Your search keyword '"Court, Donald L."' showing total 57 results

1. Evidence that bacteriophage λ lysogens may induce in response to the proton motive force uncoupler CCCP.

Author

Thomason, Lynn C. and Court, Donald L.

Subjects

*BACTERIOPHAGES, *HYDRAZINE, *OXIDATIVE phosphorylation, *PROMOTERS (Genetics), *BACTERIAL promoters

Abstract

We describe a genetic β-galactoside reporter system using a disk diffusion assay on MacConkey Lactose agar petri plates to monitor maintenance of the bacteriophage λ prophage state and viral induction in Escherichia coli K-12. Evidence is presented that the phage λ major lytic promoters, pL and pR, are activated when cells containing the reporters are exposed to the energy poison carbonyl cyanide m-chlorophenyl hydrazine, CCCP. This uncoupler of oxidative phosphorylation inhibits ATP synthesis by collapsing the proton motive force. Expression of the λ lytic promoters in response to CCCP requires host RecA function and an autocleavable CI repressor, as does SOS induction of the λ prophage that occurs by a DNA damage-dependent pathway. λ Cro function is required for CCCP-mediated activation of the λ lytic promoters. CCCP does not induce an sfi-lacZ SOS reporter. [ABSTRACT FROM AUTHOR]

Published

2016

2. RNase III: Genetics and Function; Structure and Mechanism.

Author

Court, Donald L., Gan, Jianhua, Liang, Yu-He, Shaw, Gary X., Tropea, Joseph E., Costantino, Nina, Waugh, David S., and Ji, Xinhua

Subjects

*RIBONUCLEASES, *MOLECULAR structure, *DOUBLE-stranded RNA, *GENE expression, *BACTERIAL growth, *RIBOSOMAL RNA, *ESCHERICHIA coli

Abstract

RNase III is a global regulator of gene expression in Escherichia coli that is instrumental in the maturation of ribosomal and other structural RNAs. We examine here how RNase III itself is regulated in response to growth and other environmental changes encountered by the cell and how, by binding or processing double-stranded RNA (dsRNA) intermediates, RNase III controls the expression of genes. Recent insight into the mechanism of dsRNA binding and processing, gained from structural studies of RNase III, is reviewed. Structural studies also reveal new cleavage sites in the enzyme that can generate longer 3′ overhangs. [ABSTRACT FROM AUTHOR]

Published

2013

3. Nus transcription elongation factors and RNase III modulate small ribosome subunit biogenesis in Escherichia coli.

Author

Bubunenko, Mikhail, Court, Donald L., Al Refaii, Abdalla, Saxena, Shivalika, Korepanov, Alexey, Friedman, David I., Gottesman, Max E., and Alix, Jean‐Hervé

Subjects

*ESCHERICHIA coli, *RIBOSOMAL RNA, *GENETIC transcription, *RNA polymerases, *PROTEINS

Abstract

Escherichia coli NusA and NusB proteins bind specific sites, such as those in the leader and spacer sequences that flank the 16 S region of the ribosomal RNA transcript, forming a complex with RNA polymerase that suppresses Rho-dependent transcription termination. Although antitermination has long been the accepted role for Nus factors in rRNA synthesis, we propose that another major role for the Nus-modified transcription complex in rrn operons is as an RNA chaperone insuring co-ordination of 16 S rRNA folding and RNase III processing that results in production of proper 30 S ribosome subunits. This contrarian proposal is based on our studies of nusA and nusB cold-sensitive mutations that have altered translation and at low temperature accumulate 30 S subunit precursors. Both phenotypes are suppressed by deletion of RNase III. We argue that these results are consistent with the idea that the nus mutations cause altered rRNA folding that leads to abnormal 30 S subunits and slow translation. According to this idea, functional Nus proteins stabilize an RNA loop between their binding sites in the 5′ RNA leader and on the transcribing RNA polymerase, providing a topological constraint on the RNA that aids normal rRNA folding and processing. [ABSTRACT FROM AUTHOR]

Published

2013

4. Identification of the Escherichia coli K-12 ybhE Gene as pgl, Encoding 6-Phosphogluconolactonase.

Author

Thomason, Lynn C., Court, Donald L., Datta, Atin R., Khanna, Rita, and Rosner, Judah L.

Subjects

*ESCHERICHIA coli, *ESCHERICHIA, *GENES, *PROTEINS, *ENZYMES, *PHENOTYPES

Abstract

We report identification of the Escherichia coli ybhE gene as the pg1 gene that encodes 6-phosphoglucono- lactonase. A tentative identification was first made based on the known approximate location of the pg1 gene and the similarity of the presumptive ybhE-encoded protein sequence to a known Pgl enzyme. To test this notion, the ybhE gene was deleted and replaced with a drug marker. Like previously characterized pg1 mutants, the ybhE deletion mutant had a Blu- phenotype (dark-blue staining with iodine due to accumulation of starch after growth on minimal maltose) and demonstrated impaired growth on minimal glucose medium when combined with a pgi mutation. Biochemical assay of crude extracts for 6-phosphogluconolactonase enzymatic activity showed that ybhE encodes this activity. The ybhE gene was transferred from the E. coli chromosome to an expression vector. This ybhE clone complemented both the precise deletion of the ybhE gene and a larger deletion, pglΔ8, for the Blu- phenotype and for phosphogluconolactonase activity, confirming that ybhE is the pg1 gene. A newly observed phenotype of pg1 strains is a lowered frequency of appearance of Bgl+ mutants that can utilize the β-glucoside salicin. This is likely due to poor growth of Bgl+ pg1 strains on salicin due to the accumulation of 6-phosphogluconolactone. [ABSTRACT FROM AUTHOR]

Published

2004

5. Enhanced levels of Red-mediated recombinants in mismatch repair mutants.

Author

Costantino, Nina and Court, Donald L.

Subjects

*ESCHERICHIA coli, *HOMOLOGY (Biology), *EPISOMES, *RECOMBINANT DNA, *GENES, *BACTERIOPHAGES, *CHROMOSOMES

Abstract

Homologous recombination can be used to generate recombinants on episomes or directly on the Escherichia coli chromosome with PCR products or synthetic single-stranded DNA (ssDNA) oligonucleotides (oligos). Such recombination is possible because bacteriophage A-encoded functions, called Red, efficiently recombine linear DNA with homologies as short as 20-70 bases. This technology, termed recombineering, provides ways to modify genes and segments of the chromosome as well as to study homologous recombination mechanisms. The Red Beta function, which binds and anneals ssDNA to complementary ssDNA, is able to recombine 70-base oligos with the chromosome. In E. coil, methyl-directed mismatch repair (MMR) can affect these ssDNA recombination events by eliminating the recombinant allele and restoring the original sequence. In so doing, MMR can reduce the apparent recombination frequency by >100-fold. In the absence of MMR, Red-mediated oligo recombination can incorporate a single base change into the chromosome in an unprecedented 25% of cells surviving electroporation. Our results show that Beta is the only bacteriophage function required for this level of recombination and suggest that Beta directs the ssDNA to the replication fork as it passes the target sequence. [ABSTRACT FROM AUTHOR]

Published

2003

6. Mini-λ: a tractable system for chromosome and BAC engineering

Author

Court, Donald L., Swaminathan, Srividya, Yu, Daiguan, Wilson, Helen, Baker, Teresa, Bubunenko, Mikail, Sawitzke, James, and Sharan, Shyam K.

Subjects

*BACTERIOPHAGES, *CHROMOSOMES, *MOLECULAR cloning

Abstract

The bacteriophage lambda (λ) recombination system Red has been used for engineering large DNA fragments cloned into P1 and bacterial artificial chromosomes (BAC or PAC) vectors. So far, this recombination system has been utilized by transferring the BAC or PAC clones into bacterial cells that harbor a defective λ prophage. Here we describe the generation of a mini-λ DNA that can provide the Red recombination functions and can be easily introduced by electroporation into any E. coli strain, including the DH10B-carrying BACs or PACs. The mini-λ DNA integrates into the bacterial chromosome as a defective prophage. In addition, since it retains attachment sites, it can be excised out to cure the cells of the phage DNA. We describe here the use of the mini-λ recombination system for BAC modification by introducing a selectable marker into the vector sequence of a BAC clone. In addition, using the mini-λ, we create a single missense mutation in the human BRCA2 gene cloned in a BAC without the use of any selectable marker. The ability to generate recombinants very efficiently demonstrates the usefulness of the mini-λ as a very simple mobile system for in vivo genome engineering by homologous recombination, a process named recombineering. [Copyright &y& Elsevier]

Published

2003

7. GENETIC ENGINEERING USING HOMOLOGOUS RECOMBINATION.

Author

Court, Donald L., Sawitzke, James A., and Thomason, Lynn C.

