Intensity fading MALDI mass spectrometry explained

Intensity-fading MALDI is a term coined to rename an existing method originally reported in 1999 to indirectly study a Protein–protein interaction or other protein complex[1] and the same year applied to a biological mixture to study the antigenicity of the influenza virus.[2] It involves treating a protein and a potential binding partner with a site-specific endoproteinase with the binding sites identified by their reduced area (or intensity) in a MALDI mass spectrum compared to that of non-bound protein control. It was falsely reported as new and novel in a later application by a Spanish group. The true origins of the approach and a range of applications including those employing gel based separations, drug-protein interactions and the relative affinity of such interactions, are described in a review article.[3]

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Notes and References

  1. Kiselar. Janna G.. Downard. Kevin M.. Direct Identification of Protein Epitopes by Mass Spectrometry without Immobilization of Antibody and Isolation of Antibody-Peptide Complexes. Analytical Chemistry. 71. 1999. 9 . 1792–1801. 10.1021/ac9811120. 10330909 .
  2. Kiselar. Janna G.. Downard. Kevin M.. Antigenic surveillance of the influenza virus by mass spectrometry. Biochemistry. 38. 1999. 43 . 14185–14191. 10.1021/bi991609j. 10571992 .
  3. Downard. Kevin M.. Indirect study of non-covalent protein complexes by MALDI mass spectrometry: Origins, advantages, and applications of the "intensity-fading" approach. Mass Spectrometry Reviews. 35. 2016. 5 . 559–573. 10.1002/mas.21480. 26250984 . 2016MSRv...35..559D .

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