Your search keyword '"Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics"' showing total 36 results

1. Identification of an endonuclease and N 6 -adenine methyltransferase from Ureaplasma parvum SV3F4 strain.

Author

Wu HN, Fujisawa Y, Tozuka Z, Fomenkov A, Nakura Y, Kajiyama SI, Fujiwara S, Yasukawa K, Roberts RJ, and Yanagihara I

Subjects

Recombinant Proteins metabolism, Recombinant Proteins genetics, Escherichia coli genetics, Escherichia coli enzymology, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Deoxyribonucleases, Type II Site-Specific metabolism, Deoxyribonucleases, Type II Site-Specific genetics, Methyltransferases genetics, Methyltransferases metabolism, Amino Acid Sequence, Ureaplasma genetics, Ureaplasma enzymology, Bacterial Proteins genetics, Bacterial Proteins metabolism, Bacterial Proteins chemistry

Abstract

Here, we report a novel endonuclease and N 6 -adenine DNA methyltransferase (m 6 A methyltransferase) in the Ureaplasma parvum SV3F4 strain. Our previous study found that the SV3F4 strain carries 17 unique genes, which are not encoded in the two previously reported U. parvum serovar 3 strain, OMC-P162 and ATCC 700970. Of these 17 unique genes, UP3_c0261 and UP3_c0262, were originally annotated as encoding hypothetical proteins. Comparative genomics analyses more recently indicated they encode a Type II restriction endonuclease and an m6A methyltransferase, respectively. The UP3_c0261 and UP3_c0262 genes were individually expressed and purified in Escherichia coli. The UP3_c0261 recombinant protein showed endonuclease activity on the pT7Blue vector, recognizing and cleaving a GTNAC motif, resulting in a 5 base 5' extension. The UP3_c0261 protein digested a polymerase chain reaction (PCR) product harboring the GTNAC motif. The endonuclease UP3_c0261 was designated as UpaF4I. Treatment of the PCR product with the recombinant protein UP3_c0262 completely blocked the restriction enzyme activity of UpaF4I. Analysis of the treated PCR product harboring a modified nucleotide by UP3_c0262 with HPLC-MS/MS and MS/MS showed that UP3_c0262 was an m6A methyltransferase containing a methylated A residue in both DNA strands of the GTNAC motif. Whole genome methylation analysis of SV3F4 showed that 99.9 % of the GTNAC motif was m6A modified. These results suggest the UP3_c0261 and UP3_c0262 genes may act as a novel Type II restriction-modification system in the Ureaplasma SV3F4 strain., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

2. Influence of genetic polymorphisms on arsenic methylation efficiency during pregnancy: Evidence from a Spanish birth cohort.

Author

Soler-Blasco R, Harari F, Riutort-Mayol G, Murcia M, Lozano M, Irizar A, Marina LS, Zubero MB, Fernández-Jimenez N, Braeuer S, Ballester F, and Llop S

Subjects

Pregnancy, Female, Humans, Child, Methylation, Birth Cohort, Methyltransferases genetics, Polymorphism, Single Nucleotide, Cacodylic Acid, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Arsenic metabolism

Abstract

Background: Inorganic arsenic (iAs) is a widespread toxic metalloid. It is well-known that iAs metabolism and its toxicity are mediated by polymorphisms in AS3MT and other genes. However, studies during pregnancy are scarce. We aimed to examine the role of genetic polymorphisms in AS3MT, GSTO2, N6AMT1, MTHFR, MTR, FTCD, CBS, and FOLH1 in iAs methylation efficiency during pregnancy., Methods: The study included 541 pregnant participants from the INMA (Environment and Childhood) Spanish cohort. Using high-performance liquid chromatography coupled to inductively coupled plasma-tandem mass, we measured arsenic (iAs and the metabolites monomethylarsonic acid (MMA) and dimethylarsinic acid (DMA)) in urine samples collected during the first trimester. iAs methylation efficiency was determined based on relative concentrations of the As metabolites in urine (%MMA, %DMA, and %iAs). Thirty-two single nucleotide polymorphisms (SNPs) in nine genes were determined in maternal DNA; AS3MT haplotypes were inferred. We assessed the association between genotypes/haplotypes and maternal As methylation efficiency using multivariate linear regression models., Results: The median %MMA and %DMA were 5.3 %, and 89 %, respectively. Ancestral alleles of AS3MT SNPs (rs3740393, rs3740390, rs11191453, and rs11191454) were significantly associated with higher %MMA, %iAs, and lower %DMA. Pregnant participants with zero copies of the GGCTTCAC AS3MT haplotype presented a higher %MMA. Statistically significant associations were also found for the FOLH1 SNP rs202676 (β 0.89 95%CI: 0.24, 1.55 for carriers of the G allele vs. the A allele)., Conclusions: Our study shows that ancestral alleles in AS3MT polymorphisms were associated with lower As methylation efficiency in early pregnancy and suggests that FOLH1 also plays a role in As methylation efficiency. These results support the hypothesis that As metabolism is multigenic, being a key element for identifying susceptible populations., Competing Interests: Declaration of competing interest The authors declare that they have no competing interests., (Copyright © 2023 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2023

3. Arsenic metabolism, N6AMT1 and AS3MT single nucleotide polymorphisms, and their interaction on gestational diabetes mellitus in Chinese pregnant women.

Author

Liang X, Guo G, Wang Y, Wang M, Chen X, Zhang J, Li S, Liu L, Huang Q, Cui B, Zhang M, Sun G, Tang N, Zhang X, and Zhang Q

Subjects

Humans, Female, Pregnancy, Polymorphism, Single Nucleotide, Pregnant People, Methyltransferases genetics, Methyltransferases metabolism, Cross-Sectional Studies, East Asian People, Cacodylic Acid, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Arsenic metabolism, Diabetes, Gestational genetics

Abstract

Background: Single nucleotide polymorphisms (SNPs) in N6AMT1 and AS3MT are associated with arsenic (As) metabolism, and efficient As methylation capacity has been associated with diabetes. However, little is known about the gene-As interaction on gestational diabetes mellitus (GDM)., Objective: This study aimed to explore the individual and combined effects of N6AMT1 and AS3MT SNPs with As metabolism on GDM., Methods: A cross-sectional study was performed among 385 Chinese pregnant women (86 GDM and 299 Non-GDM). Four SNPs in N6AMT1 (rs1997605 and rs1003671) and AS3MT (rs1046778 and rs11191453) were genotyped. Urinary inorganic arsenic (iAs), monomethylarsonic acid (MMA), and dimethylarsinic acid (DMA) were determined, and the percentages of As species (iAs%, MMA%, and DMA%) were calculated to assess the efficiency of As metabolism., Results: Pregnant women with N6AMT1 rs1997605 AA genotype had lower iAs% (B: 2.11; 95% CI: 4.08, -0.13) and MMA% (B: 0.21; 95% CI: 0.39, -0.04) than pregnant women with GG genotype. The AS3MT rs1046778 and rs11191453 C alleles were negatively associated with iAs% and MMA% but positively associated with DMA%. Higher urinary MMA% was significantly associated with a lower risk of GDM (OR: 0.54; 95% CI: 0.30, 0.97). The A allele in N6AMT1 rs1997605 (OR: 0.46; 95% CI: 0.26, 0.79) was associated with a decreased risk of GDM. The additive interactions between N6AMT1 rs1997605 GG genotypes and lower iAs% (AP: 0.50; 95% CI: 0.01, 0.99) or higher DMA% (AP: 0.52; 95% CI: 0.04, 0.99) were statistically significant. Similar additive interactions were also found between N6AMT1 rs1003671 GG genotypes and lower iAs% or higher DMA%., Conclusions: Genetic variants in N6AMT1 and efficient As metabolism (indicated by lower iAs% and higher DMA%) can interact to influence GDM occurrence synergistically in Chinese pregnant women., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2023 Elsevier Inc. All rights reserved.)

Published

2023

4. Phenotypic impacts and genetic regulation characteristics of the DNA adenine methylase gene (dam) in Salmonella Typhimurium biofilm forms.

