ABSTRACT
Klebsiella pneumoniae (KP) presents a global health threat, leading to significant morbidity and mortality due to its multidrug-resistant profile and the limited availability of therapeutic options. To eliminate KP lung infection, the host initiates a robust inflammatory response. One of the host's mechanisms for mitigating excessive inflammation involves the RNA-binding protein regnase-1 (Reg1, MCPIP1, or ZC3H12A). Reg1 has an RNA binding domain that recognizes stem-loop structures in the 3' untranslated region of various proinflammatory transcripts, leading to mRNA decay. However, excessive suppression of inflammation by Reg1 results in suboptimal KP control. Reg1 deficiency within the nonhematopoietic compartment confers resistance to KP in the lung. Given that lung epithelium is crucial for KP resistance, we hypothesized that selective deletion of Reg1 in lung epithelial cells might enhance proinflammatory signals, leading to a better control of KP. Our transcriptomic analysis of epithelial cells in KP-infected wild-type mice revealed the presence of three distinct alveolar type 2 cell (AT2) subpopulations (conventional, inflammatory, and cycling) and enrichment of Reg1 in inflammatory AT2 cells. We conditionally deleted Reg1 in lung AT2 cells (ΔReg1), which amplified the local inflammatory response in the lung and increased macrophage cell numbers compared with controls. However, when ΔReg1 mice were subjected to KP infection, there were no significant differences in bacterial burden or survival compared with controls. These findings suggest that the local inflammatory response enhanced by Reg1 deletion in AT2 cells is insufficient to control KP infection.
Subject(s)
Epithelial Cells , Klebsiella pneumoniae , Ribonucleases , Animals , Mice , 3' Untranslated Regions , Inflammation , Lung , Ribonucleases/geneticsABSTRACT
The leafhopper Dalbulus maidis is a harmful pest that causes severe damage to corn crops. Conventional chemical pesticides have negative environmental impacts, emphasizing the need for alternative solutions. RNA interference (RNAi) is a more specific and environmentally friendly method for controlling pests and reducing the negative impacts of current pest management practices. Previous studies have shown that orally administered double-stranded RNA (dsRNA) is less effective than injection protocols in silencing genes. This study focuses on identifying and understanding the role of double-stranded ribonucleases (dsRNases) in limiting the efficiency of oral RNAi in D. maidis. Three dsRNases were identified and characterized, with Dmai-dsRNase-2 being highly expressed in the midgut and salivary glands. An ex vivo degradation assay revealed significant nuclease activity, resulting in high instability of dsRNA when exposed to tissue homogenates. Silencing Dmai-dsRNase-2 improved the insects' response to the dsRNA targeting the gene of interest, providing evidence of dsRNases involvement in oral RNAi efficiency. Therefore, administering both dsRNase-specific and target gene-specific-dsRNAs simultaneously is a promising approach to increase the efficiency of oral RNAi and should be considered in future control strategies.
Subject(s)
Hemiptera , Ribonucleases , Animals , Ribonucleases/genetics , Ribonucleases/metabolism , RNA Interference , Zea mays/genetics , Zea mays/metabolism , Hemiptera/genetics , Hemiptera/metabolism , Insecta/genetics , RNA, Double-Stranded/geneticsABSTRACT
Type 1 conventional dendritic cells (cDC1s) are leukocytes competent to coordinate antiviral immunity, and thus, the intracellular mechanisms controlling cDC1 function are a matter of intense research. The unfolded protein response (UPR) sensor IRE1 and its associated transcription factor XBP1s control relevant functional aspects in cDC1s including antigen cross-presentation and survival. However, most studies connecting IRE1 and cDC1 function are undertaken in vivo. Thus, the aim of this work is to elucidate whether IRE1 RNase activity can also be modeled in cDC1s differentiated in vitro and reveal the functional consequences of such activation in cells stimulated with viral components. Our data show that cultures of optimally differentiated cDC1s recapitulate several features of IRE1 activation noticed in in vivo counterparts and identify the viral analog Poly(I:C) as a potent UPR inducer in the lineage. In vitro differentiated cDC1s display constitutive IRE1 RNase activity and hyperactivate IRE1 RNase upon genetic deletion of XBP1s, which regulates production of the proinflammatory cytokines IL-12p40, TNF-α and IL-6, Ifna and Ifnb upon Poly(I:C) stimulation. Our results show that a strict regulation of the IRE1/XBP1s axis regulates cDC1 activation to viral agonists, expanding the scope of this UPR branch in potential DC-based therapies.