Subjects

*GENETIC engineering, *HOMOLOGY (Biology), *GENETIC recombination

Abstract

In the past few years, in vivo technologies have emerged that, due to their efficiency and simplicity, may one day replace standard genetic engineering techniques. Constructs can be made on plasmids or directly on the Escherichia coli chromosome from PCR products or synthetic oligonucleotides by homologous recombination. This is possible because bacteriophage-encoded recombination functions efficiently recombine sequences with homologies as short as 35 to 50 base pairs. This technology, termed recombineering, is providing new ways to modify genes and segments of the chromosome. This review describes not only recombineering and its applications, but also summarizes homologous recombination in E. coli and early uses of homologous recombination to modify the bacterial chromosome. Finally, based on the premise that phage-mediated recombination functions act at replication forks, specific molecular models are proposed. [ABSTRACT FROM AUTHOR]

Published

2002

8. Crystal structure of ERA: A GTPase-dependent cell cycle regulator containing an RNA binding motif.

Author

Chen, Xin and Court, Donald L.

Subjects

*ESCHERICHIA coli, *DIME, *CRYSTALLIZATION

Abstract

Studies the crystal structure of ERA from Escherichia coli. Crystallization of the protein; X-ray data collection and processing; Overall structure and domain interactions; Crystal packing and dimerization; Results and discussion.

Published

1999

9. Transcription termination signals in the nin region of bacteriophage lambda: Identification of...

Author

Cheng, Sheau-wei C. and Court, Donald L.

Subjects

*BACTERIOPHAGE lambda, *GENETIC transcription, *GENETICS

Abstract

Suggests that the 3-kb nin region of bacteriophage lambda, located between genes P and Q contains transcription termination signals as well as 10 open reading frames. Effect of nin region deletions; Transcription termination activity of the roc region; Roc region features.

Published

1995

10. Control of ftsZ expression, cell division, and glutamine metabolism in Luria-Bertani (LB) medium...

Author

Powell, Bradford S. and Court, Donald L.

Subjects

*GLUTAMINE

Abstract

Studies the importance of supplying glutamine in cells grown in Luria-Bertani medium. Information on cell division; Detailed information on the Alarmone ppGpp in Escherichia coli; Reference to the global effects of the ppGpp-induced state; Role of the ppGpp in the regulation of glutamine metabolism; Methodology used in the study; Findings of the study.

Published

1998

11. Structural and functional analyses of the transcription-translation proteins NusB and NusE.

Author

Court, Donald L. and Patterson, Thomas A.

Subjects

*GENETIC regulation, *GENETIC mutation

Abstract

Describes the structural and functional analyses of the transcription-translation proteins NusB and NusE. Identification of mutations in nus genes that influence N antitermination without affecting bacterial viability; Determination of the sequence changes of the nusB5 and nusE71 mutations.

Published

1995

12. Amos Oppenheim (31 October 1934 to 24 September 2006).

Author

Adhya, Sankar L., Court, Donald L., Friedman, David I., and Gottesman, Max E.

Subjects

*EDUCATORS

Abstract

The article presents an obituary for educator Amos Oppenheim.

Published

2008

13. Role of an RNase III Binding Site in Transcription Termination at nutL by HK022 Nun Protein.

Author

Washburn, Robert S., Court, Donald L., and Gottesman, Max E.

Subjects

*BACTERIOPHAGES, *PROTEINS, *NUCLEOTIDES, *CELLS, *RIBONUCLEASES

Abstract

The phage HK022 Nun protein excludes phage λ by binding nascent λ pL and pR transcripts at nutL and nutR, respectively, and inducing transcription termination just downstream of these sites. Termination is more efficient at nutL than at nutR. One difference between nutL and nutR is the presence of RNase III processing sites (rIII) located immediately promoter distal to λ nutL. We found that deletion of rIII dramatically reduced Nun transcription arrest in vitro but had little effect on termination in vivo. However, consistent with the in vitro results, overexpression of a transcript carrying nutL and rIII efficiently titrated Nun, allowing λ to grow on a strain that expressed Nun, whereas a transcript carrying only nutL or nutL-rIII with nucleotides 97 to 141 deleted was ineffective. Rnc70, an RNase III mutant that binds but does not cleave rIII, also prevented Nun-mediated λ exclusion. We propose that rIII enhances the on-rate of Nun at nutL, stimulating Nun-mediated arrest in vitro. We have shown that a specific element in rIII, i.e., box C (G89GUGUGUG), strongly enhances arrest on rIII+ templates. Nun-rIII interactions do not stimulate Nun termination in vivo, presumably because formation of the Nun-nutL complex is normally not rate-limiting in the cell. In contrast to Nun, N is not occluded by Rnc70 and is not efficiently titrated by a nutL-rIII transcript. [ABSTRACT FROM AUTHOR]

Published

2006

14. Bacteriophage λ RexA and RexB functions assist the transition from lysogeny to lytic growth.

Author

Thomason, Lynn C., Schiltz, Carl J., Court, Carolyn, Hosford, Christopher J., Adams, Myfanwy C., Chappie, Joshua S., and Court, Donald L.

Subjects

*LYSOGENY, *DNA replication, *REPORTER genes, *BACTERIOPHAGES

Abstract

The CI and Cro repressors of bacteriophage λ create a bistable switch between lysogenic and lytic growth. In λ lysogens, CI repressor expressed from the PRM promoter blocks expression of the lytic promoters PL and PR to allow stable maintenance of the lysogenic state. When lysogens are induced, CI repressor is inactivated and Cro repressor is expressed from the lytic PR promoter. Cro repressor blocks PRM transcription and CI repressor synthesis to ensure that the lytic state proceeds. RexA and RexB proteins, like CI, are expressed from the PRM promoter in λ lysogens; RexB is also expressed from a second promoter, PLIT, embedded in rexA. Here we show that RexA binds CI repressor and assists the transition from lysogenic to lytic growth, using both intact lysogens and defective prophages with reporter genes under the control of the lytic PL and PR promoters. Once lytic growth begins, if the bistable switch does return to the immune state, RexA expression lessens the probability that it will remain there, thus stabilizing the lytic state and activation of the lytic PL and PR promoters. RexB modulates the effect of RexA and may also help establish phage DNA replication as lytic growth ensues. [ABSTRACT FROM AUTHOR]

Published

2021

15. A set of recombineering plasmids for gram-negative bacteria

Author

Datta, Simanti, Costantino, Nina, and Court, Donald L.

