Your search keyword '"Plasmid Construction"' showing total 1,824 results

101. Mutant T4 DNA polymerase for easy cloning and mutagenesis.

Author

Qi, Ruhu and Otting, Gottfried

Subjects

*DNA polymerase genetics, *MOLECULAR structure of DNA polymerases, *GENETIC engineering, *PLANT cloning, *MUTAGENESIS, *ESCHERICHIA coli

Abstract

The advent of high-fidelity DNA polymerases that can be used to linearize and amplify whole plasmids by PCR opened the door to greatly simplified cloning and mutagenesis protocols. Commercially available kits work well, but often have been optimized using undisclosed or proprietory components. Here we show that a mutant T4 DNA polymerase (Y320A) with attenuated 3’-exonuclease activity is uniquely suited to generate single-stranded DNA overhangs of uniform length in a more easily controllable manner than the wild-type enzyme, and this can be used to increase the yields of colonies containing correctly modified plasmids in cloning and mutagenesis experiments, which is particularly useful when E. coli cells are of relatively low competency. Standard protocols using the mutant T4 DNA polymerase are provided for the sequence and ligation independent cloning (SLIC) method and a modified QuikChange method, where the mutant enzyme enhances the yield of correctly mutated plasmid and further suppresses parental plasmid during digestion with DpnI. Single-stranded DNA overhangs generated by the mutant T4 DNA polymerase facilitate subsequent plasmid circularization, annealing and ligation in E. coli. [ABSTRACT FROM AUTHOR]

Published

2019

102. Bclaf1 critically regulates the type I interferon response and is degraded by alphaherpesvirus US3.

Author

Qin, Chao, Zhang, Rui, Lang, Yue, Shao, Anwen, Xu, Aotian, Feng, Wenhai, Han, Jun, Wang, Mengdong, He, Wanwei, Yu, Cuilian, and Tang, Jun

Subjects

*TYPE I interferons, *VIRUS diseases, *TRANSCRIPTION factors, *AUJESZKY'S disease virus, *VIRAL proteins

Abstract

Type I interferon response plays a prominent role against viral infection, which is frequently disrupted by viruses. Here, we report Bcl-2 associated transcription factor 1 (Bclaf1) is degraded during the alphaherpesvirus Pseudorabies virus (PRV) and Herpes simplex virus type 1 (HSV-1) infections through the viral protein US3. We further reveal that Bclaf1 functions critically in type I interferon signaling. Knockdown or knockout of Bclaf1 in cells significantly impairs interferon-α (IFNα) -mediated gene transcription and viral inhibition against US3 deficient PRV and HSV-1. Mechanistically, Bclaf1 maintains a mechanism allowing STAT1 and STAT2 to be efficiently phosphorylated in response to IFNα, and more importantly, facilitates IFN-stimulated gene factor 3 (ISGF3) binding with IFN-stimulated response elements (ISRE) for efficient gene transcription by directly interacting with ISRE and STAT2. Our studies establish the importance of Bclaf1 in IFNα-induced antiviral immunity and in the control of viral infections. [ABSTRACT FROM AUTHOR]

Published

2019

103. Asymmetric diversification of mating pheromones in fission yeast.

Author

Seike, Taisuke, Shimoda, Chikashi, and Niki, Hironori

Subjects

*ANIMAL sexual behavior, *PHEROMONES, *PEPTIDYLTRANSFERASE, *SCHIZOSACCHAROMYCES pombe, *GENETICS

Abstract

In fungi, mating between partners depends on the molecular recognition of two peptidyl mating pheromones by their respective receptors. The fission yeast Schizosaccharomyces pombe (Sp) has two mating types, Plus (P) and Minus (M). The mating pheromones P-factor and M-factor, secreted by P and M cells, are recognized by the receptors mating type auxiliary minus 2 (Mam2) and mating type auxiliary plus 3 (Map3), respectively. Our recent study demonstrated that a few mutations in both M-factor and Map3 can trigger reproductive isolation in S. pombe. Here, we explored the mechanism underlying reproductive isolation through genetic changes of pheromones/receptors in nature. We investigated the diversity of genes encoding the pheromones and their receptor in 150 wild S. pombe strains. Whereas the amino acid sequences of M-factor and Map3 were completely conserved, those of P-factor and Mam2 were very diverse. In addition, the P-factor gene contained varying numbers of tandem repeats of P-factor (4–8 repeats). By exploring the recognition specificity of pheromones between S. pombe and its close relative Schizosaccharomyces octosporus (So), we found that So-M-factor did not have an effect on S. pombe P cells, but So-P-factor had a partial effect on S. pombe M cells. Thus, recognition of M-factor seems to be stringent, whereas that of P-factor is relatively relaxed. We speculate that asymmetric diversification of the two pheromones might be facilitated by the distinctly different specificities of the two receptors. Our findings suggest that M-factor communication plays an important role in defining the species, whereas P-factor communication is able to undergo a certain degree of flexible adaptation–perhaps as a first step toward prezygotic isolation in S. pombe. [ABSTRACT FROM AUTHOR]

Published

2019

104. Adding function to the genome of African Salmonella Typhimurium ST313 strain D23580.

Author

Canals, Rocío, Hammarlöf, Disa L., Kröger, Carsten, Owen, Siân V., Fong, Wai Yee, Lacharme-Lora, Lizeth, Zhu, Xiaojun, Wenner, Nicolas, Carden, Sarah E., Honeycutt, Jared, Monack, Denise M., Kingsley, Robert A., Brownridge, Philip, Chaudhuri, Roy R., Rowe, Will P. M., Predeus, Alexander V., Hokamp, Karsten, Gordon, Melita A., and Hinton, Jay C. D.

Subjects

*GENOMES, *SALMONELLA typhimurium, *ENTEROBACTERIACEAE, *FOOD pathogens, *SALMONELLA enterica

Abstract

Salmonella Typhimurium sequence type (ST) 313 causes invasive nontyphoidal Salmonella (iNTS) disease in sub-Saharan Africa, targeting susceptible HIV+, malarial, or malnourished individuals. An in-depth genomic comparison between the ST313 isolate D23580 and the well-characterized ST19 isolate 4/74 that causes gastroenteritis across the globe revealed extensive synteny. To understand how the 856 nucleotide variations generated phenotypic differences, we devised a large-scale experimental approach that involved the global gene expression analysis of strains D23580 and 4/74 grown in 16 infection-relevant growth conditions. Comparison of transcriptional patterns identified virulence and metabolic genes that were differentially expressed between D23580 versus 4/74, many of which were validated by proteomics. We also uncovered the S. Typhimurium D23580 and 4/74 genes that showed expression differences during infection of murine macrophages. Our comparative transcriptomic data are presented in a new enhanced version of the Salmonella expression compendium, SalComD23580: . We discovered that the ablation of melibiose utilization was caused by three independent SNP mutations in D23580 that are shared across ST313 lineage 2, suggesting that the ability to catabolize this carbon source has been negatively selected during ST313 evolution. The data revealed a novel, to our knowledge, plasmid maintenance system involving a plasmid-encoded CysS cysteinyl-tRNA synthetase, highlighting the power of large-scale comparative multicondition analyses to pinpoint key phenotypic differences between bacterial pathovariants. [ABSTRACT FROM AUTHOR]

Published

2019

105. CDI/CDS system-encoding genes of Burkholderia thailandensis are located in a mobile genetic element that defines a new class of transposon.

Author

Ocasio, Angelica B. and Cotter, Peggy A.

Subjects

*CELL communication, *TOXINS, *ESCHERICHIA coli, *MOBILE genetic elements, *BURKHOLDERIA thailandensis

Abstract

Intercellular communication and self-recognition are critical for coordinating cooperative and competitive behaviors during sociomicrobiological community development. Contact-dependent growth inhibition (CDI) proteins are polymorphic toxin delivery systems that inhibit the growth of non-self neighboring bacteria that lack the appropriate immunity protein. In Burkholderia thailandensis, CDI system proteins (encoded by bcpAIOB genes) also induce cooperative behaviors among sibling (self) cells, a phenomenon called contact-dependent signaling (CDS). Here we describe a mobile genetic element (MGE) that carries the bcpAIOB genes in B. thailandensis E264. It is a ~210 kb composite transposon with insertion sequence (IS) elements at each end. Although the ISs are most similar to IS2 of Escherichia coli, the transposase-dependent intermediate molecule displays characteristics more similar to those of the IS26 translocatable unit (TU). A reaction requiring only the “left” IS-encoded transposase results in formation of an extrachromosomal circular dsDNA intermediate (“the megacircle”) composed of the left IS and the sequences intervening between the ISs. Insertion of the megacircle into the chromosome occurs next to a pre-existing copy of an IS2-like element, recreating a functional composite transposon. We found that BcpA activity is required for megacircle formation, and in turn, megacircle formation is required for CDS phenotypes. Our data support a model in which the bcpAIOB genes function as both helping and harming greenbeard genes, simultaneously enhancing the fitness of self bacteria that possess the same allele plus tightly linked genes that mediate cooperative behaviors, and killing non-self bacteria that do not possess the same bcpAIOB allele. Mobility of the megacircle between cells could allow bacteria invading a community to be converted to self, and would facilitate propagation of the bcpAIOB genes in the event that the invading strain is capable of overtaking the resident community. [ABSTRACT FROM AUTHOR]

Published

2019

106. CRISPR-Cas9 In Situ engineering of subtilisin E in Bacillus subtilis.

Author

Price, Marcus A., Cruz, Rita, Baxter, Scott, Escalettes, Franck, and Rosser, Susan J.

Subjects

*CRISPRS, *BACILLUS subtilis, *PLASMIDS, *PROTEOLYTIC enzymes, *POLYMERASE chain reaction

Abstract

CRISPR-Cas systems have become widely used across all fields of biology as a genome engineering tool. With its recent demonstration in the Gram positive industrial workhorse Bacillus subtilis, this tool has become an attractive option for rapid, markerless strain engineering of industrial production hosts. Previously described strategies for CRISPR-Cas9 genome editing in B. subtilis have involved chromosomal integrations of Cas9 and single guide RNA expression cassettes, or construction of large plasmids for simultaneous transformation of both single guide RNA and donor DNA. Here we use a flexible, co-transformation approach where the single guide RNA is inserted in a plasmid for Cas9 co-expression, and the donor DNA is supplied as a linear PCR product observing an editing efficiency of 76%. This allowed multiple, rapid rounds of in situ editing of the subtilisin E gene to incorporate a salt bridge triad present in the Bacillus clausii thermotolerant homolog, M-protease. A novel subtilisin E variant was obtained with increased thermotolerance and activity. [ABSTRACT FROM AUTHOR]

Published

2019

107. The spermidine acetyltransferase SpeG regulates transcription of the small RNA rprA.

Author

Hu, Linda I., Filippova, Ekaterina V., Dang, Joseph, Pshenychnyi, Sergii, Ruan, Jiapeng, Kiryukhina, Olga, Anderson, Wayne F., Kuhn, Misty L., and Wolfe, Alan J.

