ABSTRACT
The Escherichia coli AlkB protein catalyzes the direct reversal of alkylation damage to DNA; primarily 1-methyladenine (1mA) and 3-methylcytosine (3mC) lesions created by endogenous or environmental alkylating agents. AlkB is a member of the non-heme iron (II) alpha-ketoglutarate-dependent dioxygenase superfamily, which removes the alkyl group through oxidation eliminating a methyl group as formaldehyde. We have developed a fluorescence-based assay for the dealkylation activity of this family of enzymes. It uses formaldehyde dehydrogenase to convert formaldehyde to formic acid and monitors the creation of an NADH analog using fluorescence. This assay is a great improvement over the existing assays for DNA demethylation in that it is continuous, rapid and does not require radioactively labeled material. It may also be used to study other demethylation reactions including demethylation of histones. We used it to determine the kinetic constants for AlkB and found them to be somewhat different than previously reported values. The results show that AlkB demethylates 1mA and 3mC with comparable efficiencies and has only a modest preference for a single-stranded DNA substrate over its double-stranded DNA counterpart.
Subject(s)
DNA Repair Enzymes/analysis , Escherichia coli Proteins/analysis , Mixed Function Oxygenases/analysis , Spectrometry, Fluorescence/methods , DNA/chemistry , DNA/metabolism , DNA Repair Enzymes/metabolism , Escherichia coli Proteins/metabolism , Formaldehyde/analysis , Kinetics , Mixed Function Oxygenases/metabolism , NAD/analogs & derivatives , NAD/chemistry , Substrate SpecificityABSTRACT
The morbidity associated with open procedures for lumbar intervertebral disc prolapse has led to the development of minimally invasive techniques. Ho: LADD (Laser-assisted disc decompression) is a very cost-effective minimally invasive procedure. The procedure is carried out under local anesthesia. The patient can be mobilized immediately after the surgery. The study involved 36 cases treated with Ho: LADD for contained lumbar intervertebral disc prolapse. 35 cases were available for follow-up. There was a 91.5% success rate and a minimal complication rate. All cases adhered to strict inclusion and exclusion criteria and were evaluated with the modified Macnab criteria for the assessment of postoperative results.
Subject(s)
Diskectomy/methods , Intervertebral Disc Displacement/surgery , Adult , Anesthesia, Local , Follow-Up Studies , Humans , Laser Therapy , Middle Aged , Minimally Invasive Surgical ProceduresABSTRACT
Maize malic enzyme was rapidly inactivated by micromolar concentrations of cupric nitrate in the presence of ascorbate at pH, 5.0. Ascorbate or Cu2+ alone had no effect on enzyme activity. The substrate L-malate or NADP individually provided almost total protection against Cu2+-ascorbate inactivation. The loss of enzyme activity was accompanied by cleavage of the enzyme. The cleaved peptides showed molecular mass of 55 kDa, 48 kDa, 38 kDa, and 14 kDa. Addition of EDTA, histidine and imidazole provided protection. The results of protection experiments with sodium azide, DABCO and catalase suggested that reactive oxygen species were generated resulting in loss of enzyme activity. This was further supported by experiments showing that the rate of enzyme inactivation was higher in D2O than in water. It is suggested that maize malic enzyme is modified by reactive oxygen species like singlet oxygen and H2O2 generated by Cu2+-ascorbate system and the modified amino acid residue(s) may be located at or near the substrate-binding site of the enzyme.
Subject(s)
Ascorbic Acid/chemistry , Copper/chemistry , Malates/chemistry , NADP/chemistry , Zea mays/metabolism , Amino Acids/chemistry , Catalase/chemistry , Deuterium Oxide/chemistry , Edetic Acid/chemistry , Histidine/chemistry , Hydrogen Peroxide/chemistry , Hydrogen-Ion Concentration , Imidazoles/chemistry , Oxygen/chemistry , Piperazines/chemistry , Reactive Oxygen SpeciesABSTRACT
The incubation of maize malic enzyme at 37 degrees C with trypsin at a ratio of 150:1 of malic enzyme to trypsin caused rapid and complete inactivation of enzyme activity. The inactivation was caused by fairly specific cleavage of the enzyme monomer (62 kDa) into 40 kDa and 20 kDa fragments. The intensity of 40 kDa band increased with the time of treatment of enzyme with trypsin from 2 to 30 min. Substrates, especially NADP (25 microM) provided almost total protection against trypsin inactivation of the enzyme activity. The studies carried out with various other endoproteases indicated that endoprotease Lys-C was most effective in inactivating malic enzyme activity. The kinetic properties of the truncated enzyme have been studied. The Km value for malate in case of native and modified enzyme was found to be identical. Km NADP for the modified enzyme was slightly higher indicating that after proteolysis the enzyme affinity for NADP had decreased. Limited proteolysis with trypsin did not show any appreciable change in fluorescence properties of the modified enzyme. Binding of NADPH to the enzyme was not affected after modification.