Subjects

*GRAM-negative bacteria, *PLASMIDS, *CHLORAMPHENICOL, *DNA polymerases

Abstract

Abstract: We have constructed a set of plasmids that can be used to express recombineering functions in some gram-negative bacteria, thereby facilitating in vivo genetic manipulations. These plasmids include an origin of replication and a segment of the bacteriophage λ genome comprising the red genes (exo, bet and gam) under their native control. These constructs do not require the anti-termination event normally required for Red expression, making their application more likely in divergent species. Some of the plasmids have temperature-sensitive replicons to simplify curing. In creating these vectors we developed two useful recombineering applications. Any gene linked to a drug marker can be retrieved by gap-repair using only a plasmid origin and target homologies. A plasmid origin of replication can be changed to a different origin by targeted replacement, to potentially alter its copy number and host range. Both these techniques will prove useful for manipulation of plasmids in vivo. Most of the Red plasmid constructs catalyzed efficient recombination in E. coli with a low level of uninduced background recombination. These Red plasmids have been successfully tested in Salmonella, and we anticipate that that they will provide efficient recombination in other related gram-negative bacteria. [Copyright &y& Elsevier]

Published

2006

16. On the role of Cro in &lamda; prophage induction.

Author

Svenningsen, Sine L., Costantino, Nina, Court, Donald L., and Adhya, Sankar

Subjects

*NUCLEIC acids, *DNA damage, *BIOCHEMICAL genetics, *BACTERIAL genetics, *BIOMOLECULES, *PROTEINS

Abstract

The lysogenic state of bacteriophage A is exceptionally stable yet the prophage is readily induced in response to DNA damage. This delicate epigenetic switch is believed to be regulated by two proteins; the lysogenic maintenance promoting protein Cl and the early lytic protein Cro. First, we confirm, in the native configuration, the previous observation that the DNA loop mediated by oligomerization of Cl bound to two distinct operator regions (OL and OR), increases repression of the early lytic promoters and is important for stable maintenance of lysogeny. Second, we show that the presence of the cro gene might be unimportant for the lysogenic to lytic switch during induction of the A prophage. We revisit the idea that Cro's primary role in induction is instead to mediate weak repression of the early lytic promoters. [ABSTRACT FROM AUTHOR]

Published

2005

17. MOUSE GENOMIC TECHNOLOGIES: RECOMBINEERING: A POWERFUL NEW TOOL FOR MOUSE FUNCTIONAL GENOMICS.

Author

Copeland, Neal G., Jenkins, Nancy A., and Court, Donald L.

Subjects

*GENETIC recombination, *GENOMICS, *MOLECULAR genetics, *GENOMES, *ESCHERICHIA coli, *ESCHERICHIA, *MICE

Abstract

Highly efficient phage-based Escherichia coli homologous recombination systems have recently been developed that enable genomic DNA in bacterial artificial chromosomes to be modified and subcloned, without the need for restriction enzymes or DNA ligases. This new form of chromosome engineering, termed recombinogenic engineering or recombineering, is efficient and greatly decreases the time it takes to create transgenic mouse models by traditional means. Recombineering also facilitates many kinds of genomic experiment that have otherwise been difficult to carry out, and should enhance functional genomic studies by providing better mouse models and a more refined genetic analysis of the mouse genome. [ABSTRACT FROM AUTHOR]

Published

2001

18. Elements in the λ immunity region regulate phage development: beyond the 'Genetic Switch'.

Author

Thomason, Lynn C., Morrill, Kathleen, Murray, Gillian, Court, Carolyn, Shafer, Brenda, Schneider, Thomas D., and Court, Donald L.

Subjects

*BACTERIAL proteins, *BACTERIOPHAGES, *IMMUNITY, *DNA damage, *ESCHERICHIA coli

Abstract

Summary: Genetic elements in the bacteriophage λ immunity region contribute to stable maintenance and synchronous induction of the integrated Escherichia coli prophage. There is a bistable switch between lysogenic and lytic growth that is orchestrated by the CI and Cro repressors acting on the lytic (PL and PR) and lysogenic (PRM) promoters, referred to as the Genetic Switch. Other less well‐characterized elements in the phage immunity region include the PLIT promoter and the immunity terminator, TIMM. The PLIT promoter is repressed by the bacterial LexA protein in λ lysogens. LexA repressor, like the λ CI repressor, is inactivated during the SOS response to DNA damage, and this regulation ensures that the PLIT promoter and the lytic PL and PR promoters are synchronously activated. Proper RexA and RexB protein levels are critical for the switch from lysogeny to lytic growth. Mutation of PLIT reduces RexB levels relative to RexA, compromising cellular energetics and causing a 10‐fold reduction in lytic phage yield. The RexA and RexB proteins interact with themselves and each other in a bacterial two‐hybrid system. We also find that the transcription terminator, TIMM, is a Rho‐independent, intrinsic terminator. Inactivation of TIMM has minimal effect on λ lysogenization or prophage induction. [ABSTRACT FROM AUTHOR]

Published

2019

19. Requirement for NusG for Transcription Antitermination In Vivo by the λ N Protein.

Author

Ying Zhou, Filter, Joshua J., Court, Donald L., Gottesman, Max E., and Friedman, David I.

Subjects

*GENETIC transcription, *BACTERIOPHAGES, *ESCHERICHIA coli

Abstract

Examines the activation of transcription antitermination by the bacteriophage N protein by Escherichia coli NusG protein. Properties of NusG proteins; Regulation of Rho-dependent transcription termination; Effect of NusG overexpression on Rho-dependent termination.

Published

2002

20. Escherichia coli transcription factor NusG binds to 70S ribosomes.

Author

Saxena, Shivalika, Myka, Kamila K., Washburn, Robert, Costantino, Nina, Court, Donald L., and Gottesman, Max E.

Subjects

*ESCHERICHIA coli, *TRANSCRIPTION factors, *RIBOSOMES, *GENETIC mutation, *CHLORAMPHENICOL, *PHENOTYPES

Abstract

Summary: Transcription and translation are coupled processes in bacteria. A role of transcription elongation cofactor NusG in coupling has been suggested by in vitro structural studies. NMR revealed association of the NusG carboxy‐terminal domain with S10 (NusE), implying a direct role for NusG as a bridge linking RNAP and the lead ribosome. Here we present the first in vitro and in vivo evidence of full‐length NusG association with mature 70S ribosomes. Binding did not require accessory factors in vitro. Mutating the NusG:S10 binding interface at NusG F165 or NusE M88 and D97 residues weakened NusG:S10 association in vivo and completely abolished it in vitro, supporting the specificity of this interaction. Mutations in the binding interface increased sensitivity to chloramphenicol. This phenotype was suppressed by rpoB*35, an RNAP mutation that reduces replisome‐RNAP clashes. We propose that weakened NusG:S10 interaction leads to uncoupling when translation is inhibited, with resulting RNAP backtracking, replication blocks and formation of lethal DNA double‐strand breaks. [ABSTRACT FROM AUTHOR]

Published

2018

21. A Cre Transcription Fidelity Reporter Identifies GreA as a Major RNA Proofreading Factor in Escherichia coli.

Author

Bubunenko, Mikhail G., Court, Carolyn B., Rattray, Alison J., Gotte, Deanna R., Kireeva, Maria L., Irizarry-Caro, Jorge A., Xintian Li, Jin, Ding J., Court, Donald L., Strathern, Jeffrey N., and Kashlev, Mikhail

Subjects

*BACTERIAL genetics, *ESCHERICHIA coli, *TRANSCRIPTION factors, *REPORTER genes, *RNA polymerases, *GENETIC overexpression

Abstract

We made a coupled genetic reporter that detects rare transcription misincorporation errors to measure RNA polymerase transcription fidelity in Escherichia coli. Using this reporter, we demonstrated in vivo that the transcript cleavage factor GreA, but not GreB, is essential for proofreading of a transcription error where a riboA has been misincorporated instead of a riboG. A greA mutant strain had more than a 100-fold increase in transcription errors relative to wild-type or a greB mutant. However, overexpression of GreB in DgreA cells reduced the misincorporation errors to wild-type levels, demonstrating that GreB at high concentration could substitute for GreA in RNA proofreading activity in vivo. [ABSTRACT FROM AUTHOR]

Published

2017

22. Location of the unique integration site on an Escherichia coli chromosome by bacteriophage lambda DNA in vivo.

Author

Tal, Asaf, Arbel-Goren, Rinat, Costantino, Nina, Court, Donald L., and Stavans, Joel

Subjects

*ESCHERICHIA coli, *CHROMOSOMES, *GENETIC transformation, *BACTERIOPHAGES, *DNA

Abstract

The search for specific sequences on long genomes is a key process in many biological contexts. How can specific target sequences be located with high efficiency, within physiologically relevant times? We addressed this question for viral integration, a fundamental mechanism of horizontal gene transfer driving prokaryotic evolution, using the infection of Escherichia coli bacteria with bacteriophage λ and following the establishment of a lysogenic state. Following the targeting process in individual live £ coli cells in real time revealed that λ DNA remains confined near the entry point of a cell following infection. The encounter between the 15-bp-long target sequence on the chromosome and the recombination site on the viral genome is facilitated by the directed motion of bacterial DNA generated during chromosome replication, in conjunction with constrained diffusion of phage DNA. Moving the native bacterial integration site to different locations on the genome and measuring the integration frequency in these strains reveals that the frequencies of the native site and a site symmetric to it relative to tbe origin are similar, whereas both are significantly higher than when the integration site is moved near the terminus, consistent with the replication-driven mechanism we propose. This novel search mechanism is yet another example of tbe exquisite coevolution of λ with its host. [ABSTRACT FROM AUTHOR]

Published

2014

23. The Kil Peptide of Bacteriophage λ Blocks Escherichia coli Cytokinesis via ZipA-Dependent Inhibition of FtsZ Assembly.