Subject(s)
Protein Serine-Threonine Kinases , Unfolded Protein Response , Protein Serine-Threonine Kinases/genetics , Protein Serine-Threonine Kinases/metabolism , Gene Expression Regulation , Transcription Factors/metabolism , Ribonucleases/metabolismABSTRACT
In cancer, activation of the IRE1/XBP1s axis of the unfolded protein response (UPR) promotes immunosuppression and tumor growth, by acting in cancer cells and tumor infiltrating immune cells. However, the role of IRE1/XBP1s in dendritic cells (DCs) in tumors, particularly in conventional type 1 DCs (cDC1s) which are cellular targets in immunotherapy, has not been fully elucidated. Here, we studied the role of IRE1/XBP1s in subcutaneous B16/B78 melanoma and MC38 tumors by generating loss-of-function models of IRE1 and/or XBP1s in DCs or in cDC1s. Data show that concomitant deletion of the RNase domain of IRE1 and XBP1s in DCs and cDC1s does not influence the kinetics of B16/B78 and MC38 tumor growth or the effector profile of tumor infiltrating T cells. A modest effect is observed in mice bearing single deletion of XBP1s in DCs, which showed slight acceleration of melanoma tumor growth and dysfunctional T cell responses, however, this effect was not recapitulated in animals lacking XBP1 only in cDC1s. Thus, evidence presented here argues against a general pro-tumorigenic role of the IRE1/XBP1s pathway in tumor associated DC subsets.
Subject(s)
Melanoma, Experimental , Ribonucleases , Mice , Animals , Ribonucleases/metabolism , Endoribonucleases/genetics , Endoribonucleases/metabolism , Adaptive Immunity , Ribonuclease, Pancreatic/metabolism , Melanoma, Experimental/metabolism , Protein Serine-Threonine Kinases/genetics , Protein Serine-Threonine Kinases/metabolism , Dendritic CellsABSTRACT
The scale of post-transcriptional regulation and the implications of its interplay with other forms of regulation in environmental acclimation are underexplored for organisms of the domain Archaea. Here, we have investigated the scale of post-transcriptional regulation in the extremely halophilic archaeon Halobacterium salinarum NRC-1 by integrating the transcriptome-wide locations of transcript processing sites (TPSs) and SmAP1 binding, the genome-wide locations of antisense RNAs (asRNAs), and the consequences of RNase_2099C knockout on the differential expression of all genes. This integrated analysis has discovered that 54% of all protein-coding genes in the genome of this haloarchaeon are likely targeted by multiple mechanisms for putative post-transcriptional processing and regulation, with about 20% of genes likely being regulated by combinatorial schemes involving SmAP1, asRNAs, and RNase_2099C. Comparative analysis of mRNA levels (transcriptome sequencing [RNA-Seq]) and protein levels (sequential window acquisition of all theoretical fragment ion spectra mass spectrometry [SWATH-MS]) for 2,579 genes over four phases of batch culture growth in complex medium generated additional evidence for the conditional post-transcriptional regulation of 7% of all protein-coding genes. We demonstrate that post-transcriptional regulation may act to fine-tune specialized and rapid acclimation to stressful environments, e.g., as a switch to turn on gas vesicle biogenesis to promote vertical relocation under anoxic conditions and modulate the frequency of transposition by insertion sequence (IS) elements of the IS200/IS605, IS4, and ISH3 families. Findings from this study are provided as an atlas in a public Web resource (https://halodata.systemsbiology.net). IMPORTANCE While the transcriptional regulation landscape of archaea has been extensively investigated, we currently have limited knowledge about post-transcriptional regulation and its driving mechanisms in this domain of life. In this study, we collected and integrated omics data from multiple sources and technologies to infer post-transcriptionally regulated genes and the putative mechanisms modulating their expression at the protein level in Halobacterium salinarum NRC-1. The results suggest that post-transcriptional regulation may drive environmental acclimation by regulating hallmark biological processes. To foster discoveries by other research groups interested in the topic, we extended our integrated data to the public in the form of an interactive atlas (https://halodata.systemsbiology.net).