Subject(s)
Malate Dehydrogenase/chemistry , Zea mays/enzymology , Biochemistry/methods , Electrophoresis, Polyacrylamide Gel , Hydrogen-Ion Concentration , Kinetics , Lysine/chemistry , Magnesium/chemistry , Models, Chemical , Peptide Hydrolases/chemistry , Protein Conformation , Proteins/chemistry , Proteolysis , Substrate Specificity , Trypsin/chemistry , Trypsin Inhibitors/pharmacologyABSTRACT
In Escherichia coli and related bacteria, the very-short-patch (VSP) repair pathway uses an endonuclease, Vsr, to correct T-G mismatches that result from the deamination of 5-methylcytosines in DNA to C-G. The products of mutS and mutL, which are required for adenine methylation-directed mismatch repair (MMR), enhance VSP repair. Multicopy plasmids carrying mutS alleles that are dominant negative for MMR were tested for their effects on VSP repair. Some mutS mutations (class I) did not lower VSP repair in a mutS(+) background, and most class I mutations increased VSP repair in mutS cells more than plasmids containing mutS(+). Other plasmid-borne mutS mutations (class II) and mutS(+) decreased VSP repair in the mutS(+) background. Thus, MutS protein lacking functions required for MMR can still participate in VSP repair, and our results are consistent with a model in which MutS binds transiently to the mispair and then translocates away from the mispair to create a specialized structure that enhances the binding of Vsr.
Subject(s)
Adenine/metabolism , Adenosine Triphosphatases , Bacterial Proteins/genetics , Bacterial Proteins/physiology , DNA Repair , DNA-Binding Proteins , Endodeoxyribonucleases/genetics , Endodeoxyribonucleases/physiology , Escherichia coli Proteins , Alleles , Base Pair Mismatch , DNA Methylation , DNA, Bacterial/genetics , Models, Molecular , MutL Proteins , MutS DNA Mismatch-Binding Protein , MutationABSTRACT
We showed previously that transcription of a plasmid-borne kan allele increases C-to-T mutations in the nontranscribed strand. Using two new plasmid-borne kan alleles, one cmp allele, and a chromosomal kan allele, we found in this study that transcription-induced mutations are not limited to specific genes, alleles, or locations and are likely to be a general property of transcript elongation in Escherichia coli.
Subject(s)
Cytosine , DNA, Bacterial/genetics , Escherichia coli/genetics , Point Mutation , Thymine , Alleles , Chromosomes , Genes, Bacterial , Kanamycin Resistance/genetics , Plasmids , Transcription, GeneticABSTRACT
The Escherichia coli DNA glycosylase Mug excises 3,N(4)-ethenocytosines (epsilon C) and uracils from DNA, but its biological function is obscure. This is because epsilon C is not found in E. coli DNA, and uracil-DNA glycosylase (Ung), a distinct enzyme, is much more efficient at removing uracils from DNA than Mug. We find that Mug is overexpressed as cells enter stationary phase, and it is maintained at a fairly high level in resting cells. This is true of cells grown in rich or minimal media, and the principal regulation of mug is at the level of mRNA. Although the expression of mug is strongly dependent on the stationary-phase sigma factor, sigma(S), when cells are grown in minimal media, it shows only a modest dependence on sigma(S) when cells are grown in rich media. When mug cells are maintained in stationary phase for several days, they acquire many more mutations than their mug(+) counterparts. This is true in ung as well as ung(+) cells, and a majority of new mutations may not be C to T. Our results show that the biological role of Mug parallels its expression in cells. It is expressed poorly in exponentially growing cells and has no apparent role in mutation avoidance in these cells. In contrast, Mug is fairly abundant in stationary-phase cells and has an important anti-mutator role at this stage of cell growth. Thus, Mug joins a very small coterie of DNA repair enzymes whose principal function is to avoid mutations in stationary-phase cells.
