Journal of Proteome Data and Methods Volume 6

Dataset for proteome analysis by InSpIon system capable of stable nanoESI spray

We developed InSpIon system capable of stable nanoESI spray. Here, K562 cell digests were measured by DDA-MS and DIA-MS with a typical open nanoESI spray system and a spray system inserted spray tip head into an ion transfer tube, and InSpIon system.

Dataset for proteome analysis of K562 cell tryptic peptides dissolved by solutions with 12 surfactants

We evaluated the impact of surfactants on the recovery of dried peptides. Dried K562 cell digests were dissolved by solutions containing different concentrations of 12 surfactants and measured by DDA-MS and DIA-MS.

Data for proteomic analysis of sarcoma spheroids cultured with perfusion and without perfusion

This data was utilized to assess the utility of perfusion culture in cultivating spheroids of sarcoma cells. The differences between spheroids cultured with perfusion and without perfusion were analysed through mass spectrometry. The spheroids were fabricated from NCC-UPS4-C1 cell line derived from a patient with undifferentiated pleomorphic sarcoma. We found the different protein expression levels between spheroids cultured with perfusion and without perfusion.

Data for building LC-MS peak assignment algorithm based on machine learning.

For building a peak assignment algorithm using machine learning, the peptide fragment of extracted proteins from mouse liver was identified. One raw data includes the peptides with heavy- or light-labeled dimethylated lysine resides.

Dataset for co-immunoprecipitation with mass spectrometry using lauryl maltose neopentyl glycol-assisted sample preparation method

The lauryl maltose neopentyl glycol (LMNG)-assisted sample preparation (LASP) method was adapted for the process of on-beads digestion in co-immunoprecipitation with mass spectrometry (coIP-MS). In addition, to improve peptide recovery, the dried peptides were dissolved in 0.01% decyl maltose neopentyl glycol (DMNG) after desalting at the SDB Stage tip. The adapted LASP method and the lysis of dried peptides with DMNG increased the number of proteins identified in coIP-MS.

Protocol for TMT-labeling of peptides in quantitative proteomics

Isobaric tags, such as Tandem Mass Tag™ (TMT; Thermo Fisher Scientific), TMTpro™ (Thermo Fisher Scientific), or iTRAQ^® (Sciex), allow reproducible and high-throughput peptide/protein quantification in mass spectrometry-based proteomics. Herein, we introduce a practical protocol for TMT-labeling of peptide samples, with troubleshooting for possible problems and examples of important parameters in measurement by mass spectrometry.

Dataset for evaluation of the lauryl maltose neopentyl glycol assisted sample preparation method

We have developed a lauryl maltose neopentyl glycol (LMNG)-assisted sample preparation (LASP) method for reducing protein and peptide loss. LMNG was removed simply via reversed phase solid-phase extraction. LASP method was applied to the low-input SP3 method and EVOSEP ONE combined with LC-MS/MS. Furthermore, we have established sample preparation method for single cell proteomics based on the LASP method (scpLASP).

Data for the solvent-accessible surfaces of protein observed by LC-MS

For obtaining the structural data of human serum albumin (HSA) in solution using LC-MS analysis, the peptide fragments of HSA were identii ed. The raw data includes the peptides with dimethylated Lysine residues.

Dataset for proteome analysis of soleus and extensor digitorum longus muscles in mice exposed to hypergravity (3-g)

We investigated the effect of hypergravity exposure on the proteome profiles of the slow-twitch soleus and fast-twitch extensor digitorum longus muscles of mice. Mice were raised under 3-g (hypergravity) or 1-g (control) conditions, and proteins extracted from the soleus and extensor digitorum longus muscles were subjected to quantitative proteomic analysis using data-dependent acquisition mass spectrometry (DDA-MS). The proteome profiles of the soleus and extensor digitorum longus muscles suggested that biological pathways in different muscle types responded differently to hypergravity exposure.

Dataset for proteome analysis of soleus and extensor digitorum longus muscles in mice exposed to microgravity with or without fructo-oligosaccharide ingestion

The effect of microgravity (μ-g) exposure and fructo-oligosaccharide (FOS) ingestion during spaceflight was examined by determining the proteome profiles of the soleus and extensor digitorum longus muscles of mice that were launched to the International Space Station (ISS) and placed in a μ-g or centrifugal artificial 1-g (A1-g) environment for 30 days with or without FOS feeding. Quantitative analysis of proteins extracted from the soleus and extensor digitorum longus muscles suggested that in response to μ-g conditions, the soleus muscle fibers changed from a slow-twitch to a fast-twitch phenotype, and FOS ingestion mildly suppressed metabolic changes and oxidative stress.

