Your search keyword '"E. coli Cell cycle"' showing total 345 results

151. Initiator titration complex formed at datA with the aid of IHF regulates replication timing in Escherichia coli.

Author

Nozaki, Shingo, Yamada, Yoshitaka, and Ogawa, Tohru

Subjects

ESCHERICHIA coli, CHROMOSOMES, PROTEINS, DNA replication, DNA

Abstract

The initiation of replication in Escherichia coli is negatively controlled by a mechanism referred to as ‘initiator titration’, a process by which the initiator protein, DnaA, is titrated to newly replicated binding sequences on the chromosome to reduce the initiation potential for replication. Initiator titration occurs predominantly at the datA locus that binds exceptionally large amounts of DnaA molecules to prevent aberrant initiations. We found that this was enabled by integration host factor (IHF). Within datA, there is a consensus IHF recognition sequence between the two DnaA recognition sequences (DnaA boxes) essential for its function. Binding of IHF to this site was demonstrated both in vitro and in vivo. Disruption of the core sequence in the consensus of the IHF-binding resulted in increased origin concentration as observed in ΔdatA cells. Furthermore, the number of DnaA molecules bound to datA was reduced in cells carrying a disruption in the IHF-binding core sequence. The IHF-binding site and the essential DnaA boxes had to be located at a proper distance and orientation to maintain the accurate initiation timing. Therefore, IHF is a unique element in the control of replication initiation that acts negatively at datA, while known to act as a positive regulator at oriC. [ABSTRACT FROM AUTHOR]

Published

2009

152. The Stringent Response and Cell Cycle Arrest in Escherichia coli.

Author

Ferullo, Daniel J. and Lovett, Susan T.

Subjects

CELL cycle regulation, ESCHERICHIA coli, ENTEROBACTERIACEAE, CELL nuclei, AMINO acids, ESCHERICHIA coli cell cycle

Abstract

The bacterial stringent response, triggered by nutritional deprivation, causes an accumulation of the signaling nucleotides pppGpp and ppGpp. We characterize the replication arrest that occurs during the stringent response in Escherichia coli. Wild type cells undergo a RelA-dependent arrest after treatment with serine hydroxamate to contain an integer number of chromosomes and a replication origin-to-terminus ratio of 1. The growth rate prior to starvation determines the number of chromosomes upon arrest. Nucleoids of these cells are decondensed; in the absence of the ability to synthesize ppGpp, nucleoids become highly condensed, similar to that seen after treatment with the translational inhibitor chloramphenicol. After induction of the stringent response, while regions corresponding to the origins of replication segregate, the termini remain colocalized in wild-type cells. In contrast, cells arrested by rifampicin and cephalexin do not show colocalized termini, suggesting that the stringent response arrests chromosome segregation at a specific point. Release from starvation causes rapid nucleoid reorganization, chromosome segregation, and resumption of replication. Arrest of replication and inhibition of colony formation by ppGpp accumulation is relieved in seqA and dam mutants, although other aspects of the stringent response appear to be intact. We propose that DNA methylation and SeqA binding to non-origin loci is necessary to enforce a full stringent arrest, affecting both initiation of replication and chromosome segregation. This is the first indication that bacterial chromosome segregation, whose mechanism is not understood, is a step that may be regulated in response to environmental conditions. [ABSTRACT FROM AUTHOR]

Published

2008

153. Role of the bacteriophage λ exo-xis region in the virus development.

Author

Łoś, J., Łoś, M., Węgrzyn, A., and Węgrzyn, G.

Abstract

Various processes of bacteriophage λ development in Escherichia coli cells bearing either the whole λ exo-xis region (with truncated, thus nonfunctional, exo and xis genes) or particular genes from this region were investigated. The presence of either the exo-xis region or the ea8.5 gene on a plasmid resulted in formation of fuzzy plaques by infecting phage. Both efficiency of plating and efficiency of lysogenization were decreased in such hosts. On the other hand, neither the efficiency of adsorption nor intracellular lytic development of the infecting phage (measured in one-step-growth experiments) was affected while significantly more host cells survived the infection, when containing the exo-xis region. Although no effects of the exo-xis region on the activity of the p L promoter was detected, this region contributed to a decreased transcription from the cII-stimulated promoters p I, p aQ and p E. These results, together with the results of measurement of efficiency of plating of phages bearing mutations in cI, cII and cIII genes on hosts containing the exo-xis region, strongly suggest that genes from this region (especially ea8.5) are involved in the regulation of bacteriophage λ development at the stage of the lysis- vs.-lysogenization decision. [ABSTRACT FROM AUTHOR]

Published

2008

154. Dynamic events of sister chromosomes in the cell cycle of Escherichia coli.

Author

Adachi, Shun, Fukushima, Toru, and Hiraga, Sota

Subjects

CHROMOSOMES, CELL cycle, ESCHERICHIA coli, FLUORESCENCE microscopy, CELL nuclei, CYTOMETRY, ESCHERICHIA coli cell cycle

Abstract

Various events involving partitioning of sister chromosomes were precisely analyzed in asynchronously growing Escherichia coli cells in various conditions. To examine the cohesion between sister chromosomes, we analyzed living cells growing under various conditions for the number of the replication origin ( oriC) copies by flow cytometry and the foci of oriC by fluorescence microscopy. The average number of the oriC foci per cell was significantly smaller than the number of oriC copies per cell with few exceptions, suggesting cohesion of oriC sister copies. Cohesion phenomenon of oriC sister copies was also observed in a mukB null mutant cells under some growth conditions. Sister copies of the terminal region ( ter) were also found to be cohesive. Immunofluorescence microscopy for nascent DNA pulse-labeled with 5-bromo-2′-deoxyuridine (BrdU) indicated that paired replication forks acting on bidirectional replication were able to migrate toward opposite directions during ongoing replication in poor medium; however, some of them were closely associated in rich media. Analysis of the foci of MukB–GFP indicates that the number of MukB foci was always larger than the number of replication forks. The number of MukB–GFP foci increased together with cell length. The sequence of these chromosomal events in the growing cells has been depicted. [ABSTRACT FROM AUTHOR]

Published

2008

155. Mutational analysis reveals Escherichia coli oriC interacts with both DnaA-ATP and DnaA-ADP during pre-RC assembly.

Author

Grimwade, Julia E., Torgue, Julien J.-C., McGarry, Kevin C., Rozgaja, Tanya, Enloe, Sareena T., and Leonard, Alan C.