Subject(s)
DNA Glycosylases , Escherichia coli/enzymology , Escherichia coli/growth & development , Gene Expression Regulation, Bacterial , Mutation , N-Glycosyl Hydrolases/metabolism , Thymine DNA Glycosylase , Bacterial Proteins/genetics , Bacterial Proteins/metabolism , Culture Media , DNA Repair , N-Glycosyl Hydrolases/genetics , RNA, Messenger/genetics , RNA, Messenger/metabolism , Sigma Factor/genetics , Sigma Factor/metabolism , Uracil-DNA GlycosidaseABSTRACT
Maize phosphoenolpyruvate carboxylase (PEPC) was rapidly and completely inactivated by very low concentrations of trypsin at 37 degrees C. PEP+Mg2+ and several other effectors of PEP carboxylase offered substantial protection against trypsin inactivation. Inactivation resulted from a fairly specific cleavage of 20 kDa peptide from the enzyme subunit. Limited proteolysis under catalytic condition (in presence of PEP, Mg2+ and HCO3) although yielded a truncated subunit of 90 kDa, did not affect the catalytic function appreciably but desensitized the enzyme to the effectors like glucose-6-phosphate glycine and malate. However, under non-catalytic condition, only malate sensitivity was appreciably affected. Significant protection of the enzyme activity against trypsin during catalytic phase could be either due to a conformational change induced on substrate binding. Several lines of evidence indicate that the inactivation caused by a cleavage at a highly conserved C-terminal end of the subunit.
Subject(s)
Phosphoenolpyruvate Carboxylase/metabolism , Trypsin/pharmacology , Zea mays/enzymology , Bicarbonates/pharmacology , Fluorescence , Glucose-6-Phosphate/pharmacology , Glycine/pharmacology , Kinetics , Magnesium/pharmacology , Malates/pharmacology , Phosphoenolpyruvate Carboxylase/antagonists & inhibitors , Phosphorylation , Protein Conformation , Sulfhydryl Compounds/chemistryABSTRACT
The enzymes that transfer a methyl group to C5 of cytosine within specific sequences (C5 Mtases) deaminate the target cytosine to uracil if the methyl donor S-adenosylmethionine (SAM) is omitted from the reaction. Recently, it was shown that cytosine deamination caused by C5 Mtases M.HpaII, M.SssI and M.MspI is enhanced in the presence of several analogues of SAM, and a mechanism for this analogue-promoted deamination was proposed. According to this mechanism, the analogues protonate C5 of the target cytosine, creating a dihydrocytosine intermediate that is susceptible to deamination. We show here that one of these analogues, 5'-aminoadenosine (AA), enhances cytosine deamination by the Mtase M. EcoRII, but it does so without enhancing protonation of C5. Further, we show that uracil is an intermediate in the mutational pathway and propose an alternate mechanism for the analogue-promoted deamination. The new mechanism involves a facilitated water attack at C4 but does not require attack at C6 by the enzyme. The latter feature of the mechanism was tested by using M.EcoRII mutants defective in the nucleophilic attack at C6 in the deamination assay. We find that although these proteins are defective in methyl transfer and cytosine deamination, they cause cytosine deaminations in the presence of AA in the reaction. Our results point to a possible connection between the catalytic mechanism of C5 Mtases and of enzymes that transfer methyl groups to N(4) of cytosine. Further, they provide an unusual example where a coenzyme activates an otherwise "dead" enzyme to perform catalysis by a new reaction pathway.
