Simultaneous Monitoring of Multiple Kinase Activities by SELDI-TOF Mass Spectrometry

Thulasiraman, Vanitha; Wang, Zheng; Katrekar, Anjali; Lomas, Lee; Yip, Tai‐Tung

doi:10.1385/1-59259-759-9:205

Cited by 4 publications

(4 citation statements)

References 3 publications

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“…Ciphergen Biosystems (Palo Alto, CA) developed a ProteinChip System that consists of a ProteinChip Reader (i.e., MALDI linear TOF mass spectrometer), ProteinChip Software, and related accessories that are used in conjunction with ProteinChip Arrays (Tang, Tornatore, & Weinberger, 2004). A number of reports described the use of these chips for phosphorylated peptide and protein purification (Cardone et al, 1998; Davies, 2000; Laine et al, 2000; Roig et al, 2000; Mortier et al, 2001; Stoica et al, 2001; Tassi et al, 2001; Espina et al, 2004; Liu et al, 2004; Thulasiraman et al, 2004; Bowley et al, 2005; Ge, Gibbs, & Masse, 2005; Head et al, 2005; Righetti et al, 2005; Wu, Jin, & Marsh, 2005; Le Bihan et al, 2006; Bodega et al, 2007; Akashi & Yamori, 2007; Akashi et al, 2007). One example was the use of an IMAC‐Gallium ProteinChip Array (IMAC chips were charged with a solution of 50 mM gallium nitrate) for the simultaneous analysis of a mixture of three synthetic monophosphorylated peptides, KRPpSQRHGSKY, TRDIYETDYpYRK, and KRELVEPLpTPSGEAPNQALLR, and their nonphosphorylated counterparts (Thulasiraman et al, 2004).…”

Section: New Platforms Aimed To Simplify the Enrichment Proceduresmentioning

confidence: 99%

Techniques for phosphopeptide enrichment prior to analysis by mass spectrometry

Dunn

Reid

Bruening

2009

Mass Spectrometry Reviews

197

192

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Mass spectrometry is the tool of choice to investigate protein phosphorylation, which plays a vital role in cell regulation and diseases such as cancer. However, low abundances of phosphopeptides and low degrees of phosphorylation typically necessitate isolation and concentration of phosphopeptides prior to MS analysis. This review discusses the enrichment of phosphopeptides with immobilized metal affinity chromatography, reversible covalent binding, and metal oxide affinity chromatography. Capture of phosphopeptides on TiO(2) seems especially promising in terms of selectivity and recovery, but the success of all methods depends on careful selection of binding, washing, and elution solutions. Enrichment techniques are complementary, such that a combination of methods greatly enhances the number of phosphopeptides isolated from complex samples. Development of a standard series of phosphopeptides in a highly complex mixture of digested proteins would greatly aid the comparison of different enrichment methods. Phosphopeptide binding to magnetic beads and on-plate isolation prior to MALDI-MS are emerging as convenient methods for purification of small (microL) samples. On-plate enrichment can yield >70% recoveries of phosphopeptides in mixtures of a few digested proteins and can avoid sample-handling steps, but this technique is likely limited to relatively simple samples such as immunoprecipitates. With recent advances in enrichment techniques in hand, MS analysis should provide important insights into phosphorylation pathways.

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Section: New Platforms Aimed To Simplify the Enrichment Proceduresmentioning

confidence: 99%

Techniques for phosphopeptide enrichment prior to analysis by mass spectrometry

Dunn

Reid

Bruening

2009

Mass Spectrometry Reviews

197

192

View full text Add to dashboard Cite

show abstract

“…The analysis of reaction mixtures by mass spectrometry methods makes the use of chromophores and radiolabelling unnecessary, since even the addition of a phosphate group to a large protein can be detected as a precise mass shift in the spectra. In vitro multiplexed assays can be performed on protein chips that are then directly analyzed by surface-enhanced laser desorption/ionization time-of-flight mass spectrometry (SELDI-TOF MS) to monitor enzyme activities [82]. Alternatively complex protein mixtures can be immobilized on micro-beads, where the enzymatic reactions can take place and be monitored by MALDI mass spectrometry [83].…”