Subject(s)
Archaea , Transcriptome , Humans , Archaea/genetics , Transcriptome/genetics , Genome , RNA, Antisense/genetics , Ribonucleases/geneticsABSTRACT
The PumAB type-II toxin-antitoxin (TA) system is encoded by pumAB genes that are organized into an operon. This system is encoded by the pUM505 plasmid, isolated from a Pseudomonas aeruginosa clinical strain. The pumA gene encodes a putative RelE toxin protein (toxic component), whereas the pumB gene encodes a putative HTH antitoxin protein. The expression of the PumAB system in Escherichia coli confers plasmid stability. In addition, PumA toxin overexpression in P. aeruginosa possesses the capability to increase bacterial virulence, an effect that is neutralized by the PumB antitoxin. The aim of this study was to establish the mechanism of regulation of the PumAB toxin-antitoxin system from pUM505. By an in silico analysis of the putative regulatory elements, we identified two putative internal promoters, PpumB and PpumB-AlgU (in addition to the already reported PpumAB), located upstream of pumB. By RT-qPCR assays, we determined that the pumAB genes are transcribed differentially, in that the mRNA of pumB is more abundant than the pumA transcript. We also observed that pumB could be expressed individually and that its mRNA levels decreased under oxidative stress, during individual expression as well as co-expression of pumAB. However, under stressful conditions, the pumA mRNA levels were not affected. This suggests the negative regulation of pumB by stressful conditions. The PumB purified protein was found to bind to a DNA region located between the PpumAB and the pumA coding region, and PumA participates in PumB binding, suggesting that a PumA-PumB complex co-regulates the transcription of the pumAB operon. Interestingly, the pumA mRNA levels decreased after incubation in vitro with PumB protein. This effect was repressed by ribonuclease inhibitors, suggesting that PumB could function as an RNAse toward the mRNA of the toxin. Taken together, we conclude that the PumAB TA system possesses multiple mechanisms to regulate its expression, as well as that the PumB antitoxin generates a decrease in the mRNA toxin levels, suggesting an RNase function. Our analysis provides new insights into the understanding of the control of TA systems from mobile plasmid-encoded genes from a human pathogen.
Subject(s)
Antitoxins , Bacterial Toxins , Toxin-Antitoxin Systems , Humans , Antitoxins/genetics , Antitoxins/metabolism , Bacterial Toxins/genetics , Toxin-Antitoxin Systems/genetics , Apoptosis Regulatory Proteins/metabolism , Escherichia coli/genetics , Escherichia coli/metabolism , Endoribonucleases/genetics , Endoribonucleases/metabolism , RNA, Messenger , Ribonucleases/genetics , Ribonucleases/metabolism , Bacterial Proteins/genetics , Bacterial Proteins/metabolism , Gene Expression Regulation, BacterialABSTRACT
HIV-1 transactivator (Tat) protein plays a critical role in neurological disorders resulting from viral infection, commonly known as HIV-1-associated neurocognitive disorders (HAND). Previous studies have shown that circulant Tat induces M1 microglial activation, one of the hallmark features of HAND, and this is coupled with ER stress and subsequent Unfolded Protein Response (UPR) triggering. Here, we demonstrate that bystander stimuli of Tat in microglial cells result in the simultaneous overexpression of IRE1-related markers and production of M1-typed proinflammatory mediators. We also show that blocking IRE1/XBP-1 signaling using 4µ8C diminishes such inflammatory response. These findings reinforce a role for the IRE1/XBP-1 pathway in HIV-1 Tat neuropathology and suggest that targeting IRE1 RNase activity using 4µ8C or analogue compounds may provide a therapeutic intervention to mitigate against neuroinflammation in HAND.
Subject(s)
HIV-1 , Endoribonucleases , Microglia , Protein Serine-Threonine Kinases , RibonucleasesABSTRACT
Venezuelan equine encephalitis virus (VEEV) is an Alphavirus in the Togaviridae family of positive-strand RNA viruses. The viral genome of positive-strand RNA viruses is infectious, as it produces infectious virus upon introduction into a cell. VEEV is a select agent and samples containing viral RNA are subject to additional regulations due to their infectious nature. Therefore, RNA isolated from cells infected with BSL-3 select agent strains of VEEV or other positive-strand viruses must be inactivated before removal from high-containment laboratories. In this study, we tested the inactivation of the viral genome after RNA fragmentation or cDNA synthesis, using the Trinidad Donkey and TC-83 strains of VEEV. We successfully inactivated VEEV genomic RNA utilizing these two protocols. Our cDNA synthesis method also inactivated the genomic RNA of eastern and western equine encephalitis viruses (EEEV and WEEV). We also tested whether the purified VEEV genomic RNA can produce infectious virions in the absence of transfection. Our result showed the inability of the viral genome to cause infection without being transfected into the cells. Overall, this work introduces RNA fragmentation and cDNA synthesis as reliable methods for the inactivation of samples containing the genomes of positive-strand RNA viruses.
Subject(s)
Encephalitis Virus, Venezuelan Equine/genetics , Genome, Viral , RNA, Viral , Virus Inactivation , Animals , Cells, Cultured , Chlorocebus aethiops , Cytopathogenic Effect, Viral , DNA, Complementary/biosynthesis , Encephalitis Virus, Eastern Equine/genetics , Encephalitis Virus, Eastern Equine/physiology , Encephalitis Virus, Venezuelan Equine/physiology , Encephalitis Virus, Western Equine/genetics , Encephalitis Virus, Western Equine/physiology , RNA, Viral/chemistry , RNA, Viral/physiology , Ribonucleases/metabolism , Vero CellsABSTRACT
The conventional function described for platelets is maintaining vascular integrity. Nevertheless, increasing evidence reveals that platelets can additionally play a crucial role in responding against microorganisms. Activated platelets release molecules with antimicrobial activity. This ability was first demonstrated in rabbit serum after coagulation and later in rabbit platelets stimulated with thrombin. Currently, multiple discoveries have allowed the identification and characterization of PMPs (platelet microbicidal proteins) and opened the way to identify kinocidins and CHDPs (cationic host defense peptides) in human platelets. These molecules are endowed with microbicidal activity through different mechanisms that broaden the platelet participation in normal and pathologic conditions. Therefore, this review aims to integrate the currently described platelet molecules with antimicrobial properties by summarizing the pathways towards their identification, characterization, and functional evaluation that have promoted new avenues for studying platelets based on kinocidins and CHDPs secretion.
