Large-Scale Quantitative Assessment of Different In-Solution Protein Digestion Protocols Reveals Superior Cleavage Efficiency of Tandem Lys-C/Trypsin Proteolysis over Trypsin Digestion

Glatter, Timo; Ludwig, Christina; Ahrné, Erik; Aebersold, Ruedi; Heck, Albert J. R.; Schmidt, Alexander

doi:10.1021/pr300273g

Cited by 289 publications

(279 citation statements)

References 29 publications

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“…The centrosome preparations were analyzed by shotgun proteomics as described previously (Glatter et al , 2012) with minor modifications. The hybrid Orbitrap‐Velos mass spectrometer was interfaced to a nanoelectrospray ion source coupled online to an Easy‐nLC 1000 system (all Thermo Scientific, Waltham, MA, USA).…”

Section: Methodsmentioning

confidence: 99%

“…The database search results were filtered using the ion score to set the false discovery rate (FDR) to 1% on the peptide and protein level, respectively, based on the number of reverse protein sequence hits in the datasets. After normalizing the quantitative data of the technical replicates using the SafeQuant software tool (Glatter et al , 2012), the summed precursor intensities obtained from Progenesis for each centrosome preparation were aligned with the absolute protein concentrations determined by SRM analysis according to the iBAQ method (Schwanhausser et al , 2011), respectively. The resulting models were applied to estimate absolute protein levels for all proteins quantified in two centrosome preparations, and data were combined by calculating mean protein levels.…”

Section: Methodsmentioning

confidence: 99%

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Quantitative analysis of human centrosome architecture by targeted proteomics and fluorescence imaging

et al. 2016

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Centrioles are essential for the formation of centrosomes and cilia. While numerical and/or structural centrosomes aberrations are implicated in cancer, mutations in centriolar and centrosomal proteins are genetically linked to ciliopathies, microcephaly, and dwarfism. The evolutionarily conserved mechanisms underlying centrosome biogenesis are centered on a set of key proteins, including Plk4, Sas‐6, and STIL, whose exact levels are critical to ensure accurate reproduction of centrioles during cell cycle progression. However, neither the intracellular levels of centrosomal proteins nor their stoichiometry within centrosomes is presently known. Here, we have used two complementary approaches, targeted proteomics and EGFP‐tagging of centrosomal proteins at endogenous loci, to measure protein abundance in cultured human cells and purified centrosomes. Our results provide a first assessment of the absolute and relative amounts of major components of the human centrosome. Specifically, they predict that human centriolar cartwheels comprise up to 16 stacked hubs and 1 molecule of STIL for every dimer of Sas‐6. This type of quantitative information will help guide future studies of the molecular basis of centrosome assembly and function.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Quantitative analysis of human centrosome architecture by targeted proteomics and fluorescence imaging

et al. 2016

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“…Some proteomic studies use a first endoproteolytic cleavage step with the enzyme Lys-C, which is still active at higher urea concentrations such as 4 M [39] followed by a second digestion step with trypsin.…”

Section: Hydrolysis Of Protein and Rnamentioning

confidence: 99%

Analysis of protein–RNA interactions in CRISPR proteins and effector complexes by UV-induced cross-linking and mass spectrometry

Sharma

Hrle

Kramer

et al. 2015

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a b s t r a c tRibonucleoprotein (RNP) complexes play important roles in the cell by mediating basic cellular processes, including gene expression and its regulation. Understanding the molecular details of these processes requires the identification and characterization of protein-RNA interactions. Over the years various approaches have been used to investigate these interactions, including computational analyses to look for RNA binding domains, gel-shift mobility assays on recombinant and mutant proteins as well as co-crystallization and NMR studies for structure elucidation. Here we report a more specialized and direct approach using UV-induced cross-linking coupled with mass spectrometry. This approach permits the identification of cross-linked peptides and RNA moieties and can also pin-point exact RNA contact sites within the protein. The power of this method is illustrated by the application to different singleand multi-subunit RNP complexes belonging to the prokaryotic adaptive immune system, CRISPR-Cas (CRISPR: clustered regularly interspaced short palindromic repeats; Cas: CRISPR associated). In particular, we identified the RNA-binding sites within three Cas7 protein homologs and mapped the cross-linking results to reveal structurally conserved Cas7 -RNA binding interfaces. These results demonstrate the strong potential of UV-induced cross-linking coupled with mass spectrometry analysis to identify RNA interaction sites on the RNA binding proteins.

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“…Cells were collected by centrifugation at 400g at 4°C, washed twice with 2 ml ice--cold PBS buffer, harvested by centrifugation at 500g and the pellet was snap frozen in liquid nitrogen and stored at --80°C until further processing. For S. pombe, cultures of wild type 972 h+ cells were grown in YE medium [24,30] at 25˚C to concentrations of 3.5x10 6 cells/ml and around 10^8 cells of each sample were collected by centrifugation at 2,000xg, washed twice with PBS buffer and harvested by centrifugation at 2,000xg. Cells were resuspended in 100µl lysis buffer (100 mM ammoniumbicarbonate, 2% sodium deoxycholate, 5mM TCEP), disrupted by strong indirect sonication (100% amplitude, 0.5 cycle, 2 × 10 s) in a Vial Tweeter (Hielscher) and reduced for 15min at 95°C.…”

Section: Cell Lysis and Proteolysismentioning

confidence: 99%

“…Then, the samples were diluted with 100mM ammoniumbicarbonate buffer to a final sodium deoxycholate concentration of 1% and further digested by incubation with sequencing--grade modified trypsin (1/50, w/w; Promega, Madison, Wisconsin) over night at 37°C. The sequential double Lys--C/trypsin digestion has been recently shown to be more efficient in generating fully cleaved peptides than tryptic digest alone [30] and is therefore recommended for all protein samples analyzed by LC--MS. Sodium deoxycholate is one of a few LC--MS compatible detergents, since it precipitates after acidification [25,33,38] using 2M HCl to a final concentration of 50mM and can then be easily removed by centrifugation at 10,000g for 15min before LC--MS analysis.…”

Section: Cell Lysis and Proteolysismentioning

confidence: 99%

Exploiting the multiplexing capabilities of tandem mass tags for high-throughput estimation of cellular protein abundances by mass spectrometry

Ahrné

Martínez-Segura

Syed

et al. 2015

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Large-Scale Quantitative Assessment of Different In-Solution Protein Digestion Protocols Reveals Superior Cleavage Efficiency of Tandem Lys-C/Trypsin Proteolysis over Trypsin Digestion

Cited by 289 publications

References 29 publications

Quantitative analysis of human centrosome architecture by targeted proteomics and fluorescence imaging

Quantitative analysis of human centrosome architecture by targeted proteomics and fluorescence imaging

Analysis of protein–RNA interactions in CRISPR proteins and effector complexes by UV-induced cross-linking and mass spectrometry

Exploiting the multiplexing capabilities of tandem mass tags for high-throughput estimation of cellular protein abundances by mass spectrometry

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