On-line bioaffinity-electrospray mass spectrometry for simultaneous detection, identification, and quantification of protein-ligand interactions

Drăguşanu, M; Petre, Brînduşa Alina; Slamnoiu, Stefan; Vlad, Camelia; Tu, Tingting; Przybylski, Michael

doi:10.1016/j.jasms.2010.06.011

Cited by 32 publications

(51 citation statements)

References 22 publications

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“…The chip surface was prepared and cleaned before binding and affinity determinations by 45 min washing with a 1:1 mixture (v/v) of concentrated sulphuric acid and hydrogen peroxide (30%). Immobilization of proteins was performed by covalent binding of a monolayer (SAM) of 16-mercaptohexadecanoic acid as previously described [13].…”

Section: Saw Biosensor and Sample Preparation For Affinity Determinatmentioning

confidence: 99%

“…We have developed a new interface for on-line bioaffinity-mass spectrometry coupling of a surface acoustic wave (SAW) biosensor to electrospray ionization mass spectrometry (SAW-MS) [13], which provides both affinity detection and quantification and the mass spectrometric chemical structure analysis of ligands. Key element of the on-line biosensor-MS is a microfluidic interface enabling affinity-enrichment, desalting of samples from the biosensor, and transfer of ligands to the ESI-MS source.…”

Section: Introductionmentioning

confidence: 99%

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Identification and Affinity-Quantification of ß-Amyloid and α-Synuclein Polypeptides Using On-Line SAW-Biosensor-Mass Spectrometry

Slamnoiu

Vlad

Stumbaum

et al. 2014

J. Am. Soc. Mass Spectrom.

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Abstract. Bioaffinity analysis using a variety of biosensors has become an established tool for detection and quantification of biomolecular interactions.Biosensors, however, are generally limited by the lack of chemical structure information of affinity-bound ligands. On-line bioaffinity-mass spectrometry using a surface-acoustic wave biosensor (SAW-MS) is a new combination providing the simultaneous affinity detection, quantification, and mass spectrometric structural ({"' characterization of ligands. We describe here an on-line SAW-MS combination for direct identification and affinity determination, using a new interface for MS of the affinity-isolated ligand eluate. Key element of the SAW-MS combination is a microfluidic interface that integrates affinity-isolation on a gold chip, in-situ sample concentration, and desalting with a microcolumn forMS of the ligand eluate from the biosensor. Suitable MSacquisition software has been developed that provides coupling of the SAW-MS interface to a Bruker Daltonics ion trap-MS, FTICR-MS, and Waters Synapt-QTOF-MS systems. Applications are presented for mass spectrometric identifications and affinity (K 0 ) determinations of the neurodegenerative polypeptides, r..-amyloid (AI1), and pathophysiological and physiological synucleins (a-and r..-synucleins), two key polypeptide systems for Alzheimer's disease and Parkinson's disease, respectively. Moreover, first in vivo applications of aSyn polypeptides from brain homogenate show the feasibility of on-line affinity-MS to the direct analysis of biological material. These results demonstrate on-line SAW-bioaffinity-MS as a powerful tool for structural and quantitative analysis of biopolymer interactions.

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Section: Saw Biosensor and Sample Preparation For Affinity Determinatmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Identification and Affinity-Quantification of ß-Amyloid and α-Synuclein Polypeptides Using On-Line SAW-Biosensor-Mass Spectrometry

Slamnoiu

Vlad

Stumbaum

et al. 2014

J. Am. Soc. Mass Spectrom.

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“…N-α-Fmoc protected amino acids attached to NovaSyn TGA resin was from NovaBiochem (Laufelfingen, Switzerland). A K5-Ssens Biosensor (SAW-Instruments, Bonn, Germany) was used for online bioaffinity-MS with an interface developed in our laboratory, as previously described [50]. The antibody was immobilized on a gold chip, following formation of a self-assembled monolayer (SAM) surface of 16-mercaptohexadecanoic acid for 12 h at 25°C.…”

Section: Site Selectivity Of Tyrosine Nitration In Proteinsmentioning

confidence: 99%

“…Following ligand association, elution was carried out with glycine buffer, and removal of salts was performed by washing with 0.3 % HCOOH. Elution and transfer into the ESI source of a Bruker Esquire 3000+ mass spectrometer was performed as previously described [50]. Determination of dissociation constants was performed with 150 μL (300 nM) immobilized antibody at a 20 μL min -1 flow rate in PBS buffer, pH 7.5, followed by regeneration with 150 μL glycine buffer, pH 2.…”

Section: Site Selectivity Of Tyrosine Nitration In Proteinsmentioning

confidence: 99%

“…A direct online combination of bioaffinity and mass spectrometry [50], a new method recently developed in our laboratory was employed for the simultaneous characterization and quantification of the interaction of tyrosine-nitrated peptides with the anti-3NT-antibody. The online affinity-MS approach utilized a surface-acoustic wave (SAW) biosensor [51], with the anti-3NT antibody immobilized on the biosensor chip surface via a self-assembled monolayer.…”

Section: Site Selectivity Of Tyrosine Nitration In Proteinsmentioning

confidence: 99%

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When is Mass Spectrometry Combined with Affinity Approaches Essential? A Case Study of Tyrosine Nitration in Proteins

Petre

Ulrich

Stumbaum

et al. 2012

J. Am. Soc. Mass Spectrom.

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Tyrosine nitration in proteins occurs under physiologic conditions and is increased at disease conditions associated with oxidative stress, such as inflammation and Alzheimer's disease. Identification and quantification of tyrosine-nitrations are crucial for understanding nitration mechanism(s) and their functional consequences. Mass spectrometry (MS) is best suited to identify nitration sites, but is hampered by low stabilities and modification levels and possible structural changes induced by nitration. In this insight, we discuss methods for identifying and quantifying nitration sites by proteolytic affinity extraction using nitrotyrosine (NT)-specific antibodies, in combination with electrospray-MS. The efficiency of this approach is illustrated by identification of specific nitration sites in two proteins in eosinophil granules from several biological samples, eosinophil-cationic protein (ECP) and eosinophil-derived neurotoxin (EDN). Affinity extraction combined with Edman sequencing enabled the quantification of nitration levels, which were found to be 8 % and 15 % for ECP and EDN, respectively. Structure modeling utilizing available crystal structures and affinity studies using synthetic NT-peptides suggest a tyrosine nitration sequence motif comprising positively charged residues in the vicinity of the NT-residue, located at specific surface-accessible sites of the protein structure. Affinities of Tyr-nitrated peptides from ECP and EDN to NT-antibodies, determined by online bioaffinity-MS, provided nanomolar K D values. In contrast, false-positive identifications of nitrations were obtained in proteins from cystic fibrosis patients upon using NT-specific antibodies, and were shown to be hydroxy-tyrosine modifications. These results demonstrate affinity-mass spectrometry approaches to be essential for unequivocal identification of biological tyrosine nitrations.

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Mass Spectrometry

Przybylski¹

2014

Handbook of Spectroscopy

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On-line bioaffinity-electrospray mass spectrometry for simultaneous detection, identification, and quantification of protein-ligand interactions

Cited by 32 publications

References 22 publications

Identification and Affinity-Quantification of ß-Amyloid and α-Synuclein Polypeptides Using On-Line SAW-Biosensor-Mass Spectrometry

Identification and Affinity-Quantification of ß-Amyloid and α-Synuclein Polypeptides Using On-Line SAW-Biosensor-Mass Spectrometry

When is Mass Spectrometry Combined with Affinity Approaches Essential? A Case Study of Tyrosine Nitration in Proteins

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