Subject(s)
Anti-Infective Agents/blood , Blood Platelets/chemistry , Blood Platelets/microbiology , Animals , Anti-Infective Agents/chemistry , Anti-Infective Agents/classification , Anti-Infective Agents/immunology , Antimicrobial Cationic Peptides/immunology , Antiparasitic Agents/immunology , Antiviral Agents/immunology , Blood Platelets/immunology , Humans , Ribonucleases/immunologyABSTRACT
Mating system transitions from self-incompatibility (SI) to self-compatibility (SC) are common in plants. In the absence of high levels of inbreeding depression, SC alleles are predicted to spread due to transmission advantage and reproductive assurance. We characterized mating system and pistil-expressed SI factors in 20 populations of the wild tomato species Solanum habrochaites from the southern half of the species range. We found that a single SI to SC transition is fixed in populations south of the Rio Chillon valley in central Peru. In these populations, SC correlated with the presence of the hab-6 S-haplotype that encodes a low activity S-RNase protein. We identified a single population segregating for SI/SC and hab-6. Intrapopulation crosses showed that hab-6 typically acts in the expected codominant fashion to confer SC. However, we found one specific S-haplotype (hab-10) that consistently rejects pollen of the hab-6 haplotype, and results in SI hab-6/hab-10 heterozygotes. We suggest that the hab-10 haplotype could act as a genetic mechanism to stabilize mixed mating in this population by presenting a disadvantage for the hab-6 haplotype. This barrier may represent a mechanism allowing for the persistence of SI when an SC haplotype appears in or invades a population.
Subject(s)
Self-Incompatibility in Flowering Plants , Solanum , Flowers , Peru , Pollen/genetics , Ribonucleases , Self-Incompatibility in Flowering Plants/geneticsABSTRACT
A major proportion of extracellular RNAs (exRNAs) do not copurify with extracellular vesicles (EVs) and remain in ultracentrifugation supernatants of cell-conditioned medium or mammalian blood serum. However, little is known about exRNAs beyond EVs. We have previously shown that the composition of the nonvesicular exRNA fraction is highly biased toward specific tRNA-derived fragments capable of forming RNase-protecting dimers. To solve the problem of stability in exRNA analysis, we developed a method based on sequencing the size exclusion chromatography (SEC) fractions of nonvesicular extracellular samples treated with RNase inhibitors (RI). This method revealed dramatic compositional changes in exRNA population when enzymatic RNA degradation was inhibited. We demonstrated the presence of ribosomes and full-length tRNAs in cell-conditioned medium of a variety of mammalian cell lines. Their fragmentation generates some small RNAs that are highly resistant to degradation. The extracellular biogenesis of some of the most abundant exRNAs demonstrates that extracellular abundance is not a reliable input to estimate RNA secretion rates. Finally, we showed that chromatographic fractions containing extracellular ribosomes are probably not silent from an immunological perspective and could possibly be decoded as damage-associated molecular patterns.
