Application of an End-to-End Biomarker Discovery Platform to Identify Target Engagement Markers in Cerebrospinal Fluid by High Resolution Differential Mass Spectrometry

Paweletz, Cloud P.; Wiener, Matthew C.; Bondarenko, Andrey; Yates, Nathan A.; Song, Qinghua; Liaw, Andy; Lee, Anita Y. H.; Hunt, Brandon T.; Henle, Ernst S.; Meng, Fanyu; Sleph, Holly Funk; Holahan, Marie A.; Sankaranarayanan, Sethu; Simon, Adam J.; Settlage, Robert E.; Sachs, Jeffrey R.; Shearman, Mark S.; Sachs, Alan B.; Cook, Jacquelynn J.; Hendrickson, Ronald C.

doi:10.1021/pr900925d

Cited by 45 publications

(33 citation statements)

References 28 publications

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“…For robust peak detection and labelfree alignment of individual peptides across all sample injections, the commercial package Rosetta Elucidator v3.3 (Rosetta Biosoftware) with the PeakTeller algorithm (76) was used, in a manner similar to a number of recent publications (77)(78)(79)(80)(81)(82)(83)(84). After alignment and annotation, chromatographic peak intensities belonging to the same precursor mass in the MS E aligned chromatograms were then used to calculate the relative peptide and protein abundance on a sample-by-sample basis.…”

Section: Methodsmentioning

confidence: 99%

The protein expression landscape of the Arabidopsis root

Petricka

Schauer

Megraw

et al. 2012

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

132

157

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Because proteins are the major functional components of cells, knowledge of their cellular localization is crucial to gaining an understanding of the biology of multicellular organisms. We have generated a protein expression map of the Arabidopsis root providing the identity and cell type-specific localization of nearly 2,000 proteins. Grouping proteins into functional categories revealed unique cellular functions and identified cell type-specific biomarkers. Cellular colocalization provided support for numerous protein-protein interactions. With a binary comparison, we found that RNA and protein expression profiles are weakly correlated. We then performed peak integration at cell type-specific resolution and found an improved correlation with transcriptome data using continuous values. We performed GeLC-MS/MS (in-gel tryptic digestion followed by liquid chromatography-tandem mass spectrometry) proteomic experiments on mutants with ectopic and no root hairs, providing complementary proteomic data. Finally, among our root hair-specific proteins we identified two unique regulators of root hair development.plant proteome | cell-type expression | FACS | RNA-protein correlation | root hair mutant M ulticellular organisms use specialized cell types to perform activities that are integral to their function. Cellular tasks are usually achieved by proteins, which act in signaling cascades, provide structural support, and catalyze enzymatic reactions vital to growth and metabolism. Knowledge of protein cellular localization and abundance using proteomic approaches is thus crucial to our understanding of biological systems (1, 2). Proteome data can be visually represented in a map, which highlights the spatial relationships of proteins at the level of cell type, tissue, or organ. Proteome maps are useful representations of the complex "building plan" of a biological system and also serve as valuable tools for the discovery of new cellular functions (2, 3). Proteomic studies of single cell populations isolated from a variety of multicellular organisms have recently been achieved, including the oocytes of worms and mice (4-6); pollen grains (consisting of two sperm and one vegetative cell) and stomatal guard cells of plants (7,8); and sperm cells of mice and flies (9, 10). These cell types were relatively accessible because they either reside on the surface and can be purified in large quantities using biochemical fractionation (e.g., guard cells) or are large and can easily be collected (e.g., Caenorhabditis elegans oocytes). However, similar proteomic studies of internal cell populations have been more difficult and are usually only partially represented in proteomes of whole organs owing to signal dilution (e.g., refs. 11-16).The Arabidopsis thaliana root is an excellent model for investigating cellular functions internal to an organ because it is transparent, radially symmetric, and cell types can be isolated by FACS to allow molecular profiling (17). The goal of this study was to investigate cell-type function by genera...

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Section: Methodsmentioning

confidence: 99%

The protein expression landscape of the Arabidopsis root

Petricka

Schauer

Megraw

et al. 2012

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

132

157

View full text Add to dashboard Cite

show abstract

“…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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“…This undertaking takes advantage of the "label-free" dMS approach, which is a commonly used comparative method in proteomics studies for finding differentially expressed proteins/peptides under different conditions (23)(24)(25). In the design of this study, by analogy, differential clotting conditions with regard to the extent of cross-linking were established for fibrin, and the cross-linked fibrin peptides were "differentially expressed" as a result.…”

mentioning

confidence: 99%

Identification of Respective Lysine Donor and Glutamine Acceptor Sites Involved in Factor XIIIa-catalyzed Fibrin α Chain Cross-linking

Wang

2011

Journal of Biological Chemistry

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Background: Factor XIIIa catalyzes ⑀-(␥-glutamyl)-lysyl bonds between glutamine and lysine residues on fibrin ␣ and ␥ chains. Results: Site-specific determinations of intermolecular glutamine-lysine pairs on fibrin ␣ chains were accomplished using modern mass spectrometry methods. Conclusion: Nine specific cross-links between four glutamine and five lysine residues on fibrin ␣ chains were identified. Significance: The findings advance the current understanding of molecular packing in fibrin.

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Application of an End-to-End Biomarker Discovery Platform to Identify Target Engagement Markers in Cerebrospinal Fluid by High Resolution Differential Mass Spectrometry

Cited by 45 publications

References 28 publications

The protein expression landscape of the Arabidopsis root

The protein expression landscape of the Arabidopsis root

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

Identification of Respective Lysine Donor and Glutamine Acceptor Sites Involved in Factor XIIIa-catalyzed Fibrin α Chain Cross-linking

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