Subjects

ESCHERICHIA coli, DNA synthesis, GENETIC mutation, GENES, MOLECULES, ADENOSINE triphosphate

Abstract

Prior to initiating DNA synthesis, Escherichia coli oriC switches from ORC, comprising initiator DnaA bound at three high-affinity sites, to pre-RC, when additional DnaA molecules interact with low-affinity sites. Two types of low-affinity sites exist: R boxes that bind DnaA-ATP and DnaA-ADP with equal affinity, and I-sites with a three- to fourfold preference for DnaA-ATP. To assess the regulatory role of weak DnaA interactions during pre-RC assembly in vivo, we compared the behaviour of plasmid-borne wild-type oriC with mutants having an increased or decreased number of DnaA-ATP discriminatory I-sites. Increasing the number of discriminatory sites by replacing R5M with I2 inactivated extrachromosomal oriC function. Mutants with no discriminatory sites perturbed host growth and rapidly replaced wild-type chromosomal oriC, but normal function returned if one I-site was restored at either the I2, I3 or R5M position. These observations are consistent with assembly of E. coli pre-RC in vivo from mixtures of DnaA-ATP and DnaA-ADP, with I-site interactions coupling pre-RC assembly to DnaA-ATP levels. [ABSTRACT FROM AUTHOR]

Published

2007

156. Global analysis of host response to induction of a latent bacteriophage.

Subjects

BACTERIOPHAGE induction

Published

2007

157. Copy-number control of the Escherichia coli chromosome: a plasmidologist's view.

Author

Nordström, Kurt and Dasgupta, Santanu

Subjects

PLASMIDS, CHROMOSOME replication, CELL cycle, RNA, ESCHERICHIA coli, BACTERIA

Abstract

The homeostatic system that sets the copy number, and corrects over-replication and under-replication, seems to be different for chromosomes and plasmids in bacteria. Whereas plasmid replication is random in time, chromosome replication is tightly coordinated with the cell cycle such that all origins are initiated synchronously at the same cell mass per origin once per cell cycle. In this review, we propose that despite their apparent differences, the copy-number control of the Escherichia coli chromosome is similar to that of plasmids. The basic mechanism that is shared by both systems is negative-feedback control of the availability of a protein or RNA positive initiator. Superimposed on this basic mechanism are at least three systems that secure the synchronous initiation of multiple origins; however, these mechanisms are not essential for maintaining the copy number. [ABSTRACT FROM AUTHOR]

Published

2006

158. Noise in transcription negative feedback loops: simulation and experimental analysis.

Author

Dublanche, Yann, Michalodimitrakis, Konstantinos, Kümmerer, Nico, Foglierini, Mathilde, and Serrano, Luis

Subjects

GENETIC transcription, EXPRESSIVE behavior, COMPUTER simulation, TRANSCRIPTION factors, NOISE

Abstract

Negative feedback loops have been invoked as a way to control and decrease transcriptional noise. Here, we have built three circuits to test the effect of negative feedback loops on transcriptional noise of an autoregulated gene encoding a transcription factor (TF) and a downstream gene (DG), regulated by this TF. Experimental analysis shows that self-repression decreases noise compared to expression from a non-regulated promoter. Interestingly enough, we find that noise minimization by negative feedback loop is optimal within a range of repression strength. Repression values outside this range result in noise increase producing a U-shaped behaviour. This behaviour is the result of external noise probably arising from plasmid fluctuations as shown by simulation of the network. Regarding the target gene of a self-repressed TF (sTF), we find a strong decrease of noise when repression by the sTF is strong and a higher degree of noise anti-correlation between sTF and its target. Simulations of the circuits indicate that the main source of noise in these circuits could come from plasmid variation and therefore that negative feedback loops play an important role in suppressing both external and internal noise. An important observation is that DG expression without negative feedback exhibits bimodality at intermediate TF repression values. This bimodal behaviour seems to be the result of external noise as it can only be found in those simulations that include plasmid variation. [ABSTRACT FROM AUTHOR]

Published

2006

159. Maturation of theEscherichia colidivisome occurs in two steps.

Author

Aarsman, Mirjam E. G., Piette, André, Fraipont, Claudine, Vinkenvleugel, Thessa M. F., Nguyen-Distéche, Martine, and den Blaauwen, Tanneke

Subjects

ESCHERICHIA, ESCHERICHIA coli, BACTERIOLOGY, MOLECULAR biology, MOLECULAR microbiology, MICROBIOLOGY, BIOLOGY

Abstract

Cell division proteins FtsZ (FtsA, ZipA, ZapA), FtsE/X, FtsK, FtsQ, FtsL/B, FtsW, PBP3, FtsN and AmiC localize at mid cell inEscherichia coliin an interdependent order as listed. To investigate whether this reflects a time dependent maturation of the divisome, the average cell age at which FtsZ, FtsQ, FtsW, PBP3 and FtsN arrive at their destination was determined by immuno- and GFP-fluorescence microscopy of steady state grown cells at a variety of growth rates. Consistently, a time delay of 14–21 min, depending on the growth rate, between Z-ring formation and the mid cell recruitment of proteins down stream of FtsK was found. We suggest a two-step model for bacterial division in which the Z-ring is involved in the switch from cylindrical to polar peptidoglycan synthesis, whereas the much later localizing cell division proteins are responsible for the modification of the envelope shape into that of two new poles. [ABSTRACT FROM AUTHOR]

Published

2005

160. Compartmentalization of prokaryotic DNA replication.

Author

Bravo, Alicia, Serrano-Heras, Gemma, and Salas, Margarita

Subjects

PROKARYOTES, DNA, BIOLOGICAL membranes, ESCHERICHIA coli, BACILLUS subtilis, GENES

Abstract

It becomes now apparent that prokaryotic DNA replication takes place at specific intracellular locations. Early studies indicated that chromosomal DNA replication, as well as plasmid and viral DNA replication, occurs in close association with the bacterial membrane. Moreover, over the last several years, it has been shown that some replication proteins and specific DNA sequences are localized to particular subcellular regions in bacteria, supporting the existence of replication compartments. Although the mechanisms underlying compartmentalization of prokaryotic DNA replication are largely unknown, the docking of replication factors to large organizing structures may be important for the assembly of active replication complexes. In this article, we review the current state of this subject in two bacterial species, Eseheriehia coli and Bacillus subtilis, focusing our attention in both chromosomal and extrachromosomal DNA replication. A comparison with eukaryotic systems is also presented. [ABSTRACT FROM AUTHOR]

Published

2005

161. A Complete Set of Escherichia coli Open Reading Frames in Mobile Plasmids Facilitating Genetic Studies.

Author

Saka, Kimiko, Tadenuma, Maki, Nakade, Shinsuke, Tanaka, Noriko, Sugawara, Hideaki, Nishikawa, Ken, Ichiyoshi, Nobuyuki, Kitagawa, Masanari, Mori, Hirotada, Ogasawara, Naotake, and Nishimura, Akiko