Author

Keçeli Oğuz S, Has EG, Akçelik N, and Akçelik M

Subjects

Humans, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Caco-2 Cells, Biofilms, Gene Expression Regulation, Bacterial, Bacterial Proteins genetics, Salmonella typhimurium genetics, Salmonella typhimurium metabolism, MicroRNAs metabolism

Abstract

In this study, transcriptional level gene expression changes in biofilm forms of Salmonella Typhimurium ATCC 14028 and its dam mutant were investigated by performing RNAseq analysis. As a result of these analyzes, a total of 233 differentially expressed genes (DEGs) were identified in the dam mutant, of which 145 genes were downregulated and 88 genes were upregulated compared to the wild type. According to data from miRNA sequence analysis, of 13 miRNAs differentially expressed in dam mutant, 9 miRNAs were downregulated and 4 miRNAs were upregulated. These data provide the first evidence that the dam gene is a global regulator of biofilm formation in Salmonella. In addition, phenotypic analyses revealed that bacterial swimming and swarming motility and cellulose production were highly inhibited in the dam mutant. It was determined that bacterial adhesion in Caco-2 and HEp-2 cell lines was significantly reduced in dam mutant. At the end of 90 min, the adhesion rate of wild type strain was 43.3% in Caco-2 cell line, while this rate was 14.9% in dam mutant. In the HEp-2 cell line, while 45.5% adherence was observed in the wild-type strain, this rate decreased to 15.3% in the dam mutant., Competing Interests: Declaration of competing interest The authors declare no conflict of interest., (Copyright © 2022 Institut Pasteur. Published by Elsevier Masson SAS. All rights reserved.)

Published

2023

5. DNA adenine methylase, not the PstI restriction-modification system, regulates virulence gene expression in Shiga toxin-producing Escherichia coli.

Author

Carter MQ, Pham A, Huynh S, Parker CT, Miller A, He X, Hu B, and Chain PSG

Subjects

Deoxyribonucleases, Type II Site-Specific genetics, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Gene Expression Regulation, Bacterial, Humans, Prophages genetics, Shiga Toxin 2 genetics, Shiga Toxin 2 metabolism, Shiga-Toxigenic Escherichia coli genetics, Shiga-Toxigenic Escherichia coli pathogenicity, Shiga-Toxigenic Escherichia coli virology, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Viral Proteins genetics, Virulence, Virulence Factors metabolism, Deoxyribonucleases, Type II Site-Specific metabolism, Escherichia coli Infections microbiology, Prophages enzymology, Shiga-Toxigenic Escherichia coli enzymology, Viral Proteins metabolism, Virulence Factors genetics

Abstract

We previously reported a distinct methylome between the two Shiga toxin-producing Escherichia coli (STEC) O145:H28 strains linked to the 2010 U.S. lettuce-associated outbreak (RM13514) and the 2007 Belgium ice cream-associated outbreak (RM13516), respectively. This difference was thought to be attributed to a prophage encoded type II restriction-modification system (PstI R-M) in RM13514. Here, we characterized this PstI R-M system in comparison to DNA adenine methylase (Dam), a highly conserved enzyme in γ proteobacteria, by functional genomics. Deficiency in Dam led to a differential expression of over 1000 genes in RM13514, whereas deficiency in PstI R-M only impacted a few genes transcriptionally. Dam regulated genes involved in diverse functions, whereas PstI R-M regulated genes mostly encoding transporters and adhesins. Dam regulated a large number of genes located on prophages, pathogenicity islands, and plasmids, including Shiga toxin genes, type III secretion system (TTSS) genes, and enterohemolysin genes. Production of Stx2 in dam mutant was significantly higher than in RM13514, supporting a role of Dam in maintaining lysogeny of Stx2-prophage. However, following mitomycin C treatment, Stx2 in RM13514 was significantly higher than that of dam or PstI R-M deletion mutant, implying that both Dam and PstI R-M contributed to maximum Stx2 production., (Published by Elsevier Ltd.)

Published

2021

6. Tetramerization at Low pH Licenses DNA Methylation Activity of M.HpyAXI in the Presence of Acid Stress.

Author

Narayanan N, Banerjee A, Jain D, Kulkarni DS, Sharma R, Nirwal S, Rao DN, and Nair DT

Subjects

Acids metabolism, Adenine chemistry, Adenine metabolism, Amino Acid Sequence genetics, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, Helicobacter Infections enzymology, Helicobacter Infections microbiology, Helicobacter pylori pathogenicity, Humans, Hydrogen-Ion Concentration, Kinetics, Protein Multimerization genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, Stress, Physiological genetics, Substrate Specificity, DNA Methylation genetics, Helicobacter Infections genetics, Helicobacter pylori enzymology, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

Methylation of genomic DNA can influence the transcription profile of an organism and may generate phenotypic diversity for rapid adaptation in a dynamic environment. M.HpyAXI is a Type III DNA methyltransferase present in Helicobacter pylori and is upregulated at low pH. This enzyme may alter the expression of critical genes to ensure the survival of this pathogen at low pH inside the human stomach. M.HpyAXI methylates the adenine in the target sequence (5'-GCAG-3') and shows maximal activity at pH 5.5. Type III DNA methyltransferases are found to form an inverted dimer in the functional form. We observe that M.HpyAXI forms a nonfunctional dimer at pH 8.0 that is incapable of DNA binding and methylation activity. However, at pH 5.5, two such dimers associate to form a tetramer that now includes two functional dimers that can bind and methylate the target DNA sequence. Overall, we observe that the pH-dependent tetramerization of M.HpyAXI ensures that the enzyme is licensed to act only in the presence of acid stress., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2020

7. Two different restriction-modification systems for degrading exogenous DNA in Paenibacillus polymyxa.

Author

Shen M, Chen Z, Mao X, Wang L, Liang J, Huo Q, Yin X, Qiu J, and Sun D

Subjects

Bacillus subtilis genetics, Cell-Free System, DNA Methylation, DNA Restriction-Modification Enzymes metabolism, Epigenesis, Genetic, Escherichia coli genetics, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Gene Expression Regulation, Bacterial, Plasmids genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, DNA metabolism, DNA Restriction-Modification Enzymes genetics, Genetic Engineering methods, Paenibacillus polymyxa genetics

Abstract

Accompanied by benefits from horizontally transferred genes, bacteria have to face the risk of the invasion of dangerous genes. Bacteria often use the restriction-modification (R-M) system, which is consisted of methyl transferase (MEase) and restrictase (REase), to protect self-DNA and defend against foreign DNA. Paenibacillus polymyxa, widely used as growth promoting rhizobacteria in agriculture, can also produce compounds of medical and industrial interests. It is unclear whether R-M systems exist in P. polymyxa. In this study, we used a shuttle plasmid with epigenetic modification from different bacteria to explore R-M systems in P. polymyxa. We found that DNA which is methylated by DNA adenine methyltransferase (Dam) in E. coli was strongly restricted, indicating the presence of a Dam-methylation-dependent R-M system in P. polymyxa. Whereas, DNA from a dam - E. coli strain was also moderately restricted, indicating the presence of a Dam-methylation-independent R-M system. Degradation of plasmid DNA with Dam methylation by cell-free protein extract of P. polymyxa provides additional evidence for the presence of Dam-methylation-dependent R-M system. Taken together, our work showed that there are two different types of R-M system in P. polymyxa, providing a foundation for the study of innate immunity in P. polymyxa and for the development of genetic engineering tools in P. polymyxa., (Copyright © 2018 Elsevier Inc. All rights reserved.)

Published

2018

8. DNA adenine hypomethylation leads to metabolic rewiring in Deinococcus radiodurans.

Author

Shaiwale NS, Basu B, Deobagkar DD, Deobagkar DN, and Apte SK

Subjects

Adenine metabolism, Bacterial Proteins genetics, DNA, Bacterial genetics, Deinococcus genetics, Gene Deletion, Methylation, Proteomics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Bacterial Proteins metabolism, DNA, Bacterial metabolism, Deinococcus metabolism

Abstract

The protein encoded by DR_0643 gene from Deinococcus radiodurans was shown to be an active N-6 adenine-specific DNA methyltransferase (Dam). Deletion of corresponding protein reduced adenine methylation in the genome by 60% and resulted in slow-growth phenotype. Proteomic changes induced by DNA adenine hypomethylation were mapped by two-dimensional protein electrophoresis coupled with mass spectrometry. As compared to wild type D. radiodurans cells, at least 54 proteins were differentially expressed in Δdam mutant. Among these, 39 metabolic enzymes were differentially expressed in Δdam mutant. The most prominent change was DNA adenine hypomethylation induced de-repression of pyruvate dehydrogenase complex, E1 component (aceE) gene resulting in 10 fold increase in the abundance of corresponding protein. The observed differential expression profile of metabolic enzymes included increased abundance of enzymes involved in fatty acid and amino acid degradation to replenish acetyl Co-A and TCA cycle intermediates and diversion of phosphoenolpyruvate and pyruvate into amino acid biosynthesis, a metabolic rewiring attempt by Δdam mutant to restore energy generation via glycolysis-TCA cycle axis. This is the first report of DNA adenine hypomethylation mediated rewiring of metabolic pathways in prokaryotes., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2015