Author

Haeusser, Daniel P., Hoashi, Marina, Weaver, Anna, Brown, Nathan, Pan, James, Sawitzke, James A., Thomason, Lynn C., Court, Donald L., and Margolin, William

Subjects

*PEPTIDES, *BACTERIOPHAGE lambda, *ESCHERICHIA coli, *CYTOKINESIS, *CELL division

Abstract

Assembly of the essential, tubulin-like FtsZ protein into a ring-shaped structure at the nascent division site determines the timing and position of cytokinesis in most bacteria and serves as a scaffold for recruitment of the cell division machinery. Here we report that expression of bacteriophage λ kil, either from a resident phage or from a plasmid, induces filamentation of Escherichia coli cells by rapid inhibition of FtsZ ring formation. Mutant alleles of ftsZ resistant to the Kil protein map to the FtsZ polymer subunit interface, stabilize FtsZ ring assembly, and confer increased resistance to endogenous FtsZ inhibitors, consistent with Kil inhibiting FtsZ assembly. Cells with the normally essential cell division gene zipA deleted (in a modified background) display normal FtsZ rings after kil expression, suggesting that ZipA is required for Kil-mediated inhibition of FtsZ rings in vivo. In support of this model, point mutations in the C-terminal FtsZ-interaction domain of ZipA abrogate Kil activity without discernibly altering FtsZ-ZipA interactions. An affinity-tagged-Kil derivative interacts with both FtsZ and ZipA, and inhibits sedimentation of FtsZ filament bundles in vitro. Together, these data inspire a model in which Kil interacts with FtsZ and ZipA in the cell to prevent FtsZ assembly into a coherent, division-competent ring structure. Phage growth assays show that kil+ phage lyse ∼30% later than kil mutant phage, suggesting that Kil delays lysis, perhaps via its interaction with FtsZ and ZipA. [ABSTRACT FROM AUTHOR]

Published

2014

24. Bacterial DNA polymerases participate in oligonucleotide recombination.

Author

Li, Xin‐tian, Thomason, Lynn C., Sawitzke, James A., Costantino, Nina, and Court, Donald L.

Subjects

*OLIGONUCLEOTIDES, *GENOMICS, *ESCHERICHIA coli, *GENETIC markers

Abstract

Synthetic single-strand oligonucleotides (oligos) with homology to genomic DNA have proved to be highly effective for constructing designed mutations in targeted genomes, a process referred to as recombineering. The cellular functions important for this type of homologous recombination have yet to be determined. Towards this end, we have identified Escherichia coli functions that process the recombining oligo and affect bacteriophage λ Red-mediated oligo recombination. To determine the nature of oligo processing during recombination, each oligo contained multiple nucleotide changes: a single base change allowing recombinant selection, and silent changes serving as genetic markers to determine the extent of oligo processing during the recombination. Such oligos were often not incorporated into the host chromosome intact; many were partially degraded in the process of recombination. The position and number of these silent nucleotide changes within the oligo strongly affect both oligo processing and recombination frequency. Exonucleases, especially those associated with DN A Polymerases I and III, affect inheritance of the silent nucleotide changes in the oligos. We demonstrate for the first time that the major DNA polymerases ( Pol I and Pol III) and DNA ligase are directly involved with oligo recombination. [ABSTRACT FROM AUTHOR]

Published

2013

25. Isolation and Characterization of RNA Polymerase rpoB Mutations That Alter Transcription Slippage during Elongation in Escherichia coli.

Author

Zhou, Yan Ning, Lubkowska, Lucyna, Hui, Monica, Court, Carolyn, Shuo Chen, Court, Donald L., Strathern, Jeffrey, Ding Jun Jin, and Kashlev, Mikhail

Subjects

*ESCHERICHIA coli, *RNA polymerases, *ISOLATION of biotechnological microorganisms, *PHENOTYPES, *HELIX-loop-helix motifs, *MESSENGER RNA

Abstract

Transcription fidelity is critical for maintaining the accurate flow of genetic information. The study of transcription fidelity has been limited because the intrinsic error rate of transcription is obscured by the higher error rate of translation, making identification of phenotypes associated with transcription infidelity challenging. Slippage of elongatingRNApolymerase (RNAP) on homopolymeric A/T tracts in DNA represents a special type of transcription error leading to disruption of open reading frames in Escherichia coli mRNA. However, the regions in RNAP involved in elongation slippage and its molecular mechanism are unknown. We constructed an A/T tract that is out of frame relative to a downstream lacZ gene on the chromosome to examine transcriptional slippage during elongation. Further, we developed a genetic system that enabled us for the first time to isolate and characterize E. coliRNAPmutants with altered transcriptional slippage in vivo. We identified several amino acid residues in the β subunit of RNAP that affect slippage in vivo and in vitro. Interestingly, these highly clustered residues are located near the RNA strand of the RNA-DNA hybrid in the elongation complex. Our E. coli study complements an accompanying study of slippage by yeast RNAP II and provides the basis for future studies on the mechanism of transcription fidelity. [ABSTRACT FROM AUTHOR]

Published

2013

26. The Era GTPase recognizes the GAUCACCUCC sequence and binds helix 45 near the 3' end of 165 rRNA.

Author

Chao Tu, Xiaomei Zhou, Tarasov, Sergey G., Tropea, Joseph E., Austin, Brian P., Waugh, David S., Court, Donald L., and Xinhua Ji

Subjects

*RNA, *NUCLEOTIDES, *GUANOSINE triphosphatase, *PROTEINS, *PHENOTYPES

Abstract

Era, composed of a GTPase domain and a K homology domain, is essential for bacterial cell viability. It is required for the maturation of 16S rRNA and assembly of the 30S ribosomal subunit. We showed previously that the protein recognizes nine nucleotides (1531AUCACCUCC1539) near the 3' end of 16S rRNA, and that this recognition stimulates GTP-hydrolyzing activity of Era. In all three kingdoms of life, the 1530GAUCA1534 sequence and helix 45 (h45) (nucleotides 1506-1529) are highly conserved. It has been shown that the 1530GA1531 to 1530AG1531 double mutation severely affects the viability of bacteria. However, whether Era interacts with G1530 and/or h45 and whether such interactions (if any) contribute to the stimulation of Era's GTPase activity were not known. Here, we report two RNA structures that contain nucleotides 1506-1542 (RNA301), one in complex with Era and GDPNP (GNP), a nonhydrolysable GTP-analogue, and the other in complex with Era, GNP, and the KsgA methyltransferase. The structures show that Era recognizes 10 nucleotides, including G1530, and that Era also binds h45. Moreover, GTPase assay experiments show that G1530 does not stimulate Era's GTPase activity. Rather, A1531 and A1534 are most important for stimulation and h45 further contributes to the stimulation. Although G1530 does not contribute to the intrinsic GTPase activity of Era, its interaction with Era is important for binding and is essential for the protein to function, leading to the discovery of a new cold-sensitive phenotype of Era. [ABSTRACT FROM AUTHOR]

Published

2011

27. Probing Cellular Processes with Oligo-Mediated Recombination and Using the Knowledge Gained to Optimize Recombineering

Author

Sawitzke, James A., Costantino, Nina, Li, Xin-tian, Thomason, Lynn C., Bubunenko, Mikhail, Court, Carolyn, and Court, Donald L.