Abstract

To facilitate genetic studies of Escherichia coli, we constructed a complete set of mobile plasmid clones of intact open reading frames (ORFs). Their expression is strictly controlled by Ptac/lacIq. The plasmids carrying each ORF were introduced into an F+ recA strain and stored in 96-well microtiter plates. In this way, 96 clones can be transferred simultaneously to F−bacteria using the conjugative system. This provides a convenient procedure for systematic identification of ORFs that suppress or complement mutations. We created two types of clone sets: the original set contained individual clones in 45 microtiter plates, and a second set contained pools of 48 clones stored in a single microtiter plate. Using these clone sets, we have identified 403 genes that can correct in trans the temperature-sensitive defect of cell division mutants, which would suggest multiple global regulators for bacterial cell division. [ABSTRACT FROM PUBLISHER]

Published

2005

162. Genetic recombination and the cell cycle: what we have learned from chromosome dimers.

Author

Lesterlin, Christian, Barre, François-Xavier, and Cornet, François

Subjects

GENETIC recombination, DNA, CHROMOSOMES, CELL cycle, DIMERS, RECOMBINANT DNA, GENES

Abstract

Genetic recombination is central to DNA metabolism. It promotes sequence diversity and maintains genome integrity in all organisms. However, it can have perverse effects and profoundly influence the cell cycle. In bacteria harbouring circular chromosomes, recombination frequently has an unwanted outcome, the formation of chromosome dimers. Dimers form by homologous recombination between sister chromosomes and are eventually resolved by the action of two site-specific recombinases, XerC and XerD, at their target site,dif, located in the replication terminus of the chromosome. Studies of the Xer system and of the modalities of dimer formation and resolution have yielded important knowledge on how both homologous and site-specific recombination are controlled and integrated in the cell cycle. Here, we briefly review these advances and highlight the important questions they raise. [ABSTRACT FROM AUTHOR]

Published

2004

163. Recombination and chromosome segregation.

Author

David J. Sherratt, Britta Søballe, François-Xavier Barre, Sergio Filipe, Ivy Lau, Thomas Massey, and James Yates

Published

2004

164. Titration of the Escherichia coli DnaA protein to excess datA sites causes destabilization of replication forks, delayed replication initiation and delayed cell division.

Author

Løbner-Olesen, Anders and Skarstad, Kirsten

Subjects

ESCHERICHIA coli, CELL division, GENETICS

Abstract

Summary In Escherichia coli , the level of the initiator protein DnaA is limiting for initiation of replication at oriC . A high-affinity binding site for DnaA, datA , plays an important role. Here, the effect of extra datA sites was studied. A moderate increase in datA dosage (≈ fourfold) delayed initiation of replication and cell division, but increased the rate of replication fork movement about twofold. At a further increase in the datA gene dosage, the SOS response was induced, and incomplete rounds of chromosome replication were detected. Overexpression of DnaA protein suppressed the SOS response and restored normal replication timing and rate of fork movement. In the presence of extra datA sites, cells showed a dependency on PriA and RecA proteins, indicating instability of the replication fork. The results suggest that wild-type replication fork progression normally includes controlled pausing, and that this is a prerequisite for normal replication fork function. [ABSTRACT FROM AUTHOR]

Published

2003

165. Transcriptional control for initiation of chromosomal replication in Escherichia coli: fluctuation of the level of origin transcription ensures timely initiation.

Author

Masayuki Su'etsugu, et al, Akiko Emotoa, et al, Kazuyuki Fujimitsu, et al, Kenji Keyamura, et al, and Tsutomu Katayama, et al

Subjects

ESCHERICHIA coli, CHROMOSOME analysis, CYTOLOGICAL research, GENETICS

Abstract

Abstract Background: During the cell cycle, the initiation of chromosomal replication is strictly controlled. In Escherichia coli , the initiator DnaA and the replication origin oriC are major targets for this regulation. Here, we assessed the role of transcription of the mioC gene, which reads through the adjacent oriC region. This mioC-oriC transcription is regulated in coordination with the replication cycle so that it is activated after initiation and repressed before initiation. Results: We isolated a strain bearing a mioC promoter mutation that causes constitutive mioC-oriC transcription from the chromosome. A quantitative S1 nuclease assay indicated that in this mutant, the level of transcription does not fluctuate. Introduction of this mutation suppressed the growth defect of an overinitiation-type dnaAcos mutant, and severely inhibited the growth of initiation-defective dnaA mutants at semipermissive temperatures in a dnaA allele-specific manner. These results suggest that mioC-oriC transcription inhibits initiation at oriC . Indeed, flow cytometry analysis and quantification of DNA replication in synchronized cultures revealed that the mioC promoter mutation alters the control of the initiation of chromosomal replication, for instance by delaying replication within the cell cycle. Conclusions: These results suggest that the transcriptional regulation of the mioC gene is required for cell cycle-coordinated initiation of chromosomal replication. [ABSTRACT FROM AUTHOR]

Published

2003

166. The bacterial replication initiator DnaA. DnaA and oriC, the bacterial mode to initiate DNA replication

Author

Messer, Walter

Subjects

DNA replication, BACTERIAL genetics

Abstract

The initiation of replication is the central event in the bacterial cell cycle. Cells control the rate of DNA synthesis by modulating the frequency with which new chains are initiated, like all macromolecular synthesis. The end of the replication cycle provides a checkpoint that must be executed for cell division to occur. This review summarizes recent insight into the biochemistry, genetics and control of the initiation of replication in bacteria, and the central role of the initiator protein DnaA. [Copyright &y& Elsevier]

Published

2002

167. CONTROL OF CHROMOSOME REPLICATION IN CAULOBACTER CRESCENTUS.

Author

Marczynski, Gregory T. and Shapiro, Lucy

Subjects

CHROMOSOME replication, CELL cycle

Abstract

Caulobacter crescentus permits detailed analysis of chromosome replication control during a developmental cell cycle. Its chromosome replication origin (Cori) may be prototypical of the large and diverse class of alpha-proteobacteria. Cori has features that both affiliate and distinguish it from the Escherichia coli chromosome replication origin. For example, requirements for DnaA protein and RNA transcription affiliate both origins. However, Cori is distinguished by several features, and especially by five binding sites for the CtrA response regulator protein. To selectively repress and limit chromosome replication, CtrA receives both protein degradation and protein phosphorylation signals. The signal mediators, proteases, response regulators, and kinases, as well as Cori DNA and the replisome, all show distinct patterns of temporal and spatial organization during cell cycle progression. Future studies should integrate our knowledge of biochemical activities at Cori with our emerging understanding of cytological dynamics in C. crescentus and other bacteria. [ABSTRACT FROM AUTHOR]

Published

2002

168. Competitive interaction of the OxyR DNA-binding protein and the Dam methylase at the antigen 43 gene regulatory region in Escherichia coli.