9. Dam methylation regulates the expression of SPI-5-encoded sopB gene in Salmonella enterica serovar Typhimurium.

Author

Giacomodonato MN, Llana MN, Castañeda Mdel R, Buzzola F, García MD, Calderón MG, Sarnacki SH, and Cerquetti MC

Subjects

Animals, Bacterial Proteins biosynthesis, Blotting, Western, Disease Models, Animal, Epithelial Cells microbiology, Gene Deletion, Genomic Islands, Lymph Nodes microbiology, Mice, Inbred BALB C, Real-Time Polymerase Chain Reaction, Reverse Transcriptase Polymerase Chain Reaction, Salmonella Infections, Animal, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Virulence Factors biosynthesis, Bacterial Proteins metabolism, DNA Methylation, Gene Expression Regulation, Bacterial, Salmonella typhimurium genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism

Abstract

DNA adenine methylation is an essential factor in Salmonella virulence. Here, we investigate the involvement of DNA adenine methylase (Dam) in the expression and translocation of a SPI-5-encoded effector of S. Typhimurium. SopB expression and secretion were determined using SopB-FLAG-tagged wild type and dam strains of S. Typhimurium. Western blot and quantitative reverse transcriptase PCR analysis showed that the dam mutant expresses lower levels of SopB protein and sopB mRNA than the wild type strain under SPI-1 and SPI-2 inducing conditions in vitro. SopB secretion was also considerably impaired in the absence of dam. In agreement with in vitro experiments, SopB synthesis in dam mutants recovered from infected epithelial cells and from murine mesenteric lymph nodes was reduced by 40% respect to the wild type strain (p < 0.05). SopB translocation was neither detected in the cytosol of epithelial cells nor in the cytosol of cells isolated from mesenteric lymph nodes infected with the dam mutant. Taken together, our results demonstrate that, in S. Typhimurium, Dam methylation modulates the expression and translocation of SPI-5-encoded SopB effector., (Copyright © 2014 Institut Pasteur. Published by Elsevier Masson SAS. All rights reserved.)

Published

2014

10. Lipoprotein lipase gene HindIII polymorphism and risk of myocardial infarction in South Indian population.

Author

Tanguturi PR, Pullareddy B, Rama Krishna BS, and Murthy DK

Subjects

Age Distribution, Aged, Analysis of Variance, Case-Control Studies, Confidence Intervals, Female, Gene Expression Regulation, Genotype, Humans, Incidence, India epidemiology, Logistic Models, Male, Middle Aged, Multivariate Analysis, Myocardial Infarction diagnosis, Risk Assessment, Sex Distribution, Survival Rate, Genetic Predisposition to Disease epidemiology, Lipoprotein Lipase genetics, Myocardial Infarction epidemiology, Myocardial Infarction genetics, Polymorphism, Genetic, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

Introduction: Studies have reported an association between lipoprotein lipase (LPL) gene and myocardial infarction in some populations. Therefore, the present study aimed to investigate the association of the HindIII polymorphism of the (LPL) gene with myocardial infarction and to explore its potential role in susceptibility in a South Indian population., Subjects and Methods: We included a total of 412 subjects (202 myocardial infarction patients and 210 age- and sex-matched controls). Demographic and clinical characteristics were collected. Lipid profiles were estimated. DNA was isolated and the LPL gene HindIII polymorphism was determined by polymerase chain reaction., Results: Comparison of the lipid profiles between patients and controls showed that patients had statistically high significant values (p = 0.0001). The H(+) H(+) genotype of the LPL gene is associated with myocardial infarction. H(+) H(+) vs. H(-) H(-) was χ2 = 19.4, OR 3.1, CI 95% 1.8-5.2, p < 0.0001., Conclusion: Our study strongly suggests that the LPL gene HindIII Hþ Hþ genotype is an independent risk factor for first MI., (Copyright © 2013 Cardiological Society of India. Published by Elsevier B.V. All rights reserved.)

Published

2013

11. Structural insights into the assembly and shape of Type III restriction-modification (R-M) EcoP15I complex by small-angle X-ray scattering.

Author

Gupta YK, Yang L, Chan SH, Samuelson JC, Xu SY, and Aggarwal AK

Subjects

Holoenzymes genetics, Hydrolysis, Models, Molecular, Protein Subunits, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Ultracentrifugation, X-Rays, DNA metabolism, Holoenzymes chemistry, Holoenzymes metabolism, Scattering, Small Angle, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism

Abstract

EcoP15I is the prototype of the Type III restriction enzyme family, composed of two modification (Mod) subunits to which two (or one) restriction (Res) subunits are then added. The Mod subunits are responsible for DNA recognition and methylation, while the Res subunits are responsible for ATP hydrolysis and cleavage. Despite extensive biochemical and genetic studies, there is still no structural information on Type III restriction enzymes. We present here small-angle X-ray scattering (SAXS) and analytical ultracentrifugation analysis of the EcoP15I holoenzyme and the Mod(2) subcomplex. We show that the Mod(2) subcomplex has a relatively compact shape with a radius of gyration (R(G)) of ∼37.4 Å and a maximal dimension of ∼110 Å. The holoenzyme adopts an elongated crescent shape with an R(G) of ∼65.3 Å and a maximal dimension of ∼218 Å. From reconstructed SAXS envelopes, we postulate that Mod(2) is likely docked in the middle of the holoenzyme with a Res subunit at each end. We discuss the implications of our model for EcoP15I action, whereby the Res subunits may come together and form a "sliding clamp" around the DNA., (Copyright © 2012 Elsevier Ltd. All rights reserved.)

Published

2012

12. The effect of methylation on some biological parameters in Salmonella enterica serovar Typhimurium.

Author

Aloui A, Tagourti J, El May A, Joseleau Petit D, and Landoulsi A

Subjects

DNA Replication genetics, DNA, Bacterial chemistry, DNA, Bacterial metabolism, Hot Temperature, Mutation, Salmonella typhimurium genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, DNA Methylation, Salmonella typhimurium growth & development

Abstract

Cell growth is tightly coupled to DNA replication and its methylation [Proc Natl Acad Sci U S A 93 (1996) 12206-12211]. In a culture medium, growing of Salmonella Typhimurium (S. Typhimurium) mutant cells (dam⁻) decreased (2.5 fold) relative to the wild type strain (dam⁺). In this study, we show that the reason for this growth deficiency is due to the DNA methylation. The absence of a Dam methyltransferase protein results in poor growth efficiency and disturbs the synchrony of replication initiation in vivo, as evaluated by flow cytometry. On the other hand, we show that lack of methylation could increase the DNA response to thermal stress (decreasing the DNA melting temperature, T(m)), and the reason for this effect is due to the methylation status and not to the number of guanine and cytosine bases (G+C) in the duplex DNA. Our results show that methylation is an epigenetic factor that may play a key role in the cell growth, the synchrony of DNA replication [C R Biologies 330 (2007) 576-580] and the stress protection., (Copyright © 2009. Published by Elsevier SAS.)

Published

2011

13. Identification of holocarboxylase synthetase chromatin binding sites in human mammary cell lines using the DNA adenine methyltransferase identification technology.

Author

Singh D, Pannier AK, and Zempleni J

Subjects

Binding Sites, Carbon-Nitrogen Ligases chemistry, Carbon-Nitrogen Ligases genetics, Cell Line, Humans, Mammary Glands, Human cytology, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Carbon-Nitrogen Ligases metabolism, Chromatin chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism

Abstract

Holocarboxylase synthetase (HCS) is a chromatin protein that is essential for mediating the covalent binding of biotin to histones. Biotinylation of histones plays crucial roles in the repression of genes and repeats in the human genome. We tested the feasibility of DNA adenine methyltransferase identification (DamID) technology to map HCS binding sites in human mammary cell lines. Full-length HCS was fused to DNA adenine methyltransferase (Dam) for subsequent transfection into breast cancer (MCF-7) and normal breast (MCF-10A) cells. HCS docking sites in chromatin were identified by using the unique adenine methylation sites established by Dam in the fusion construct; docking sites were unambiguously identified using methylation-sensitive digestion, cloning, and sequencing. In total, 15 novel HCS binding sites were identified in the two cell lines, and the following 4 of the 15 overlapped between MCF-7 and MCF-10A cells: inositol polyphosphate-5-phosphatase A, corticotropin hormone precursor, ribosome biogenesis regulatory protein, and leptin precursor. We conclude that DamID is a useful technology to map HCS binding sites in human chromatin and propose that the entire set of HCS binding sites could be mapped by combining DamID with microarray technology., (Copyright © 2011 Elsevier Inc. All rights reserved.)