Subjects

*OLIGONUCLEOTIDES, *ESCHERICHIA coli, *DNA repair, *GENOMES, *MUTAGENESIS, *DNA replication, *GENETIC recombination

Abstract

Abstract: Recombination with single-strand DNA oligonucleotides (oligos) in Escherichia coli is an efficient and rapid way to modify replicons in vivo. The generation of nucleotide alteration by oligo recombination provides novel assays for studying cellular processes. Single-strand exonucleases inhibit oligo recombination, and recombination is increased by mutating all four known exonucleases. Increasing oligo concentration or adding nonspecific carrier oligo titrates out the exonucleases. In a model for oligo recombination, λ Beta protein anneals the oligo to complementary single-strand DNA at the replication fork. Mismatches are created, and the methyl-directed mismatch repair (MMR) system acts to eliminate the mismatches inhibiting recombination. Three ways to evade MMR through oligo design include, in addition to the desired change (1) a C·C mismatch  6 bp from that change; (2) four or more adjacent mismatches; or (3) mismatches at four or more consecutive wobble positions. The latter proves useful for making high-frequency changes that alter only the target amino acid sequence and even allows modification of essential genes. Efficient uptake of DNA is important for oligo-mediated recombination. Uptake of oligos or plasmids is dependent on media and is 10,000-fold reduced for cells grown in minimal versus rich medium. Genomewide engineering technologies utilizing recombineering will benefit from both optimized recombination frequencies and a greater understanding of how biological processes such as DNA replication and cell division impact recombinants formed at multiple chromosomal loci. Recombination events at multiple loci in individual cells are described here. [Copyright &y& Elsevier]

Published

2011

28. Oligonucleotide recombination in Gram-negative bacteria.

Author

Swingle, Bryan, Markel, Eric, Costantino, Nina, Bubunenko, Mikhail G., Cartinhour, Samuel, and Court, Donald L.

Subjects

*DNA, *OLIGONUCLEOTIDES, *BACTERIA, *CHROMOSOMES, *GRAM-negative bacteria, *GENOMES

Abstract

This report describes several key aspects of a novel form of RecA-independent homologous recombination. We found that synthetic single-stranded DNA oligonucleotides (oligos) introduced into bacteria by transformation can site-specifically recombine with bacterial chromosomes in the absence of any additional phage-encoded functions. Oligo recombination was tested in four genera of Gram-negative bacteria and in all cases evidence for recombination was apparent. The experiments presented here were designed with an eye towards learning to use oligo recombination in order to bootstrap identification and development of phage-encoded recombination systems for recombineering in a wide range of bacteria. The results show that oligo concentration and sequence have the greatest influence on recombination frequency, while oligo length was less important. Apart from the utility of oligo recombination, these findings also provide insights regarding the details of recombination mediated by phage-encoded functions. Establishing that oligos can recombine with bacterial genomes provides a link to similar observations of oligo recombination in archaea and eukaryotes suggesting the possibility that this process is evolutionary conserved. [ABSTRACT FROM AUTHOR]

Published

2010

29. Structure of ERA in complex with the 3′ end of 165 rRNA: Implications for ribosome biogenesis.

Author

Chao Tu, Xiaomei Zhou, Tropea, Joseph E., Austin, Brian P., Waugh, David S., Court, Donald L., and Xinhua Ji

Subjects

*BACTERIAL cell surfaces, *RIBOSOMAL DNA, *CELL membrane formation, *HYDROLYSIS, *PROTEINS

Abstract

ERA, composed of an N-terminal GTPase domain followed by an RNA-binding KH domain, is essential for bacterial cell viability. It binds to 165 rRNA and the 305 ribosomal subunit. However, its RNA-binding site, the functional relationship between the two domains, and its role in ribosome biogenesis remain unclear. We have determined two crystal structures of ERA, a binary complex with GDP and a ternary complex with a GTP-analog and the 1531AUCACCUCCUUA1542 sequence at the 3′ end of 165 rRNA. In the ternary complex, the first nine of the 12 nucleotides are recognized by the protein. We show that GTP binding is a prerequisite for RNA recognition by ERA and that RNA recognition stimulates its GTP-hydrolyzing activity. Based on these and other data, we propose a functional cycle of ERA, suggesting that the protein serves as a chaperone for processing and maturation of 16S rRNA and a checkpoint for assembly of the 305 ribosomal subunit. The AUCA sequence is highly conserved among bacteria, archaea, and eukaryotes, whereas the CCUCC, known as the anti-Shine-Dalgarno sequence, is conserved in noneukaryotes only. Therefore, these data suggest a common mechanism for a highly conserved ERA function in all three kingdoms of life by recognizing the AUCA, with a "twist" for noneukaryotic ERA proteins by also recognizing the CCUCC. [ABSTRACT FROM AUTHOR]

Published

2009

30. Structural Basis for Binding of RNA and Cofactor by a KsgA Methyltransferase

Author

Tu, Chao, Tropea, Joseph E., Austin, Brian P., Court, Donald L., Waugh, David S., and Ji, Xinhua

Subjects

*LIGAND binding (Biochemistry), *RNA, *METHYLTRANSFERASES, *HOMOCYSTEINE, *MOLECULAR structure, *MOLECULAR recognition, *CONFORMATIONAL analysis

Abstract

Summary: Among methyltransferases, KsgA and the reaction it catalyzes are conserved throughout evolution. However, the specifics of substrate recognition by the enzyme remain unknown. Here we report structures of Aquifex aeolicus KsgA, in its ligand-free form, in complex with RNA, and in complex with both RNA and S-adenosylhomocysteine (SAH, reaction product of cofactor S-adenosylmethionine), revealing critical structural information on KsgA-RNA and KsgA-SAH interactions. Moreover, the structures show how conformational changes that occur upon RNA binding create the cofactor-binding site. There are nine conserved functional motifs (motifs I–VIII and X) in KsgA. Prior to RNA binding, motifs I and VIII are flexible, each exhibiting two distinct conformations. Upon RNA binding, the two motifs become stabilized in one of these conformations, which is compatible with the binding of SAH. Motif X, which is also stabilized upon RNA binding, is directly involved in the binding of SAH. [Copyright &y& Elsevier]

Published

2009

31. Structural and Functional Analysis of the E. coli NusB-S10 Transcription Antitermination Complex

Author

Luo, Xiao, Hsiao, He-Hsuan, Bubunenko, Mikhail, Weber, Gert, Court, Donald L., Gottesman, Max E., Urlaub, Henning, and Wahl, Markus C.

Subjects

*BACTERIAL genetics, *ESCHERICHIA coli, *GENETIC transcription, *PROKARYOTES, *FUNCTIONAL analysis, *PROTEIN S, *RIBOSOMES, *MICROBIOLOGICAL assay, *TRANSCRIPTION factors

Abstract

Summary: Protein S10 is a component of the 30S ribosomal subunit and participates together with NusB protein in processive transcription antitermination. The molecular mechanisms by which S10 can act as a translation or a transcription factor are not understood. We used complementation assays and recombineering to delineate regions of S10 dispensable for antitermination, and determined the crystal structure of a transcriptionally active NusB-S10 complex. In this complex, S10 adopts the same fold as in the 30S subunit and is blocked from simultaneous association with the ribosome. Mass spectrometric mapping of UV-induced crosslinks revealed that the NusB-S10 complex presents an intermolecular, composite, and contiguous binding surface for RNAs containing BoxA antitermination signals. Furthermore, S10 overproduction complemented a nusB null phenotype. These data demonstrate that S10 and NusB together form a BoxA-binding module, that NusB facilitates entry of S10 into the transcription machinery, and that S10 represents a central hub in processive antitermination. [Copyright &y& Elsevier]

Published

2008

32. Host responses influence on the induction of lambda prophage.

Author

Rokney, Assaf, Kobiler, Oren, Amir, Amnon, Court, Donald L., Stavans, Joel, Adhya, Sankar, and Oppenheim, Amos B.

