2009
DOI: 10.1093/nar/gkp827
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Profiling the selectivity of DNA ligases in an array format with mass spectrometry

Abstract: 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 … Show more

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Cited by 36 publications
(28 citation statements)
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“…As the DP length is decreased, the specificity increases because the rate of ligation on mismatched RNA templates decreases at a faster rate than the rate of ligation on the target RNA template. Previously, 25 the use of [g-thio]-triphosphate as a substrate for T4 DNA ligase in DNA array profiling found a delayed rate of ligation reactions. We show that CPs with pre-adenylated 1-Thio-AMP groups improve the specificity of ligation reactions on RNA when mismatches are present.…”
Section: Discussionmentioning
confidence: 99%
“…As the DP length is decreased, the specificity increases because the rate of ligation on mismatched RNA templates decreases at a faster rate than the rate of ligation on the target RNA template. Previously, 25 the use of [g-thio]-triphosphate as a substrate for T4 DNA ligase in DNA array profiling found a delayed rate of ligation reactions. We show that CPs with pre-adenylated 1-Thio-AMP groups improve the specificity of ligation reactions on RNA when mismatches are present.…”
Section: Discussionmentioning
confidence: 99%
“…Surfaces are stabilized on the surface layer, and a minimal amount of matrix is required for measurement. 12) and inhibitors of the anthrax lethal factor. 13) The process may maximize the utility of LDI-MS, and its usefulness and future potential have been confirmed.…”
Section: Self-assembling Monolayer For Maldi-msmentioning
confidence: 99%
“…The SAMs can be customized to use a variety of immobilization chemistries, including maleimide and azide (or alkyne) for covalent capture, and biotin for streptavidin-biotin capture. [8][9][10] Monolayers specifically bind and capture the intended analytes, allowing for isolation of the analyte from 384 samples in parallel-by using the standard microtiter plates-and we are now transitioning to 1536-well plates. Furthermore, the intrinsic compatibility of SAMDI with essentially any enzyme activity (provided the activity results in a change in the molecular weight of the substrate) permits the screening of posttranslational modifications using peptide substrates.…”
Section: Introductionmentioning
confidence: 99%