Published

2011

14. DNA methylation and mutator genes in Escherichia coli K-12.

Author

Marinus MG

Subjects

DNA Mismatch Repair, Recombination, Genetic, DNA Methylation, DNA, Bacterial metabolism, Escherichia coli genetics, Genes, Bacterial, Methylnitronitrosoguanidine pharmacology, Mutation, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

Mutator strains of Escherichia coli have been used to define mechanisms that account for the high fidelity of chromosome duplication and chromosome stability. Mutant strains defective in post-replicative mismatch repair display a strong mutator phenotype consistent with a role for correction of mismatches arising from replication errors. Inactivation of the gene (dam) encoding DNA adenine methyltransferase results in a mutator phenotype consistent with a role for DNA methylation in strand discrimination during mismatch repair. This review gives a personal perspective on the discovery of dam mutants in E. coli and their relationship to mismatch repair and mutator phenotypes., (Copyright © 2010 Elsevier B.V. All rights reserved.)

Published

2010

15. Fusion of GFP to the M.EcoKI DNA methyltransferase produces a new probe of Type I DNA restriction and modification enzymes.

Author

Chen K, Roberts GA, Stephanou AS, Cooper LP, White JH, and Dryden DT

Subjects

DNA chemistry, Deoxyribonucleases, Type I Site-Specific genetics, Fluorescence Resonance Energy Transfer, Green Fluorescent Proteins genetics, Recombinant Fusion Proteins genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Deoxyribonucleases, Type I Site-Specific chemistry, Green Fluorescent Proteins chemistry, Recombinant Fusion Proteins chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry

Abstract

We describe the fusion of enhanced green fluorescent protein to the C-terminus of the HsdS DNA sequence-specificity subunit of the Type I DNA modification methyltransferase M.EcoKI. The fusion expresses well in vivo and assembles with the two HsdM modification subunits. The fusion protein functions as a sequence-specific DNA methyltransferase protecting DNA against digestion by the EcoKI restriction endonuclease. The purified enzyme shows Förster resonance energy transfer to fluorescently-labelled DNA duplexes containing the target sequence and to fluorescently-labelled ocr protein, a DNA mimic that binds to the M.EcoKI enzyme. Distances determined from the energy transfer experiments corroborate the structural model of M.EcoKI., (Copyright (c) 2010 Elsevier Inc. All rights reserved.)

Published

2010

16. Epigenetic modification of rhizobial genome is essential for efficient nodulation.

Author

Ichida H, Yoneyama K, Koba T, and Abe T

Subjects

DNA Methylation, Genome, Bacterial, Symbiosis, Epigenesis, Genetic, Nitrogen Fixation genetics, Rhizobium genetics, Root Nodules, Plant microbiology, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

CcrM is one of the solitary bacterial DNA methyltransferases which does not have corresponding restriction enzymes. We established a stable ccrM-overexpressing mutant of Mesorhizobium loti, MlccrM-OX, and performed molecular and phenotypic characterization of this strain. In the M. loti MlccrM-OX infected plants, nodulation was apparently delayed at 7 days after inoculation (dai), however, the nodules that eventually formed on the MlccrM-OX roots showed nitrogen fixing ability by at least 21 dai. These results suggest that the initial morphogenic events were affected by ccrM-overexpression and that the correct pattern of DNA methylation of the bacterial genome is not essential for plant-microbe symbiosis, but are required for efficient nodulation.

Published

2009

17. Competitive Lrp and Dam assembly at the pap regulatory region: implications for mechanisms of epigenetic regulation.

Author

Peterson SN and Reich NO

Subjects

Base Sequence, Binding Sites genetics, Binding, Competitive, DNA Methylation, DNA Primers genetics, DNA, Bacterial genetics, DNA, Bacterial metabolism, Escherichia coli Proteins genetics, Kinetics, Leucine-Responsive Regulatory Protein genetics, Models, Biological, Operon, Protein Binding, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Epigenesis, Genetic, Escherichia coli genetics, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Fimbriae Proteins genetics, Leucine-Responsive Regulatory Protein metabolism, Regulatory Sequences, Nucleic Acid, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism

Abstract

Escherichia coli DNA adenine methyltransferase (Dam) and Leucine-responsive regulatory protein (Lrp) are key regulators of the pap operon, which codes for the pilus proteins necessary for uropathogenic E. coli cellular adhesion. The pap operon is regulated by a phase variation mechanism in which the methylation states of two GATC sites in the pap regulatory region and the binding position of Lrp determine whether the pilus genes are expressed. The post-replicative reassembly of Dam, Lrp, and the local regulator PapI onto a hemimethylated pap intermediate is a critical step of the phase variation switching mechanism and is not well understood. We show that Lrp, in the presence and in the absence of PapI and nonspecific DNA, specifically protects pap regulatory GATC sites from Dam methylation when allowed to compete with Dam for assembly on unmethylated and hemimethylated pap DNA. The methylation protection is dependent upon the concentration of Lrp and does not occur with non-regulatory GATC sites. Our data suggest that only at low Lrp concentrations will Dam compete effectively for binding and methylation of the proximal GATC site, leading to a phase switch resulting in the expression of pili.

Published

2008

18. Mismatch repair proteins collaborate with methyltransferases in the repair of O(6)-methylguanine.

Author

Rye PT, Delaney JC, Netirojjanakul C, Sun DX, Liu JZ, and Essigmann JM

Subjects

Electroporation, Escherichia coli, Escherichia coli Proteins genetics, Guanine metabolism, Oligonucleotides genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, DNA Mismatch Repair, DNA-Binding Proteins metabolism, Guanine analogs & derivatives, Methyltransferases metabolism

Abstract

DNA repair is essential for combatting the adverse effects of damage to the genome. One example of base damage is O(6)-methylguanine (O(6)mG), which stably pairs with thymine during replication and thereby creates a promutagenic O(6)mG:T mismatch. This mismatch has also been linked with cellular toxicity. Therefore, in the absence of repair, O(6)mG:T mismatches can lead to cell death or result in G:C-->A:T transition mutations upon the next round of replication. Cysteine thiolate residues on the Ada and Ogt methyltransferase (MTase) proteins directly reverse the O(6)mG base damage to yield guanine. When a cytosine is opposite the lesion, MTase repair restores a normal G:C pairing. However, if replication past the lesion has produced an O(6)mG:T mismatch, MTase conversion to a G:T mispair must still undergo correction to avoid mutation. Two mismatch repair pathways in E. coli that convert G:T mispairs to native G:C pairings are methyl-directed mismatch repair (MMR) and very short patch repair (VSPR). This work examined the possible roles that proteins in these pathways play in coordination with the canonical MTase repair of O(6)mG:T mismatches. The possibility of this repair network was analyzed by probing the efficiency of MTase repair of a single O(6)mG residue in cells deficient in individual mismatch repair proteins (Dam, MutH, MutS, MutL, or Vsr). We found that MTase repair in cells deficient in Dam or MutH showed wild-type levels of MTase repair. In contrast, cells lacking any of the VSPR proteins MutS, MutL, or Vsr showed a decrease in repair of O(6)mG by the Ada and Ogt MTases. Evidence is presented that the VSPR pathway positively influences MTase repair of O(6)mG:T mismatches, and assists the efficiency of restoring these mismatches to native G:C base pairs.

Published

2008

19. Structure and substrate recognition of the Escherichia coli DNA adenine methyltransferase.

Author

Horton JR, Liebert K, Bekes M, Jeltsch A, and Cheng X

Subjects

DNA Methylation, DNA, Bacterial genetics, Fluorescence, Kinetics, Mutagenesis, Site-Directed, S-Adenosylhomocysteine metabolism, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Substrate Specificity, Escherichia coli enzymology, Escherichia coli genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism

Abstract

The structure of the Escherichia coli Dam DNA-(adenine-N6)-methyltransferase in complex with cognate DNA was determined at 1.89 A resolution in the presence of S-adenosyl-L-homocysteine. DNA recognition and the dynamics of base-flipping were studied by site-directed mutagenesis, DNA methylation kinetics and fluorescence stopped-flow experiments. Our data illustrate the mechanism of coupling of DNA recognition and base-flipping. Contacts to the non-target strand in the second (3') half of the GATC site are established by R124 to the fourth base-pair, and by L122 and P134 to the third base-pair. The aromatic ring of Y119 intercalates into the DNA between the second and third base-pairs, which is essential for base-flipping to occur. Compared to previous published structures of bacteriophage T4 Dam, three major new observations are made in E.coli Dam. (1) The first Gua is recognized by K9, removal of which abrogates the first base-pair recognition. (2) The flipped target Ade binds to the surface of EcoDam in the absence of S-adenosyl-L-methionine, which illustrates a possible intermediate in the base-flipping pathway. (3) The orphaned Thy residue displays structural flexibility by adopting an extrahelical or intrahelical position where it is in contact to N120.