Author

Waldron, Denise E, Owen, Peter, and Dorman, Charles J

Subjects

PROTEIN binding, METHYLTRANSFERASES, ANTIGENS, DNA replication

Abstract

Summary The antigen 43 surface protein of Escherichia coli is expressed in a phase-variable manner by a mechanism involving alternative activation and repression of transcription of the agn43 gene. The repressor is the OxyR DNA-binding protein, and its binding site was found to be located downstream of the agn43 transcription start site in a region of DNA that encompasses three 5′ -GATC-3′ sequences that are subject to Dam-mediated DNA methylation. It has been suggested previously that the phase-variable expression of antigen 43 results from a competition between Dam methylase and the OxyR repressor for these sites. The 5′ -GATC-3′ sequences were inactivated for methylation by site-directed mutagenesis, and all possible combinations of inactive and active sites were assessed for effects on phase-variable expression of the agn43 gene. Inactivation of any 5′ -GATC-3′ site individually had no effect; at least two sites had to be inactivated to disrupt the normal pattern of expression. Studies of OxyR interaction with agn43 DNA showed that methylation of any two 5′ -GATC-3′ sites was necessary and sufficient to block binding of the repressor. It was also found that the adenines of the second and third 5′ -GATC-3′ sites are required for OxyR binding, demonstrating that the sites for Dam methylation and for repressor binding are intimately associated. This is consistent with a competition model in which Dam and OxyR share a preference for specific DNA sequences in the regulatory region of the agn43 gene. [ABSTRACT FROM AUTHOR]

Published

2002

169. Fractionation of Escherichia coli cell populations at different stages during growth transition to stationary phase.

Author

Makinoshima, Hideki, Nishimura, Akiko, and Ishihama, Akira

Subjects

ESCHERICHIA coli, GREEN fluorescent protein

Abstract

Summary Cultures of Escherichia coli could be separated into more than 15 cell populations, each forming a discrete band after Percoll gradient centrifugation. The cell separation was found to result from the difference in buoyant density but not the size difference. The cell density increases upon transition from exponential growth to stationary phase. Exponential phase cultures formed at least five discrete bands with lower densities, whereas stationary phase cultures formed more than 10 bands with higher densities. Two molecular markers characterizing each cell population were identified: the functioning promoter species, as identified by measuring the expression of green fluorescent protein under the control of test promoters; and the expressed protein species, as monitored by quantitative immunoblotting. These findings together suggest that the growth phase-coupled transition of E. coli phenotype is discontinuous. [ABSTRACT FROM AUTHOR]

Published

2002

170. Escherichia coli cell cycle control genes affect chromosome superhelicity.

Author

Weitao, Tao, Nordström, Kurt, and Dasgupta, Santanu

Subjects

GENETIC mutation, GENETICS, CELL nuclei, GENES, HEREDITY, PROTEINS

Abstract

We have used ethidium bromide titration for direct measurement of the changes in the negative supercoiling of Esdieridiia coli chromosome caused by mutations inactivating the cell cycle functions mukB and seqA. The amounts of the intercalative agent required to relax the supercoiled chromosome in mukB and seqA mutants were lower and higher, respectively, than for the wild-type parent, confirming that these cell cycle genes modulate the topology of the L coli chromosome. Plasmid superhelicity measured in these mutant strains showed similar effects albeit of reduced magnitude. As the effects of mukB and segA mutations were not restricted to the chromosome alone, MukB and SeqA proteins possibly interact with factors involved in the maintenance of intracellular DNA topology. To our knowledge, this is the first direct demonstration of the influence of mukB and segA genes on the superhelicity of the L coli chromosome. [ABSTRACT FROM AUTHOR]

Published

2000

171. Fusion expression of Escherichia coli prlC gene and preparation of PrlC proteinase affinity column.

Author

Xueyuan Jiang, Zhicheng Jin, Ni Cheng, and Dexu Zhu

Subjects

PROTEINASES, ESCHERICHIA coli, PROTEOLYTIC enzymes, PHYSICAL & theoretical chemistry, DIGESTIVE enzymes, AMINO acids

Abstract

Escherichia coli PrlC is a trypsin-like proteinase regulating the cell cycle. The Escherichia coli prlC gene has been cloned into the pET28a prokaryotic expression vector. The recombinant fusion protein was produced mostly in the soluble, active form and the expression level amounted to approximately 70% of total protein. The recombinant proteinase was efficiently adsorbed to a resin containing immobilized Ni2+ via its amino terminal fusion hexahistidine tail to give a PrlC proteinase affinity column. The adsorbed fusion proteinase hydrolyzed 4-methylcoumaryl-7-amide of tert-butoxycarbonyl-l-valyl-l-prolyl-l-arginine (Boc-Val-Pro-Arg-NH-Mec), the specific substrate for the trypsin-like proteinase activity of E. coli PrlC. [ABSTRACT FROM AUTHOR]

Published

2000

172. New genes with old modus operandi.

Author

Dasgupta, Santanu, Maisnier-Patin, Sophie, and Nordström, Kurt

Subjects

ESCHERICHIA coli, GENETICS, CHROMOSOMES, PROTEINS, GENES, CELLS

Abstract

The process of partitioning bacterial sister chromosomes into daughter cells seems to be distinct from chromatid segregation during eukaryotic mitosis. In Escherichia coli, partitioning starts soon after initiation of replication, when the two newly replicated oriCs move from the cell centre to quarter positions within the cell. As replication proceeds, domains of the compact, supercoiled chromosome are locally decondensed ahead of the replication fork. The nascent daughter chromosomes are recondensed and moved apart through the concerted activities of topoisomerases and the SeqA (sequestration) and MukB (chromosome condensation) proteins, all of which modulate nucleoid superhelicity. Thus, genes involved in chromosome topology, once set aside as 'red herrings' in the search for 'true' partition functions, are again recognized as being important for chromosome partitioning in E. coli. [ABSTRACT FROM AUTHOR]

Published

2000

173. Suppression of a DnaX temperature-sensitive polymerization defect by mutation in the initiation gene, dnaA, requires functional oriC.

Author

Blinkova, Alexandra, Ginés-Candelaria, Edwin, Ross, Julie D., and Walker, James R.

Subjects

ESCHERICHIA coli, DNA polymerases, MICROBIAL mutation, EFFECT of temperature on microorganisms

Abstract

Temperature sensitivity of DNA polymerization and growth, resulting from mutation of the τ and γ subunits of Escherichia coli DNA polymerase III, are suppressed by Cs,Sx mutations of the initiator gene, dnaA. These mutations simultaneously cause defective initiation at 20°C. Efficient suppression, defined as restoration of normal growth rate at 39°C to essentially all the cells, depends on functional oriC. Increasing DnaA activity in a strain capable of suppression, by introducing a copy of the wild-type allele, increasing the suppressor gene dosage or introducing a seqA mutation, reversed the suppression. This suggests that the suppression mechanism depends on reduced activity of DnaACs,Sx. Models that assume that suppression results from an initiation defect or from DnaACs,Sx interaction with polymerization proteins during nascent strand synthesis are proposed. [ABSTRACT FROM AUTHOR]

Published

2000

174. IHF redistributes bound initiator protein, DnaA, on supercoiled oriC ofEscherichia coli.

Author

Grimwade, Julia E., Ryan, Valorie T., and Leonard, Alan C.