Subjects

*SPERMIDINE acetyltransferase, *GENETIC transcription regulation, *NON-coding RNA, *POLYAMINES, *MICROBIAL virulence

Abstract

Spermidine N-acetyltransferase (SpeG) acetylates and thus neutralizes toxic polyamines. Studies indicate that SpeG plays an important role in virulence and pathogenicity of many bacteria, which have evolved SpeG-dependent strategies to control polyamine concentrations and survive in their hosts. In Escherichia coli, the two-component response regulator RcsB is reported to be subject to Nε-acetylation on several lysine residues, resulting in reduced DNA binding affinity and reduced transcription of the small RNA rprA; however, the physiological acetylation mechanism responsible for this behavior has not been fully determined. Here, we performed an acetyltransferase screen and found that SpeG inhibits rprA promoter activity in an acetylation-independent manner. Surface plasmon resonance analysis revealed that SpeG can physically interact with the DNA-binding carboxyl domain of RcsB. We hypothesize that SpeG interacts with the DNA-binding domain of RcsB and that this interaction might be responsible for SpeG-dependent inhibition of RcsB-dependent rprA transcription. This work provides a model for SpeG as a modulator of E. coli transcription through its ability to interact with the transcription factor RcsB. This is the first study to provide evidence that an enzyme involved in polyamine metabolism can influence the function of the global regulator RcsB, which integrates information concerning envelope stresses and central metabolic status to regulate diverse behaviors. [ABSTRACT FROM AUTHOR]

Published

2018

108. Protein engineering strategies for improving the selective methylation of target CpG sites by a dCas9-directed cytosine methyltransferase in bacteria.

Author

Xiong, Tina, Rohm, Dahlia, Workman, Rachael E., Roundtree, Lauren, Novina, Carl D., Timp, Winston, and Ostermeier, Marc

Subjects

*PROTEIN engineering, *METHYLTRANSFERASES, *DNA methylation, *CPG nucleotides, *GENE expression in mammals

Abstract

Mammalian gene expression is a complex process regulated in part by CpG methylation. The ability to target methylation for de novo gene regulation could have therapeutic and research applications. We have previously developed a dCas9-MC/MN protein for targeting CpG methylation. dCas9-MC/MN is composed of an artificially split M.SssI methyltransferase (MC/MN), with the MC fragment fused to a nuclease-null CRISPR/Cas9 (dCas9). Guide RNAs directed dCas9-MC/MN to methylate target sites in E. coli and human cells but also caused some low-level off-target methylation. Here, in E. coli, we show that shortening the dCas9-MC linker increases methylation of CpG sites located at select distances from the dCas9 binding site. Although a shortened linker decreased methylation of other CpGs proximal to the target site, it did not reduce off-target methylation of more distant CpG sites. Instead, targeted mutagenesis of the methyltransferase’s DNA binding domain, designed to reduce DNA affinity, significantly and preferentially reduced methylation of such sites. [ABSTRACT FROM AUTHOR]

Published

2018

109. Nab3’s localization to a nuclear granule in response to nutrient deprivation is determined by its essential prion-like domain.

Author

Loya, Travis J., O’Rourke, Thomas W., Simke, William C., Kelley, Joshua B., and Reines, Daniel

Subjects

*NUCLEOPROTEINS, *NUCLEAR energy, *GRANULE cells, *CYTOPLASMIC granules, *AMYLOID

Abstract

Ribonucleoprotein (RNP) granules are higher order assemblies of RNA, RNA-binding proteins, and other proteins, that regulate the transcriptome and protect RNAs from environmental challenge. There is a diverse range of RNP granules, many cytoplasmic, which provide various levels of regulation of RNA metabolism. Here we present evidence that the yeast transcription termination factor, Nab3, is targeted to intranuclear granules in response to glucose starvation by Nab3’s proline/glutamine-rich, prion-like domain (PrLD) which can assemble into amyloid in vitro. Localization to the granule is reversible and sensitive to the chemical probe 1,6 hexanediol suggesting condensation is driven by phase separation. Nab3’s RNA recognition motif is also required for localization as seen for other PrLD-containing RNA-binding proteins that phase separate. Although the PrLD is necessary, it is not sufficient to localize to the granule. A heterologous PrLD that functionally replaces Nab3’s essential PrLD, directed localization to the nuclear granule, however a chimeric Nab3 molecule with a heterologous PrLD that cannot restore termination function or viability, does not form granules. The Nab3 nuclear granule shows properties similar to well characterized cytoplasmic compartments formed by phase separation, suggesting that, as seen for other elements of the transcription machinery, termination factor condensation is functionally important. [ABSTRACT FROM AUTHOR]

Published

2018

110. CDHR3 extracellular domains EC1-3 mediate rhinovirus C interaction with cells and as recombinant derivatives, are inhibitory to virus infection.

Author

Watters, Kelly and Palmenberg, Ann C.

Subjects

*VIRUSES, *RHINOVIRUSES, *VERY low-density lipoproteins, *RECOMBINANT proteins, *GENOTYPES, *GENETIC polymorphisms

Abstract

Viruses in the rhinovirus C species (RV-C) are more likely to cause severe wheezing illnesses and asthma exacerbations in children than related isolates of the RV-A or RV-B. The RV-C capsid is structurally distinct from other rhinoviruses and does not bind ICAM-1 or VLDL receptors. The RV-C receptor is instead, human cadherin-related family member 3 (CDHR3), a protein unique to the airway epithelium. A single nucleotide polymorphism (rs6967330, encoding C529Y) in CDHR3 regulates the display density of CDHR3 on cell surfaces and is among the strongest known genetic correlates for childhood virus-induced asthma susceptibility. CDHR3 immunoprecipitations from transfected or transduced cell lysates were used to characterize the RV-C interaction requirements. The C529 and Y529 variations in extracellular repeat domain 5 (EC5), bound equivalently to virus. Glycosylase treatment followed by mass spectrometry mapped 3 extracellular N-linked modification sites, and further detected surface-dependent, α2–6 sialyation unique to the Y529 format. None of these modifications were required for RV-C recognition, but removal or even dilution of structurally stabilizing calcium ions from the EC junctions irreversibly abrogated virus binding. CDHR3 deletions expressed in HeLa cells or as bacterial recombinant proteins, mapped the amino-terminal EC1 unit as the required virus contact. Derivatives containing the EC1 domain, could not only recapitulate virus:receptor interactions in vitro, but also directly inhibit RV-C infection of susceptible cells for several virus genotypes (C02, C15, C41, and C45). We propose that all RV-C use the same EC1 landing pad, interacting with putative EC3-mediated multimerization formats of CDHR3. [ABSTRACT FROM AUTHOR]

Published

2018

111. Conserved mRNA-granule component Scd6 targets Dhh1 to repress translation initiation and activates Dcp2-mediated mRNA decay in vivo.

Author

Zeidan, Quira, Zhang, Fan, Zhang, Hongen, Hinnebusch, Alan G., He, Feng, and Jacobson, Allan

Subjects

*MESSENGER RNA, *PROTEINS, *RNA-protein interactions, *PROTEIN expression, *RIBOSOMES, *RNA sequencing

Abstract

Scd6 protein family members are evolutionarily conserved components of translationally silent mRNA granules. Yeast Scd6 interacts with Dcp2 and Dhh1, respectively a subunit and a regulator of the mRNA decapping enzyme, and also associates with translation initiation factor eIF4G to inhibit translation in cell extracts. However, the role of Scd6 in mRNA turnover and translational repression in vivo is unclear. We demonstrate that tethering Scd6 to a GFP reporter mRNA reduces mRNA abundance via Dcp2 and suppresses reporter mRNA translation via Dhh1. Thus, in a dcp2Δ mutant, tethered Scd6 reduces GFP protein expression with little effect on mRNA abundance, whereas tethered Scd6 has no impact on GFP protein or mRNA expression in a dcp2Δ dhh1Δ double mutant. The conserved LSm domain, but not the RGG domain, of Scd6 is required for translational repression and mRNA turnover by tethered Scd6. Both functions are enhanced in a ccr4Δ mutant, suggesting that the deadenylase function of Ccr4-Not complex interferes with a more efficient repression pathway enlisted by Scd6. Ribosome profiling and RNA-Seq analysis of scd6Δ and dhh1Δ mutants suggests that Scd6 cooperates with Dhh1 in translational repression and turnover of particular native mRNAs, with both processes dependent on Dcp2. Our results suggest that Scd6 can (i) recruit Dhh1 to confer translational repression and (ii) activate mRNA decapping by Dcp2 with attendant degradation of specific mRNAs in vivo, in a manner dependent on the Scd6 LSm domain and modulated by Ccr4. [ABSTRACT FROM AUTHOR]

Published

2018

112. Essentiality of Plasmodium falciparum plasmepsin V.

Author

Boonyalai, Nonlawat, Collins, Christine R., Hackett, Fiona, Withers-Martinez, Chrislaine, and Blackman, Michael J.