Published

2006

20. GATC flanking sequences regulate Dam activity: evidence for how Dam specificity may influence pap expression.

Author

Peterson SN and Reich NO

Subjects

DNA Methylation, Fimbriae Proteins biosynthesis, Fimbriae, Bacterial, Gene Expression Regulation, Bacterial, Models, Molecular, Mutation, Operon, Promoter Regions, Genetic, Protein Binding, Regulatory Sequences, Nucleic Acid, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Escherichia coli enzymology, Fimbriae Proteins genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry

Abstract

Escherichia coli DNA adenine methyltransferase (Dam) plays essential roles in DNA replication, mismatch repair and gene regulation. The differential methylation by Dam of the two GATC sequences in the pap promoter regulates the expression of pili genes necessary for uropathogenic E.coli cellular adhesion. Dam processively methylates GATC sites in various DNA substrates, yet the two pap GATC sites are not processively methylated. We previously proposed that the flanking sequences surrounding the two pap GATC sites contribute to the enzyme's distributive methylation. We show here that replacement of the poorly methylated pap GATC sites with sites predicted to be processively methylated indeed results in an increase in Dam processivity. The increased processivity is due to a change in the methyltransfer kinetics and not the binding efficiency of Dam. A competition experiment in which the flanking sequences of only one pap GATC site were altered demonstrates that the GATC flanking sequences directly regulate the enzyme's catalytic efficiency. The GATC flanking sequences in Dam-regulated promoters in E.coli and other bacteria are similar to those in the pap promoter. Gene regulation from some of these promoters involves mechanisms and proteins that are quite different from those in the pap operon. Further, GATC sequences previously identified to remain unmethylated within the E.coli genome, but whose function remains largely unassigned, are flanked by sequences predicted to be poorly methylated. We conclude that the GATC flanking sequences may be critical for expression of pap and other Dam-regulated genes by affecting the activity of Dam at such sites and, thus, its processivity. A model is proposed, illustrating how the sequences flanking the GATC sites in Dam-regulated promoters may contribute to this epigenetic mechanism of gene expression, and how flanking sequences contribute to the diverse biological roles of Dam.

Published

2006

21. Cisplatin induces DNA double-strand break formation in Escherichia coli dam mutants.

Author

Nowosielska A and Marinus MG

Subjects

Adenosine Triphosphatases genetics, DNA Helicases genetics, DNA Repair genetics, DNA, Bacterial drug effects, Escherichia coli drug effects, Escherichia coli enzymology, Escherichia coli Proteins genetics, Exodeoxyribonuclease V genetics, Mutation, Recombination, Genetic genetics, Antineoplastic Agents toxicity, Cisplatin toxicity, DNA Damage, Escherichia coli genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

Escherichia coli dam cells are more susceptible to the cytotoxic action of cisplatin than wildtype. Dam mutS or dam mutL bacteria, however, are resistant to this agent indicating that active mismatch repair sensitizes dam cells to cisplatin toxicity. Genetic data, obtained previously, were consistent with the generation and repair of cisplatin-induced double-strand breaks (DSBs). We measured DSB formation in temperature-sensitive dam recB mutants, after exposure to cisplatin, using pulse field gel electrophoresis and observed an increase in linear 100-300 kb DNA fragments corresponding to approximately 15-45 double strand breaks per genome. The formation of these DSBs was temperature and dose-dependent and was decreased in recBC bacteria at the permissive temperature or in dam(+) or mutS control strains. There was a three-fold increase in circa 2 mb linear chromosomal fragments in dam recBC strains at the non-permissive temperature compared to recBC alone. We show that dam priA strains are not viable suggesting that DSB formation is dependent on DNA replication restart. The sensitivity of priA mutants to cisplatin is also consistent with this conclusion.

Published

2005

22. Stopped-flow and mutational analysis of base flipping by the Escherichia coli Dam DNA-(adenine-N6)-methyltransferase.

Author

Liebert K, Hermann A, Schlickenrieder M, and Jeltsch A

Subjects

Amino Acid Sequence, Base Pair Mismatch, Conserved Sequence, DNA, Bacterial chemistry, Molecular Sequence Data, Mutagenesis, Site-Directed, S-Adenosylmethionine metabolism, Sequence Homology, Amino Acid, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, DNA Mutational Analysis, DNA, Bacterial genetics, Escherichia coli enzymology, Mutation genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

By stopped-flow kinetics using 2-aminopurine as a probe to detect base flipping, we show here that base flipping by the Escherichia coli Dam DNA-(adenine-N6)-methyltransferase (MTase) is a biphasic process: target base flipping is very fast (k(flip)>240 s(-1)), but binding of the flipped base into the active site pocket of the enzyme is slow (k=0.1-2 s(-1)). Whereas base flipping occurs in the absence of S-adenosyl-l-methionine (AdoMet), binding of the target base in the active site pocket requires AdoMet. Our data suggest that the tyrosine residue in the DPPY motif conserved in the active site of DNA-(adenine-N6)-MTases stacks to the flipped target base. Substitution of the aspartic acid residue of the DPPY motif by alanine abolished base flipping, suggesting that this residue contacts and stabilizes the flipped base. The exchange of Ser188 located in a loop next to the active center by alanine led to a seven- to eightfold reduction of k(flip), which was also reduced with substrates having altered GATC recognition sites and in the absence of AdoMet. These findings provide evidence that the enzyme actively initiates base flipping by stabilizing the transition state of the process. Reduced rates of base flipping in substrates containing the target base in a non-canonical sequence demonstrate that DNA recognition by the MTase starts before base flipping. DNA recognition, cofactor binding and base flipping are correlated and efficient base flipping takes place only if the enzyme has bound to a cognate target site and AdoMet is available.

Published

2004

23. Engineering of restriction endonucleases: using methylation activity of the bifunctional endonuclease Eco57I to select the mutant with a novel sequence specificity.

Author

Rimseliene R, Maneliene Z, Lubys A, and Janulaitis A

Subjects

Amino Acid Motifs, Binding Sites, DNA Methylation, DNA, Bacterial genetics, DNA, Bacterial metabolism, Deoxyribonucleases, Type II Site-Specific, Escherichia coli metabolism, Models, Genetic, Mutagenesis, Site-Directed, Protein Binding, Restriction Mapping, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Structure-Activity Relationship, Escherichia coli enzymology, Mutation genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

Type II restriction endonucleases (REs) are widely used tools in molecular biology, biotechnology and diagnostics. Efforts to generate new specificities by structure-guided design and random mutagenesis have been unsuccessful so far. We have developed a new procedure called the methylation activity-based selection (MABS) for generating REs with a new specificity. MABS uses a unique property of bifunctional type II REs to methylate DNA targets they recognize. The procedure includes three steps: (1) conversion of a bifunctional RE into a monofunctional DNA-modifying enzyme by cleavage center disruption; (2) mutagenesis and selection of mutants with altered DNA modification specificity based on their ability to protect predetermined DNA targets; (3) reconstitution of the cleavage center's wild-type structure. The efficiency of the MABS technique was demonstrated by altering the sequence specificity of the bifunctional RE Eco57I from 5'-CTGAAG to 5'-CTGRAG, and thus generating the mutant restriction endonuclease (and DNA methyltransferase) of a specificity not known before. This study provides evidence that MABS is a promising technique for generation of REs with new specificities.

Published

2003

24. A novel cholesteryl ester transfer protein promoter polymorphism (-971G/A) associated with plasma high-density lipoprotein cholesterol levels. Interaction with the TaqIB and -629C/A polymorphisms.