Subject(s)
Extracellular Vesicles/genetics , RNA, Transfer/genetics , RNA/genetics , Ribosomes/genetics , Animals , Culture Media, Conditioned/pharmacology , Enzyme Inhibitors/pharmacology , High-Throughput Nucleotide Sequencing , Humans , Ribonucleases/antagonists & inhibitors , Ribonucleases/geneticsABSTRACT
BACKGROUND: Some multifunctional cellular proteins, as the monocyte chemotactic protein-induced protein 1 (ZC3H12A/MCPIP1) and the cyclin-dependent kinase inhibitor CDKN1A/p21, are able to modulate the cellular susceptibility to the human immunodeficiency virus type 1 (HIV-1). Several studies showed that CDKN1A/p21 is expressed at high levels ex vivo in cells from individuals who naturally control HIV-1 replication (HIC) and a recent study supports a coordinate regulation of ZC3H12A/MCPIP1 and CDKN1A/p21 transcripts in a model of renal carcinoma cells. Here, we explored the potential associations between mRNA expression of ZC3H12A/MCPIP1 and CDKN1A/p21 in HIC sustaining undetectable (elite controllers-EC) or low (viremic controllers-VC) viral loads. RESULTS: We found a selective upregulation of ZC3H12A/MCPIP1 and CDKN1A/p21 mRNA levels in PBMC from HIC compared with both ART-suppressed and HIV-negative control groups (P≤ 0.02) and higher MCPIP1 and p21 proteins levels in HIC than in HIV-1 negative subjects. There was a moderate positive correlation (r ≥ 0.57; P ≤ 0.014) between expressions of both transcripts in HIC and in HIC combined with control groups. We found positive correlations between the mRNA level of CDKN1A/p21 with activated CD4+ T cells levels in HIC (r ≥ 0.53; P ≤ 0.017) and between the mRNA levels of both CDKN1A/p21 (r = 0.74; P = 0.005) and ZC3H12A/MCPIP1 (r = 0.58; P = 0.040) with plasmatic levels of sCD14 in EC. Reanalysis of published transcriptomic data confirmed the positive association between ZC3H12A/MCPIP1 and CDKN1A/p21 mRNA levels in CD4+ T cells and monocytes from disparate cohorts of HIC and other HIV-positive control groups. CONCLUSIONS: These data show for the first time the simultaneous upregulation of ZC3H12A/MCPIP1 and CDKN1A/p21 transcripts in the setting of natural suppression of HIV-1 replication in vivo and the positive correlation of the expression of these cellular factors in disparate cohorts of HIV-positive individuals. The existence of a common regulatory pathway connecting ZC3H12A/MCPIP1 and CDKN1A/p21 could have a synergistic effect on HIV-1 replication control and pharmacological manipulation of these multifunctional host factors may open novel therapeutic perspectives to prevent HIV-1 replication and disease progression.
Subject(s)
Cyclin-Dependent Kinase Inhibitor p21/metabolism , HIV Infections/immunology , HIV-1/physiology , Ribonucleases/metabolism , Transcription Factors/metabolism , CD4-Positive T-Lymphocytes/immunology , CD4-Positive T-Lymphocytes/metabolism , Cyclin-Dependent Kinase Inhibitor p21/genetics , Female , HIV Infections/genetics , HIV Infections/metabolism , HIV Infections/virology , Humans , Leukocytes, Mononuclear/metabolism , Monocytes/immunology , Monocytes/metabolism , RNA, Messenger/metabolism , Ribonucleases/genetics , Transcription Factors/genetics , Up-Regulation , Viral LoadABSTRACT
Thioredoxins are regulatory proteins that reduce disulfide bonds on target proteins. NaTrxh, which belongs to the plant thioredoxin family h subgroup 2, interacts and reduces the S-RNase enhancing its ribonuclease activity seven-fold, resulting an essential protein for pollen rejection inNicotiana.Here, the crystal structure of NaTrxh at 1.7 Å by X-ray diffraction is reported. NaTrxh conserves the typical fold observed in other thioredoxins from prokaryotes and eukaryotes, but it contains extensions towards both N- and C-termini.The NaTrxh N-terminal extension participates in the reduction of S-RNase, and in the structure reported here, this is orientated towards the reactive site. The interaction between SF11-RNase and the NaTrxh N-terminal was simulated and the short-lived complex observed lasted for a tenth of ns. Moreover, we identified certain amino acids as SF11-RNase-E155 and NaTrxh-M104 as good candidates to contribute to the stability of the complex. Furthermore, we simulated the reduction of the C153-C186 SF11-RNase disulfide bond and observed subtle changes that affect the entire core, which might explain the increase in the ribonuclease activity of S-RNase when it is reduced by NaTrxh.
Subject(s)
Nicotiana/metabolism , Plant Proteins/metabolism , Ribonucleases/metabolism , Binding Sites/physiology , Eukaryota/metabolism , Prokaryotic Cells/metabolism , Protein Transport/physiologyABSTRACT
Fibrillarin is a highly conserved nucleolar methyltransferase responsible for ribosomal RNA methylation across evolution from Archaea to humans. It has been reported that fibrillarin is involved in the methylation of histone H2A in nucleoli and other processes, including viral progression, cellular stress, nuclear shape, and cell cycle progression. We show that fibrillarin has an additional activity as a ribonuclease. The activity is affected by phosphoinositides and phosphatidic acid and insensitive to ribonuclease inhibitors. Furthermore, the presence of phosphatidic acid releases the fibrillarin-U3 snoRNA complex. We show that the ribonuclease activity localizes to the GAR (glycine/arginine-rich) domain conserved in a small group of RNA interacting proteins. The introduction of the GAR domain occurred in evolution in the transition from archaea to eukaryotic cells. The interaction of this domain with phospholipids may allow a phase separation of this protein in nucleoli.
