Kinetic Analysis of Yersinia pestis DNA Adenine Methyltransferase Activity Using a Hemimethylated Molecular Break Light Oligonucleotide

Wood, R.J.K.; Maynard-Smith, Michael D.; Robinson, Victoria; Oyston, Petra C. F.; Titball, Richard W.; Roach, Peter L.

doi:10.1371/journal.pone.0000801

Cited by 6 publications

(6 citation statements)

References 31 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Cleavage of the stem leads to the melting of the short cleaved sequence and separation of fluorophore and quencher resulting in an increase in fluorescence. This assay format has been applied to DNA adenine-N6 methyltransferase activity (Dam) ( 38–40 ), in all cases the oligonucleotide stem contains the 5′-GATC-3′ Dam recognition sequence. The most recent assay coupled a hemimethylated substrate with a restriction enzyme (DpnI), which will preferentially cleave the fully methylated substrate, so that one methylation event by Dam is reported by a proportional increase in fluorescence because of DpnI cleavage.…”

Section: Introductionmentioning

confidence: 99%

A real-time assay for CpG-specific cytosine-C5 methyltransferase activity

Wood¹,

McKelvie²,

Maynard-Smith³

et al. 2010

Nucleic Acids Research

Self Cite

View full text Add to dashboard Cite

A real-time assay for CpG-specific cytosine-C5 methyltransferase activity has been developed. The assay applies a break light oligonucleotide in which the methylation of an unmethylated 5′-CG-3′ site is enzymatically coupled to the development of a fluorescent signal. This sensitive assay can measure rates of DNA methylation down to 0.34 ± 0.06 fmol/s. The assay is reproducible, with a coefficient of variation over six independent measurements of 4.5%. Product concentration was accurately measured from fluorescence signals using a linear calibration curve, which achieved a goodness of fit (R2) above 0.98. The oligonucleotide substrate contains three C5-methylated cytosine residues and one unmethylated 5′-CG-3′ site. Methylation yields an oligonucleotide containing the optimal substrate for the restriction enzyme GlaI. Cleavage of the fully methylated oligonucleotide leads to separation of fluorophore from quencher, giving a proportional increase in fluorescence. This method has been used to assay activity of DNMT1, the principle maintenance methyltransferase in human cells, and for the kinetic characterization of the bacterial cytosine-C5 methyltransferase M.SssI. The assay has been shown to be suitable for the real-time monitoring of DNMT1 activity in a high-throughput format, with low background signal and the ability to obtain linear rates of methylation over long periods, making this a promising method of high-throughput screening for inhibitors.

show abstract

Section: Introductionmentioning

confidence: 99%

A real-time assay for CpG-specific cytosine-C5 methyltransferase activity

Wood¹,

McKelvie²,

Maynard-Smith³

et al. 2010

Nucleic Acids Research

Self Cite

View full text Add to dashboard Cite

show abstract

“…Such competition binding assays took up to 1 h to complete, and the ‐term stability of Dam during these experiments was therefore an important consideration. Kinetic analysis of Y. pestis Dam inactivation has shown the enzyme to be particularly unstable (Wood et al ., ) and the more stable E. coli enzyme was used for these measurements. Both compounds 3 and 13 were found to fully displace oligonucleotide 4 in the presence and absence of AdoHcy, resulting in a drop in fluorescence anisotropy values to that of free‐labelled 4 in solution.…”

Section: Resultsmentioning

confidence: 99%

“…Fluorescence measurements were recorded in a Tecan Safire II (Reading, UK) microplate reader using 10 readings per well (each measurement) a Z-position of 12 000 mM and an integration time of 20 ms. Fluorescence measurements were made using an excitation wavelength of 486 nM with a bandwidth of 5 nM, and an emission wavelength of 518 nM with a bandwidth of 10 nM and the gain was set at 170, unless otherwise stated. Calibration plots were prepared as described previously (Wood et al, 2007) and in Supplementary Section S2 to enable conversion of rate of change in fluorescence to change of rate of reaction ( Supplementary Table S1 and Figure S1). The activity of Y. pestis Dam was measured in triplicate (unless otherwise stated) in black, flat bottomed, 384 Well Small Volume TM HiBase polystyrene microplates (Greiner, Stonehouse, UK), with a total assay volume of 20 mL, maintained at 30°C.…”

Section: Dam Activity Assaymentioning

confidence: 99%

“…Both these mutants were attenuated in mouse infection models. In order to facilitate the development of Dam-specific inhibitors, we developed a continuous fluorescence-based assay for monitoring Dam activity that is suitable for the high-throughput screening (HTS) of potential Dam inhibitors (Wood et al, 2007). In this current study, we describe the screening of an inhibitor library and identification of compounds with specific activity against Dam in this assay, providing a lead for the development of antimicrobials against this target.…”