Author

Le Goff W, Guerin M, Nicaud V, Dachet C, Luc G, Arveiler D, Ruidavets JB, Evans A, Kee F, Morrison C, Chapman MJ, and Thillet J

Subjects

Adult, Aged, Base Sequence, Cardiovascular Diseases prevention & control, Cholesterol Ester Transfer Proteins, Female, Gene Expression Regulation, Genotype, Humans, Male, Middle Aged, Molecular Sequence Data, Polymerase Chain Reaction, Probability, Registries, Sampling Studies, Sensitivity and Specificity, Site-Specific DNA-Methyltransferase (Adenine-Specific) analysis, Cardiovascular Diseases genetics, Carrier Proteins genetics, Cholesterol, HDL blood, Cholesterol, HDL genetics, Glycoproteins, Polymorphism, Genetic, Promoter Regions, Genetic, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

The plasma cholesteryl ester transfer protein (CETP) plays a key role in reverse cholesterol transport (RCT) by mediating the transfer of cholesteryl ester (CE) from high-density lipoprotein (HDL) to atherogenic ApoB-containing lipoproteins, including VLDL, IDL and LDL. We describe a new polymorphism located at position -971 in the human CETP gene promoter, which corresponds to a G/A substitution at a potential AvaI restriction site. The relationship between the -971G/A polymorphism, plasma lipid parameters and plasma CETP concentration was evaluated in the Etude Cas-Témoins de l'Infarctus du Myocarde (control-myocardial infarction cases) cohort, and revealed that the -971G/A polymorphism (A allele frequency: 0.491) was significantly associated with both plasma high-density lipoprotein cholesterol (HDL-C) levels and CETP concentration (P=0.006 and 0.009, respectively). Subjects with genotype -971GG displayed both low HDL-C levels and high plasma CETP concentration, while genotype -971AA subjects displayed the inverse relationship. Evaluation of potential interactions between the -971G/A and the -629C/A or TaqIB polymorphisms demonstrated that the -971G/A polymorphism interacts significantly with the functional -629C/A site and the TaqIB polymorphism with respect to plasma HDL-C levels (P=0.0014 and 0.012, respectively), but does not affect plasma CETP concentration. These results clearly suggest that the interaction between the 971G/A polymorphism and either the -629C/A or the TaqIB polymorphism on plasma CETP concentration is different than that implicated in HDL-C levels. Transient transfection of HepG2 cells revealed that the -971G/A polymorphism did not modulate transcriptional activity of the human CETP gene promoter. The -971G/A promoter polymorphism therefore constitutes a non-functional marker. Furthermore, the observed effects of the -971G/A polymorphism on both plasma CETP concentration and HDL-C levels are due to functional variants in linkage disequilibrium with it. Our findings strongly suggest the existence of as yet unidentified functional polymorphisms in the CETP gene promoter that could explain the association between specific polymorphisms of the CETP gene and both plasma HDL-C and CETP concentrations.

Published

2002

25. Target recognition by EcoKI: the recognition domain is robust and restriction-deficiency commonly results from the proteolytic control of enzyme activity.

Author

O'Neill M, Powell LM, and Murray NE

Subjects

Adenosine Triphosphatases metabolism, Amino Acid Sequence, Amino Acid Substitution genetics, Binding Sites, Chromosomes, Bacterial genetics, DNA Restriction Enzymes genetics, DNA Restriction Enzymes isolation & purification, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, DNA-Binding Proteins isolation & purification, DNA-Binding Proteins metabolism, Endopeptidase Clp, Enzyme Activation, Escherichia coli genetics, Escherichia coli virology, Fluorescence Polarization, Molecular Sequence Data, Mutation genetics, Phenotype, Plasmids genetics, Plasmids metabolism, Protein Structure, Tertiary, Serine Endopeptidases metabolism, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) isolation & purification, Substrate Specificity, Transduction, Genetic, DNA Restriction Enzymes chemistry, DNA Restriction Enzymes metabolism, Escherichia coli enzymology, Escherichia coli Proteins, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism

Abstract

We report a genetic and biochemical analysis of a target recognition domain (TRD) of EcoKI, a type I restriction and modification enzyme. The TRDs of type I R-M systems are within the specificity subunit (HsdS) and HsdS confers sequence specificity to a complex endowed with both restriction and modification activities. Random mutagenesis has revealed that most substitutions within the amino TRD of EcoKI, a region comprising 157 amino acid residues, have no detectable effect on the phenotype of the bacterium, even when the substitutions are non- conservative. The structure of the TRD appears to be robust. All but one of the six substitutions that confer a restriction-deficient, modification-deficient (r(-)m(-)) phenotype were found to be in the interval between residues 80 and 110, a region predicted by sequence comparisons to form part of the protein-DNA interface. Additional site-directed mutations affecting this interval commonly impair both restriction and modification. However, we show that an r(-) phenotype cannot be taken as evidence that the EcoKI complex lacks endonuclease activity; in response to even a slightly impaired modification efficiency, the endonuclease activity of EcoKI is destroyed by a process dependent upon the ClpXP protease. Enzymes from mutants with an r(-)m(-) phenotype commonly retain some sequence-specific activity; methylase activity can be detected on hemimethylated DNA substrates and residual endonuclease activity is implied whenever the viability of the r(-)m(-) bacterium is dependent on ClpXP. Conversely, the viability of ClpX(-) r(-)m(-) bacteria can be used as evidence for little, or no, endonuclease activity. Of 14 mutants with an r(-)m(-) phenotype, only six are viable in the absence of ClpXP. The significance of four of the six residues (G91, G105, F107 and G141) is enhanced by the finding that even conservative substitutions for these residues impair modification, thereby conferring an r(-)m(-) phenotype., (Copyright 2001 Academic Press.)

Published

2001

26. Bacterial DNA methylation and gene transfer efficiency.

Author

Allamane S, Jourdes P, Ratel D, Vicat JM, Dupré I, Lainé M, Berger F, Benabid AL, and Wion D

Subjects

5-Methylcytosine, Adenine metabolism, Animals, Cell Line, Cells, Cultured, Cytosine metabolism, DNA Modification Methylases genetics, DNA Modification Methylases metabolism, Escherichia coli enzymology, Escherichia coli Proteins, Fibroblasts, Gene Amplification, Gene Deletion, Gene Silencing, Genes, Reporter genetics, Genetic Therapy methods, Luciferases genetics, Luciferases metabolism, Mice, Plasmids genetics, Plasmids metabolism, Promoter Regions, Genetic genetics, Rats, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Transfection, Adenine analogs & derivatives, Cytosine analogs & derivatives, DNA Methylation, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression Regulation, Gene Transfer Techniques, Transgenes genetics

Abstract

The necessary amplification step in bacteria of any plasmid currently used in DNA immunization or gene therapy introduces modification in the nucleotide sequence of plasmid DNA used in gene transfer. These changes affect the adenine and the internal cytosine in respectively all of the GATC and CC(A/T)GG sequences. These modifications which introduce 6-methyladenine and 5-methylcytosine in plasmidic DNA are the consequence of the existence of the bacterial modification systems Dam and Dcm. In eucaryotes, the presence of 5-methylcytosine at dinucleotides -CG- is involved in silencing gene expression, but the possible consequences of the presence of the bacterial G(m)ATC and C(m)C(A/T)GG sequences in the plasmids used in gene transfer experiments are presently unknown. Since the possibility exists to obtain plasmid DNA lacking this specific bacterial pattern of methylation by using (dam(-), dcm(-)) bacteria we performed experiments to compare in vitro and in vivo gene transfer efficiency of a pCMV-luc reporter plasmid amplified either in the JM109 (dam(+), dcm(+)) or JM110 (dam(-), dcm(-)) bacteria. Data obtained demonstrated that the presence of 6-methyladenine in GATC sequences and 5-methylcytosine in the second C of CC(A/T)GG motifs does not reduce the levels of luciferase activity detected following in vitro or in vivo gene transfer. On the contrary, gene transfer with a pCMV-luc amplified in JM109 (dam(+), dcm(+)) bacteria gives greater amounts of luciferase than the same transfection performed with a plasmid amplified in the mutated JM110 (dam(-), dcm(-)) counterpart. Therefore, these data do not suggest that the use of (dam(-), dcm(-)) bacteria to amplify plasmid DNA may increase gene transfer efficiency. However, the persistence of the use of (dam(+), dcm(+)) bacteria in order to amplify plasmid DNA raises the question of the possible biological consequences of the introduction of the bacterial G(m)ATC and C(m)C(A/T)GG sequences in eukaryotic cells or organisms., (Copyright 2000 Academic Press.)

