negative bacteria is an essential compartment containing a specific complement of lipids and proteins that constitute a protective, selective permeability barrier. Outer membrane β-barrel proteins are assembled into the membrane by the essential hetero-oligomeric BAM complex, which contains the lipoprotein BamE. We have identified a homologue of BamE, encoded by CC1365, which is located in the outer membrane of the stalked alpha-proteobacterium Caulobacter crescentus. BamE associates with proteins whose homologues in other bacteria are known to participate in outer membrane protein assembly: BamA (CC1915), BamB (CC1653) and BamD (CC1984). Caulobacter cells lacking BamE grow slowly in rich medium and are hypersensitive to anionic detergents, some antibiotics and heat exposure, which suggest that the membrane integrity of the mutant is compromised. Membranes of the ΔbamE mutant have normal amounts of the outer membrane protein RsaF, a TolC homologue, but are deficient in CpaC*, an aggregated form of the outer membrane secretin for type IV pili. ΔbamE membranes also contain greatly reduced amounts of three TonB-dependent receptors that are abundant in wild-type cells. Cells lacking BamE have short stalks and are delayed in stalk outgrowth during the cell cycle. Based on these findings, we propose that Caulobacter BamE participates in the assembly of outer membrane β-barrel proteins, including one or more substrates required for the initiation of stalk biogenesis.

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“…After RT reaction had been performed at 40˚C for 15 min, PCR consisting of denaturing at 82˚C for 1 min, annealing at a fixed temperature, 5 degrees lower than T m , which was calculated by the rule of thumb Sequencing of pdc gene method [18], for 1 min and extension at 72˚C for 1 min was carried out using the two primers for each gene. The PCR products after 20, 25, 30 and 35 cycles for each gene were analyzed by 0.9% agarose gel electrophoresis, and the relative intensity of the products was densitometrically estimated by using a Bio-Rad molecular imager [19,20]. Under our conditions, the RNA-selective RT-PCR was able to specifically detect mRNA, because no band was observed when reverse transcriptase was omitted.…”

Section: Rt-pcr Analysismentioning

confidence: 99%

Thermotolerant Zymomonas mobilis: Comparison of Ethanol Fermentation Capability with that of an Efficient Type Strain

Sootsuwan¹,

Irie²,

Murata³

et al. 2007

TOBIOTJ

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Abstract:Zymomonas mobilis is an alternative microorganism to Saccharomyces cerevisiae for ethanol production. To find a thermotolerant Z. mobilis strain, the growth and ethanol production of four isolates in Thailand were compared with those of the efficient strain ZM4 (NRRL B-14023) at different temperatures. One of the selected strains, TISTR 405, was found to grow and produce ethanol even at 39˚C to an extent similar to that at 30˚C, and the growth and ethanol productivity at 39˚C were better than those of ZM4 at 30˚C, suggesting that TISTR 405 is suitable for ethanol fermentation at high temperatures. Analysis of genes directly related to ethanol formation or degradation, adhA, adhB and pdc, encoding alcohol dehydrogenase (Adh) A, AdhB and pyruvate decarboxylase, respectively, revealed that these genes were highly conserved in both strains. Comparison of their gene expression and activity of the products in both TISTR 405 and ZM4 at different temperatures or growth phases indicated that there was not a great difference at the transcriptional level, but the total activity of AdhA and AdhB in TISTR 405 was higher than that in ZM4. Both strains showed a significant increase in AdhB activity in the stationary phase.

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Cell lysis directed by σ E in early stationary phase and effect of induction of the rpoE gene on global gene expression in Escherichia coli

Cited by 67 publications

References 45 publications

Appropriate Regulation of the σ ^E -Dependent Envelope Stress Response Is Necessary To Maintain Cell Envelope Integrity and Stationary-Phase Survival in Escherichia coli

Appropriate Regulation of the σ ^E -Dependent Envelope Stress Response Is Necessary To Maintain Cell Envelope Integrity and Stationary-Phase Survival in Escherichia coli

The BAM complex subunit BamE (SmpA) is required for membrane integrity, stalk growth and normal levels of outer membrane β-barrel proteins in Caulobacter crescentus

Thermotolerant Zymomonas mobilis: Comparison of Ethanol Fermentation Capability with that of an Efficient Type Strain

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Cell lysis directed by σ E in early stationary phase and effect of induction of the rpoE gene on global gene expression in Escherichia coli

Cited by 67 publications

References 45 publications

Appropriate Regulation of the σ E -Dependent Envelope Stress Response Is Necessary To Maintain Cell Envelope Integrity and Stationary-Phase Survival in Escherichia coli

Appropriate Regulation of the σ E -Dependent Envelope Stress Response Is Necessary To Maintain Cell Envelope Integrity and Stationary-Phase Survival in Escherichia coli

The BAM complex subunit BamE (SmpA) is required for membrane integrity, stalk growth and normal levels of outer membrane β-barrel proteins in Caulobacter crescentus

Thermotolerant Zymomonas mobilis: Comparison of Ethanol Fermentation Capability with that of an Efficient Type Strain

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Appropriate Regulation of the σ ^E -Dependent Envelope Stress Response Is Necessary To Maintain Cell Envelope Integrity and Stationary-Phase Survival in Escherichia coli

Appropriate Regulation of the σ ^E -Dependent Envelope Stress Response Is Necessary To Maintain Cell Envelope Integrity and Stationary-Phase Survival in Escherichia coli