Evaluation of a Surface Sampling Probe Electrospray Mass Spectrometry System for the Analysis of Surface Deposited and Affinity Captured Proteins

Van Berkel, Gary J; Ford, Michael J; Doktycz, Mitchel John; Kennel, Steve J

doi:10.1002/rcm.2428

Title: Evaluation of a Surface Sampling Probe Electrospray Mass Spectrometry System for the Analysis of Surface Deposited and Affinity Captured Proteins

Journal Article · Sun Jan 01 00:00:00 EST 2006 · Rapid Communications in Mass Spectrometry

DOI:https://doi.org/10.1002/rcm.2428· OSTI ID:1003314

Van Berkel, Gary J ^[1]; Ford, Michael J ^[1]; Doktycz, Mitchel John ^[1]; Kennel, Steve J ^[1]

ORNL

A combined self-aspirating electrospray emitter/surfacing-sampling probe coupled with an ion trap mass spectrometer was used to sample and mass analyze proteins from surfaces. The sampling probe mass spectrometer system was used to sample and detect lysozyme that had been deposited onto a glass slide using a piezoelectric spotter or murine gamma-interferon affinity captured on a glass slide using surface-immobilized anti-gamma-interferon antibody. The detection level for surface-deposited lysozyme (spot size {le}200 {micro}m) was approximately 1.0 fmol ({approx}100 fmol/mm{sup 2}) as determined from the ability to measure accurately the protein molecular mass from the mass spectrum acquired by sampling the deposit. These detection limits may be sufficient for certain applications in which protein fractions from a separation method are collected onto a surface. Radiolabeled proteins were used to quantify the surface density of immobilized antibody and the efficiency of capture of the gamma-interferon on glass and higher surface area ceramic supports. The capture density of gamma-interferon at surface saturation ranged from about 23 to 50 fmol/mm{sup 2} depending on the capture surface. Nonetheless, mass spectrometric detection of affinity capture protein was successful in some cases, but the results were not reproducible. Thus, improvement of the sampling system, ionization efficiency and/or capture density will be necessary for practical sampling of affinity-captured proteins. The means to accomplish improved sampling system detection limits and to increase the absolute amounts of protein captured per unit area are discussed.

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Research Organization:: Oak Ridge National Lab. (ORNL), Oak Ridge, TN (United States)

Sponsoring Organization:: Work for Others (WFO)

DOE Contract Number:: DE-AC05-00OR22725

OSTI ID:: 1003314

Journal Information:: Rapid Communications in Mass Spectrometry, Vol. 20, Issue 7; ISSN 0951--4198

Country of Publication:: United States

Language:: English

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59 BASIC BIOLOGICAL SCIENCES
99 GENERAL AND MISCELLANEOUS//MATHEMATICS, COMPUTING, AND INFORMATION SCIENCE
AFFINITY
CERAMICS
DETECTION
EFFICIENCY
EVALUATION
GLASS
IONIZATION
LYSOZYME
MASS SPECTROMETERS
MASS SPECTROSCOPY
PROBES
PROTEINS
SAMPLING
SATURATION
SENSITIVITY
SURFACE AREA

Title: Evaluation of a Surface Sampling Probe Electrospray Mass Spectrometry System for the Analysis of Surface Deposited and Affinity Captured Proteins

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