Subjects

*PLASMODIUM falciparum, *GENE amplification, *RECOMBINANT DNA, *MICROBIAL virulence, *POLYMERASE chain reaction

Abstract

The malaria parasite replicates within erythrocytes. The pathogenesis of clinical malaria is in large part due to the capacity of the parasite to remodel its host cell. To do this, intraerythrocytic stages of Plasmodium falciparum export more than 300 proteins that dramatically alter the morphology of the infected erythrocyte as well as its mechanical and adhesive properties. P. falciparum plasmepsin V (PfPMV) is an aspartic protease that processes proteins for export into the host erythrocyte and is thought to play a key role in parasite virulence and survival. However, although standard techniques for gene disruption as well as conditional protein knockdown have been previously attempted with the pfpmv gene, complete gene removal or knockdown was not achieved so direct genetic proof that PMV is an essential protein has not been established. Here we have used a conditional gene excision approach combining CRISPR-Cas9 gene editing and DiCre-mediated recombination to functionally inactivate the pfpmv gene. The resulting mutant parasites displayed a severe growth defect. Detailed phenotypic analysis showed that development of the mutant parasites was arrested early in the ring-to-trophozoite transition in the erythrocytic cycle following gene excision. Our findings are the first to elucidate the effects of PMV gene disruption, showing that it is essential for parasite viability in asexual blood stages. The mutant parasites can now be used as a platform to further dissect the Plasmodium protein export pathway. [ABSTRACT FROM AUTHOR]

Published

2018

113. Construction, expression, and characterization of AG11−843 and AG11−1581.

Author

Xie, Yan, Yang, Yan-Tao, Shi, Wei, Ai, Xia, and Xi, Xu-Guang

Subjects

*PROTEIN expression, *DNA copy number variations, *RECOMBINANT proteins, *PROTEIN structure, *GENETIC code

Abstract

Abstract AG1, a member of the DUF1220 protein family, exhibits the most extreme human lineage-specific copy number expansion of any protein-coding sequence in the genome. These variations in copy number have been linked to both brain evolution among primates and brain size in humans. Unfortunately, our current understanding of the structure and function of these proteins is limited because current cloning and expression techniques fail to consistently produce recombinant protein for in vitro studies. The present work describes a method for amino acid and DNA sequence optimization and synthesis, recombinant protein expression and analysis of two AG1 fragments, AG11−843 and AG11−1581. It was first necessary to modify the nucleotide sequence, while holding the GC content at 52.9%. The genes were then sectionally synthesized by overlap PCR. The resulting segments were cloned into the pET-15 b-sumo expression vector and subsequently transformed into BL21 (DE3) cells. After inducing their expression, the AG11−843 and AG11−1581 proteins were isolated and purified. Furthermore, using dynamic light scattering and gel filtration analysis, AG11−843 and AG11−1581 were shown to be present in tetrameric and dimeric forms in solution. To our knowledge, this is the first study to synthesize and express fragments of the DUF1220 protein family for in vitro analysis. Taken together, the proven utility and versatility of this method indicate that it can be used as an effective technique to construct and express other proteins with complicated sequences, thus providing the means to study their function and structure in vitro. Highlights • A method of DNA codon optimization, synthesis, recombinant protein expression with complicated sequences was provided. • Sequence analysis and synonymous codon substitution was used for sequence optimization. • Overlap PCR was used for the sequence synthesis. • The recombinant proteins AG11−843 and AG11−1581 were over expressed and purified for further analysis. • The existence state in solution of AG11−843 and AG11−1581 were analyzed by DLS and gel filtration. [ABSTRACT FROM AUTHOR]

Published

2018

114. The effect of proteotoxic stress on human tau protein aggregation and toxicity expressed in yeast Saccharomyces cerevisiae

Author

Zubčić, Karla, Boban, Mirta, Šimić, Goran, Višnjić, Dora, Šalković-Petrišić, Melita, Švob Štrac, Dubravka, Jazvinšćak Jembrek, Maja, and Pećina-Šlaus, Nives

Subjects

molecular cloning, protein quality control system, proteotoxic stress, luminescent reporter Tau-NanoBit, plasmid construction, yeast Saccharomyces cerevisiae, genetic screening, Alzheimer's disease, tau protein, tau protein agregation

Abstract

Nakupljanje agregata proteina tau u neurofibrilarne snopiće najistaknutije je histopatološko obilježje Alzheimerove bolesti. U zdravim neuronima tau ima karakteristike topljivog proteina te je uglavnom vezan za mikrotubule aksona, dok u neuronima zahvaćenim patologijom tvori agregate i akumulira se u somi i dendritima. Količina agregata i širenje neurofibrilarnih promjena u mozgu u izravnoj su korelaciji s napredovanjem bolesti i stupnjem kognitivnog oštećenja. Glavni rizični čimbenik za nastanak Alzheimerove bolesti je starenje, no točni uzroci agregacije tau još nisu potpuno razjašnjeni. Budući da su putevi agregacije proteina evolucijski konzervirani, radi genetičkog pristupa otkrivanju čimbenika agregacije i toksičnosti proteina tau, u ovom smo radu kao stanični model odabrali kvasac Saccharomyces cerevisiae. Kako bismo bolje razumjeli rane korake u tau patologiji, uspostavili smo i upotrijebili molekularni alat za proučavanje oligomerizacije tau u živim stanicama, temeljen na luminiscenciji, u kojem interakcija dvaju tau proteina rezultira komplementacijom luciferaze NanoLuc i luminiscencijom. Istražili smo dovode li različiti čimbenici, napose proteotoksični stres, do agregacije tau te smo ispitali toksičnost proteina tau u stanicama kvasca u uvjetima stresa. Pokazali smo da proteotoksični stres ne doprinosi oligomerizaciji i toksičnosti tau u stanicama kvasca. Uspostavljeni reporter tau-NanoBiT omogućit će genetički probir čimbenika agregacije i toksičnosti tau proteina u daljnjim istraživanjima., The main histopathological hallmark of Alzheimer’s disease are neurofibrillary tangles - large aggregates of protein tau. In healthy neurons, tau is a soluble protein mostly bound to the microtubules in axons, however in the affected neurons, tau accumulates in the soma and dendrites and forms aggregates. The number of tangles and the spread of neurofibrillary changes in the brain are directly correlated with the progression of the disease. The causes of tau aggregation are not completely clear. Since many molecular pathways of protein aggregation are evolutionarily conserved, we have chosen yeast Saccharomyces cerevisiae as a cell model to study the factors of tau aggregation. To better understand the early steps in tau pathology, we used a molecular tool for studying tau oligomerization in living cells, based on the luminescent reporter NanoBiT, in which tau protein interaction results in complementation of NanoLuc luciferase. We investigated how different factors, especially proteotoxic stress, affect tau aggregation and examined the toxicity of tau in yeast cells under stress conditions. We have shown that proteotoxic stress does not contribute to tau oligomerization and toxicity in yeast cells. The established tau-NanoBiT reporter will enable genetic screens for the aggregation factors and tau protein toxicity in future research.

Published

2023

115. Rapid Deletion Plasmid Construction Methods for Protoplast and Agrobacterium-based Fungal Transformation Systems

Author

García-Pedrajas, María D., Paz, Zahi, Andrews, David L., Baeza-Montañez, Lourdes, Gold, Scott E., Gupta, Vijai Kumar, editor, Tuohy, Maria G., editor, Ayyachamy, Manimaran, editor, Turner, Kevin M., editor, and O’Donovan, Anthonia, editor

Published

2013

116. BLM prevents instability of structure-forming DNA sequences at common fragile sites.

Author

Wang, Hailong, Li, Shibo, Zhang, Huimin, Wang, Ya, Hao, Shuailin, and Wu, Xiaohua

Subjects

*NUCLEOTIDE sequence, *GENETIC recombination, *MITOSIS, *GENE expression, *HELICASES

Abstract

Genome instability often arises at common fragile sites (CFSs) leading to cancer-associated chromosomal rearrangements. However, the underlying mechanisms of how CFS protection is achieved is not well understood. We demonstrate that BLM plays an important role in the maintenance of genome stability of structure-forming AT-rich sequences derived from CFSs (CFS-AT). BLM deficiency leads to increased DSB formation and hyper mitotic recombination at CFS-AT and induces instability of the plasmids containing CFS-AT. We further showed that BLM is required for suppression of CFS breakage upon oncogene expression. Both helicase activity and ATR-mediated phosphorylation of BLM are important for preventing genetic instability at CFS-AT sequences. Furthermore, the role of BLM in protecting CFS-AT is not epistatic to that of FANCM, a translocase that is involved in preserving CFS stability. Loss of BLM helicase activity leads to drastic decrease of cell viability in FANCM deficient cells. We propose that BLM and FANCM utilize different mechanisms to remove DNA secondary structures forming at CFS-AT on replication forks, thereby preventing DSB formation and maintaining CFS stability. [ABSTRACT FROM AUTHOR]

Published

2018

117. De novo biosynthesis of myricetin, kaempferol and quercetin in Streptomyces albus and Streptomyces coelicolor.

Author

Marín, Laura, Gutiérrez-del-Río, Ignacio, Entrialgo-Cadierno, Rodrigo, Villar, Claudio J., and Lombó, Felipe

Subjects

*BIOSYNTHESIS, *MYRICETIN, *QUERCETIN, *STREPTOMYCES coelicolor, *FLAVONOLS

Abstract

Flavonols are a flavonoid subfamily widely distributed in plants, including several ones of great importance in human and animal diet (apple, tomato, broccoli, onion, beans, tea). These polyphenolic nutraceuticals exert potent antimicrobial (membrane potential disruptors), antioxidant (free-radical scavengers), pharmacokinetic (CYP450 modulators), anti-inflammatory (lipoxygenase inhibitors), antiangiogenic (VEGF inhibitors) and antitumor (cyclin inhibitors) activities. Biotechnological production of these nutraceuticals, for example via heterologous biosynthesis in industrial actinomycetes, is favored since in plants these polyphenols appear as inactive glycosylated derivatives, in low concentrations or as part of complex mixtures with other polyphenolic compounds. In this work, we describe the de novo biosynthesis of three important flavonols, myricetin, kaempferol and quercetin, in the industrially relevant actinomycetes Streptomyces coelicolor and S. albus. De novo biosynthesis of kaempferol, myricetin and quercetin in actinomycetes has not been described before. [ABSTRACT FROM AUTHOR]

Published

2018

118. RepB C-terminus mutation of a pRi-repABC binary vector affects plasmid copy number in Agrobacterium and transgene copy number in plants.

Author

Vaghchhipawala, Zarir, Radke, Sharon, Nagy, Ervin, Russell, Mary L., Johnson, Susan, Gelvin, Stanton B., Gilbertson, Larry A., and Ye, Xudong

Subjects

*GENETIC mutation, *PLASMIDS, *AGROBACTERIUM, *BOTANY, *VIRAL replication, *NUCLEOTIDE sequencing

Abstract

A native repABC replication origin from pRiA4b was previously reported as a single copy plasmid in Agrobacterium tumefaciens and can improve the production of transgenic plants with a single copy insertion of transgenes when it is used in binary vectors for Agrobacterium-mediated transformation. A high copy pRi-repABC variant plasmid, pTF: :Ri, which does not improve the frequency of single copy transgenic plants, has been reported in the literature. Sequencing the high copy pTF: :Ri repABC operon revealed the presence of two mutations: one silent mutation and one missense mutation that changes a tyrosine to a histidine (Y299H) in a highly conserved area of the C-terminus of the RepB protein (RepBY299H). Reproducing these mutations in the wild-type pRi-repABC binary vector showed that Agrobacterium cells with the RepBY299H mutation grow faster on both solidified and in liquid medium, and have higher plasmid copy number as determined by ddPCR. In order to investigate the impact of the RepBY299H mutation on transformation and quality plant production, the RepBY299H mutated pRi-repABC binary vector was compared with the original wild-type pRi-repABC binary vector and a multi-copy oriV binary vector in canola transformation. Molecular analyses of the canola transgenic plants demonstrated that the multi-copy pRi-repABC with the RepBY299H mutation provides no advantage in generating high frequency single copy, backbone-free transgenic plants in comparison with the single copy wild-type pRi-repABC binary vector. [ABSTRACT FROM AUTHOR]

Published

2018

119. The “speed gene” effect of myostatin arises in Thoroughbred horses due to a promoter proximal SINE insertion.

Author

Rooney, Mary F., Hill, Emmeline W., Kelly, Vincent P., and Porter, Richard K.