Section: Experimental Measures Of Kinetic Parametersmentioning

confidence: 99%

Parameter estimate of signal transduction pathways

2006

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BackgroundThe "inverse" problem is related to the determination of unknown causes on the bases of the observation of their effects. This is the opposite of the corresponding "direct" problem, which relates to the prediction of the effects generated by a complete description of some agencies. The solution of an inverse problem entails the construction of a mathematical model and takes the moves from a number of experimental data. In this respect, inverse problems are often ill-conditioned as the amount of experimental conditions available are often insufficient to unambiguously solve the mathematical model. Several approaches to solving inverse problems are possible, both computational and experimental, some of which are mentioned in this article. In this work, we will describe in details the attempt to solve an inverse problem which arose in the study of an intracellular signaling pathway.ResultsUsing the Genetic Algorithm to find the sub-optimal solution to the optimization problem, we have estimated a set of unknown parameters describing a kinetic model of a signaling pathway in the neuronal cell. The model is composed of mass action ordinary differential equations, where the kinetic parameters describe protein-protein interactions, protein synthesis and degradation. The algorithm has been implemented on a parallel platform. Several potential solutions of the problem have been computed, each solution being a set of model parameters. A sub-set of parameters has been selected on the basis on their small coefficient of variation across the ensemble of solutions.ConclusionDespite the lack of sufficiently reliable and homogeneous experimental data, the genetic algorithm approach has allowed to estimate the approximate value of a number of model parameters in a kinetic model of a signaling pathway: these parameters have been assessed to be relevant for the reproduction of the available experimental data.

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“…In addition, it can also simplify the construction and execution of target selectivity panels. Although the use of multiplexing in hit discovery has been previously reported for kinases, nuclear receptors, and GPCRs, 11,[16][17][18] there are few examples of multiplexed assay systems used for large-scale HTS and none using Ca 2+ flux assays for GPCRs. Therefore, the benefits and liabilities of multiplexed Ca 2+ flux assays to large-scale screening are unknown.…”

Section: Introductionmentioning

confidence: 99%

Multiplexed G-Protein–Coupled Receptor Ca2+ Flux Assays for High-Throughput Screening

Miret¹,

Zhang²,

Min³

et al. 2005

SLAS Discovery

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An early drug discovery approach focusing on gene families can benefit from strategies that exploit common signaling mechanisms to more effectively identify and characterize novel chemical lead structures. Multiplexing, defined as the screening of multiple targets within the same experiment, is an example of this strategy. Here, the authors describe a technique that allows multiplexing of a common assay type used to study G-protein-coupled receptors: changes in intracellular Ca2+ levels as measured by Molecular Device's fluorometric imaging plate reader (FLIPR). The multiplexed FLIPR assays showed the expected pharmacological properties of single assays, with good reproducibility and Z* factors. The authors used them to screen large compound libraries in 2 multiplexed assay designs. The 1st used a single-cell line expressing 2 different receptors and the 2nd a mixture of 2 cell lines of the same type each expressing distinct receptors. Screening using these multiplexed assays produced significant savings in reagents, time, and human resources and allowed the authors to quickly identify specific and selective hits.

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Simultaneous Monitoring of Multiple Kinase Activities by SELDI-TOF Mass Spectrometry

Cited by 4 publications

References 3 publications

Techniques for phosphopeptide enrichment prior to analysis by mass spectrometry

Techniques for phosphopeptide enrichment prior to analysis by mass spectrometry

Parameter estimate of signal transduction pathways

Multiplexed G-Protein–Coupled Receptor Ca2+ Flux Assays for High-Throughput Screening

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