Subjects

BACTERIAL genetics, ESCHERICHIA coli, CHROMOSOME replication

Abstract

In Escherichia coli, initiation of chromosome replication requires that DnaA binds to R boxes (9-mer repeats) in oriC, the unique chromosomal replication origin. At the time of initiation, integration host factor (IHF) also binds to a specific site in oriC. IHF stimulates open complex formation by DnaA on supercoiled oriC in cell-free replication systems, but it is unclear whether this stimulation involves specific changes in the oriC nucleoprotein complex. Using dimethylsulphate (DMS) footprinting on supercoiled oriC plasmids, we observed that IHF redistributed prebound DnaA, stimulating binding to sites R2, R3 and R5(M), as well as to three previously unidentified non-R sites with consensus sequence (A/T)G(G/C) (A/T)N(G/C)G(A/T)(A/T)(T/C)A. Redistribution was dependent on IHF binding to its cognate site and also required a functional R4 box. By reducing the DnaA level required to separate DNA strands and trigger initiation of DNA replication at each origin, IHF eliminates competition between strong and weak sites for free DnaA and enhances the precision of initiation synchrony during the cell cycle. [ABSTRACT FROM AUTHOR]

Published

2000

175. Molecular Modeling the Proteins from the exo-xis Region of Lambda and Shigatoxigenic Bacteriophages.

Author

Donaldson, Logan W.

Subjects

BACTERIOPHAGE lambda, PROTEIN models, GENETIC transcription regulation, RNA regulation, RNA polymerases

Abstract

Despite decades of intensive research on bacteriophage lambda, a relatively uncharacterized region remains between the exo and xis genes. Collectively, exo-xis region genes are expressed during the earliest stages of the lytic developmental cycle and are capable of affecting the molecular events associated with the lysogenic-lytic developmental decision. In Shiga toxin-producing E. coli (STEC) and enterohemorragic E. coli (EHEC) that are responsible for food- and water-borne outbreaks throughout the world, there are distinct differences of exo-xis region genes from their counterparts in lambda phage. Together, these differences may help EHEC-specific phage and their bacterial hosts adapt to the complex environment within the human intestine. Only one exo-xis region protein, Ea8.5, has been solved to date. Here, I have used the AlphaFold and RoseTTAFold machine learning algorithms to predict the structures of six exo-xis region proteins from lambda and STEC/EHEC phages. Together, the models suggest possible roles for exo-xis region proteins in transcription and the regulation of RNA polymerase. [ABSTRACT FROM AUTHOR]

Published

2021

176. The role of c-myc in cellular growth control.

Author

Schmidt, Emmett V

Subjects

DNA, CELL division

Abstract

Cell division is coupled to cell growth. Since some c-myc target genes are regulators of cell growth while others function in cell division pathways, c-myc is apparently poised at the interface of these processes. Cell culture systems have shown specific myc-associated growth phenotypes. Increased cell growth precedes DNA synthesis after myc activation in cells expressing myc-estrogen receptor fuson constructs and cells lacking c-myc exhibit a marked loss of protein synthesis. A number of candidate c-myc target genes regulate processes required for cell growth including rRNA transcription and processing, ribosomal protein transcription and translation, and translation initiation. These interactions all have the potential to account for the growth phenotypes in c-myc mutant cells. The ability of translation initiation factors, including eIF4E, to transform cells makes them particularly interesting targets of c-myc. Further evaluation of these target genes will provide important insights into growth control and c-myc's functions in cellular proliferation. [ABSTRACT FROM AUTHOR]

Published

1999

177. Transcription level of operon ftsYEX and activity of promoter P1 of rpoH during the cell cycle in Escherichia coli.

Author

Gómez-Eichelmann, M. Carmen and Helmstetter, Charles E.

Published

1999

178. FtsZ dimerization in vivo.

Author

Di Lallo, Anderluzzi, Ghelardini, Paolozzi, and Paolozzi

Subjects

POLYMERIZATION, ESCHERICHIA coli

Abstract

A hybrid assay, based on the properties of the λ repressor, was developed to detect FtsZ dimerization in Escherichia coli in vivo. A gene fusion comprising the N-terminal end of the λ cI repressor gene and the complete E. coli ftsZ gene was constructed. The fused protein resulted in a functional λ repressor and was able to complement the thermosensitive mutant ftsZ84. Using the same strategy, a series of 10 novel mutants of FtsZ that are unable to dimerize was selected, and a deletion analysis of the protein was carried out. Characterization of these mutants allowed the identification of three separate FtsZ portions: the N-terminal of about 150 amino acids; the C-terminal of about 60 amino acids, which corresponds to the less conserved portion of the protein; and a central region of about 150 residues. Mutants belonging to this region would define the dimerization domain of FtsZ. [ABSTRACT FROM AUTHOR]

Published

1999

179. Adenylate pool sizes and succinate dehydrogenase activity increase continuously throughout the cell cycle of Escherichia coli.

Author

Misri, Ravinder and Poole, Robert K.

Published

1986

180. Chromosome and Plasmid Partition in Escherichia Coli.

Author

Hiraga, Sota

Published

1992

181. Plasmid replication and partition in <em>Escherichia coli</em>: is the cell membrane the key?

Author

Firshein, William and Kim, Peter

Subjects

PLASMIDS, ESCHERICHIA coli, CELL membranes, DNA replication, CELL cycle

Abstract

The DNA-membrane complex has been the subject of intensive investigation for over 35 years as the possible site for DNA replication in the prokaryotic cell and the site through which newly synthesized chromosomes are segregated into daughter cells. However, the molecular mechanisms which control these phenomena are, for the most part, poorly understood despite genetic, biochemical, and morphologic evidence in favour of their existence. This is probably due to the transient nature and non-covalent interactions that occur between DNA and the membrane. In addition, there is a paucity of knowledge concerning the nature of the membrane receptors for DNA and whether the membrane plays simply a structural or metabolic role in the two processes. Plasmids can provide important insights into the role of the membrane in replication and partitioning because the plasmid life cycle is relatively simple, with replication occurring during the cell cycle and partitioning during cell division. The replicon model of Jacob et al. (1963, Cold Spring Harbor Symp Quant Biol 28: 329-348) still represents a good conceptual framework (with modifications) to explain how plasmid replication and partitioning are linked by the membrane. In its simplest form, the model focuses on specific membrane binding sites (possibly along the equator of the cell) for plasmid (or bacterial) replication, with the membrane acting as a motive force to separate the newly synthesized replicons and their attached sites into daughter cells. Indeed, proteins involved in both plasmid replication and partitioning have been found in membrane fractions and some plasmids require membrane binding for initiation and an active partitioning. We propose that several factors are critical for both plasmid DNA replication and partitioning. One factor is the extent of negative supercoiling (brought about by an interplay of various topoisomerases, but most importantly by DNA gyrase). Supercoiling is known to be critical for initiation of DNA replication but may also be important for the formation of a partition complex in contact with the cell membrane. Another factor is the presence of specific subdomains of the membrane which can interact specifically with origin DNA and possibly other regions involved in partitioning. Such domains may be induced transiently or be present at all times during the cell cycle. [ABSTRACT FROM AUTHOR]