Subjects

*MYOSTATIN, *THOROUGHBRED horse, *GENETIC polymorphisms, *GENE expression, *AEROBIC capacity, *SKELETAL muscle

Abstract

Thoroughbred horses are finely-tuned athletes with a high aerobic capacity relative to skeletal muscle mass, attributable to centuries of genetic selection for speed and stamina. Polymorphisms in the myostatin gene (MSTN), a pronounced inhibitor of skeletal muscle growth, have been shown to almost singularly account for gene-based race distance aptitude in racehorses. In Thoroughbreds, two MSTN polymorphisms, a single nucleotide variation in the first intron (SNP g.66493737C>T) and a non-coding transposable element within the promoter region (a 227 bp SINE insertion) are of particular interest. Until now, it has not been clear which of these variants affect skeletal muscle phenotypes or whether both can impact racing performance. In a large cohort of Thoroughbreds, we observed a complete concordance between the SNP and the SINE insertion. By means of in vitro assays in C2C12 myoblasts, we isolated the SNP variant from the SINE polymorphism and showed the latter is exclusively responsible for adversely affecting transcription initiation and gene expression thereby limiting myostatin protein production. Mapping the MSTN transcription start site in horse skeletal muscle likewise revealed anomalous transcription initiation in the presence of the SINE insertion. Our data provides mechanistic evidence that the SINE insertion uniquely accounts for the MSTN “speed gene” effect on race distance aptitude in the Thoroughbred horse. [ABSTRACT FROM AUTHOR]

Published

2018

120. The yeast stress inducible Ssa Hsp70 reduces α-synuclein toxicity by promoting its degradation through autophagy.

Author

Gupta, Arpit, Puri, Anuradhika, Singh, Prashant, Sonam, Surabhi, Pandey, Richa, and Sharma, Deepak

Subjects

*AUTOPHAGY, *BIOCHEMISTRY, *CARBOHYDRATES, *SYNUCLEINS, *CARRIER proteins, *MOLECULAR biology

Abstract

The mechanism underlying the role of Hsp70s in toxicity associated with intracellular accumulation of toxic protein inclusions is under intense investigation. In current study, we examined the roles of all different isoforms of yeast cytosolic Ssa Hsp70 on α-synuclein mediated cellular toxicity. The study showed that yeast cells expressing stress-inducible Ssa3 or Ssa4 as sole Ssa Hsp70 isoforms, reduced α-synuclein toxicity better than those expressing a constitutive counterpart. The protective effect of stress-inducible Ssa Hsp70s was not α-syn specific, but more general to other inclusion forming proteins such as polyQ. We show that the protective effect is not by induction of a general stress response in Ssa3 cells rather by promoting α-synuclein degradation through autophagy. The present study revealed that effect of Hsp70s was isoform dependent, and that autophagy protects Ssa3 cells from the deleterious effects of toxic protein inclusions. [ABSTRACT FROM AUTHOR]

Published

2018

121. Development of reverse genetics systems and investigation of host response antagonism and reassortment potential for Cache Valley and Kairi viruses, two emerging orthobunyaviruses of the Americas.

Author

Dunlop, James I., Szemiel, Agnieszka M., Navarro, Aitor, Wilkie, Gavin S., Tong, Lily, Modha, Sejal, Mair, Daniel, Sreenu, Vattipally B., Da Silva Filipe, Ana, Li, Ping, Huang, Yan-Jang S., Brennan, Benjamin, Hughes, Joseph, Vanlandingham, Dana L., Higgs, Stephen, Elliott, Richard M., and Kohl, Alain

Subjects

*TYPE I interferons, *REVERSE genetics, *LAMB carcasses, *CELL lines, *ANIMAL vaccination

Abstract

Orthobunyaviruses such as Cache Valley virus (CVV) and Kairi virus (KRIV) are important animal pathogens. Periodic outbreaks of CVV have resulted in the significant loss of lambs on North American farms, whilst KRIV has mainly been detected in South and Central America with little overlap in geographical range. Vaccines or treatments for these viruses are unavailable. One approach to develop novel vaccine candidates is based on the use of reverse genetics to produce attenuated viruses that elicit immune responses but cannot revert to full virulence. The full genomes of both viruses were sequenced to obtain up to date genome sequence information. Following sequencing, minigenome systems and reverse genetics systems for both CVV and KRIV were developed. Both CVV and KRIV showed a wide in vitro cell host range, with BHK-21 cells a suitable host cell line for virus propagation and titration. To develop attenuated viruses, the open reading frames of the NSs proteins were disrupted. The recombinant viruses with no NSs protein expression induced the production of type I interferon (IFN), indicating that for both viruses NSs functions as an IFN antagonist and that such attenuated viruses could form the basis for attenuated viral vaccines. To assess the potential for reassortment between CVV and KRIV, which could be relevant during vaccination campaigns in areas of overlap, we attempted to produce M segment reassortants by reverse genetics. We were unable to obtain such viruses, suggesting that it is an unlikely event. [ABSTRACT FROM AUTHOR]

Published

2018

122. Implications of the expression of Enterococcus faecalis citrate fermentation genes during infection.

Author

Martino, Gabriela P., Perez, Cristian E., Magni, Christian, and Blancato, Víctor S.

Subjects

*ENTEROCOCCUS faecalis, *BACTERIAL diseases, *GENE expression in bacteria, *FERMENTATION, *DECARBOXYLASES

Abstract

Citrate is an ubiquitous compound in nature. However, citrate fermentation is present only in a few pathogenic or nonpathogenic microorganisms. The citrate fermentation pathway includes a citrate transporter, a citrate lyase complex, an oxaloacetate decarboxylase and a regulatory system. Enterococcus faecalis is commonly present in the gastro-intestinal microbiota of warm-blooded animals and insect guts. These bacteria can also cause infection and disease in immunocompromised individuals. In the present study, we performed whole genome analysis in Enterococcus strains finding that the complete citrate pathway is present in all of the E. faecalis strains isolated from such diverse habitats as animals, hospitals, water, milk, plants, insects, cheese, etc. These results indicate the importance of this metabolic preservation for persistence and growth of E. faecalis in different niches. We also analyzed the role of citrate metabolism in the E. faecalis pathogenicity. We found that an E. faecalis citrate fermentation-deficient strain was less pathogenic for Galleria mellonella larvae than the wild type. Furthermore, strains with deletions in the oxaloacetate decarboxylase subunits or in the α-acetolactate synthase resulted also less virulent than the wild type strain. We also observed that citrate promoters are induced in blood, urine and also in the hemolymph of G. mellonella. In addition, we showed that citrate fermentation allows E. faecalis to grow better in blood, urine and G. mellonella. The results presented here clearly indicate that citrate fermentation plays an important role in E. faecalis opportunistic pathogenic behavior. [ABSTRACT FROM AUTHOR]

Published

2018

123. A simple approach for multi-targeted shRNA-mediated inducible knockdowns using Sleeping Beauty vectors.

Author

Fink, Severin, Zugelder, Laurens, Roth, Bernhard, Brandt, Evelyn, Meloche, Sylvain, Izsvák, Zsuzsanna, Bargou, Ralf C., and Stühmer, Thorsten

Subjects

*MESSENGER RNA, *GENE expression, *PLASMIDS, *MITOGEN-activated protein kinases, *MOLECULAR biology

Abstract

shRNA expression is an established technique to transiently or permanently deplete cells of a particular mRNA/protein. In functional analyses of oncogenic pathways it can thus be used as an alternative to pharmacologic inhibitors, or as a means to address otherwise undruggable targets. Here we describe and functionally validate a simple reiterative cloning system to generate concatenated multi-shRNA expression plasmids. The multi-shRNA expression cassette can eventually be subcloned into any suitably designed vector for the stable transfection of cells, here tested with derivatives of the Sleeping Beauty transposon vector for stable transfection of multiple myeloma cell lines at the lowest biosafety level. We finally test inducible versions of such multi-cassette knockdown vectors and show their efficacy for the induced concerted knockdown of all four components of the MEK/MAPK-module in the Ras/MAPK pathway. The described vector system(s) should be useful for functional knockdown analyses in a wide array of cell line models. [ABSTRACT FROM AUTHOR]

Published

2018

124. Type II restriction modification system in Ureaplasma parvum OMC-P162 strain.

Author

Wu, Heng Ning, Nakura, Yukiko, Yoshimura, Michinobu, Gaddi Tantengco, Ourlad Alzeus, Nomiyama, Makoto, Takayanagi, Toshimitsu, Fujita, Tomio, Yasukawa, Kiyoshi, and Yanagihara, Itaru

Subjects

*UREAPLASMA, *METHYLCYTOSINE, *GESTATIONAL age, *OPERONS, *DNA methyltransferases

Abstract

Ureaplasma parvum serovar 3 strain, OMC-P162, was isolated from the human placenta of a preterm delivery at 26 weeks’ gestation. In this study, we sequenced the complete genome of OMC-P162 and compared it with other serovar 3 strains isolated from patients with different clinical conditions. Ten unique genes in OMC-P162, five of which encoded for hypothetical proteins, were identified. Of these, genes UPV_229 and UPV_230 formed an operon whose open reading frames were predicted to code for a DNA methyltransferase and a hypothetical protein, respectively. DNA modification analysis of the OMC-P162 genome identified N4-methylcytosine (m4C) and N6-methyladenine (m6A), but not 5-methylocytosine (m5C). UPV230 recombinant protein displayed endonuclease activity and recognized the CATG sequence, resulting in a blunt cut between A and T. This restriction enzyme activity was identical to that of the cultivated OMC-P162 strain, suggesting that this restriction enzyme was naturally expressed in OMC-P162. We designated this enzyme as UpaP162. Treatment of pT7Blue plasmid with recombinant protein UPV229 completely blocked UpaP162 restriction enzyme activity. These results suggest that the UPV_229 and UPV_230 genes act as a type II restriction-modification system in Ureaplasma OMC-P162. [ABSTRACT FROM AUTHOR]

Published

2018

125. Simplified inducible system for Trypanosoma brucei.

Author

Niemirowicz, Gabriela T., Cazzulo, Juan J., Álvarez, Vanina E., and Bouvier, León A.