Subject(s)
Cytosine/chemistry , DNA (Cytosine-5-)-Methyltransferases/antagonists & inhibitors , DNA (Cytosine-5-)-Methyltransferases/chemistry , S-Adenosylmethionine/chemistry , Adenosine/analogs & derivatives , Adenosine/chemistry , Alanine/genetics , Cysteine/genetics , DNA-Cytosine Methylases/chemistry , DNA-Cytosine Methylases/genetics , Deamination , Enzyme Inhibitors/chemistry , Escherichia coli/enzymology , Mutagenesis, Site-Directed , Serine/genetics , Uracil/chemistryABSTRACT
Illumination increased markedly the affinity to bicarbonate of phosphoenolpyruvate carboxylase (PEPC; EC 4.1.1.31) in leaves of Amaranthus hypochondriacus L., a C4 plant. When leaves were illuminated, the apparent Km for (HCO3-) of PEPC decreased by about 50% concurrent with a 2- to 5-fold increase in Vmax and 3- to 4-fold increase in Ki for malate. The inclusion of ethoxyzolamide, an inhibitor of carbonic anhydrase, during the assay had no effect on kinetic and regulatory properties of PEPC indicating that carbonic anhydrase was not involved during light-induced sensitization of PEPC to HCO3-. Pretreatment of leaf discs with cycloheximide (CHX), a cytosolic protein synthesis inhibitor, suppressed significantly the light-enhanced decrease in apparent Km (HCO3-). Further, in vitro phosphorylation of purified dark-form PEPC by protein kinase A (PKA) decreased the apparent Km (HCO3-) of the enzyme, in addition increasing Ki (malate) as expected. Such changes, due to in vitro phosphorylation of purified PEPC by PKA, occurred only with wild-type PEPC, but not in the mutant form of maize (S15D) which is already a mimic of the phosphorylated enzyme. These results suggest that phosphorylation of the enzyme is important during the sensitization of PEPC to HCO3- by illumination in C4 leaves. Since illumination is expected to increase the cytosolic pH and the availability of dissolved HCO3- in mesophyll cells, the sensitization by light of PEPC to HCO3- could be physiologically quite significant.
Subject(s)
Bicarbonates/metabolism , Magnoliopsida/radiation effects , Phosphoenolpyruvate Carboxylase/metabolism , Plant Leaves/radiation effects , Light , Magnoliopsida/enzymology , Malates/metabolism , Plant Leaves/enzymologyABSTRACT
We show here that transcription by the bacteriophage T7 RNA polymerase increases the deamination of cytosine bases in the non-transcribed strand to uracil, causing C to T mutations in that strand. Under optimal conditions, the mutation frequency increases about fivefold over background, and is similar to that seen with the Escherichia coli RNA polymerase. Further, we found that a mutant T7 RNA polymerase with a slower rate of elongation caused more cytosine deaminations than its wild-type parent. These results suggest that promoting cytosine deamination in the non-transcribed strand is a general property of transcription in E. coli and is dependent on the length of time the transcription bubble stays open during elongation. To see if transcription-induced mutations have influenced the evolution of bacteriophage T7, we analyzed its genome for a bias in base composition. Our analysis showed a significant excess of thymine over cytosine bases in the highly transcribed regions of the genome. Moreover, the average value of this bias correlated well with the levels of transcription of different genomic regions. Our results indicate that transcription-induced mutations have altered the composition of bacteriophage T7 genome and suggest that this may be a significant force in genome evolution.