Published

1997

182. Escherichia coli strains in which chromosome replication is controlled by a P1 or F replicon integrated into oriC.

Author

Eliasson, Åsa, Nordström, Kurt, and Bernander, Rolf

Subjects

ESCHERICHIA coli, CHROMOSOME replication, PLASMIDS, NUCLEOIDS, CHROMOSOMES

Abstract

We report the construction of intP1 and intFs strains, in which the basic replicon from either plasmid P1 or plasmid F (oriS) has been integrated in both orientations into the origin of replication, oriC, of the Escherichia coli chromosome. In these strains, oriC is no longer functional and chromosome-replication is instead controlled by the integrated plasmid replicon. The strains were viable, showing that the deviation from normal chromosome-replication control was not large enough to prohibit cell survival. The strains showed a broader cell-size distribution than a wild-type strain and were more filamentous in rich than in minimal media, although cells of wild-type size were also present. Celts which contained aberrantly shaped or aberrantly distributed nucleoids were also observed. Marker-frequency analysis indicated that chromosome replication was predominantly bidirectional in both intFs strains. In the intP1 strains, the degree of bidirectionality depended upon the orientation of the integrated replicon. [ABSTRACT FROM AUTHOR]

Published

1996

183. The Escherichia coli enzoskeleton.

Author

Norris, Vic, Turnock, Geoff, and Sigee, Dave

Subjects

CELL membranes, CYTOPLASM, PROTOPLASM, LIPIDS, MEMBRANE proteins, CELL cycle

Abstract

The nature of the structure of the bacterial cell is becoming clearer. The envelope contains periseptal annuli, a discontinuous periplasm and adhesion sites, whilst the cytoplasmic membrane is probably organized into distinct proteolipid domains by the coupled transcription-translation-insertion (transertion) of membrane proteins. The structure of the nucleoid is determined by proteins which self-associate and by attachment to membrane, which is achieved in part by transertion. Metabolic pathways form multi-enzyme complexes which channel substrates and which connect membranes and nucleic acids to create the extensive, cross-linked, intracellular structure we term the 'nzoskeleton'. This enzoskeleton includes eukaryotic-like cytoskeletal structures and elements such as the MukB and FtsZ proteins. We propose that the enzoskeleton is regulated by calcium and by protein phosphorylation during adaptation to different environments and during the cell cycle. [ABSTRACT FROM AUTHOR]

Published

1996

184. EGTA induces the synthesis in <em>Escherichia coli</em> of three proteins that cross-react with calmodulin antibodies.

Author

Laoudj, Dalila, Andersen, Catherine L., Bras, Ana, Goldberg, Martin, Jacq, Annick, and Holland, I. Barry

Subjects

ESCHERICHIA coli, VERAPAMIL, ELECTROPHORESIS, PEPTIDE hormones, CELLS

Abstract

Escherichia coli mutants, (verA, dilA) specifically resistant to the Ca2+ channel inhibitors verapamil and diltiazem, respectively, are hypersensitive to EGTA and BAPTA. We have shown, using 1-D and 2-D gel electrophoresis, that the synthesis of at least 25 polypeptides in the mutants was enhanced by treatment with Ca2+ chelators and the synthesis of at least 11 polypeptides was repressed. This pattern of induction was not observed in heat- or SDS-treated cells and therefore does not appear to be a general stress response. The majority of the induced proteins are low molecular weight, extremely heat stable and acidic, characteristic properties of caimodulin. Moreover, of the major induced species, three with apparent molecular masses of 12, 18, and 34kDa all cross-reacted with polydonal and monoclonal anti-bodies to eukaryote calmodulins or calerythrin, a heat-resistant Ca2+-binding protein from Saccharo-polyspora erythraea. The verA, dilA mutants. In being hypersensitive to EGTA and to the Ca2+ ionophore A23187 + Ca2+, may be defective in the regulation of the level of free intracellular Ca2+. [ABSTRACT FROM AUTHOR]

Published

1994

185. Correlation of gene transcription with the time of initiation of chromosome replication in Escherichia coli.

Author

Theisen, Patrick W., Grimwade, Julia E., Leonard, Alan C., Bogan, Joseph A., and Helmstetter, Charles E.

Subjects

GENETIC transcription, ESCHERICHIA coli, CHROMOSOME replication, CHROMOSOMES, NUCLEOTIDE sequence

Abstract

Transcriptional levels of the Escherichia coli mioC and gidA genes, which flank the chromosomal origin of replication (oriC) and the dnaA gene, were correlated with the time of initiation of chromosome replication. The transcripts were measured either in dnaC2(ts) mutants that had been aligned for initiation of chromosome replication by a temperature shift or in synchronous cultures of cells obtained using the baby machine technique. In both types of experiments, mioC transcription was inhibited prior to initiation of chromosome replication and resumed several minutes after initiation. Conversely, gidA and dnaA transcription were both inhibited after initiation of replication, coincident with the period of hemimethylation of oriC DNA. It is proposed that mioC transcription prevents initiation of chromosome replication, and must terminate before replication can begin. It is further proposed that the eclipse period between rounds of replication, i.e. the minimum interval between successive initiations, encompasses the time required to methylate GATC sequences in newly replicated oriC plus the time required to terminate mioC transcription. Conversely, the active transcription of gidA and dna prior to initiation is consistent with their positive effects on initiation, and their shutdown after initiation could serve to limit premature reinitiation. [ABSTRACT FROM AUTHOR]