Subjects

*TRYPANOSOMA brucei, *GENETIC transcription, *RIBOSOMAL RNA, *RNA sequencing, *PROMOTERS (Genetics)

Abstract

Nowadays, most reverse genetics approaches in Trypanosoma brucei, a protozoan parasite of medical and veterinary importance, rely on pre-established cell lines. Consequently, inducible experimentation is reduced to a few laboratory strains. Here we described a new transgene expression system based exclusively on endogenous transcription activities and a minimum set of regulatory components that can easily been adapted to different strains. The pTbFIX vectors are designed to contain the sequence of interest under the control of an inducible rRNA promoter along with a constitutive dicistronic unit encoding a nucleus targeted tetracycline repressor and puromycin resistance genes in a tandem “head-to-tail” configuration. Upon doxycycline induction, the system supports regulatable GFP expression (170 to 400 fold) in both bloodstream and procyclic T. brucei forms. Furthermore we have adapted the pTbFIX plasmid to perform RNAi experimentation. Lethal phenotypes, including α-tubulin and those corresponding to the enolase and clathrin heavy chain genes, were successfully recapitulated in procyclic and bloodstream parasites thus showing the versatility of this new tool. [ABSTRACT FROM AUTHOR]

Published

2018

126. Desiccation tolerance in Acinetobacter baumannii is mediated by the two-component response regulator BfmR.

Author

IIIFarrow, John M., Wells, Greg, and Pesci, Everett C.

Subjects

*ACINETOBACTER baumannii, *DEHYDRATION, *BACTERIAL growth, *SUGAR-free liquid medication, *HYDROGEN peroxide

Abstract

For the opportunistic pathogen Acinetobacter baumannii, desiccation tolerance is thought to contribute significantly to the persistence of these bacteria in the healthcare environment. We investigated the ability of A. baumannii to survive rapid drying, and found that some strains exhibited a profoundly desiccation-resistant phenotype, characterized by the ability of a large proportion of cells to survive on a dry surface for an extended period of time. However, this phenotype was only displayed during the stationary phase of growth. Most interestingly, we found that drying resistance could be lost after extended cultivation in liquid medium. Genome sequencing of isolates that became drying-sensitive identified mutations in bfmR, which encodes a two-component response regulator that is important for A. baumannii virulence. Additionally, BfmR was necessary for the expression of stress-related proteins during stationary phase, and one of these, KatE, was important for long-term drying survival. These results suggested that BfmR may control stress responses, and we demonstrated that the ΔbfmR mutant was more sensitive to hydrogen peroxide, nutrient starvation, and increased osmolarity. We also found that cross-protection against drying could be stimulated by either starvation, which required BfmR, or increased osmolarity. These results imply that BfmR plays a role in controlling stress responses in A. baumannii which help protect cells during desiccation, and they provide a regulatory link between this organism’s ability to persist in the environment and pathogenicity. [ABSTRACT FROM AUTHOR]

Published

2018

127. Aminoglycoside-inducible expression of the mexAB-oprM multidrug efflux operon in Pseudomonas aeruginosa: Involvement of the envelope stress-responsive AmgRS two-component system.

Author

Fruci, Michael and Poole, Keith

Subjects

*AMINOGLYCOSIDES, *PSEUDOMONAS aeruginosa, *BACTERIAL operons, *PHYSIOLOGICAL stress, *LOCUS (Genetics)

Abstract

Exposure of P. aeruginosa to the aminoglycoside (AG) paromomycin (PAR) induced expression of the PA3720-armR locus and the mexAB-oprM multidrug efflux operon that AmgR controls, although PAR induction of mexAB-oprM was independent of armR. Multiple AGs promoted mexAB-oprM expression and this was lost in the absence of the amgRS locus encoding an aminoglycoside-activated envelope stress-responsive 2-component system (TCS). Purified AmgR bound to the mexAB-oprM promoter region consistent with this response regulator directly regulating expression of the efflux operon. The thiol-active reagent, diamide, which, like AGs, promotes protein aggregation and cytoplasmic membrane damage also promoted AmgRS-dependent mexAB-oprM expression, a clear indication that the MexAB-OprM efflux system is recruited in response to membrane perturbation and/or circumstances that lead to this. Despite the AG and diamide induction of mexAB-oprM, however, MexAB-OprM does not appear to contribute to resistance to these agents. [ABSTRACT FROM AUTHOR]

Published

2018

128. Identification of a VapA virulence factor functional homolog in Rhodococcus equi isolates housing the pVAPB plasmid.

Author

Willingham-Lane, Jennifer M., Coulson, Garry B., and Hondalus, Mary K.

Subjects

*RHODOCOCCUS equi, *MICROBIAL virulence, *HOMOLOGY (Biochemistry), *IMMUNOCOMPROMISED patients, *PLASMIDS, *MACROPHAGES

Abstract

Rhodococcus equi is a facultative intracellular bacterium of macrophages and is an important pathogen of animals and immunocompromised people wherein disease results in abcessation of the lungs and other sites. Prior work has shown that the presence of the major virulence determinant, VapA, encoded on the pVAPA-type plasmid, disrupts normal phagosome development and is essential for bacterial replication within macrophages. pVAPA- type plasmids are typical of R. equi strains derived from foals while strains from pigs carry plasmids of the pVAPB-type, lacking vapA, and those from humans harbor various types of plasmids including pVAPA and pVAPB. Through the creation and analysis of a series of gene deletion mutants, we found that vapK1 or vapK2 is required for optimal intracellular replication of an R. equi isolate carrying a pVAPB plasmid type. Complementation analysis of a ΔvapA R. equi strain with vapK1 or vapK2 showed the VapK proteins of the pVAPB-type plasmid could restore replication capacity to the macrophage growth-attenuated ΔvapA strain. Additionally, in contrast to the intracellular growth capabilities displayed by an equine R. equi transconjugant strain carrying a pVAPB-type plasmid, a transconjugant strain carrying a pVAPB-type plasmid deleted of vapK1 and vapK2 proved incapable of replication in equine macrophages. Cumulatively, these data indicate that VapK1 and K2 are functionally equivalent to VapA. [ABSTRACT FROM AUTHOR]

Published

2018

129. Scavenger receptor-C acts as a receptor for Bacillus thuringiensis vegetative insecticidal protein Vip3Aa and mediates the internalization of Vip3Aa via endocytosis.

Author

Jiang, Kun, Hou, Xiao-yue, Tan, Tong-tong, Cao, Zhang-lei, Mei, Si-qi, Yan, Bing, Chang, Jin, Han, Lu, Zhao, Dan, and Cai, Jun

Subjects

*SCAVENGER receptors (Biochemistry), *VIRAL receptors, *BACILLUS thuringiensis, *ENDOCYTOSIS, *PROTEINS

Abstract

The vegetative insecticidal proteins (Vip), secreted by many Bacillus thuringiensis strains during their vegetative growth stage, are genetically distinct from known insecticidal crystal proteins (ICPs) and represent the second-generation insecticidal toxins. Compared with ICPs, the insecticidal mechanisms of Vip toxins are poorly understood. In particular, there has been no report of a definite receptor of Vip toxins to date. In the present study, we identified the scavenger receptor class C like protein (Sf-SR-C) from the Spodoptera frugiperda (Sf9) cells membrane proteins that bind to the biotin labeled Vip3Aa, via the affinity magnetic bead method coupled with HPLC-MS/MS. We then certified Vip3Aa protoxin could interact with Sf-SR-C in vitro and ex vivo. In addition, downregulation of SR-C expression in Sf9 cells and Spodoptera exigua larvae midgut reduced the toxicity of Vip3Aa to them. Coincidently, heterologous expression of Sf-SR-C in transgenic Drosophila midgut significantly enhanced the virulence of Vip3Aa to the Drosophila larvae. Moreover, the complement control protein domain and MAM domain of Sf-SR-C are involved in the interaction with Vip3Aa protoxin. Furthermore, endocytosis of Vip3Aa mediated by Sf-SR-C correlates with its insecticidal activity. Our results confirmed for the first time that Sf-SR-C acts as a receptor for Vip3Aa protoxin and provides an insight into the mode of action of Vip3Aa that will significantly facilitate the study of its insecticidal mechanism and application. [ABSTRACT FROM AUTHOR]

Published

2018

130. Light control of G protein signaling pathways by a novel photopigment.

Author

Osorno, Tomás, Arenas, Oscar, Ramírez-Suarez, Nelson J., Echeverry, Fabio A., Gomez, María del Pilar, and Nasi, Enrico

Subjects

*G proteins, *CELLULAR signal transduction, *PHOTOSYNTHETIC pigments, *MEMBRANE potential, *GENE expression, *NEUROSCIENCES

Abstract

Channelopsins and photo-regulated ion channels make it possible to use light to control electrical activity of cells. This powerful approach has lead to a veritable explosion of applications, though it is limited to changing membrane voltage of the target cells. An enormous potential could be tapped if similar opto-genetic techniques could be extended to the control of chemical signaling pathways. Photopigments from invertebrate photoreceptors are an obvious choice—as they do not bleach upon illumination -however, their functional expression has been problematic. We exploited an unusual opsin, pScop2, recently identified in ciliary photoreceptors of scallop. Phylogenetically, it is closer to vertebrate opsins, and offers the advantage of being a bi-stable photopigment. We inserted its coding sequence and a fluorescent protein reporter into plasmid vectors and demonstrated heterologous expression in various mammalian cell lines. HEK 293 cells were selected as a heterologous system for functional analysis, because wild type cells displayed the largest currents in response to the G-protein activator, GTP-γ-S. A line of HEK cells stably transfected with pScop2 was generated; after reconstitution of the photopigment with retinal, light responses were obtained in some cells, albeit of modest amplitude. In native photoreceptors pScop2 couples to Go; HEK cells express poorly this G-protein, but have a prominent Gq/PLC pathway linked to internal Ca mobilization. To enhance pScop2 competence to tap into this pathway, we swapped its third intracellular loop—important to confer specificity of interaction between 7TMDRs and G-proteins—with that of a Gq-linked opsin which we cloned from microvillar photoreceptors present in the same retina. The chimeric construct was evaluated by a Ca fluorescence assay, and was shown to mediate a robust mobilization of internal calcium in response to illumination. The results project pScop2 as a potentially powerful optogenetic tool to control signaling pathways. [ABSTRACT FROM AUTHOR]

Published

2018

131. Regulation of the NRF2 transcription factor by andrographolide and organic extracts from plant endophytes.

Author

Wong, Daphne Pei Wen, Ng, Mei Ying, Leung, Jia Yu, Boh, Boon Kim, Lim, Ee Chien, Tan, Shi Hua, Lim, Shuying, Seah, Wen Hui, Hu, Christine Zhiwen, Ho, Boon Chuan, Ng, Daphne Hui Ping, and Hagen, Thilo

Subjects

*ENDOPHYTES, *TRANSCRIPTION factors, *PROTEIN expression, *CANCER treatment, *TARGETED drug delivery, THERAPEUTIC use of plant extracts

