<i>Staphylococcus aureus</i> DNA ligase: characterization of its kinetics of catalysis and development of a high-throughput screening compatible chemiluminescent hybridization protection assay

Gul, Sheraz; Brown, Richard C. D.; May, Earl W.; Mazzulla, Marie; Smyth, Martin G.; Berry, Colin; Morby, Andrew P.; Powell, David J.

doi:10.1042/bj20040054

Cited by 8 publications

(8 citation statements)

References 41 publications

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“…16 the use of a streptavidincoated plate to capture biotinylated, ligated DNA 8,15 requires expensive assay plates and includes a washing step. the chemiluminescence assay of gul et al 14 requires a heating step, and the light output is so brief that the flash reagent must be added to one well at a time just before it is read in a plate reader equipped with an injector, a slow process not amenable to screening large libraries. 6.…”

Section: Methodsmentioning

confidence: 99%

A High-Throughput Fluorescence Resonance Energy Transfer-Based Assay for DNA Ligase

et al. 2011

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DNA ligase is the enzyme that catalyzes the formation of the backbone phosphodiester bond between the 5′-PO4 and 3′-OH of adjacent DNA nucleotides at single-stranded nicks. These nicks occur between Okazaki fragments during replication of the lagging strand of the DNA as well as during DNA repair and recombination. As essential enzymes for DNA replication, the NAD+-dependent DNA ligases of pathogenic bacteria are potential targets for the development of antibacterial drugs. For the purposes of drug discovery, a high-throughput assay for DNA ligase activity is invaluable. This article describes a straightforward, fluorescence resonance energy transfer–based DNA ligase assay that is well suited for high-throughput screening for DNA ligase inhibitors as well as for use in enzyme kinetics studies. Its use is demonstrated for measurement of the steady-state kinetic constants of Haemophilus influenzae NAD+-dependent DNA ligase and for measurement of the potency of an inhibitor of this enzyme.

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Section: Methodsmentioning

confidence: 99%

A High-Throughput Fluorescence Resonance Energy Transfer-Based Assay for DNA Ligase

et al. 2011

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“…Efforts to increase throughput have adopted homogeneous phase assays that use a secondary reaction to detect the product of the ligase reaction (17), but the use of labels and multiple steps increase the incidence of false positive and negative results.…”

Section: Introductionmentioning

confidence: 99%

“…The methods now used to assay ligase activity—which rely on gel electrophoresis of labeled oligonucleotides—have a limited throughput and are tedious when applied for profiling the activity of the ligase for a family of substrates ( 16 ). Efforts to increase throughput have adopted homogeneous phase assays that use a secondary reaction to detect the product of the ligase reaction ( 17 ), but the use of labels and multiple steps increase the incidence of false positive and negative results.…”

Section: Introductionmentioning

confidence: 99%

Profiling the selectivity of DNA ligases in an array format with mass spectrometry

Kim¹,

Mrksich²

2009

Nucleic Acids Research

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This article describes a method for the global profiling of the substrate specificities of DNA ligases and illustrates examples using the Taq and T4 DNA ligases. The method combines oligonucleotide arrays, which offer the benefits of high throughput and multiplexed assays, with mass spectrometry to permit label-free assays of ligase activity. Arrays were prepared by immobilizing ternary biotin-tagged DNA substrates to a self-assembled monolayer presenting a layer of streptavidin protein. The array represented complexes having all possible matched and mismatched base pairs at the 3′ side of the nick site and also included a number of deletions and insertions at this site. The arrays were treated with ligases and adenosine triphosphate or analogs of the nucleotide triphosphate and then analyzed by matrix-assisted laser desorption-ionization mass spectrometry to determine the yields for both adenylation of the 5′-probe strand and joining of the two probe strands. The resulting activity profiles reveal the basis for specificity of the ligases and also point to strategies that use ATP analogs to improve specificity. This work introduces a method that can be applied to profile a broad range of enzymes that operate on nucleic acid substrates.