Subject(s)
Chromosomal Proteins, Non-Histone/chemistry , Chromosomal Proteins, Non-Histone/metabolism , Phospholipids/metabolism , Ribonucleases/chemistry , Ribonucleases/metabolism , Chromosomal Proteins, Non-Histone/genetics , HeLa Cells , Humans , Mutation/genetics , Protein Domains , RNA, Small Nucleolar/metabolism , Recombinant Proteins/metabolism , Ribonucleases/genetics , Ribonucleoproteins/metabolism , Structure-Activity RelationshipABSTRACT
KEY MESSAGE: The early flowering system HSP::AtFT allowed a fast evaluation of a gene containment system based on the construct PsEND1::barnase-barstar for poplar. Transgenic lines showed disturbed pollen development and sterility. Vertical gene transfer through pollen flow from transgenic or non-native plant species into their crossable natural relatives is a major concern. Gene containment approaches have been proposed to reduce or even avoid gene flow among tree species. However, evaluation of genetic containment strategies for trees is very difficult due to the long-generation times. Early flowering induction would allow faster evaluation of genetic containment in this case. Although no reliable methods were available for the induction of fertile flowers in poplar, recently, a new early flowering approach was developed. In this study, early flowering poplar lines containing the gene construct PsEND1::barnase-barstar were obtained. The PsEND1 promoter was chosen due to its early expression pattern, its versality and efficiency for generation of male-sterile plants fused to the barnase gene. RT-PCRs confirmed barnase gene activity in flowers, and pollen development was disturbed, leading to sterile flowers. The system developed in this study represents a valuable tool for gene containment studies in forest tree species.
Subject(s)
Bacterial Proteins/genetics , Flowers/growth & development , Gene Editing/methods , Plant Infertility/genetics , Plants, Genetically Modified/growth & development , Pollen/growth & development , Populus/growth & development , Ribonucleases/genetics , Arabidopsis Proteins/genetics , Bacterial Proteins/metabolism , Flowers/genetics , Flowers/metabolism , Flowers/radiation effects , Gene Expression Regulation, Plant , Gene Flow , Genetic Vectors , Heat-Shock Response , Plants, Genetically Modified/metabolism , Plants, Genetically Modified/radiation effects , Pollen/genetics , Populus/genetics , Populus/metabolism , Populus/radiation effects , Promoter Regions, Genetic , Ribonucleases/metabolism , Temperature , Transformation, GeneticABSTRACT
Poly(A) tail shortening is a critical step in messenger RNA (mRNA) decay and control of gene expression. The carbon catabolite repressor 4 (CCR4)-associated factor 1 (CAF1) component of the CCR4-NOT deadenylase complex plays an essential role in mRNA deadenylation in most eukaryotes. However, while CAF1 has been extensively investigated in yeast and animals, its role in plants remains largely unknown. Here, we show that the Citrus sinensis CAF1 (CsCAF1) is a magnesium-dependent deadenylase implicated in resistance against the citrus canker bacteria Xanthomonas citri. CsCAF1 interacted with proteins of the CCR4-NOT complex, including CsVIP2, a NOT2 homologue, translin-associated factor X (CsTRAX) and the poly(A)-binding proteins CsPABPN and CsPABPC. CsCAF1 also interacted with PthA4, the main X. citri effector required for citrus canker elicitation. We also present evidence suggesting that PthA4 inhibits CsCAF1 deadenylase activity in vitro and stabilizes the mRNA encoded by the citrus canker susceptibility gene CsLOB1, which is transcriptionally activated by PthA4 during canker formation. Moreover, we show that an inhibitor of CsCAF1 deadenylase activity significantly enhanced canker development, despite causing a reduction in PthA4-dependent CsLOB1 transcription. These results thus link CsCAF1 with canker development and PthA4-dependent transcription in citrus plants.