Abstract

The transcription factor NF-E2 Related Factor-2 (NRF2) is an important drug target. Activation of NRF2 has chemopreventive effects in cancer and exerts beneficial effects in a number of diseases, including neurodegenerative diseases, inflammatory diseases, hepatosteatosis, obesity and insulin resistance. Hence, there have been great efforts to discover and characterize novel NRF2 activators. One reported NRF2 activator is the labdane diterpenoid andrographolide. In this study, we identified the mechanism through which andrographolide activates NRF2. We showed that andrographolide inhibits the function of KEAP1, a protein that together with CUL3 and RBX1 forms an E3 ubiquitin ligase that polyubiquitinates NRF2. Andrographolide partially inhibits the interaction of KEAP1 with CUL3 in a manner dependent on Cys151 in KEAP1. This suggests that andrographolide forms Michael acceptor dependent adducts with Cys151 in KEAP1 in vivo, leading to inhibition of NRF2 ubiquitination and consequently accumulation of the transcription factor. Interestingly, we also showed that at higher concentrations andrographolide increases NRF2 protein expression in a Cys151 independent, but likely KEAP1 dependent manner, possibly through modification of other Cys residues in KEAP1. In this study we also screened secondary metabolites produced by endophytes isolated from non-flowering plants for NRF2-inducing properties. One of the extracts, ORX 41, increased both NRF2 protein expression and transcriptional activity markedly. These results suggest that endophytes isolated from non-flowering or other plants may be a good source of novel NRF2 inducing compounds. [ABSTRACT FROM AUTHOR]

Published

2018

132. 单质粒哺乳动物单杂交系统的构建及功能评价.

Author

陈凡, 林木贵, 程亚丽, and 林梅西

Abstract

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Published

2018

133. Identification of putative effectors of the Type IV secretion system from the Wolbachia endosymbiont of Brugia malayi.

Author

Carpinone, Emily M., Li, Zhiru, Mills, Michael K., Foltz, Clemence, Brannon, Emma R., Carlow, Clotilde K. S., and Starai, Vincent J.

Subjects

*WOLBACHIA, *SECRETION, *BRUGIA malayi, *VERTICAL transmission (Communicable diseases), *FILARIASIS

Abstract

Wolbachia is an unculturable, intracellular bacterium that persists within an extremely broad range of arthropod and parasitic nematode hosts, where it is transmitted maternally to offspring via vertical transmission. In the filarial nematode Brugia malayi, a causative agent of human lymphatic filariasis, Wolbachia is an endosymbiont, and its presence is essential for proper nematode development, survival, and pathogenesis. While the elucidation of Wolbachia:nematode interactions that promote the bacterium’s intracellular persistence is of great importance, research has been hampered due to the fact that Wolbachia cannot be cultured in the absence of host cells. The Wolbachia endosymbiont of B. malayi (wBm) has an active Type IV secretion system (T4SS). Here, we have screened 47 putative T4SS effector proteins of wBm for their ability to modulate growth or the cell biology of a typical eukaryotic cell, Saccharomyces cerevisiae. Five candidates strongly inhibited yeast growth upon expression, and 6 additional proteins showed toxicity in the presence of zinc and caffeine. Studies on the uptake of an endocytic vacuole-specific fluorescent marker, FM4-64, identified 4 proteins (wBm0076 wBm00114, wBm0447 and wBm0152) involved in vacuole membrane dynamics. The WAS(p)-family protein, wBm0076, was found to colocalize with yeast cortical actin patches and disrupted actin cytoskeleton dynamics upon expression. Deletion of the Arp2/3-activating protein, Abp1p, provided resistance to wBm0076 expression, suggesting a role for wBm0076 in regulating eukaryotic actin dynamics and cortical actin patch formation. Furthermore, wBm0152 was found to strongly disrupt endosome:vacuole cargo trafficking in yeast. This study provides molecular insight into the potential role of the T4SS in the Wolbachia endosymbiont:nematode relationship. [ABSTRACT FROM AUTHOR]

Published

2018

134. Cyclin-dependent kinase modulates budding yeast Rad5 stability during cell cycle.

Author

Hayashi, Masafumi, Keyamura, Kenji, and Hishida, Takashi

Subjects

*CYCLIN-dependent kinases, *IMMUNOMODULATORS, *CELL cycle, *DNA damage, *DNA synthesis

Abstract

The DNA damage tolerance (DDT) pathway facilitates the bypass of the fork-blocking lesions without removing them through either translesion DNA synthesis or error-free damage bypass mechanism. The Saccharomyces cerevisiae Rad5 is a multi-functional protein involved in the error-free branch of the DDT pathway, and its protein level periodically fluctuates through the cell cycle; however, the mechanistic basis and functional importance of the Rad5 level for the cell cycle regulation remain unclear. Here, we show that Rad5 is predominantly phosphorylated on serine 130 (S130) during S/G2 phase and that this modification depends on the cyclin-dependent kinase Cdc28/CDK1. We also show that the phosphorylated Rad5 species at S130 exhibit a relatively short half-life compared with non-phosphorylated Rad5 moiety, and that the Rad5 protein is partially stabilized in phosphorylation-defective rad5 S130A cells. Importantly, the elimination of this modification results in a defective cell-cycle dependent Rad5 oscillation pattern. Together, our results demonstrate that CDK1 modulates Rad5 stability by phosphorylation during the cell cycle, suggesting a crosstalk between the phosphorylation and degradation of Rad5. [ABSTRACT FROM AUTHOR]

Published

2018

135. Highly multiplexed genome engineering using CRISPR/Cas9 gRNA arrays.

Author

Kurata, Morito, Wolf, Natalie K., Lahr, Walker S., Weg, Madison T., Kluesner, Mitchell G., Lee, Samantha, Hui, Kai, Shiraiwa, Masano, Webber, Beau R., and Moriarity, Branden S.

Subjects

*GENETIC engineering, *CRISPRS, *RIBONUCLEASES, *NUCLEOTIDE sequence, *PROMOTERS (Genetics)

Abstract

The CRISPR/Cas9 system is an RNA guided nuclease system that evolved as a mechanism of adaptive immunity in bacteria. This system has been adopted for numerous genome engineering applications in research and recently, therapeutics. The CRISPR/Cas9 system has been largely implemented by delivery of Cas9 as protein, RNA, or plasmid along with a chimeric crRNA-tracrRNA guide RNA (gRNA) under the expression of a pol III promoter, such as U6. Using this approach, multiplex genome engineering has been achieved by delivering several U6-gRNA plasmids targeting multiple loci. However, this approach is limited due to the efficiently of delivering multiple plasmids to a single cell at one time. To augment the capability and accessibility of multiplexed genome engineering, we developed an efficient golden gate based method to assemble gRNAs linked by optimal Csy4 ribonuclease sequences to deliver up to 10 gRNAs as a single gRNA array transcript. Here we report the optimal expression of our guide RNA array under a strong pol II promoter. This system can be implemented alongside the myriad of CRISPR applications, allowing users to model complex biological processes requiring numerous gRNAs. [ABSTRACT FROM AUTHOR]

Published

2018

136. 基质金属蛋白酶2基因野生型和G1207A突变型质粒构建与鉴定.

Author

罗家明, 朱红, 张微, 王成芳, and 陈蓉

Abstract

Objective To study the function of matrix metalloproteinase 2( MMP2) gene, and to construct the wild type and G1207 A mutant plasmids of MMP2 gene. Methods Wild type and mutation site G1207 A of MMP2 gene were amplified by polymerase chain reaction( PCR) and site-directed mutagenesis, and then we cloned into p UC57 plasmid and identified them by DNA restriction endonuclease profiling and plasmid sequencing. Results The length of PCR amplification products of MMP2 gene wild type and G1207 A mutation was 3 416 bp, which was consistent with the theoretical value.By the DNA restriction endonuclease analysis and gene sequencing, the sequences of recombinant plasmids p UC57-MMP2 and p UC57-p. Arg403 His were consistent with those of the Gen Bank( NCCT000016. 10). Among the G1207 A mutants, except that the G of 1 207 site was substituted by A, the other sequences were identical to the wild type sequences of the MMP2 gene. Conclusion The wild type plasmid p UC57-MMP2 and the mutant plasmid p UC57-p. Arg403 His are successfully constructed. [ABSTRACT FROM AUTHOR]

Published

2018

137. Filamentation and restoration of normal growth in Escherichia coli using a combined CRISPRi sgRNA/antisense RNA approach.

Author

Mückl, Andrea, Schwarz-Schilling, Matthaeus, Fischer, Katrin, and Simmel, Friedrich C.

Subjects

*ESCHERICHIA coli growth, *CRISPRS, *ANTISENSE RNA, *BACTERIAL cell cycle, *PROTEIN expression

Abstract

CRISPR interference (CRISPRi) using dCas9-sgRNA is a powerful tool for the exploration and manipulation of gene functions. Here we quantify the reversible switching of a central process of the bacterial cell cycle by CRISPRi and an antisense RNA mechanism. Reversible induction of filamentous growth in E. coli has been recently demonstrated by controlling the expression levels of the bacterial cell division proteins FtsZ/FtsA via CRISPRi. If FtsZ falls below a critical level, cells cannot divide. However, the cells remain metabolically active and continue with DNA replication. We surmised that this makes them amenable to an inducible antisense RNA strategy to counteract FtsZ inhibition. We show that both static and inducible thresholds can adjust the characteristics of the switching process. Combining bulk data with single cell measurements, we characterize the efficiency of the switching process. Successful restoration of division is found to occur faster in the presence of antisense sgRNAs than upon simple termination of CRISPRi induction. [ABSTRACT FROM AUTHOR]

Published

2018

138. Design and characterization of a synthetic minimal promoter for heterocyst-specific expression in filamentous cyanobacteria.