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“…LigA is well conserved among eubacterial species, is architecturally and biochemically distinct from the ATP-dependent DNA ligases of eukaryotic cells, and has been found to be essential for bacterial viability wherever examined (13,14,15,17,31). Moreover, the DNA ligation reaction has been dissected mechanistically, mutationally, and structurally (8,20,25,26,33,34,35), and screening assays have been reported for the complete reaction cycle and for individual component steps (2,11,18).DNA ligation activities are essential for multiple DNA processes in replication and repair, including the joining of Okazaki fragments into a continuous strand during chromosomal DNA replication. Enzymatically, DNA ligation proceeds via three successive adenylyl transfer steps (Fig.…”

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confidence: 99%

Mechanistic Assessment of DNA Ligase as an Antibacterial Target in Staphylococcus aureus

Podos

Thanassi

Pucci

2012

Antimicrob Agents Chemother

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We report the use of a known pyridochromanone inhibitor with antibacterial activity to assess the validity of NAD ؉ -dependent DNA ligase (LigA) as an antibacterial target in Staphylococcus aureus. Potent inhibition of purified LigA was demonstrated in a DNA ligation assay (inhibition constant [K i ] ‫؍‬ 4.0 nM) and in a DNA-independent enzyme adenylation assay using full-length LigA (50% inhibitory concentration [IC 50 ] ‫؍‬ 28 nM) or its isolated adenylation domain (IC 50 ‫؍‬ 36 nM). Antistaphylococcal activity was confirmed against methicillin-susceptible and -resistant S. aureus (MSSA and MRSA) strains (MIC ‫؍‬ 1.0 g/ml). Analysis of spontaneous resistance potential revealed a high frequency of emergence (4 ؋ 10 ؊7 ) of high-level resistant mutants (MIC > 64) with associated ligA lesions. There were no observable effects on growth rate in these mutants. N ADϩ -dependent DNA ligase (LigA) has been identified by numerous authors as an attractive potential target for broadspectrum antibacterial chemotherapy (7,23). LigA is well conserved among eubacterial species, is architecturally and biochemically distinct from the ATP-dependent DNA ligases of eukaryotic cells, and has been found to be essential for bacterial viability wherever examined (13,14,15,17,31). Moreover, the DNA ligation reaction has been dissected mechanistically, mutationally, and structurally (8,20,25,26,33,34,35), and screening assays have been reported for the complete reaction cycle and for individual component steps (2,11,18).DNA ligation activities are essential for multiple DNA processes in replication and repair, including the joining of Okazaki fragments into a continuous strand during chromosomal DNA replication. Enzymatically, DNA ligation proceeds via three successive adenylyl transfer steps (Fig. 1) (32): first, DNA-independent covalent adenylation of the catalytic lysine by the NAD ϩ substrate; second, adenylyl transfer to the free 5= phosphate at the nicked DNA ligation site; and third, the covalent sealing of the DNA nick with concomitant AMP release. Biochemical functions of distinct domains in the modular enzyme structure have been assigned to particular reaction steps. The DNA-independent adenylyl transfer activity resides within the amino-terminal adenylation domain, which comprises an amino-terminal Ia region that is specific to NAD ϩ -dependent DNA ligases and a nucleotidyl transferase (NTase) region that is universal among DNA and RNA ligases. The subsequent coupling of adenylation to DNA ligation depends upon downstream DNA-binding domains, which include an oligonucleotide-binding fold (OB fold) and a helix-hairpin-helix (HhH) domain. Structural studies of the adenylation domain have revealed conformational transitions that accompany the adenylation cycle (8), and structural study of the full-length enzyme bound to DNA-adenylate has identified specific contacts between the DNA-binding domains and the DNA duplex substrate near the nicked ligation site (20).Numerous LigA inhibitors have been reported to date, including ary...

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Staphylococcus aureus DNA ligase: characterization of its kinetics of catalysis and development of a high-throughput screening compatible chemiluminescent hybridization protection assay

Cited by 8 publications

References 41 publications

A High-Throughput Fluorescence Resonance Energy Transfer-Based Assay for DNA Ligase

A High-Throughput Fluorescence Resonance Energy Transfer-Based Assay for DNA Ligase

Profiling the selectivity of DNA ligases in an array format with mass spectrometry

Mechanistic Assessment of DNA Ligase as an Antibacterial Target in Staphylococcus aureus

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