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Inhibition of Yersinia pestisDNA adenine methyltransferase in vitro by a stibonic acid compound: identification of a potential novel class of antimicrobial agents

McKelvie

Richards

Harmer

et al. 2012

British J Pharmacology

View full text Add to dashboard Cite

BACKGROUND AND PURPOSEMultiple antibiotic resistant strains of plague are emerging, driving a need for the development of novel antibiotics effective against Yersinia pestis. DNA adenine methylation regulates numerous fundamental processes in bacteria and alteration of DNA adenine methlytransferase (Dam) expression is attenuating for several pathogens, including Y. pestis. The lack of a functionally similar enzyme in humans makes Dam a suitable target for development of novel therapeutics for plague. EXPERIMENTAL APPROACHCompounds were evaluated for their ability to inhibit Dam activity in a high-throughput screening assay. DNA was isolated from Yersinia grown in the presence of lead compounds and restricted to determine the effect of inhibitors on DNA methylation. Transcriptional analysis was undertaken to determine the effect of an active inhibitor on virulence-associated phenotypes. KEY RESULTSWe have identified a series of aryl stibonic acids which inhibit Dam in vitro. The most active, 4-stibonobenzenesulfonic acid, exhibited a competitive mode of inhibition with respect to DNA and a Ki of 6.46 nM. One compound was found to inhibit DNA methylation in cultured Y. pestis. The effects of this inhibition on the physiology of the cell were widespread, and included altered expression of known virulence traits, including iron acquisition and Type III secretion. CONCLUSIONS AND IMPLICATIONSWe have identified a novel class of potent Dam inhibitors. Treatment of bacterial cell cultures with these inhibitors resulted in a decrease in DNA methylation. Expression of virulence factors was affected, suggesting these inhibitors may attenuate bacterial infectivity and function as antibiotics. AbbreviationsAdoHcy, S-adenosylhomocysteine; A m , N6-methyladenine; D, dabcyl quencher; Dam, DNA adenine methyltransferase

show abstract

“…Most of these approaches are discontinuous and laborious. For real-time monitoring of DNA methyltransferase activity fluorescence-based assays based on either fluorescence quenching or fluorescence resonance energy transfer (FRET) have been proposed. − However, the proposed fluorescence sensors require double-labeled oligonucleotide substrates which will not only increase the cost of sensing system but also probably reduce the cleavage efficiency, and these bulky fluorescent groups might interfere with the kinetic behavior of the substrate molecules. Fluorescent assays require the proper design of DNA probes which may limit the versatility of such methods.…”

mentioning

confidence: 99%

Nanopore-Based, Label-Free, and Real-Time Monitoring Assay for DNA Methyltransferase Activity and Inhibition

et al. 2017

View full text Add to dashboard Cite

DNA methylation catalyzed by DNA methyltransferase plays an important role in many biological processes. However, conventional assays proposed for DNA methyltransferase activity are laborious and discontinuous. We have proposed a novel method for real-time monitoring of the activity and kinetics of Escherichia coli DNA adenine methyltransferase (Dam) using nanopore technique coupled with enzyme-linkage reactions. A double-stranded DNA probe AB having a recognition sequence 5'-GATC-3' for both Dam and MboI restriction endonuclease was prepared. Dam catalyzed the methylation of substrate probe AB, which blocked the cleavage reaction of MboI, while the absence of Dam resulted in cleavage of nonmethylated probe AB into four ssDNA fragments by MboI. When tested with nanopore, double-stranded methylated probe AB generated long-lived events, distinguished clearly from MboI-cleavage-mediated ssDNA fragments that generated only spikelike events. The proposed method has a detection limit of 0.03 U/mL for Dam in a short assay time of about 150 min. This sensing system is easy to perform, simple to design and circumvents the use of radioactive substances, resulting in efficient detection of the activity of Dam even in complex matrixes like human serum sample. Furthermore, it has the potential to screen Dam-targeted inhibitor drugs which may assist in the discovery of new anticancer medicines. This method is general and could be extended easily for monitoring activity of a wide variety of methyltransferases by coupling with their corresponding methylation-sensitive endonucleases.

show abstract

Kinetic Analysis of Yersinia pestis DNA Adenine Methyltransferase Activity Using a Hemimethylated Molecular Break Light Oligonucleotide

Cited by 6 publications

References 31 publications

A real-time assay for CpG-specific cytosine-C5 methyltransferase activity

A real-time assay for CpG-specific cytosine-C5 methyltransferase activity

Inhibition of Yersinia pestisDNA adenine methyltransferase in vitro by a stibonic acid compound: identification of a potential novel class of antimicrobial agents

Nanopore-Based, Label-Free, and Real-Time Monitoring Assay for DNA Methyltransferase Activity and Inhibition

Contact Info

Product

Resources

About