Subject(s)
Bacteriophage T7/enzymology , Bacteriophage T7/genetics , DNA-Directed RNA Polymerases/metabolism , Genome, Viral , Mutagenesis/genetics , Transcription, Genetic/genetics , Amination , Amino Acid Substitution/genetics , Base Composition , Cytosine/metabolism , DNA-Directed RNA Polymerases/genetics , Escherichia coli/enzymology , Escherichia coli/genetics , Evolution, Molecular , Genes, Viral/genetics , Kinetics , RNA, Bacterial/biosynthesis , RNA, Bacterial/genetics , RNA, Messenger/biosynthesis , RNA, Messenger/genetics , Templates, Genetic , Thymine/metabolism , Viral ProteinsABSTRACT
The human thymine-DNA glycosylase has a sequence homolog in Escherichia coli that is described to excise uracils from U.G mismatches (Gallinari, P., and Jiricny, J. (1996) Nature 383, 735-738) and is named mismatched uracil glycosylase (Mug). It has also been described to remove 3,N(4)-ethenocytosine (epsilonC) from epsilonC.G mismatches (Saparbaev, M., and Laval, J. (1998) Proc. Natl. Acad. Sci. U. S. A. 95, 8508-8513). We used a mug mutant to clarify the role of this protein in DNA repair and mutation avoidance. We find that inactivation of mug has no effect on C to T or 5-methylcytosine to T mutations in E. coli and that this contrasts with the effect of ung defect on C to T mutations and of vsr defect on 5-methylcytosine to T mutations. Even under conditions where it is overproduced in cells, Mug has little effect on the frequency of C to T mutations. Because uracil-DNA glycosylase (Ung) and Vsr are known to repair U.G and T.G mismatches, respectively, we conclude that Mug does not repair U.G or T.G mismatches in vivo. A defect in mug also has little effect on forward mutations, suggesting that Mug does not play a role in avoiding mutations due to endogenous damage to DNA in growing E. coli. Cell-free extracts from mug(+) ung cells show very little ability to remove uracil from DNA, but can excise epsilonC. The latter activity is missing in extracts from mug cells, suggesting that Mug may be the only enzyme in E. coli that can remove this mutagenic adduct. Thus, the principal role of Mug in E. coli may be to help repair damage to DNA caused by exogenous chemical agents such as chloroacetaldehyde.
Subject(s)
Cytosine/analogs & derivatives , DNA Repair , DNA, Bacterial/metabolism , Escherichia coli/enzymology , Escherichia coli/genetics , N-Glycosyl Hydrolases/metabolism , Thymine DNA Glycosylase , 5-Methylcytosine , Base Pair Mismatch , Cytosine/metabolism , DNA, Bacterial/genetics , Endodeoxyribonucleases/metabolism , Humans , Mutagenesis , N-Glycosyl Hydrolases/genetics , Open Reading Frames , Point Mutation , Substrate Specificity , ThymineABSTRACT
Repair synthesis catalysed by DNA polymerase beta at 1 nt gaps occurs in the main pathway of mammalian base excision repair. DNA polymerase beta has no exonucleolytic proof-reading ability, and exhibits high error frequency during DNA synthesis. Consequently, continuous correction of endogenous DNA damage by short-patch repair synthesis might lead to a high spontaneous mutation rate, unless subsequent steps in the repair pathway allow for selective removal of incorporation errors. We show here that both human DNA ligase I and III discriminate strongly between a correctly paired versus a mispaired residue at the 3' position of a nick in DNA, when assayed in the presence of physiological concentrations of KCl. The resulting delay in joining after misincorporation by DNA polymerase beta during gap filling could allow for removal of the mismatched terminal residue by a distinct 3' exonuclease.
Subject(s)
DNA Ligases/metabolism , DNA Repair , Base Sequence , Catalysis , DNA Ligase ATP , Humans , Kinetics , Molecular Sequence Data , Poly-ADP-Ribose Binding Proteins , Potassium Chloride , Substrate Specificity , Xenopus ProteinsABSTRACT
In Escherichia coli and human cells, many sites of cytosine methylation in DNA are hot spots for C to T mutations. It is generally believed that T.G mismatches created by the hydrolytic deamination of 5-methylcytosines (5meC) are intermediates in the mutagenic pathway. A number of hypotheses have been proposed regarding the source of the mispaired thymine and how the cells deal with the mispairs. We have constructed a genetic reversion assay that utilizes a gene on a mini-F to compare the frequency of occurrence of C to T mutations in different genetic backgrounds in exponentially growing E. coli. The results identify at least two causes for the hot spot at a 5meC: (1) the higher rate of deamination of 5meC compared to C generates more T.G than uracil.G (U.G) mismatches, and (2) inefficient repair of T.G mismatches by the very short-patch (VSP) repair system compared to the repair of U. G mismatches by the uracil-DNA glycosylase (Ung). This combination of increased DNA damage when the cytosines are methylated coupled with the relative inefficiency in the post-replicative repair of T.G mismatches can be quantitatively modeled to explain the occurrence of the hot spot at 5meC. This model has implications for mutational hot and cold spots in all organisms.