Subject(s)
Citrus sinensis/enzymology , Citrus sinensis/microbiology , Disease Resistance/immunology , Plant Diseases/immunology , Plant Diseases/microbiology , Plant Proteins/metabolism , Ribonucleases/metabolism , Amino Acid Sequence , Bacterial Proteins/metabolism , Citrus sinensis/genetics , Citrus sinensis/immunology , Gene Expression Regulation, Plant/drug effects , Magnesium/pharmacology , Plant Diseases/genetics , Plant Proteins/genetics , Poly A/metabolism , Protein Binding/drug effects , Pyrazoles/chemistry , Pyrazoles/pharmacology , RNA Stability/drug effects , Transcription, Genetic/drug effects , Xanthomonas/drug effects , Xanthomonas/physiologyABSTRACT
The golden mussel, Limnoperna fortunei, is a mollusk native to Southeast Asia and a highly invasive species in South American countries such as Brazil, Uruguay, and Argentina. In order to better understand the biological behavior of the species and develop alternative control methods, genetic studies involving the optimization of DNA isolation procedures are of utmost importance.The objective of the present study was to develop a simple, reproducible, free of contaminants, and cheap protocol to extract DNA from L. fortunei using the adductor muscle of the mussel as the source. Four DNA extraction protocols were compared: extraction with SDS and proteinase K (P1); extraction with SDS, proteinase K and phenol (P2); TRIzol extraction (P3); and NaCl, SDS and RNase extraction (P4). DNA concentration (ng μL-1) and purity (at 260/280 nm) were measured using a spectrophotometer. DNA purity and amplification were verified by electrophoresis and PCR, respectively. P1 resulted in samples with low DNA concentrations or without any DNA, as revealed by the quantification and purity analysis; P2 had low efficiency, given the absence of DNA in most of the samples subjected to electrophoresis. On the other hand, P3 showed contamination with proteins, as indicated by an absorbance of <1.8 and by the low-quality electrophoresis results. Finally, P4 resulted in well-defined bands, absorbance between 1.8 and 2.0, and successful amplification by PCR. In conclusion, the extraction protocol P4 is a practical, fast, free of contaminants, and efficient method for the isolation of L. fortunei DNA.
O mexilhão dourado, Limnoperna fortunei é um molusco originário do sudeste da Ásia, altamente invasor em países Sul-Americanos como Brasil, Uruguai e Argentina. Para compreender melhor o comportamento biológico da espécie e criar alternativas de controle é indispensável a realização de estudos genéticos, onde a otimização dos procedimentos de isolamento do DNA é fundamental.O objetivo desse estudo foi obter um protocolo simples, reproduzível, não contaminante e barato para a extração do DNA de L. fortunei. Foram comparados quatro protocolos experimentais de extração de DNA, utilizando como material biológico o músculo abdutor: extração por SDS e proteinase K (P1), extração por SDS, proteinase K e fenol (P2), extração por Trizol (P3) e extração por NaCl (P4). A quantificação (ng μL-1) e a pureza (260/280 nm) do DNA foram obtidas por espectrofotometria. A integridade e a amplificação do DNA foram verificadas através de eletroforese e PCR, respectivamente. P1 demonstrou baixas concentrações e ausência de DNA nas amostras, identificado pela quantificação e teste de integridade. P2 apresentou baixa eficácia, visualizada pela ausência de DNA na maioria das amostras na eletroforese. Por outro lado, P3 exibiu sinais de contaminação por proteínas, identificado pela razão de absorbância <1.8 e pela baixa qualidade da eletroforese. Finalmente, P4 mostrou um padrão na formação das bandas, absorbância entre 1,8 2,0 e sucesso na amplificação pela PCR. Conclui-se que o protocolo de extração P4 mostrou-se como um método prático, rápido, não contaminante e eficiente para obtenção do DNA de L. fortunei.
Subject(s)
Animals , DNA , Bioaccumulation/legislation & jurisprudence , Perna/genetics , Sodium Dodecyl Sulfate , Endopeptidase K/administration & dosage , Polymerase Chain Reaction/veterinary , Ribonucleases/administration & dosageABSTRACT
The golden mussel, Limnoperna fortunei, is a mollusk native to Southeast Asia and a highly invasive species in South American countries such as Brazil, Uruguay, and Argentina. In order to better understand the biological behavior of the species and develop alternative control methods, genetic studies involving the optimization of DNA isolation procedures are of utmost importance.The objective of the present study was to develop a simple, reproducible, free of contaminants, and cheap protocol to extract DNA from L. fortunei using the adductor muscle of the mussel as the source. Four DNA extraction protocols were compared: extraction with SDS and proteinase K (P1); extraction with SDS, proteinase K and phenol (P2); TRIzol extraction (P3); and NaCl, SDS and RNase extraction (P4). DNA concentration (ng μL-1) and purity (at 260/280 nm) were measured using a spectrophotometer. DNA purity and amplification were verified by electrophoresis and PCR, respectively. P1 resulted in samples with low DNA concentrations or without any DNA, as revealed by the quantification and purity analysis; P2 had low efficiency, given the absence of DNA in most of the samples subjected to electrophoresis. On the other hand, P3 showed contamination with proteins, as indicated by an absorbance of <1.8 and by the low-quality electrophoresis results. Finally, P4 resulted in well-defined bands, absorbance between 1.8 and 2.0, and successful amplification by PCR. In conclusion, the extraction protocol P4 is a practical, fast, free of contaminants, and efficient method for the isolation of L. fortunei DNA.(AU)
