Quantitative analysis of complex peptide mixtures using FTMS and differential mass spectrometry

Meng, Fanyu; Wiener, Matthew C.; Sachs, Jeffrey R.; Burns, Chrissina; Verma, Priyanka; Paweletz, Cloud P.; Mazur, Matthew T.; Deyanova, Ekaterina G.; Yates, Nathan A.; Hendrickson, Ronald C.

doi:10.1016/j.jasms.2006.09.014

Cited by 70 publications

(65 citation statements)

References 22 publications

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“…LC-MS Data Processing-For robust peak detection and label-free alignment of individual peptides across all 72 sample injections, we utilized the Rosetta Elucidator® v3.3 software (Rosetta Biosoftware, Inc., Seattle, WA) with PeakTeller algorithm, in a similar manner to several recent publications (24,(31)(32)(33)(34)(35)(36)(37). Following alignment and annotation, chromatographic peak intensities belonging to the same precursor mass in the MS E aligned chromatograms were used to calculate the relative peptide and protein abundance on a sectionby-section basis.…”

Section: Methodsmentioning

confidence: 99%

Proteomic Profiling of a Layered Tissue Reveals Unique Glycolytic Specializations of Photoreceptor Cells

Reidel

Thompson

Farsiu

et al. 2011

Molecular & Cellular Proteomics

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The retina is a highly ordered tissue whose outermost layers are formed by subcellular compartments of photoreceptors generating light-evoked electrical responses. We studied protein distributions among individual photoreceptor compartments by separating the entire photoreceptor layer of a flat-mounted frozen retina into a series of thin tangential cryosections and analyzing protein compositions of each section by label-free quantitative mass spectrometry. Based on 5038 confidently identified peptides assigned to 896 protein database entries, we generated a quantitative proteomic database (a "map") correlating the distribution profiles of identified proteins with the profiles of marker proteins representing individual compartments of photoreceptors and adjacent cells. We evaluated the applicability of several common peptide-toprotein quantification algorithms in the context of our database and found that the highest reliability was obtained by summing the intensities of all peptides representing a given protein, using at least the 5-6 most intense peptides when applicable. We used this proteome map to investigate the distribution of glycolytic enzymes, critical in fulfilling the extremely high metabolic demands of photoreceptor cells, and obtained two major findings. First, unlike the majority of neurons rich in hexokinase I, but similar to other highly metabolically active cells, photoreceptors express hexokinase II. Hexokinase II has a very high catalytic activity when associated with mitochondria, and indeed we found it colocalized with mitochondria in photoreceptors. Second, photoreceptors contain very little triosephosphate isomerase, an enzyme converting dihydroxyacetone phosphate into glyceraldehyde-3-phosphate. This may serve as a functional adaptation because dihydroxyacetone phosphate is a major precursor in phospholipid biosynthesis, a process particularly active in photoreceptors because of the constant renewal of their lightsensitive membrane disc stacks. Overall, our approach for proteomic profiling of very small tissue amounts at a resolution of a few microns, combining cryosectioning and liquid chromatography-tandem MS, can be applied for quantitative investigation of proteomes where spatial resolution is paramount.

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Section: Methodsmentioning

confidence: 99%

Proteomic Profiling of a Layered Tissue Reveals Unique Glycolytic Specializations of Photoreceptor Cells

Reidel

Thompson

Farsiu

et al. 2011

Molecular & Cellular Proteomics

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“…Subjects were monitored at 5 different times, before and after the end of exercise. Plasma underwent glycopeptide enrichment, followed by LC MS/MS [98][99][100]. Potential protein markers with at least 2 distinct peptide components increasing during exercise as a function of work load and duration, were selected.…”

Section: Effects Of Eccentric Upper Extremity Exercise On Plasma Protmentioning

confidence: 99%

Diversity of human skeletal muscle in health and disease: Contribution of proteomics

Gelfi

Vasso

Cerretelli

2011

Journal of Proteomics

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“…Differential mass spectrometry has been successfully applied for the relative quantitation of complex peptide mixtures (17,18). To adapt dMS to the analysis of intact protein mixtures, two primary requirements to retain are a reproducible biochemical sample processing method and a robust LC-MS analysis.…”

Section: Resultsmentioning

confidence: 99%

“…To identify proteins of interest (as defined by m∕z ratio, intensity and retention time) we used dMS, a label-free LC-MS method for finding ions that exhibit a statistically significant difference in abundance in complex mixtures of peptides or proteins as previously described (8,17,18). Expression profiles generated from the highresolution LC-MS data above were analyzed using the Rosetta Elucidator™ system (version 3.2) (40).…”

Section: Methodsmentioning

confidence: 99%

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Quantitative analysis of intact apolipoproteins in human HDL by top-down differential mass spectrometry

Mazur¹,

Cardasis²,

Spellman³

et al. 2010

Proc. Natl. Acad. Sci. U.S.A.

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Top-down mass spectrometry holds tremendous potential for the characterization and quantification of intact proteins, including individual protein isoforms and specific posttranslationally modified forms. This technique does not require antibody reagents and thus offers a rapid path for assay development with increased specificity based on the amino acid sequence. Top-down MS is efficient whereby intact protein mass measurement, purification by mass separation, dissociation, and measurement of product ions with ppm mass accuracy occurs on the seconds to minutes time scale. Moreover, as the analysis is based on the accurate measurement of an intact protein, top-down mass spectrometry opens a research paradigm to perform quantitative analysis of "unknown" proteins that differ in accurate mass. As a proof of concept, we have applied differential mass spectrometry (dMS) to the top-down analysis of apolipoproteins isolated from human HDL 3 . The protein species at 9415.45 Da demonstrates an average fold change of 4.7 (p-value 0.017) and was identified as an O-glycosylated form of apolipoprotein C-III [NANA-ð2 → 3Þ-Gal-βð1 → 3Þ-GalNAc, þ656.2037 Da], a protein associated with coronary artery disease. This work demonstrates the utility of top-down dMS for quantitative analysis of intact protein mixtures and holds potential for facilitating a better understanding of HDL biology and complex biological systems at the protein level.quantitative proteomics | Fourier-transfrom mass spectrometry | electron transfer dissociation | top-down proteomics | posttranslational modifications

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Quantitative analysis of complex peptide mixtures using FTMS and differential mass spectrometry

Cited by 70 publications

References 22 publications

Proteomic Profiling of a Layered Tissue Reveals Unique Glycolytic Specializations of Photoreceptor Cells

Proteomic Profiling of a Layered Tissue Reveals Unique Glycolytic Specializations of Photoreceptor Cells

Diversity of human skeletal muscle in health and disease: Contribution of proteomics

Quantitative analysis of intact apolipoproteins in human HDL by top-down differential mass spectrometry

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