Published

1993

186. Cell division in Escherichia coli minB mutants.

Author

Akerlund, Thomas, Bernander, Rolf, and Nordström, Kurt

Subjects

ESCHERICHIA coli, CELL division, CELLS, GENETIC mutation, CHROMOSOMES

Abstract

In Escherichia coli minB mutants, cell division can take place at the cell poles as well as non-polarly in the cell. We have examined growth, division patterns, and nucleoid distribution in individual cells of a minC point mutant and a minBdeletion mutant, and compared them to the corresponding wild-type strain and an intR1 strain in which the chromosome is over-replicated. The main findings were as follows. In the minBmutants, polar and non-polar divisions appeared to occur independently of each other. Furthermore, the timing of cell division in the cell cycle was found to be severely affected. In addition, nucleold conformation and distribution were considerably disturbed. The results obtained call for a reevaluation of the role of the MinB system in the E. coli cell cycle, and of the concept that limiting quanta of cell division factors are regularly produced during the cell cycle. [ABSTRACT FROM AUTHOR]

Published

1992

187. Escherichia coli prlC Gene Encodes a Trypsin-Like Proteinase Regulating the Cell Cycle.

Author

Jiang, Xueyuan, Zhang, Minyue, Ding, Yi, Yao, Jun, Chen, Hao, Zhu, Dexu, and Muramatu, Mutumi

Subjects

ESCHERICHIA coli, FOODBORNE diseases, AMINO acids, MOLECULAR weights, PROTEINASES

Abstract

Proteinase In has previously been described as displaying a trypsin-like proteinase activity that momentarily appears immediately before DNA synthesis in the cell cycle of Escherichia coli synchronized by phosphate starvation and which is closely related to the initiation of DNA replication [Kato, M., Irisawa, T., Ohtani, M., and Muramatu, M. (1992) Eur. J. Biochem. 210, 1007–1014]. We purified the proteinase In from E. coli C600 and found that the 15 amino acid residues of its amino-terminal were identical with those of oligopeptidase A (OpdA), the product of the E. coli prIC gene. The purified proteinase had a molecular mass of approximately 67 kDa, which was also the same as that of oligopeptidase A. To further elucidate the relationship between proteinase in and oligopeptidase A, we assembled an expression vector to direct the synthesis of E. coli oligopeptidase A. The protein was expressed at a high level in E. coli BL21(DE3) and was produced mostly in the soluble, active form. Both the recombinant enzyme (rPrlC) and the purified proteinase In could hydrolyze trypsin substrates for proteinase In as well as benzyloxycarbonyl AlaAla-Leu p-nitroanilide (Z-AALpNA), described as a synthetic substrate for oligopeptidase A. The effects of various protease inhibitors on rPrlC were also very similar to those on proteinase in. The trypsin inhibitors 4-guanidino benzoic acid 4-tert-butylphenyl ester and antipain strongly inhibited the trypsin-like proteinase activity of the recombinant enzyme, but had no effect on its Z-AALpNA hydrolyzing activity. Cobalt ion, which greatly enhanced the OpdA activity, slightly inhibited the trypsin-like activity of the recombinant enzyme. These results strongly suggest that proteinase in is encoded by the E. coli prlC gene and is a multi-functional proteinase with two separate active sites. [ABSTRACT FROM AUTHOR]

Published

1998

188. A second gene for Type I signal peptidase in Bradyrhizobium japonicum, sipF, is located near genes involved in RNA processing and cell division.

Author

Bairl, A. and Müller, P.

Abstract

The Tn phoA-induced Bradyrhizobium japonicum mutant 184 shows slow growth and aberrant colonization of soybean nodules. Using a DNA fragment adjacent to the transposon insertion site as a probe, a 3.4-kb BglII fragment of B. japonicum 110 spc4 DNA was identified and cloned. Sequence analysis indicated that two truncated ORFs and three complete ORFs were encoded on this fragment. A database search revealed homologies to several other prokaryotic proteins: PdxJ (an enzyme involved in vitamin B6 biosynthesis), AcpS (acyl carrier protein synthase), Lep or Sip (prokaryotic type I signal peptidase), RNase III (an endoribonuclease which processes double-stranded rRNA precursors and mRNA) and Era (a GTP-binding protein required for cell division). The mutation in strain 184 was found to lie within the signal peptidase gene, which was designated sipF. Therefore, sipF is located in a region that encodes gene products involved in posttranscriptional and posttranslational processing processes. By complementation of the lepts E. coli mutant strain IT41 it was demonstrated that sipF indeed encodes a functional signal peptidase, and genetic complementation of B. japonicum mutant 184 by a 2.8-kb SalI fragment indicated that sipF is expressed from a promoter located directly upstream of sipF. Using a non-polar kanamycin resistance cassette, a specific sipF– mutant was constructed which exhibited defects in symbiosis similar to those of the original mutant 184. [ABSTRACT FROM AUTHOR]

Published

1998

189. Increased sensitivity of E. coli to novobiocin, EDTA and the anticalmodulin drug W7 following overproduction of DjlA requires a functional transmembrane domain.

Author

Bernard, S., Clarke, D. J., Chen, M. X., Holland, I. B., and Jacq, A.

Abstract

In earlier studies we found that E. coli is sensitive to anticalmodulin drugs such as W7. Mutants that are resistant to this drug were isolated, including wseA1. In an attempt to clone the wseA gene, we isolated a clone that restored sensitivity to the drug in the mutant. We found that this clone in fact suppresses W7 resistance through expression of djlA, which encodes a novel DnaJ-like protein. It was found previously that overproduction of DjlA could induce capsule synthesis via activation of the two-component regulatory pathway RcsC/B. In addition to suppression of wseA1, djlA overexpression increases the sensitivity of cells to EDTA and novobiocin, but not to other drugs tested. Although overexpression of a form of the protein carrying a mutation in, or lacking, the J-region of DjlA also led to increased sensitivity, indicating that the chaperone activity of this protein was not strictly required, the full-length, wild- type protein had a more pronounced effect. In contrast, a point mutation which affects the function of the transmembrane domain but not the localisation or stability of DjlA abolished the effects of DjlA overproduction. [ABSTRACT FROM AUTHOR]

Published

1998

190. Does replication-induced transcription regulate synthesis of the myriad low copy number proteins of Escherichia coli?

Author

Guptasarma, Purnananda

Published

1995

191. Overview of controls in the Escherichia coli cell cycle.

Author

Vinella, Daniel and D'Ari, Richard

Published

1995

192. ppGpp-mediated regulation of DNA replication and cell division in Escherichia coli.