Subjects

*BACTERIOPHAGES, *VIRUSES, *BACTERIOPHAGE lambda, *EPISOMES, *DNA damage, *BIOCHEMICAL genetics

Abstract

Inactivation of bacteriophage lambda CI repressor leads almost exclusively to lytic development. Prophage induction can be initiated either by DNA damage or by heat treatment of a temperature-sensitive repressor. These two treatments also cause a concurrent activation of either the host SOS or heat-shock stress responses respectively. We studied the effects of these two methods of induction on the lytic pathway by monitoring the activation of different lambda promoters, and found that the lambda genetic network co-ordinates information from the host stress response networks. Our results show that the function of the CII transcriptional activator, which facilitates the lysogenic developmental pathway, is not observed following either method of induction. Mutations in the cro gene restore the CII function irrespective of the induction method. Deletion of the heat-shock protease gene ftsH can also restore CII function following heat induction but not following SOS induction. Our findings highlight the importance of the elimination of CII function during induction as a way to ensure an efficient lytic outcome. We also show that, despite the common inhibitory effect on CII function, there are significant differences in the heat- and SOS-induced pathways leading to the lytic cascade. [ABSTRACT FROM AUTHOR]

Published

2008

33. Identification and analysis of recombineering functions from Gram-negative and Gram-positive bacteria and their phages.

Author

Datta, Simanti, Costantino, Nina, Xiaomei Zhou, and Court, Donald L.

Subjects

*FUNCTIONAL analysis, *BACTERIA, *BACTERIOPHAGES, *GENES, *ESCHERICHIA coli, *EXONUCLEASES, *OLIGONUCLEOTIDES

Abstract

We report the identification and functional analysis of nine genes from Gram-positive and Gram-negative bacteria and their phages that are similar to lambda (λ) bet or Escherichia coli recT. Beta and RecT are single-strand DNA annealing proteins, referred to here as recombinases. Each of the nine other genes when expressed in E. coli carries out oligonucleotide-mediated recombination. To our knowledge, this is the first study showing single-strand recombinase activity from diverse bacteria. Similar to bet and recT, most of these other recombinases were found to be associated with putative exonuclease genes. Beta and RecT in conjunction with their cognate exonucleases carry out recombination of linear double-strand DNA. Among four of these foreign recombinase/exonuclease pairs tested for recombination with double-strand DNA, three had activity, albeit barely detectable. Thus, although these recombinases can function in E. coli to catalyze oligonucleotide recombination, the double-strand DNA recombination activities with their exonuclease partners were inefficient. This study also demonstrated that Gam, by inhibiting host ReBCD nuclease activity. helps to improve the efficiency of λ Red-mediated recombination with linear double-strand DNA, but Gam is not absolutely essential. Thus, in other bacterial species where Gam analogs have not been identified, double-strand DNA recombination may still work in the absence of a Gam-like function. We anticipate that at least some of the recombineering systems studied here will potentiate oligonucleotide and double-strand DNA-mediated recombineering in their native or related bacteria. [ABSTRACT FROM AUTHOR]

Published

2008

34. A stepwise model for double-stranded RNA processing by ribonuclease III.

Author

Jianhua Gan, Shaw, Gary, Tropea, Joseph E., Waugh, David S., Court, Donald L., and Xinhua Ji

Subjects

*RNA, *HYDROLYSIS, *NUCLEIC acids, *RIBOSE, *SOLVOLYSIS, *RIBONUCLEASES

Abstract

RNA interference is mediated by small interfering RNAs produced by members of the ribonuclease III (RNase III) family represented by bacterial RNase III and eukaryotic Rnt1p, Drosha and Dicer. For mechanistic studies, bacterial RNase III has been a valuable model system for the family. Previously, we have shown that RNase III uses two catalytic sites to create the 2-nucleotide (nt) 3′ overhangs in its products. Here, we present three crystal structures of RNase III in complex with double-stranded RNA, demonstrating how Mg2+ is essential for the formation of a catalytically competent protein–RNA complex, how the use of two Mg2+ ions can drive the hydrolysis of each phosphodiester bond, and how conformational changes in both the substrate and the protein are critical elements for assembling the catalytic complex. Moreover, we have modelled a protein–substrate complex and a protein–reaction intermediate (transition state) complex on the basis of the crystal structures. Together, the crystal structures and the models suggest a stepwise mechanism for RNase III to execute the phosphoryl transfer reaction. [ABSTRACT FROM AUTHOR]

Published

2008

35. The Structure of the R184A Mutant of the Inositol Monophosphatase Encoded by suhB and Implications for Its Functional Interactions in Escherichia coli.

Author

Yanling Wang, Stieglitz, Kimberly A., Bubunenko, Mikhail, Court, Donald L., Boguslaw Stec, and Roberts, Mary F.

Subjects

*ESCHERICHIA coli, *ESCHERICHIA, *INOSITOL, *INOSITOL phosphates, *GENETIC mutation

Abstract

The Escherichia coil product of the suhB gene, SuhB, is an inositol monophosphatase (IMPase) that is best known as a suppressor of temperature-sensitive growth phenotypes in E. coli. To gain insights into these biological diverse effects, we determined the structure of the SuhB R184A mutant protein. The structure showed a dimer organization similar to other IMPases, but with an altered interface suggesting that the presence of Arg-184 in the wild-type protein could shift the monomer-dimer equilibrium toward monomer. In parallel, a gel shift assay showed that SuhB forms a tight complex with RNA polymerase (RNA pol) that inhibits the IMPase catalytic activity of SuhB. A variety of SuhB mutant proteins designed to stabilize the dimer interface did not show a clear correlation with the ability of a specific mutant protein to complement the ΔsuhB mutation when introduced extragenically despite being active IMPases. However, the loss of sensitivity to RNA pol binding, i.e. in G173V, R1841, and L96F/R1841, did correlate strongly with loss of complementation of ΔsuhB. Because residue 184 forms the core of the SuhB dimer, it is likely that the interaction with RNA polymerase requires monomeric SuhB. The exposure of specific residues facilitates the interaction of SuhB with RNA pol (or another target with a similar binding surface) and it is this heterodimer formation that is critical to the ability of SuhB to rescue temperature-sensitive phenotypes in E. coli. [ABSTRACT FROM AUTHOR]

Published

2007

36. Multicopy plasmid modification with phage λ Red recombineering

Author

Thomason, Lynn C., Costantino, Nina, Shaw, Dana V., and Court, Donald L.

Subjects

*GENETIC recombination, *TRANSGENIC organisms, *PLASMIDS, *CYTOPLASMIC inheritance

Abstract

Abstract: Recombineering, in vivo genetic engineering using the bacteriophage λ Red generalized recombination system, was used to create various modifications of a multicopy plasmid derived from pBR322. All genetic modifications possible on the Escherichia coli chromosome and on bacterial artificial chromosomes (BACs) are also possible on multicopy plasmids and are obtained with similar frequencies to their chromosomal counterparts, including creation of point mutations (5–10% unselected frequency), deletions and substitutions. Parental and recombinant plasmids are nearly always present as a mixture following recombination, and circular multimeric plasmid molecules are often generated during the recombineering. [Copyright &y& Elsevier]

Published

2007

37. Importance of the 5 S rRNA-binding Ribosomal Proteins for Cell Viability and Translation in Escherichia coli

Author

Korepanov, Alexey P., Gongadze, George M., Garber, Maria B., Court, Donald L., and Bubunenko, Mikhail G.

Subjects

*ESCHERICHIA coli, *NON-coding RNA, *CHROMOSOMES, *RIBOSOMES

Abstract

Abstract: A specific complex of 5 S rRNA and several ribosomal proteins is an integral part of ribosomes in all living organisms. Here we studied the importance of Escherichia coli genes rplE, rplR and rplY, encoding 5 S rRNA-binding ribosomal proteins L5, L18 and L25, respectively, for cell growth, viability and translation. Using recombineering to create gene replacements in the E. coli chromosome, it was shown that rplE and rplR are essential for cell viability, whereas cells deleted for rplY are viable, but grow noticeably slower than the parental strain. The slow growth of these L25-defective cells can be stimulated by a plasmid expressing the rplY gene and also by a plasmid bearing the gene for homologous to L25 general stress protein CTC from Bacillus subtilis. The rplY mutant ribosomes are physically normal and contain all ribosomal proteins except L25. The ribosomes from L25-defective and parental cells translate in vitro at the same rate either poly(U) or natural mRNA. The difference observed was that the mutant ribosomes synthesized less natural polypeptide, compared to wild-type ribosomes both in vivo and in vitro. We speculate that the defect is at the ribosome recycling step. [Copyright &y& Elsevier]

Published

2007

38. Structural Insight into the Mechanism of Double-Stranded RNA Processing by Ribonuclease III

Author

Gan, Jianhua, Tropea, Joseph E., Austin, Brian P., Court, Donald L., Waugh, David S., and Ji, Xinhua

