SRM can be used for targeted
quantitative proteomics by
mass spectrometry. Following
ionization in, for example, an
electrospray source, a
peptide precursor is first isolated to obtain a substantial
ion population of mostly the intended species. This population is then
fragmented to yield product ions whose signal abundances are indicative of the abundance of the peptide in the sample. This experiment can be performed on
triple quadrupole mass spectrometers, where mass-resolving Q1 isolates the precursor, q2 acts as a collision cell, and mass-resolving Q3 is cycled through the product ions which are detected upon exiting the last
quadrupole by an
electron multiplier. A precursor/product pair is often referred to as a
transition. Much work goes into ensuring that transitions are selected that have maximum specificity. Using
isotopic labeling with heavy-labeled (e.g.,
D,
13C, or
15N) peptides to a complex matrix as
concentration standards, SRM can be used to construct a
calibration curve that can provide the absolute quantification (i.e., copy number per
cell) of the native, light peptide, and by extension, its parent
protein. SRM has also been used as a method of triggering full product ion scans of peptides to either a) confirm the specificity of the SRM transition, or b) detect specific
post-translational modifications which are below the limit of detection of standard MS analyses. In 2017, SRM has been developed to be a highly sensitive and reproducible mass spectrometry-based protein targeted detection platform (entitled "SAFE-SRM"), and it has been demonstrated that the SRM-based new pipeline has major advantages in clinical proteomics applications over traditional SRM pipelines, and it has demonstrated a dramatically improved diagnostic performance over that from antibody-based protein biomarker diagnostic methods, such as
ELISA. ==See also==