Author

Wegelius, Adam, Li, Xin, Turco, Federico, and Stensjö, Karin

Subjects

*CYANOBACTERIA, *HETEROCYSTS, *MICROBIAL cells, *HYDROGEN production, *HYDROGENASE, *PROMOTERS (Genetics)

Abstract

Short and well defined promoters are essential for advancing cyanobacterial biotechnology. The heterocyst of Nostoc sp. is suggested as a microbial cell factory for oxygen sensitive catalysts, such as hydrogenases for hydrogen production, due to its microoxic environment. We identified and predicted promoter elements of possible significance through a consensus strategy using a pool of heterocyst-induced DIF+ promoters known from Anabaena sp. PCC 7120. To test if these conserved promoter elements were crucial for heterocyst-specific expression, promoter-yfp reporter constructs were designed. The characterization was accomplished by replacing, -35 and -10 regions and the upstream element, with well described elements from the trc promoter of Escherichia coli, which is also functional in Nostoc sp. From the in vivo spatial fluorescence of the different promoter-yfp reporters in Nostoc punctiforme ATCC 29133, we concluded that both the consensus -35 and extended -10 regions were important for heterocyst-specific expression. Further that the promoter strength could be improved by the addition of an upstream element. We designed a short synthetic promoter of 48 nucleotides, PsynDIF, including a consensus DIF1 sequence, a 17 base pair stretch of random nucleotides and an extended consensus -10 region, and thus generated the shortest promoter for heterocyst-specific expression to date. [ABSTRACT FROM AUTHOR]

Published

2018

139. A Bordetella pertussis MgtC homolog plays a role in the intracellular survival.

Author

Cafiero, Juan Hilario, Lamberti, Yanina Andrea, Surmann, Kristin, Vecerek, Branislav, and Rodriguez, Maria Eugenia

Subjects

*BORDETELLA pertussis, *HOMOLOGY (Biology), *INTRACELLULAR membranes, *PHAGOSOMES, *PH standards

Abstract

Bordetella pertussis, the causative agent of whooping cough, has the capability to survive inside the host cells. This process requires efficient adaptation of the pathogen to the intracellular environment and the associated stress. Among the proteins produced by the intracellular B. pertussis we identified a protein (BP0414) that shares homology with MgtC, a protein which was previously shown to be involved in the intracellular survival of other pathogens. To explore if BP0414 plays a role in B. pertussis intracellular survival a mutant strain defective in the production of this protein was constructed. Using standard in vitro growth conditions we found that BP0414 is required for B. pertussis growth under low magnesium availability or low pH, two environmental conditions that this pathogen might face within the host cell. Intracellular survival studies showed that MgtC is indeed involved in B. pertussis viability inside the macrophages. The use of bafilomycin A1, which inhibits phagosome acidification, abolished the survival defect of the mgtC deficient mutant strain suggesting that in intracellular B. pertussis the role of MgtC protein is mainly related to the bacterial adaptation to the acidic conditions found inside the of phagosomes. Overall, this work provides an insight into the importance of MgtC in B. pertussis pathogenesis and its contribution to bacterial survival within immune cells. [ABSTRACT FROM AUTHOR]

Published

2018

140. Efficient genome editing using tRNA promoter-driven CRISPR/Cas9 gRNA in Aspergillus niger.

Author

Song, Letian, Ouedraogo, Jean-Paul, Kolbusz, Magdalena, Nguyen, Thi Truc Minh, and Tsang, Adrian

Subjects

*FUNGAL genetics, *ASPERGILLUS niger, *GENOME editing, *TRANSFER RNA, *PROMOTERS (Genetics), *CRISPRS

Abstract

As a powerful tool for fast and precise genome editing, the CRISPR/Cas9 system has been applied in filamentous fungi to improve the efficiency of genome alteration. However, the method of delivering guide RNA (gRNA) remains a bottleneck in performing CRISPR mutagenesis in Aspergillus species. Here we report a gRNA transcription driven by endogenous tRNA promoters which include a tRNA gene plus 100 base pairs of upstream sequence. Co-transformation of a cas9-expressing plasmid with a linear DNA coding for gRNA demonstrated that 36 of the 37 tRNA promoters tested were able to generate the intended mutation in A. niger. When gRNA and cas9 were expressed in a single extra-chromosomal plasmid, the efficiency of gene mutation was as high as 97%. Co-transformation with DNA template for homologous recombination, the CRISPR/Cas9 system resulted ~42% efficiency of gene replacement in a strain with a functioning non-homologous end joining machinery (kusA+), and an efficiency of >90% gene replacement in a kusA- background. Our results demonstrate that tRNA promoter-mediated gRNA expressions are reliable and efficient in genome editing in A. niger. [ABSTRACT FROM AUTHOR]

Published

2018

141. Characterization of diverse homoserine lactone synthases in Escherichia coli.

Author

Daer, René, Barrett, Cassandra M., Melendez, Ernesto Luna, Wu, Jiaqi, Tekel, Stefan J., Xu, Jimmy, Dennison, Brady, Muller, Ryan, and Haynes, Karmella A.

Subjects

*SYNTHASES, *ESCHERICHIA coli, *SMALL molecules, *QUORUM sensing, *PHYSICAL sciences

Abstract

Quorum sensing networks have been identified in over one hundred bacterial species to date. A subset of these networks regulate group behaviors, such as bioluminescence, virulence, and biofilm formation, by sending and receiving small molecules called homoserine lactones (HSLs). Bioengineers have incorporated quorum sensing pathways into genetic circuits to connect logical operations. However, the development of higher-order genetic circuitry is inhibited by crosstalk, in which one quorum sensing network responds to HSLs produced by a different network. Here, we report the construction and characterization of a library of ten synthases including some that are expected to produce HSLs that are incompatible with the Lux pathway, and therefore show no crosstalk. We demonstrated their function in a common lab chassis, Escherichia coli BL21, and in two contexts, liquid and solid agar cultures, using decoupled Sender and Receiver pathways. We observed weak or strong stimulation of a Lux receiver by longer-chain or shorter-chain HSL-generating Senders, respectively. We also considered the under-investigated risk of unintentional release of incompletely deactivated HSLs in biological waste. We found that HSL-enriched media treated with bleach were still bioactive, while autoclaving deactivates LuxR induction. This work represents the most extensive comparison of quorum signaling synthases to date and greatly expands the bacterial signaling toolkit while recommending practices for disposal based on empirical, quantitative evidence. [ABSTRACT FROM AUTHOR]

Published

2018

142. Cellular reagents for diagnostics and synthetic biology.

Author

Bhadra, Sanchita, Pothukuchy, Arti, Shroff, Raghav, Cole, Austin W., Byrom, Michelle, Ellefson, Jared W., Gollihar, Jimmy D., and Ellington, Andrew D.

Subjects

*ENZYMES, *MOLECULAR biology, *FREEZE-drying, *CELLS, *SYNTHETIC biology

Abstract

We have found that the overproduction of enzymes in bacteria followed by their lyophilization leads to 'cellular reagents' that can be directly used to carry out numerous molecular biology reactions. We demonstrate the use of cellular reagents in a variety of molecular diagnostics, such as TaqMan qPCR with no diminution in sensitivity, and in synthetic biology cornerstones such as the Gibson assembly of DNA fragments, where new plasmids can be constructed solely based on adding cellular reagents. Cellular reagents have significantly reduced complexity and cost of production, storage and implementation, features that should facilitate accessibility and use in resource-poor conditions. [ABSTRACT FROM AUTHOR]

Published

2018

143. Characterization of biochemical properties of an apurinic/apyrimidinic endonuclease from Helicobacter pylori.

Author

Turgimbayeva, Aigerim, Abeldenov, Sailau, Zharkov, Dmitry O., Ishchenko, Alexander A., Ramankulov, Yerlan, Saparbaev, Murat, and Khassenov, Bekbolat

Subjects

*APURINIC acid, *ENDONUCLEASES, *DNA, *HELICOBACTER pylori, *ESCHERICHIA coli

Abstract

Apurinic/apyrimidinic (AP) endonucleases play critical roles in the repair of abasic sites and strand breaks in DNA. Complete genome sequences of Helicobacter pylori reveal that this bacterial specie has a single AP endonuclease. An H. pylori homolog of Xth (HpXth) is a member of exonuclease III family, which is represented by Escherichia coli Xth. Currently, it remains unknown whether this single AP endonuclease has DNA repair activities similar to those of its counterpart in E. coli and other bacteria. We report that HpXth possesses efficient AP site cleavage, 3’-repair phosphodiesterase, and 3’-phosphatase activities but not the nucleotide incision repair function. Optimal reaction conditions for HpXth’s AP endonuclease activity are low ionic strength, high Mg2+ concentration, pH in the range 7–8, and temperature 30 °C. The kinetic parameters measured under steady-state conditions showed that HpXth removes the AP site, 3’-blocking sugar-phosphate, and 3’-terminal phosphate in DNA strand breaks with good efficiency (kcat/KM = 1240, 44, and 5,4 μM–1·min–1, respectively), similar to that of E. coli Xth. As expected, the presence of HpXth protein in AP endonuclease—deficient E. coli xth nfo strain significantly reduced the sensitivity to an alkylating agent and H2O2. Mutation of active site residue D144 in HpXth predicted to be essential for catalysis resulted in a complete loss of enzyme activities. Several important structural features of HpXth were uncovered by homology modeling and phylogenetic analysis. Our data show the DNA substrate specificity of H. pylori AP endonuclease and suggest that HpXth counteracts the genotoxic effects of DNA damage generated by endogenous and host-imposed factors. [ABSTRACT FROM AUTHOR]

Published

2018

144. MiR-221 negatively regulates innate anti-viral response.

Author

Du, Hongqiang, Cui, Shuang, Li, Yunfei, Yang, Guang, Wang, Peiyan, Fikrig, Erol, and You, Fuping

Subjects

*IMMUNE system, *ANTIVIRAL agents, *VIRUS diseases, *RNA sequencing, *GENETIC overexpression, *MICRORNA

Abstract

The innate immune system plays a critical role in the initial antiviral response. However, the timing and duration of these responses must be tightly regulated during infection to ensure appropriate immune cell activation and anti-viral defenses. Here we demonstrate that during antiviral response, a negative regulator miR-221 was also induced in an ELF4-dependent manner. We further show that ELF4 promotes miR-221 expression through direct binding to its promoter. Overexpression and knockdown assay show that miR-221 can negatively regulate IFNβ production in time of virus infection. RNA-seq analysis of miR-221 overexpressed cells revealed multiple candidate targets. Taken together, our study identified a novel negative microRNA regulator of innate antiviral response, which is dependent on ELF4. [ABSTRACT FROM AUTHOR]

Published

2018

145. Interaction between the cellular E3 ubiquitin ligase SIAH-1 and the viral immediate-early protein ICP0 enables efficient replication of Herpes Simplex Virus type 2 in vivo.