Subjects

*RNA-protein interactions, *DOUBLE-stranded RNA, *RNA, *RIBONUCLEASES, *SMALL interfering RNA, *CATALYTIC RNA

Abstract

Summary: Members of the ribonuclease III (RNase III) family are double-stranded RNA (dsRNA) specific endoribonucleases characterized by a signature motif in their active centers and a two-base 3′ overhang in their products. While Dicer, which produces small interfering RNAs, is currently the focus of intense interest, the structurally simpler bacterial RNase III serves as a paradigm for the entire family. Here, we present the crystal structure of an RNase III-product complex, the first catalytic complex observed for the family. A 7 residue linker within the protein facilitates induced fit in protein-RNA recognition. A pattern of protein-RNA interactions, defined by four RNA binding motifs in RNase III and three protein-interacting boxes in dsRNA, is responsible for substrate specificity, while conserved amino acid residues and divalent cations are responsible for scissile-bond cleavage. The structure reveals a wealth of information about the mechanism of RNA hydrolysis that can be extrapolated to other RNase III family members. [Copyright &y& Elsevier]

Published

2006

39. Switches in Bacteriophage Lambda Development.

Author

Oppenheim, Amos B., Kobiler, Oren, Stavans, Joel, Court, Donald L., and Adhya, Sankar

Subjects

*BACTERIOPHAGE lambda, *LYSOGENY, *BACTERIAL genetics, *GENETIC transcription, *GENETIC research

Abstract

The lysis-lysogeny decision of bacteriophage lambda (λ) is a paradigm for developmental genetic networks. There are three key features, which characterize the network. First, after infection of the host bacterium, a decision between lytic or lysogenic development is made that is dependent upon environmental signals and the number of infecting phages per cell. Second, the lysogenic prophage state is very stable. Third, the prophage enters lytic development in response to DNA-damaging agents. The CI and Cro regulators define the lysogenic and lytic states, respectively, as a bistable genetic switch. Whereas CI maintains a stable lysogenic state, recent studies indicate that Cro sets the lytic course not by directly blocking CI expression but indirectly by lowering levels of CII which activates cI transcription. We discuss how a relatively simple phage like λ employs a complex genetic network in decision-making processes, providing a challenge for theoretical modeling. [ABSTRACT FROM AUTHOR]

Published

2005

40. Intermediate States of Ribonuclease III in Complex with Double-Stranded RNA

Author

Gan, Jianhua, Tropea, Joseph E., Austin, Brian P., Court, Donald L., Waugh, David S., and Ji, Xinhua

Subjects

*NUCLEIC acids, *CARRIER proteins, *GENETIC regulation, *AFTERLIFE

Abstract

Summary: Bacterial ribonuclease III (RNase III) can affect RNA structure and gene expression in either of two ways: as a processing enzyme that cleaves double-stranded (ds) RNA, or as a binding protein that binds but does not cleave dsRNA. We previously proposed a model of the catalytic complex of RNase III with dsRNA based on three crystal structures, including the endonuclease domain of RNase III with and without bound metal ions and a dsRNA binding protein complexed with dsRNA. We also reported a noncatalytic assembly observed in the crystal structure of an RNase III mutant, which binds but does not cleave dsRNA, complexed with dsRNA. We hypothesize that the RNase III•dsRNA complex can exist in two functional forms, a catalytic complex and a noncatalytic assembly, and that in between the two forms there may be intermediate states. Here, we present four crystal structures of RNase III complexed with dsRNA, representing possible intermediates. [Copyright &y& Elsevier]

Published

2005

41. Quantitative kinetic analysis of the bacteriophage &lamda; genetic network.

Author

Kobiler, Oren, Rokney, Assaf, Friedman, Nir, Court, Donald L., Stavans, Joel, and Oppenheim, Amos B.

Subjects

*PROTEINS, *BACTERIAL genetics, *MICROBIAL genetics, *BACTERIOPHAGES, *BACTERIOLOGY, *ORGANIC compounds

Abstract

The lysis-lysogeny decision of bacteriophage λ has been a paradigm for a developmental genetic network, which is composed of interlocked positive and negative feedback loops. This genetic network is capable of responding to environmental signals and to the number of infecting phages. An interplay between Cl and Cro functions suggested a bistable switch model for the lysis-lysogeny decision. Here, we present a real-time picture of the execution of lytic and lysogenic pathways with unprecedented temporal resolution. We monitor, in vivo, both the level and function of the CII and Q gene regulators. These activators are cotranscribed yet control opposite developmental pathways. Conditions that favor the lysogenic response show severe delay and down-regulation of Q activity, in both CII-dependent and CII-independent ways. Whereas CII activity correlates with its protein level, Q shows a pronounced threshold before its function is observed. Our quantitative analyses suggest that by regulating CII and CIII, Cro plays a key role in the ability of the λ genetic network to sense the difference between one and more than one phage particles infecting a cell. Thus, our results provide an improved framework to explain the longstanding puzzle of the decision process. [ABSTRACT FROM AUTHOR]

Published

2005

42. Translation repression by an RNA polymerase elongation complex.

Author

Wilson, Helen R., Jian-guang Zhou, Daigun Yu, and Court, Donald L.

Subjects

*BACTERIOPHAGES, *VIRUSES, *PROTEINS, *RNA polymerases, *GENETICS, *MICROBIOLOGY

Abstract

Bacteriophage λ N and bacterial Nus proteins together with a unique site NUT in the leader of the early viral N gene transcript bind RNA polymerase (RNAP) and form a highly processive antitermination complex; N bound at NUT also represses N translation. In this study, we investigate whether N and NUT cause N translation repression as part of the antitermination complex by testing conditions that inhibit the formation of the N-modified transcription complex for their effect on N-mediated translation repression. We show that nus and nut mutations that in combination destabilize multiple interactions in the antitermination complex prevent N-mediated translation repression. Likewise, transcription of the nut-N region by T7 RNAP, which does not lead to the assembly of an effective antitermination complex when N is supplied, eliminates translation repression. We also demonstrate that a unique mutant β subunit of RNAP reduces N-mediated translation repression, and that overexpression of transcription factor NusA suppresses this defect. We conclude that the N-modified RNAP transcription complex is necessary to repress N translation. [ABSTRACT FROM AUTHOR]

Published

2004

43. Noncatalytic Assembly of Ribonuclease III with Double-Stranded RNA

Author

Blaszczyk, Jaroslaw, Gan, Jianhua, Tropea, Joseph E., Court, Donald L., Waugh, David S., and Ji, Xinhua

Subjects

*DOUBLE-stranded RNA, *GENE expression, *CARRIER proteins, *ENDONUCLEASES

Abstract

Ribonuclease III (RNase III) represents a family of double-stranded RNA (dsRNA) endonucleases. The simplest bacterial enzyme contains an endonuclease domain (endoND) and a dsRNA binding domain (dsRBD). RNase III can affect RNA structure and gene expression in either of two ways: as a dsRNA-processing enzyme that cleaves dsRNA, or as a dsRNA binding protein that binds but does not cleave dsRNA. We previously determined the endoND structure of Aquifex aeolicus RNase III (Aa-RNase III) and modeled a catalytic complex of full-length Aa-RNase III with dsRNA. Here, we present the crystal structure of Aa-RNase III in complex with dsRNA, revealing a noncatalytic assembly. The major differences between the two functional forms of RNase III·dsRNA are the conformation of the protein and the orientation and location of dsRNA. The flexibility of a 7 residue linker between the endoND and dsRBD enables the transition between these two forms. [Copyright &y& Elsevier]

Published

2004

44. In vivo recombineering of bacteriophage λ by PCR fragments and single-strand oligonucleotides

Author

Oppenheim, Amos B., Rattray, Alison J., Bubunenko, Mikhail, Thomason, Lynn C., and Court, Donald L.