O mexilhão dourado, Limnoperna fortunei é um molusco originário do sudeste da Ásia, altamente invasor em países Sul-Americanos como Brasil, Uruguai e Argentina. Para compreender melhor o comportamento biológico da espécie e criar alternativas de controle é indispensável a realização de estudos genéticos, onde a otimização dos procedimentos de isolamento do DNA é fundamental.O objetivo desse estudo foi obter um protocolo simples, reproduzível, não contaminante e barato para a extração do DNA de L. fortunei. Foram comparados quatro protocolos experimentais de extração de DNA, utilizando como material biológico o músculo abdutor: extração por SDS e proteinase K (P1), extração por SDS, proteinase K e fenol (P2), extração por Trizol (P3) e extração por NaCl (P4). A quantificação (ng μL-1) e a pureza (260/280 nm) do DNA foram obtidas por espectrofotometria. A integridade e a amplificação do DNA foram verificadas através de eletroforese e PCR, respectivamente. P1 demonstrou baixas concentrações e ausência de DNA nas amostras, identificado pela quantificação e teste de integridade. P2 apresentou baixa eficácia, visualizada pela ausência de DNA na maioria das amostras na eletroforese. Por outro lado, P3 exibiu sinais de contaminação por proteínas, identificado pela razão de absorbância <1.8 e pela baixa qualidade da eletroforese. Finalmente, P4 mostrou um padrão na formação das bandas, absorbância entre 1,8 2,0 e sucesso na amplificação pela PCR. Conclui-se que o protocolo de extração P4 mostrou-se como um método prático, rápido, não contaminante e eficiente para obtenção do DNA de L. fortunei.(AU)
Subject(s)
Animals , Perna/genetics , DNA/isolation & purification , DNA/chemical synthesis , Bioaccumulation/legislation & jurisprudence , Polymerase Chain Reaction/veterinary , Sodium Dodecyl Sulfate , Ribonucleases/administration & dosage , Endopeptidase K/administration & dosageABSTRACT
A perchloric acid-soluble protein (PSP), named here tv-psp1, was identified in Trichomonas vaginalis. It is expressed under normal culture conditions according to expressed sequence tag (EST) analysis. On the other hand, Tv-PSP1 protein was identified by mass spectrometry with a 40% of identity to human PSP (p14.1). Polyclonal antibodies against recombinant Tv-PSP1 (rTv-PSP1) recognized a single band at 13.5 kDa in total protein parasite extract by SDS-PAGE and a high molecular weight band analyzed by native PAGE. Structural analysis of Tv-PSP1, using dynamic light scattering, size exclusion chromatography, and circular dichroism spectroscopy, showed a trimeric structure stable at 7 M urea with 38% α-helix and 14% ß-sheet in solution and a molecular weight of 40.5 kD. Tv-PSP1 models were used to perform dynamic simulations over 100 ns suggesting a stable homotrimeric structure. Tv-PSP1 was located in the nucleus, cytoplasm, and hydrogenosomes of T. vaginalis, and the in silico analysis by Search Tool for the Retrieval of Interacting Genes/Proteins (STRING) showed interactions with RNA binding proteins. The preliminary results of RNA degradation analysis with the recombinant Tv-PSP1 showed RNA partial deterioration suggesting a possible putative ribonuclease function.
Subject(s)
Perchlorates/metabolism , Protozoan Proteins/analysis , RNA-Binding Proteins/analysis , Ribonucleases/analysis , Trichomonas vaginalis/metabolism , Amino Acid Sequence , Animals , Circular Dichroism , Electrophoresis, Polyacrylamide Gel , Heat-Shock Proteins/genetics , Humans , Mice , Mice, Inbred BALB C , Molecular Dynamics Simulation , Protozoan Proteins/genetics , RNA-Binding Proteins/genetics , Ribonucleases/geneticsABSTRACT
We have previously shown that 5' halves from tRNAGlyGCC and tRNAGluCUC are the most enriched small RNAs in the extracellular space of human cell lines, and especially in the non-vesicular fraction. Extracellular RNAs are believed to require protection by either encapsulation in vesicles or ribonucleoprotein complex formation. However, deproteinization of non-vesicular tRNA halves does not affect their retention in size-exclusion chromatography. Thus, we considered alternative explanations for their extracellular stability. In-silico analysis of the sequence of these tRNA-derived fragments showed that tRNAGly 5' halves can form homodimers or heterodimers with tRNAGlu 5' halves. This capacity is virtually unique to glycine tRNAs. By analyzing synthetic oligonucleotides by size exclusion chromatography, we provide evidence that dimerization is possible in vitro. tRNA halves with single point substitutions preventing dimerization are degraded faster both in controlled nuclease digestion assays and after transfection in cells, showing that dimerization can stabilize tRNA halves against the action of cellular nucleases. Finally, we give evidence supporting dimerization of endogenous tRNAGlyGCC 5' halves inside cells. Considering recent reports have shown that 5' tRNA halves from Ala and Cys can form tetramers, our results highlight RNA intermolecular structures as a new layer of complexity in the biology of tRNA-derived fragments.