Subject(s)
DNA Methylation , Models, Genetic , Point Mutation , 5-Methylcytosine , Cell Division/genetics , Cytosine/analogs & derivatives , Cytosine/chemistry , DNA Damage , DNA Repair , DNA, Bacterial/genetics , DNA, Bacterial/metabolism , Escherichia coli/cytology , Escherichia coli/genetics , Escherichia coli/growth & development , Humans , Replicon , Thymine/chemistryABSTRACT
We recently showed that transcription can promote C to T mutations in the non-transcribed strand in E. coli. To study the relationship between the level of transcription and mutant frequency, an inactive allele of the kanamycin-resistance gene was expressed under the control of a hybrid promoter consisting of an UP element and the tac promoter. When this promoter is induced, the frequency of C to T mutations in the non-transcribed strand increases in rough proportion to the amount of mRNA. At the highest level of transcription at which cell growth is not affected, there is about a 10-fold increase in the frequency of mutations. This result is consistent with the hypothesis that transcription forces the non-transcribed strand to be in a single-stranded state and that this results in frequent C to T mutations.
Subject(s)
Cytosine , DNA, Bacterial , Escherichia coli/genetics , Mutation , Thymine , Transcription, Genetic , Cell LineABSTRACT
The cytosine methyltransferases (MTases) M. HhaI and M. HpaII bind substrates in which the target cytosine is replaced by uracil or thymine, i.e. DNA containing a U:G or a T:G mismatch. We have extended this observation to the EcoRII MTase (M. EcoRII) and determined the apparent Kd for binding. Using a genetic assay we have also tested the possibility that MTase binding to U:G mismatches may interfere with repair of the mismatches and promote C:G to T:A mutations. We have compared two mutants of M. EcoRII that are defective for catalysis by the wild-type enzyme for their ability to bind DNA containing U:G or T:G mismatches and for their ability to promote C to T mutations. We find that although all three proteins are able to bind DNAs with mismatches, only the wild-type enzyme promotes C:G to T:A mutations in vivo. Therefore, the ability of M. EcoRII to bind U:G mismatched duplexes is not sufficient for their mutagenic action in cells.
Subject(s)
DNA, Bacterial/metabolism , DNA-Cytosine Methylases/metabolism , Nucleic Acid Heteroduplexes/metabolism , Point Mutation , 5-Methylcytosine , Binding Sites , Cytosine/analogs & derivatives , Cytosine/metabolism , DNA Methylation , DNA Repair , DNA-Cytosine Methylases/genetics , Drug Resistance, Microbial , Escherichia coli/drug effects , Escherichia coli/enzymology , Escherichia coli/genetics , Kanamycin/pharmacology , Mutation , Oligodeoxyribonucleotides/metabolismABSTRACT
Maize leaf NADP-malic enzyme was rapidly inactivated by micromolar concentrations of Woodward's reagent K (WRK). The inactivation followed pseudo-first order reaction kinetics. The order of reaction with respect to WRK was 1, suggesting that inactivation was a consequence of the modification of a single residue per active site. The modified enzyme showed a characteristic absorbance at 346 nm due to carboxyl group modification and also exhibited altered surface charge as seen from the elution profile on "Mono Q" anion exchange column and the mobility on native polyacrylamide gel electrophoresis. Substrate NADP and NADP + Mg2+ strongly protected the enzyme against WRK inactivation indicating that the modified residue may be located at or near the active site. Binding affinity of NADPH to the malic enzyme was studied by the fluorescence technique. The native enzyme binds NADPH strongly resulting in enhancement of the fluorescence emission and also causes a blue shift in the emission maximum of NADPH from 465 nm to 450 nm, however, the modified enzyme neither exhibited the enhancement of fluorescence emission nor the blue shift, indicating loss of NADPH binding site on modification. The essential carboxyl group may be involved in NADPH binding during catalysis by the enzyme.