Subjects

*BACTERIOPHAGES, *OLIGONUCLEOTIDES, *GENES, *DNA

Abstract

We demonstrate that the bacteriophage λ Red functions efficiently recombine linear DNA or single-strand oligonucleotides (ss-oligos) into bacteriophage λ to create specific changes in the viral genome. Point mutations, deletions, and gene replacements have been created. While recombineering with oligonucleotides, we encountered other mutations accompanying the desired point mutational change. DNA sequence analysis suggests that these unwanted mutations are mainly frameshift deletions introduced during oligonucleotide synthesis. [Copyright &y& Elsevier]

Published

2004

45. Recombineering with overlapping single-stranded DNA oligonucleotides: Testing a recombination intermediate.

Author

Daiguan Yu, Sawitzke, James A., Ellis, Hilary, and Court, Donald L.

Subjects

*GENETIC recombination, *OLIGONUCLEOTIDES, *DNA

Abstract

A phage λ-based recombination system, Red, can be used for high-efficiency mutagenesis, repair, and engineering of chromosomal or episomal DNA in vivo in Escherichia coli. When long linear double-stranded DNA with short flanking homologies to their targets are used for the recombination, the λ Exo, Beta, and Gam proteins are required. The current model is: (i) Gam inhibits the host RecBCD activity, thereby protecting the DNA substrate for recombination; (ii) Exo degrades from each DNA end in a 5' → 3' direction, creating double-stranded DNA with 3' single-stranded DNA tails; and (iii) Beta binds these 3' overhangs to protect and anneal them to complementary sequences. We have tested this model for Red recombination by using electroporation to introduce overlapping, complementary oligonucleotides that when annealed in vivo approximate the recombination intermediate that Exo should create. Using this technique we found Exo-independent recombination. Surprisingly, a similarly constructed substrate with 5' overhangs recombined more efficiently. This 5' overhang recombination required both Exo and Beta for high levels of recombination and the two oligonucleotides need to overlap by only 6 bp on their 3' ends. Results indicate that Exo may load Beta onto the 3' overhang it produces. In addition, multiple overlapping oligonucleotides were successfully used to generate recombinants in vivo, a technique that could prove useful for many genetic engineering procedures. [ABSTRACT FROM AUTHOR]

Published

2003

46. Phage HK022 Nun protein represses translation of phage λ N (transcription termination/translation repression).

Author

Kim, Hyeong C., Jian-guang Zhou, Wilson, Helen R., Mogilnitskiy, Grigoriy, Court, Donald L., and Gottesman, Max E.

Subjects

*BACTERIOPHAGE lambda, *RNA polymerases, *GENES

Abstract

The N-terminal arginine-rich motif of phage HK022 Nun protein binds to NUT sequences in phage λ nascent transcripts and induces transcription termination. Interactions between the Nun C terminus and RNA polymerase as well as the DNA template are required for termination. We have isolated Nun C-terminal point and deletion mutants that are unable to block transcription. The mutants bind NUT RNA and inhibit translation of the λ N gene. Thus HK022 excludes λ both by terminating transcription on the phage chromosome and by preventing translation of the essential λ N gene. Like N autoregulation, translation repression by Nun requires host RNaseIII deficiency (rnc) or a mutation in the RNaseIII processing site (rIII) located between NUTL and the beginning of the N coding sequence. Our data support the idea that Nun bound at NUTL causes steric interference with ribosome attachment to the nearby N coding sequence. Two models, Nun acting alone or in complex with host proteins, are discussed. [ABSTRACT FROM AUTHOR]

Published

2003

47. A Spring-Loaded State of NusG in Its Functional Cycle Is Suggested by X-ray Crystallography and Supported by Site-Directed Mutants.

Author

Knowlton, J. Randy, Bubunenko, Mikhail, Andrykovitch, Michelle, Wei Guo, Routzahn, Karen M., Waugh, David S., Court, Donald L., and Xinhua Ji

Subjects

*TRANSCRIPTION factors, *MOLECULAR structure, *CRYSTALLOGRAPHY, *SITE-specific mutagenesis

Abstract

Transcription factor NusG is present in all prokaryotes, and orthologous proteins have also been identified in yeast and humans. NusG contains a 27-residue KOW motif, found in ribosomal protein L24 where it interacts with rRNA. NusG in Escherichia coli (EcNusG) is an essential protein and functions as a regulator of Rho-dependent transcription termination, phage λ, N and rRNA transcription antitermination, and phage HK022 Nun termination. Relative to EcNusG, Aquifex aeolicus NusG (AaNusG) and several other bacterial NusG proteins contain a variable insertion sequence of ∼70 residues in the central region of the molecule. Recently, crystal structures of AaNusG in space groups P2[sub 1] and I222 have been reported; the authors conclude that there are no conserved dimers among the contacting molecules in the crystals [Steiner, T., Kaiser, J. T., Marinkovic, S., Huber, R., and Wahl, M. C. (2002) EMBO J. 21, 4641-4653]. We have independently determined the structures of AaNusG also in two crystal forms, P2[sub 1] and C222[sub 1], and surprisingly found that AaNusG molecules form domain-swapped dimers in both crystals. Additionally, polymerization is also observed in the P2[sub 1] crystal. A unique "ball-and-socket" junction dominates the intermolecular interactions within both oligomers. We believe that this interaction is a clue to the function of the molecule and propose a spring-loaded state in the functional cycle of NusG. The importance of the ball-and-socket junction for the function of NusG is supported by the functional analysis of site-directed mutants. [ABSTRACT FROM AUTHOR]

Published

2003

48. The global regulator RNase III modulates translation repression by the transcription elongation factor N.

Author

Wilson, Helen R., Daiguan Yu, Peters, III., Howard K., Jian-guang Zhou, and Court, Donald L.

Subjects

*BACTERIOPHAGES, *GENETIC regulation, *GENETIC transcription, *GENE expression, *RNA, *GENETIC code

Abstract

Efficient expression of most bacteriophage &lamda; early genes depends upon the formation of an antiterminating transcription complex to overcome transcription terminators in the early operons, PL and PR. Formation of this complex requires the phage-encoded protein N, the first gene product expressed from the PL operon. The N leader RNA contains, in this order: the NUTL site, an RNase III-sensitive hairpin and the N ribosome-binding site. N bound to NUTL RNA is part of both the antitermination complex and an auto-regulatory complex that represses the translation of the N gene. In this study, we show that cleavage of the N leader by RNase III does not inhibit antitermination but prevents N-mediated translation repression of N gene expression. In fact, by preventing N auto- regulation, RNase III activates N gene translation at least 200-fold. N-mediated translation repression is extremely sensitive to growth rate, reflecting the growth rate regulation of RNase III expression itself. Given N protein's critical role in &lamda; development, the level of RNase III activity therefore serves as an important sensor of physiological conditions for the bacteriophage. [ABSTRACT FROM AUTHOR]

Published

2002

49. High efficiency mutagenesis, repair, and engineering of chromosomal DNA using single-stranded....

Author

Ellis, Hilary M., Daiguan Yu, DiTizio, Tina, and Court, Donald L.

Subjects

*OLIGONUCLEOTIDES, *MUTAGENESIS, *DNA replication, *GENETIC recombination

Abstract

Examines the use of single-stranded (ss) oligonucleotides in mutagenesis, repair, and engineering of chromosomal DNA. Results of ssDNA homologous recombination; Need for beta protein to recombine ssDNA; Correlation between strand bias and direction of replication.

Published

2001

50. The structure of the transcriptional antiterminator NusB from Escherichia coli.

Author

Altieri, Amanda S., Mazzulla, Marie J., Horita, David A., Heath Coats, R., Wingfield, Paul T., Das, Asis, Court, Donald L., and Andrew Byrd, R.

Subjects

*ESCHERICHIA coli, *PROTEINS, *RNA, *MYCOBACTERIUM tuberculosis

Abstract

We have determined the solution structure of NusB, a transcription antitermination protein from Escherichia coli. The structure reveals a novel, all α-helical protein fold. NusB mutations that cause a loss of function (NusB5) or alter specificity for RNA targets (NusB101) are localized to surface residues and likely affect RNA?protein or protein?protein interactions. Residues that are highly conserved among homologs stabilize the protein core. The solution structure of E. coli NusB presented here resembles that of Mycobacterium tuberculosis NusB determined by X-ray diffraction, but differs substantially from a solution structure of E. coli NusB reported earlier. [ABSTRACT FROM AUTHOR]

Published

2000