Author

Schreiber, Gideon, Ron, Eliora, and Glaser, Gad

Abstract

ppGpp serves as an alarmon in prokaryotes, distributing and coordinating different cellular processes according to the nutritional potential of the growth medium. This work is interpreted as favoring the view that, in addition to its previously documented role in regulating the rate of ribosome synthesis [4], ppGpp participates in coordinating DNA replication and cell division. We studied the effects of ppGpp on the cell division cycle, using cells containing plasmid pSM11 that codes for the 55-kDa truncated RelA protein under the inducible Ptac promoter. In this system it was found that the rate of initiation of new rounds of DNA replication is inversely correlated with the intracellular level of ppGpp. Furthermore, ppGpp levels similar to those found during the activation of stringent control inhibited replication initiation, in a manner comparable to that resulting from inhibition of protein synthesis by amino acid starvation or by chloramphenicol addition. However, in contrast to chloramphenicol treatment, elevated ppGpp levels did not block septum formation, and, in fact, there is some evidence for enhanced septation. As a result, the residual cell division following elevation in ppGpp levels was higher than after chloramphenicol treatment, resulting in cells with a size similar to that of stationary phase cells. [ABSTRACT FROM AUTHOR]

Published

1995

193. Molecular cloning of the EnvC gene of Escherichia coli.

Author

Robert Klein, Jürgen, Henrich, Bernhard, and Plapp, Roland

Abstract

DNA fragments complementing the envC mutation could be isolated by cloning chromosomal DNA in the vector pUH84. When the frequencies of transformation and the frequencies of restoring the envC phenotype were compared, the high copy number hybrid plasmids complemented with a frequency of 10. After subcloning the envC-complementing DNA fragment into the low copy number plasmid pLG339, efficient complementation was achieved by spontaneous integration of the IS2 element of Escherichia coli. By nucleotide sequence analysis, a potential promoter, a ribosome-binding site, and an unidentified reading frame were detected in the respective DNA fragment. [ABSTRACT FROM AUTHOR]

Published

1990

194. The cell cycle of Escherichia coli.

Author

Donachie, William D.

Subjects

ESCHERICHIA coli, CELL cycle

Abstract

Studies the cell cycle of Escherichia coli. Modeling initiation control; Proteins controlling initiation; Other factors that influence initiation timing; Process of partition; Partition mutants; Cytokinesis; Septation; Septum splitting and the completion of division; Regulating cell-division proteins; Timing and localization of division; Housekeeping proteins that are essential for cell division; Intrinsic division inhibitors.

Published

1993

195. Bacterial chromosomes.

Published

1995

196. Cell elongation and septation are two mutually exclusive processes in Escherichia coli.

Author

Canepari, P., Signoretto, Caterina, Boaretti, Marzia, and Lleò, Maria Del Mar

Abstract

Bacterial rod morphogenesis was studied in synchronously growing cells of Escherichia coli C600 during the reshaping process that follows the removal of mecillinam, a β-lactam antibiotic that specifically inhibits lateral wall formation of gram-negative rods and causes transition to coccal shape. Removal of mecillinam after 30 min of action did not affect the timing of subsequent cell division, but removal after 50 min delayed resumption of cell division for approximately one generation time. In order to study the interplay between lateral wall elongation and septum formation in determining and maintaining the bacterial rod shape, we evaluated the effect of re-adding mecillinam or of adding aztreonam (a specific inhibitor of septum formation) at various stages of the reshaping process. We conclude that mecillinam was active only during the reshaping process, while aztreonam was active only later when the cells were close to dividing again. These results provide further evidence for our previous proposal according to which elongation and septation are two alternating and competing events of the cell cycle and are linked to each other to force bacterial rods to grow to a given length. [ABSTRACT FROM AUTHOR]

Published

1997

197. The cell cycle of Bacillus subtilis as studied by electron microscopy.

Author

Nanninga, N., Koppes, L., and Vries-Tijssen, F.

Abstract

Bacillus subtilis strain Marburg was grown exponentially with a doubling time of 65 min. To follow the time course of various cell cycle events, cells were collected by agar filtration and were then classified according to length. The DNA replication cycle was determined by a quantitative analysis of radioautograms of tritiated thymidine pulse labeled cells. The DNA replication period was found to be 45 min. This period is preceded and followed by periods without DNA synthesis of about 10 min. The morphology and segregation of nucleoplasmic bodies was studied in thin sections. B. subtilis contains two sets of genomes. DNA replication and DNA segregation seem to go hand in hand and DNA segregation is completed shortly after termination of DNA replication. Cell division and cell separation were investigated in whole mount preparations (agar filtration) and in thin sections. Cell division starts about 20 min after cell birth; cell separation starts at about 45 min and before completion of the septum. [ABSTRACT FROM AUTHOR]

Published

1979

198. Resistance to trifluoroperazine, a calmodulin inhibitor, maps to the fabD locus in Escherichia coli.

Author

Bouquin, Nicolas, Tempete, Marc, Barry Holland, I., and Séror, Simone

Published

1995

199. Two pathways of division inhibition in UV-irradiated E. coli.

Author

Burton, Paul and Holland, I.

Published

1983

200. Coordination of Growth, Chromosome Replication/Segregation, and Cell Division in E. coli

Author

Mathieu Stouf, Nancy Kleckner, Martin White, Jay K. Fisher, and Katerina E. Chatzi

Subjects

0301 basic medicine, Microbiology (medical), cell division, licensing, Cell division, lcsh:QR1-502, Review, Biology, Permission, DNA replication, Microbiology, lcsh:Microbiology, Chromosome segregation, 03 medical and health sciences, 0302 clinical medicine, Nucleoid, chromosome, bacteria, E. coli, Chromosome, Cell cycle, Cell biology, 030104 developmental biology, Replication Initiation, cell cycle coordination, 030217 neurology & neurosurgery

Abstract

Bacterial cells growing in steady state maintain a 1:1:1 relationship between an appropriate mass increase, a round of DNA replication plus sister chromosome segregation, and cell division. This is accomplished without the cell cycle engine found in eukaryotic cells. We propose here a formal logic, and an accompanying mechanism, for how such coordination could be provided in E. coli. Completion of chromosomal and divisome-related events would lead, interactively, to a “progression control complex” (PCC) which provides integrated physical coupling between sister terminus regions and the nascent septum. When a cell has both (i) achieved a sufficient mass increase, and (ii) the PCC has developed, a conformational change in the PCC occurs. This change results in “progression permission,” which triggers both onset of cell division and release of terminus regions. Release of the terminus region, in turn, directly enables a next round of replication initiation via physical changes transmitted through the nucleoid. Division and initiation are then implemented, each at its own rate and timing, according to conditions present. Importantly: (i) the limiting step for progression permission may be either completion of the growth requirement or the chromosome/divisome processes required for assembly of the PCC; and, (ii) the outcome of the proposed process is granting of permission to progress, not determination of the absolute or relative timings of downstream events. This basic logic, and the accompanying mechanism, can explain coordination of events in both slow and fast growth conditions; can accommodate diverse variations and perturbations of cellular events; and is compatible with existing mathematical descriptions of the E. coli cell cycle. Also, while our proposition is specifically designed to provide 1:1:1 coordination among basic events on a “per-cell cycle” basis, it is a small step to further envision permission progression is also the target of basic growth rate control. In such a case, the rate of mass accumulation (or its equivalent) would determine the length of the interval between successive permission events and, thus, successive cell divisions and successive replication initiations.

Published

2018