Subject(s)
Isoxazoles/pharmacology , Malate Dehydrogenase/antagonists & inhibitors , Binding Sites , Enzyme Inhibitors/pharmacology , Isoxazoles/metabolism , Kinetics , Magnesium/pharmacology , Malate Dehydrogenase/isolation & purification , Malate Dehydrogenase/metabolism , Malates/metabolism , Malates/pharmacology , NADP/metabolism , NADP/pharmacology , Zea mays/enzymologyABSTRACT
Cytosines in single-stranded DNA deaminate to uracils at 140 times the rate for cytosines in double-stranded DNA. If resulting uracils are not replaced with cytosine, C to T mutations occur. These facts suggest that cellular processes such as transcription that create single-stranded DNA should promote C to T mutations. We tested this hypothesis with the Escherichia coli tac promoter and found that induction of transcription causes approximately 4-fold increase in the frequency of C to U or 5-methylcytosine to T deaminations in the nontranscribed strand. Excess mutations caused by C to U deaminations were reduced, but not eliminated, by uracil-DNA glycosylase. Similarly, mutations caused by 5-methylcytosine to T deaminations were only partially reduced by the very short-patch repair process in E.coli. These effects are unlikely to be caused by differential repair of the two strands, and our results suggest that all actively transcribed genes in E. coli should acquire more C to T mutations in the nontranscribed strand.
Subject(s)
Escherichia coli/genetics , Escherichia coli/metabolism , Point Mutation , Promoter Regions, Genetic , Transcription, Genetic , Base Sequence , Cytosine , DNA Methylation , DNA Primers , DNA, Single-Stranded/genetics , DNA, Single-Stranded/metabolism , Escherichia coli/drug effects , Isopropyl Thiogalactoside/pharmacology , Kanamycin Resistance/genetics , Polymerase Chain Reaction , ThymineABSTRACT
In Escherichia coli and related bacteria, the product of gene dcm methylates the second cytosine of 5'-CCWGG sequences (where W is A or T). Deamination of 5-methylcytosine (5meC) results in C to T mutations. The mutagenic potential of 5meC is reduced by a system called very short patch (VSP) repair, which replaces T with C. T:G and U:G mispairs in the methylatable sequence and in related sequences are recognized by the product of vsr, a gene adjacent to dcm. Vsr creates a nick just 5' of the mispaired pyrimidine to initiate the repair. Additional products known to be required for VSP repair are DNA polymerase I and DNA ligase. MutS and MutL have a stimulatory role but are not required. The ability of Vsr to recognize T:G mispairs in sequences related to CCWGG is probably responsible for over- and under-representation of certain tetranucleotides in the E. coli genome. Although VSP repair reduces spontaneous mutations at 5meCs in replicating bacteria, mutation hot-spots persist at these sites. Under conditions that more accurately mimic the natural environment of E. coli, VSP repair appears to be effective in preventing mutation at 5meC.
Subject(s)
Cytosine , DNA Repair , Endodeoxyribonucleases/metabolism , Amino Acid Sequence , Base Sequence , DNA, Bacterial , Endodeoxyribonucleases/chemistry , Endodeoxyribonucleases/genetics , Escherichia coli/genetics , Escherichia coli/metabolism , Genome, Bacterial , Humans , Methylation , Molecular Sequence Data , Mutation , OligonucleotidesABSTRACT
Multicopy clones of Escherichia coli cytosine methyltransferases Dcm and EcoRII methylase (M. EcoRII) cause an approximately 50-fold increase in C --> T mutations at their canonical site of methylation, 5'-CmeCAGG (meC is 5-methylcytosine). These plasmids also cause transition mutations at the second cytosine in the sequences CCGGG at approximately 10-fold lower frequency. Similarly, M. HpaII was found to cause a significant increase in C --> T mutations at a CCAG site, in addition to causing mutations at its canonical site of methylation, CCGG. Using a plasmid that substantially overproduces M. EcoRII, in vivo methylation at CCSGG (S is C or G) and other non-canonical sites could be detected using a gel electrophoretic assay. There is a direct correlation between the level of M. EcoRII activity in cells, the extent of methylation at non-canonical sites and frequency of mutations at these same sites. Overproduction of M. EcoRII in cells also causes degradation of DNA and induction of the SOS response. In vitro, M. EcoRII methylates an oligonucleotide duplex containing a CCGGG site at a slow rate, suggesting that overproduction of the enzyme is essential for significant amounts of such methylation to occur. Together these results show that cytosine methyltransferases occasionally methylate cellular DNA at non-canonical sites and suggest that in E. coli, methylation-specific restriction systems and sequence specificity of the DNA mismatch correction systems may have evolved to accommodate this fact. These results also suggest that mutational effects of cytosine methyltransferases may be much broader than previously imagined.