Author

Czechowicz, Julia S., Nagel, Claus-Henning, Voges, Maike, Spohn, Michael, Eibl, Martha M., and Hauber, Joachim

Subjects

*HERPES simplex virus, *UBIQUITIN ligases, *AMINO acid analysis, *PROTEIN synthesis, *PROTEIN metabolism

Abstract

Herpes Simplex Virus type 2 (HSV-2) is a neurotropic human pathogen. Upon de novo infection, the viral infected cell protein 0 (ICP0) is immediately expressed and interacts with various cellular components during the viral replication cycle. ICP0 is a multifunctional regulatory protein that has been shown to be important for both efficient viral replication and virus reactivation from latency. In particular, as previously demonstrated in transfected tissue culture models, ICP0 interacts with the cellular E3 ubiquitin ligase SIAH-1, which targets ICP0 for proteasomal degradation. However, the consequence of this virus-host interaction during the establishment of HSV-2 infection in vivo has not yet been elucidated. Here we confirmed that ICP0 of HSV-2 interacts with SIAH-1 via two conserved PxAxVxP amino acid binding motifs. We also demonstrate in vitro that a SIAH-1 binding-deficient HSV-2 strain, constructed by homologous recombination technology, exhibits an attenuated growth curve and impaired DNA and protein synthesis. This attenuated phenotype was also confirmed in an in vivo ocular infection mouse model. Specifically, viral load of the SIAH-1 binding-deficient HSV-2 mutant was significantly reduced in the trigeminal ganglia and brain stem at day 5 and 7 post infection. Our findings indicate that the interplay between ICP0 and SIAH-1 is important for efficient HSV-2 replication in vivo, thereby affecting viral dissemination kinetics in newly infected organisms, and possibly revealing novel targets for antiviral therapy. [ABSTRACT FROM AUTHOR]

Published

2018

146. Centromeric signaling proteins boost G1 cyclin degradation and modulate cell size in budding yeast.

Author

Martínez-Láinez, Joan M., Moreno, David F., Parisi, Eva, Clotet, Josep, and Aldea, Martí

Subjects

*CELL size, *YEAST, *CENTROMERE, *CYCLINS, *PROTEINS

Abstract

Cell size scales with ploidy in a great range of eukaryotes, but the underlying mechanisms remain unknown. Using various orthogonal single-cell approaches, we show that cell size increases linearly with centromere (CEN) copy number in budding yeast. This effect is due to a G1 delay mediated by increased degradation of Cln3, the most upstream G1 cyclin acting at Start, and specific centromeric signaling proteins, namely Mad3 and Bub3. Mad3 binds both Cln3 and Cdc4, the adaptor component of the Skp1/Cul1/F-box (SCF) complex that targets Cln3 for degradation, these interactions being essential for the CEN-dosage dependent effects on cell size. Our results reveal a pathway that modulates cell size as a function of CEN number, and we speculate that, in cooperation with other CEN-independent mechanisms, it could assist the cell to attain efficient mass/ploidy ratios. [ABSTRACT FROM AUTHOR]

Published

2018

147. Proteomic analysis identifies transcriptional cofactors and homeobox transcription factors as TBX18 binding proteins.

Author

Rivera-Reyes, Reginaldo, Kleppa, Marc-Jens, and Kispert, Andreas

Subjects

*PROTEOMICS, *GENE regulatory networks, *HOMEOBOX genes, *CARRIER proteins, *INTERSTITIAL nephritis

Abstract

The TBX18 transcription factor is a crucial developmental regulator of several organ systems in mice, and loss of its transcriptional repression activity causes dilative nephropathies in humans. The molecular complexes with which TBX18 regulates transcription are poorly understood prompting us to use an unbiased proteomic approach to search for protein interaction partners. Using overexpressed dual tagged TBX18 as bait, we identified by tandem purification and subsequent LC-MS analysis TBX18 binding proteins in 293 cells. Clustering of functional annotations of the identified proteins revealed a highly significant enrichment of transcriptional cofactors and homeobox transcription factors. Using nuclear recruitment assays as well as GST pull-downs, we validated CBFB, GAR1, IKZF2, NCOA5, SBNO2 and CHD7 binding to the T-box of TBX18 in vitro. From these transcriptional cofactors, CBFB, CHD7 and IKZF2 enhanced the transcriptional repression of TBX18, while NCOA5 and SBNO2 dose-dependently relieved it. All tested homeobox transcription factors interacted with the T-box of TBX18 in pull-down assays, with members of the Pbx and Prrx subfamilies showing coexpression with Tbx18 in the developing ureter of the mouse. In summary, we identified and characterized new TBX18 binding partners that may influence the transcriptional activity of TBX18 in vivo. [ABSTRACT FROM AUTHOR]

Published

2018

148. Schistosoma japonicum IAP and Teg20 safeguard tegumental integrity by inhibiting cellular apoptosis.

Author

Liu, Juntao, Giri, Bikash R., Chen, Yongjun, Luo, Rong, Xia, Tianqi, Grevelding, Christoph G., and Cheng, Guofeng

Subjects

*SCHISTOSOMA, *SCHISTOSOMIASIS, *IMMUNE response, *APOPTOSIS, *CELL proliferation

Abstract

Schistosomes are causative agents of human schistosomiasis, which is endemic in tropical and subtropical areas of the world. Adult schistosomes can survive in their final hosts for several decades, and they have evolved various strategies to overcome the host immune response. Consequently, understanding the mechanisms that regulate parasitic cell survival will open avenues for developing novel strategies against schistosomiasis. Our previous study suggested that an inhibitor of apoptosis protein in Schistosoma japonicum (SjIAP) may play important roles in parasitic survival and development. Here, we demonstrated that SjIAP can negatively regulate cellular apoptosis in S. japonicum by suppressing caspase activity. Immunohistochemistry analysis indicated that SjIAP ubiquitously expressed within the worm body including the tegument. Silencing of SjIAP expression via small interfering RNA led to destruction of the tegument integrity in schistosomes. We further used co-immunoprecipitation to identify interaction partners of SjIAP and revealed the tegument protein SjTeg-20 as a putative interacting partner of SjIAP. The interaction between SjIAP and SjTeg-20 was confirmed by a yeast two-hybrid (Y2H) assay. Moreover, results of a TUNEL assay, RNA interference, scanning and transmission electron microscopy, caspase assays, transcript profiling, and protein localization of both interacting molecules provided first evidence for an essential role of SjIAP and SjTeg-20 to maintain the structural integrity of the tegument by negatively regulating apoptosis. Taken together, our findings suggest that the cooperative activities of SjIAP and SjTeg-20 belong to the strategic inventory of S. japonicum ensuring survival in the hostile environment within the vasculature of the final host. [ABSTRACT FROM AUTHOR]

Published

2018

149. Killing with proficiency: Integrated post-translational regulation of an offensive Type VI secretion system.

Author

Ostrowski, Adam, Cianfanelli, Francesca R., Porter, Michael, Mariano, Giuseppina, Peltier, Julien, Wong, Jun Jie, Swedlow, Jason R., Trost, Matthias, and Coulthurst, Sarah J.

Subjects

*ANTIBACTERIAL agents, *ANTI-infective agents, *ENTEROBACTERIACEAE, *DEPHOSPHORYLATION, *PHARMACOLOGY

Abstract

The Type VI secretion system (T6SS) is widely used by bacterial pathogens as an effective weapon against bacterial competitors and is also deployed against host eukaryotic cells in some cases. It is a contractile nanomachine which delivers toxic effector proteins directly into target cells by dynamic cycles of assembly and firing. Bacterial cells adopt distinct post-translational regulatory strategies for deployment of the T6SS. ‘Defensive’ T6SSs assemble and fire in response to incoming attacks from aggressive neighbouring cells, and can utilise the Threonine Protein Phosphorylation (TPP) regulatory pathway to achieve this control. However, many T6SSs are ‘offensive’, firing at all-comers without the need for incoming attack or other cell contact-dependent signal. Post-translational control of the offensive mode has been less well defined but can utilise components of the same TPP pathway. Here, we used the anti-bacterial T6SS of Serratia marcescens to elucidate post-translational regulation of offensive T6SS deployment, using single-cell microscopy and genetic analyses. We show that the integration of the TPP pathway with the negative regulator TagF to control core T6SS machine assembly is conserved between offensive and defensive T6SSs. Signal-dependent PpkA-mediated phosphorylation of Fha is required to overcome inhibition of membrane complex assembly by TagF, whilst PppA-mediated dephosphorylation promotes spatial reorientation and efficient killing. In contrast, the upstream input of the TPP pathway defines regulatory strategy, with a new periplasmic regulator, RtkS, shown to interact with the PpkA kinase in S. marcescens. We propose a model whereby the opposing actions of the TPP pathway and TagF impose a delay on T6SS re-assembly after firing, providing an opportunity for spatial re-orientation of the T6SS in order to maximise the efficiency of competitor cell targeting. Our findings provide a better understanding of how bacterial cells deploy competitive weapons effectively, with implications for the structure and dynamics of varied polymicrobial communities. [ABSTRACT FROM AUTHOR]

Published

2018

150. Interaction of lipoprotein QseG with sensor kinase QseE in the periplasm controls the phosphorylation state of the two-component system QseE/QseF in Escherichia coli.

Author

Göpel, Yvonne and Görke, Boris

Subjects

*LIPOPROTEINS, *HISTIDINE kinases, *PHOSPHORYLATION, *HOMEOSTASIS, *VIRULENCE of Escherichia coli, *ADRENALINE, *BACTERIA

Abstract

Histidine kinase QseE and response regulator QseF compose a two-component system in Enterobacteriaceae. In Escherichia coli K-12 QseF activates transcription of glmY and of rpoE from Sigma 54-dependent promoters by binding to upstream activating sequences. Small RNA GlmY and RpoE (Sigma 24) are important regulators of cell envelope homeostasis. In pathogenic Enterobacteriaceae QseE/QseF are required for virulence. In enterohemorrhagic E. coli QseE was reported to sense the host hormone epinephrine and to regulate virulence genes post-transcriptionally through employment of GlmY. The qseEGF operon contains a third gene, qseG, which encodes a lipoprotein attached to the inner leaflet of the outer membrane. Here, we show that QseG is essential and limiting for activity of QseE/QseF in E. coli K-12. Metabolic 32P-labelling followed by pull-down demonstrates that phosphorylation of the receiver domain of QseF in vivo requires QseE as well as QseG. Accordingly, QseG acts upstream and through QseE/QseF by stimulating activity of kinase QseE. 32P-labelling also reveals an additional phosphorylation in the QseF C-terminus of unknown origin, presumably at threonine/serine residue(s). Pulldown and two-hybrid assays demonstrate interaction of QseG with the periplasmic loop of QseE. A mutational screen identifies the Ser58Asn exchange in the periplasmic loop of QseE, which decreases interaction with QseG and concomitantly lowers QseE/QseF activity, indicating that QseG activates QseE by interaction. Finally, epinephrine is shown to have a moderate impact on QseE activity in E. coli K-12. Epinephrine slightly stimulates QseF phosphorylation and thereby glmY transcription, but exclusively during stationary growth and this requires both, QseE and QseG. Our data reveal a three-component signaling system, in which the phosphorylation state of QseE/QseF is governed by interaction with lipoprotein QseG in response to a signal likely derived from the cell envelope. [ABSTRACT FROM AUTHOR]

Published

2018