Published

2000

27. Mutational analysis of target base flipping by the EcoRV adenine-N6 DNA methyltransferase.

Author

Jeltsch A, Roth M, and Friedrich T

Subjects

Cross-Linking Reagents metabolism, DNA genetics, DNA-Binding Proteins genetics, Mutagenesis, Site-Directed genetics, Oligodeoxyribonucleotides genetics, Photolysis, Protein Binding genetics, S-Adenosylmethionine metabolism, Thermodynamics, Uracil analogs & derivatives, Uracil metabolism, DNA Mutational Analysis, Mutation genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

DNA methyltransferases flip their target base out of the DNA helix. Here, we have investigated base flipping by wild-type EcoRV DNA methyltransferase (M.EcoRV) and five M.EcoRV variants (D193A, Y196A, S229A, W231R and Y258A). These variants bind to DNA and S-adenosylmethionine but have a severely reduced catalytic efficiency or are catalytically inactive. To measure base flipping three different assays were used, viz. analysis of the yields of photocrosslinking reactions between the enzymes and a substrate in which the target base is replaced by 5-iodouracil, analysis of the binding constants to substrates containing a mismatch base-pair at the target position and analysis of the salt dependence of specific complex formation. Our data show that the Y196A, W231R and Y258A variants are not able to stabilize a flipped target base, suggesting that the aromatic amino acid residues (Tyr196, Trp231 and Tyr258) are involved in hydrophobic interactions with the flipped base. The D193A variant behaves like wild-type M.EcoRV with respect to base flipping. The fact that this variant is catalytically inactive indicates that Asp193 has a function in chemical catalysis. The S229A variant can better flip modified bases but does not tightly lock the flipped base into the adenine-binding pocket, suggesting that Ser229 could form a contact to the flipped adenine., (Copyright 1998 Academic Press.)

Published

1999

28. KpnAI, a new type I restriction-modification system in Klebsiella pneumoniae.

Author

Lee NS, Rutebuka O, Arakawa T, Bickle TA, and Ryu J

Subjects

Cloning, Molecular, Escherichia coli, Genes, Bacterial, Genetic Complementation Test, Klebsiella pneumoniae genetics, Peptides chemistry, Restriction Mapping, Sequence Analysis, DNA, Sequence Homology, Amino Acid, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, DNA Restriction-Modification Enzymes genetics, Klebsiella pneumoniae enzymology

Abstract

The KpnAI restriction-modification (R-M) system has been identified in Klebsiella pneumoniae strain M5a1. The restriction gene of KpnAI was first cloned into pBR322 using an r-m+ M5a1 derivative and phage SBS for screening. Subsequently, an adjacent DNA fragment showing modification activity was cloned into pUC19. A total of 7.2 kb DNA sequencing data revealed three open reading frames, corresponding to hsdR, hsdM and hsdS genes of type I R-M systems. The predicted hsdR, hsdM and hsdS-coded peptides shared 95%, 98% and 44% identity, respectively, with the corresponding peptides of the recently identified StySBLI system, a prototype of the type ID family. This high homology suggests that KpnAI is also a member of the type ID family. The KpnAI system seems to be the first type I system identified in Klebsiella species.

Published

1997

29. The replisome organizer (G38P) of Bacillus subtilis bacteriophage SPP1 forms specialized nucleoprotein complexes with two discrete distant regions of the SPP1 genome.

Author

Missich R, Weise F, Chai S, Lurz R, Pedré X, and Alonso JC

Subjects

Bacillus subtilis genetics, Base Sequence, Binding Sites, Chromosome Mapping, Cloning, Molecular, DNA Footprinting, DNA Replication, DNA, Viral chemistry, DNA, Viral metabolism, Microscopy, Electron, Molecular Sequence Data, Nucleic Acid Conformation, Nucleoproteins genetics, Repetitive Sequences, Nucleic Acid, Replication Origin, Sequence Homology, Nucleic Acid, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Viral Proteins chemistry, Bacillus Phages genetics, Nucleoproteins metabolism, Viral Proteins genetics, Viral Proteins metabolism

Abstract

Initiation of Bacillus subtilis bacteriophage SPP1 DNA replication requires the products of genes 38, 39 and 40 (G38P, G39P and G40P). G38P specifically binds two discrete regions, which are 32.1 kb apart in a linear map of the SPP1 genome. One of these target sites, which maps at the left end of the phage genome, within gene 38, was shown to function as an origin of replication and was therefore termed left origin (oriL). The other site, which lies within a non-coding segment in the late transcribed region on the right end of the genome, was termed oriR. Both sites contain two types of repeated elements (termed Box AB and A + T-rich region). The K(app) for the G38P-oriL DNA and G38P-oriR DNA complexes was estimated to be 1 nM and 4 nM, respectively. G38P binds to the distant oriL and oriR sites cooperatively. DNase I footprinting experiments showed protection by G38P in Box AB, but not in the A + T-rich region. Electron microscopy analysis showed that G38P forms a higher-order nucleoprotein structure with the SPP1 oriL and oriR sites through protein-protein interaction. G38P binding at its cognate sites does not seem to modify the length of the DNA, but to bend it. These results suggest that G38P forms a nucleoprotein complex on the regions where the SPP1 replication origins were previously predicted.

Published

1997

30. Functional analysis of conserved motifs in EcoP15I DNA methyltransferase.

Author

Ahmad I and Rao DN

Subjects

Base Sequence, Binding Sites, Cloning, Molecular, Cross-Linking Reagents, DNA metabolism, DNA Primers, Molecular Sequence Data, Mutagenesis, Site-Directed, S-Adenosylmethionine, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Ultraviolet Rays, Conserved Sequence, Escherichia coli enzymology, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism

Abstract

EcoP15I DNA methyltransferase recognizes the sequence 5'-CAGCAG-3' and transfers a methyl group to N-6 of the second adenine residue in the recognition sequence. All N-6 adenine methyltransferases contain two highly conserved sequences, FxGxG (motif I), postulated to form part of the S-adenosyl-L-methionine binding site and (D/N/S)PP(Y/F) (motif IV) involved in catalysis. We have altered the second glycine residue in motif I to arginine and serine, and substituted tyrosine in motif IV with tryptophan in EcoP15I DNA methyltransferase, using site-directed mutagenesis. The mutant enzymes were overexpressed, purified and characterized by biochemical methods. The mutations in motif I completely abolished AdoMet binding but left target DNA recognition unaltered. Although the mutation in motif IV resulted in loss of enzyme activity, we observed enhanced crosslinking of S-adenosyl-L-methionine and DNA. This implies that DNA and AdoMet binding sites are close to motif IV. Taken together, these results reinforce the importance of motif I in AdoMet binding and motif IV in catalysis. Additionally, limited proteolysis and UV crosslinking experiments with EcoP15I DNA methyltransferase imply that DNA binds in a cleft formed by two domains in the protein. Methylation protection analysis provides evidence for the fact that EcoP15I DNA MTase makes contacts in the major groove of its substrate DNA. Interestingly, hypermethylation of the guanine residue next to the target adenine residue indicates that the protein probably flips out the target adenine residue.

Published

1996

31. An extended -10 promoter alone directs transcription of the DpnII operon of Streptococcus pneumoniae.

Author

Sabelnikov AG, Greenberg B, and Lacks SA

Subjects

Base Sequence, Genes, Bacterial genetics, Molecular Sequence Data, Operon genetics, Point Mutation physiology, RNA, Bacterial biosynthesis, RNA, Bacterial genetics, RNA, Messenger biosynthesis, RNA, Messenger genetics, Sequence Deletion physiology, Streptococcus pneumoniae enzymology, Deoxyribonucleases, Type II Site-Specific genetics, Promoter Regions, Genetic genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Streptococcus pneumoniae genetics, Transcription, Genetic genetics

Abstract

The genetic cassette encoding the DpnII restriction-modification system of Streptococcus pneumoniae gave transcription products of approximately 2.7 and 1.8 kilobases. The larger, mRNA1, covered both of the methylase genes, dpnM and dpnA, and the endonuclease gene dpnB; the smaller, mRNA2, covered only the dpnA and dpnB genes. Transcription of mRNA1 was shown to begin at the translation start site for dpnM, thereby producing an mRNA without any apparent ribosome-binding site for translation of the DpnM methylase. The promoter for mRNA1 was shown by base substitution and deletion analysis to consist of an extended -10 site, TaTGgTATAAT, with no required -35 site. A possible promoter further upstream with close matches to a -35 site and a nonextended -10 site was not used. A survey of 36 proven and putative promoters used by S. pneumoniae revealed that 61% of them contained the full -10 extension, although, other than the dpnM promoter, they matched at a -35 site, as well. It appears that, unlike those found in Escherichia coli, S. pneumoniae promoters frequently require an extended -10 site, and such a site can function naturally without a -35 site.

