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Dichroïsme circulaire×MALDI-TOF×Résonance des Plasmons de Surface×
DomaineSpectroscopieSpectroscopieSpectroscopie
FamilleProcess / pipelineProcess / pipelineProcess / pipeline
Année d'origine196919881971
Auteur d'origineJean-Claude FasmanMichael KarasErich Kretschmann
TypeSpectroscopic methodIonization and mass analysis techniqueOptical technique
Source fondatriceGreenfield, N. J., & Fasman, G. D. (1969). Computed circular dichroism spectra for protein secondary structures. Biochemistry, 8(10), 4108-4116. DOI ↗Karas, M., & Hillenkamp, F. (1988). Laser desorption ionization of proteins with molecular masses exceeding 10,000 daltons. Analytical Chemistry, 60(20), 2299-2301. DOI ↗Kretschmann, E. (1971). Determination of optical constants of metals by excitation of surface plasmons. Zeitschrift für Physik, 241(4), 313-324. link ↗
AliasCD spectroscopy, circular dichroism, CD analysisMALDI mass spectrometry, MALDI-TOF-MS, laser desorption mass spectrometrySPR, surface plasmon, SPR biosensing
Apparentées333
RésuméCircular Dichroism (CD) spectroscopy measures the differential absorption of left- and right-circularly polarized light by optically active molecules, particularly proteins and nucleic acids. Introduced by Greenfield and Fasman in 1969, CD is a rapid, non-destructive technique for characterizing secondary structure (alpha-helix, beta-sheet), monitoring protein folding transitions, and assessing conformational changes in response to pH, temperature, or ligand binding.Matrix-Assisted Laser Desorption/Ionization (MALDI) combined with Time-of-Flight (TOF) mass analysis, or MALDI-TOF, is a soft ionization mass spectrometry technique that gently ionizes intact biomolecules and volatile organic compounds, then measures their mass-to-charge ratio by measuring flight time through a field-free drift region. Introduced independently by Karas, Hillenkamp, and Tanaka in 1988, MALDI-TOF revolutionized proteomics, microbiology, and organic analysis by enabling mass determination of proteins and polymers exceeding 100 kDa.Surface Plasmon Resonance (SPR) is a real-time, label-free technique for detecting and monitoring biomolecular interactions at a sensor surface by measuring changes in the refractive index caused by ligand binding. Developed by Kretschmann in 1971 and applied to biosensing by Liedberg, Nylander, and Lundström in 1983, SPR is now a gold standard for measuring binding kinetics (association and dissociation rates) and equilibrium binding constants in protein interactions, antibody-antigen recognition, and drug discovery.
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ScholarGateComparer des méthodes: Circular Dichroism · MALDI-TOF · Surface Plasmon Resonance. Consulté le 2026-06-19 sur https://scholargate.app/fr/compare