Published

1995

32. Deletions within the DNA recognition subunit of M.EcoR124I that identify a region involved in protein-protein interactions between HsdS and HsdM.

Author

Abadjieva A, Webb M, Patel J, Zinkevich V, and Firman K

Subjects

Amino Acid Sequence, Amino Acids chemistry, Base Sequence, Conserved Sequence, DNA, Viral metabolism, Deoxyribonucleases, Type I Site-Specific chemistry, Genetic Complementation Test, Molecular Sequence Data, Peptide Fragments chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, Deoxyribonucleases, Type I Site-Specific genetics, Deoxyribonucleases, Type I Site-Specific metabolism, Sequence Deletion physiology

Abstract

The DNA recognition subunit (HsdS) of type I restriction endonucleases can be divided into domains by means of amino acid identity between subunits from the same family. It has been proposed that DNA-protein interactions occur within the variable domains of the subunit and that protein-protein interactions involve the conserved domains. We have constructed a number of deletion mutants of HsdS that have allowed us to investigate protein-protein interactions. Using a combination of a "competitive" complementation assay and the ability of HsdM to "solubilize" HsdS, we have defined a region within the central conserved domain of HsdS that is responsible for HsdS-HsdM interaction. Computer analysis of amino acid identity between the N-terminal half and the C-terminal half of HsdS identifies a region (repeated in both conserved domains), one copy of which overlaps the region we have identified as essential for HsdS-HsdM interactions, which may be responsible for such protein-protein interactions.

Published

1994

33. The Escherichia coli prr region encodes a functional type IC DNA restriction system closely integrated with an anticodon nuclease gene.

Author

Tyndall C, Meister J, and Bickle TA

Subjects

Amino Acid Sequence, Bacteriophage lambda growth & development, Base Sequence, Cloning, Molecular, Cosmids, DNA Modification Methylases chemistry, DNA Modification Methylases isolation & purification, DNA Modification Methylases metabolism, DNA, Viral metabolism, Methylation, Molecular Sequence Data, Mutagenesis, Insertional, Restriction Mapping, Sequence Analysis, DNA, Sequence Homology, Amino Acid, Sequence Homology, Nucleic Acid, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry, Site-Specific DNA-Methyltransferase (Adenine-Specific) isolation & purification, Site-Specific DNA-Methyltransferase (Adenine-Specific) metabolism, DNA Modification Methylases genetics, Escherichia coli genetics, Genes, Bacterial genetics, Ribonucleases genetics, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics

Abstract

The prr locus was originally described as coding a ribonuclease that is activated after phage T4 infection to cut within the anticodon of a specific tRNA, inactivating protein synthesis and thus blocking phage development. Wild-type T4 phage has two genes coding the enzymes polynucleotide kinase and RNA ligase, whose only function seems to be to repair the damage done by the anticodon nuclease. As the only apparent function of the prr ribonuclease is to combat phage infection, it can be considered as an RNA-based restriction enzyme. In non-infected cells, the prr enzyme is kept inactive in a complex with three other proteins which were predicted on the basis of DNA homologies to be the subunits of a type IC DNA restriction and modification system. Unlike other type IC systems so far characterized, prr is chromosomally rather than plasmid coded. However, sequences upstream from prr also have homology with sequences from the plasmid R124 and the prophage P1. We have now investigated the prr system and shown that it is indeed a bona fide type IC system which we call EcoprrI, and which is active both in vivo and in vitro. The system is fully functional even in the absence of the anticodon nuclease and seems to be a typical type I enzyme. EcoprrI recognizes the sequence CCA(N7)RTGC. One peculiarity is that, with low efficiency, EcoprrI will recognize and methylate variants of its recognition sequence such as CCT(N7)ATGC, which is methylated in one strand of the DNA only.

Published

1994

34. The domains of a type I DNA methyltransferase. Interactions and role in recognition of DNA methylation.

Author

Cooper LP and Dryden DT

Subjects

Amino Acid Sequence, Base Sequence, Binding Sites, DNA genetics, Escherichia coli enzymology, Molecular Sequence Data, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments isolation & purification, Protein Conformation, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Substrate Specificity, Site-Specific DNA-Methyltransferase (Adenine-Specific) chemistry

Abstract

The DNA methyltransferases of type I restriction-modification systems are trimeric enzymes composed of one DNA specificity (S) subunit and two modification (M) subunits. The S subunit contains two large regions, each of which recognizes one part of the split, asymmetrical DNA target sequence. Each M subunit contains an amino acid motif for binding the methyl group donor and cofactor, S-adenosyl methionine. The EcoKI methyltransferase has a strong preference for methylating a hemimethylated DNA target rather than an unmodified target. We have used partial proteolytic digestion of EcoKI methyltransferase to generate polypeptide domains that we have identified by amino acid sequencing. The S subunit was cut into two large, folded domains each containing one DNA binding region. Binding of DNA partially protected the S subunit from digestion. The M subunit was also cut into two large domains joined together by a short flexible loop, and a C-terminal tail region. The short loop contained part of the S-adenosyl methionine binding motif, and cofactor binding protected the loop and the two large domains from proteolysis. The C-terminal domain of M remained associated with the N-terminal domain of the S subunit even after the rest of the protein had been digested. The conformation of the tail region of the M subunit was sensitive to the methylation state of DNA in ternary complexes also containing S-adenosyl methionine, and could differentiate between unmethylated and hemimethylated DNA substrates.

Published

1994

35. A Caulobacter DNA methyltransferase that functions only in the predivisional cell.

Author

Zweiger G, Marczynski G, and Shapiro L

Subjects

Amino Acid Sequence, Base Sequence, Caulobacter crescentus cytology, Cell Division genetics, Gene Expression physiology, Genes, Bacterial physiology, Lac Operon physiology, Methylation, Molecular Sequence Data, Promoter Regions, Genetic physiology, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Caulobacter crescentus enzymology, DNA, Bacterial metabolism, Site-Specific DNA-Methyltransferase (Adenine-Specific) physiology

Abstract

Caulobacter crescentus was found to have a DNA methyltransferase, CcrM, that methylates the adenine base of the HinfI recognition sequence, GANTC. The ccrM gene was cloned, and DNA sequence analysis revealed that the predicted amino acid sequence has 49% identity with the Haemophilus influenzae methyltransferase HinfM. Expression of the ccrM gene was found to be restricted to the portion of the cell cycle immediately prior to cell division. At three separate chromosomal sites the CcrM recognition sequence is fully methylated in swarmer cells, becomes hemimethylated upon DNA replication in stalked cells, and does not become remethylated until just prior to cell division. The time of methyltransferase expression coincides with the time of methylation of these three chromosomal sites and of plasmid DNA in the predivisional cell. When ccrM gene expression is placed under control of a constitutive promoter, these chromosomal sites are fully methylated throughout the cell cycle. A high proportion of morphologically aberrant cells, and cells that have undergone an additional chromosome replication initiation, are found in this population. Thus, the temporal control of this methyltransferase appears to contribute to the accurate cell-cycle control of DNA replication and cellular morphology.

Published

1994

36. A mutation in the dam gene of Vibrio cholerae: 2-aminopurine sensitivity with intact GATC methylase activity.

Author

Bandyopadhyay R, Sengupta A, and Das J

Subjects

Aminacrine pharmacology, Bacteriophages genetics, Base Sequence, Conjugation, Genetic, Escherichia coli genetics, Kinetics, Methyl Methanesulfonate pharmacology, Plasmids, Substrate Specificity, Ultraviolet Rays, Vibrio cholerae drug effects, Vibrio cholerae radiation effects, 2-Aminopurine pharmacology, Adenine analogs & derivatives, Genes, Bacterial, Mutation, Site-Specific DNA-Methyltransferase (Adenine-Specific) genetics, Vibrio cholerae genetics

Abstract

Vibrio cholerae mutants sensitive to 2-aminopurine (2AP) but with DNA adenine methylase activity similar to parental cells have been isolated. The mutant strains were sensitive to ultraviolet light (UV), methyl methane sulphonate (MMS) and 9-aminoacridine. The spontaneous mutation frequency of the mutants were not significantly affected. Attempts to isolate dam V. cholerae cells by screening 2AP sensitive cells have not been successful. All the mutant phenotypes could be suppressed by introducing the plasmid pRB103 carrying the dam gene of Escherichia coli into the mutant cells.

Published

1989