Dataset for proteomic analyses of mouse soleus muscle in three model experiments under different gravity environments

We collectively evaluated the results of proteomic analysis of the soleus muscle from three mouse models exposed to different gravity environments (hindlimb unloading, spaceflight, and hypergravity), and identified gravity-responsive muscle proteins.

Dataset for gravity-responsive proteins in the bone tissue of spaceflight mice obtained by data-independent acquisition mass spectrometry (DIA-MS)

The microgravity (μ-g) environment during spaceflight can cause severe acute bone loss. To identify gravity-response proteins involved in bone metabolism, we analyzed the proteome of the femur and mandible collected from spaceflight mice raised in a μ-g or artificial 1-gravity (A1-g) environment on the International Space Station in orbit. The bone mass of the femur diaphysis decreased in response to gravity unloading, whereas that of the mandible remained unchanged due to mastication stimuli. Collective evaluation of the dataset of the proteome of the femur and mandible obtained by data-independent acquisition mass spectrometry (DIA-MS) identified the bone proteins that were altered by the μ-g environment and involved in bone loss.

Data for proteomic analysis of in situ digestion of alcohol-fixed cells for quantitative proteomics

We have developed a novel method for the preparation of proteome samples by direct digestion of methanol-fixed cells with trypsin, named in situ digestion of alcohol-fixed cells for quantitative proteomics (iSDAC). In this method, the cells are fixed in methanol and digested directly with trypsin without solubilizing cells with detergents. The elimination of the detergent removal step allows for easy and rapid sample preparation. This method’s digestion efficiency and reproducibility are comparable to those of commonly used proteome sample preparation methods.

Protocol for phosphoproteomic analysis

Protein phosphorylation is one of the most major post-translational modifications which is involved in regulation of various cellular functions. The number of phosphorylation sites identified has dramatically increased with the development of phosphoproteome analysis technology by mass spectrometry. The remarkable development of this technology has been supported mainly by the development and improvement of pretreatment methods such as phosphopeptide enrichment, the evolution of mass spectrometers, and the development of data analysis methods and software. In this paper we focus on pretreatment methods and present an example of clinical phosphoproteome analysis with limited sample amounts.

Data for peptidomic analysis of a single mouse hypothalamus

In this study, the differential solubilization method was modified to extract peptides from small amounts of frozen tissue. As a result, we successfully identified a total of 1,535 peptides including 35 bioactive peptides from 135 μg of mouse hypothalamus in three measurements.

Dataset for proteome analysis of serum purified by 35 lectins

Serum proteins enriched with 35 different lectins were analyzed by LC-MS/MS. The results showed that enrichment with Solanum tuberosum lectin (STL) and Lycopersicon esculentum lectin (LEL) resulted in the detection of many trace proteins in the serum. The combination of lectins was also examined, and the combination of STL and LEL was found to be the best for observing serum trace proteins. We aplied the STL/LEL method to sera from systemic lupus erythematosus (SLE) model mice and control mice, and compared them.

Astronaut serum proteome analysis dataset obtained by data-independent acquisition mass spectrometry (DIA-MS)

To elucidate the mechanisms involved in the adaptation to microgravity environments, we performed quantitative proteomic analysis of serum collected from astronauts before, during, and after prolonged spaceflight missions on the International Space Station (ISS) in orbit using data-independent acquisition mass spectrometry (DIA-MS). Quantitative analysis at each sampling point provided information on the characteristic serum protein profiles for several time points.

Dataset for proteome analysis of the gastrocnemius muscle in mice exposed to microgravity

The effects of exposure to microgravity (μ-g) during prolonged spaceflight were examined by comparing the proteome profiles of the gastrocnemius muscle in mice that were launched to the International Space Station (ISS) and placed in a μ-g or centrifugal artificial 1-g (A1-g) environment for 30 days. Alterations in the proteome profile of the gastrocnemius from μ-g–exposed mice indicated the activation of fibrinolysis, blood coagulation, and negative regulation of endopeptidases and peptidases.

Dataset for gravity-responsive serum proteins in spaceflight mice using data-independent ac-quisition mass spectrometry (DIA-MS)

In this study, quantitative serum proteomic analysis of spaceflight and hindlimb unloading (HU) mice was performed using data-independent acquisition mass spectrometry (DIA-MS). Collective eval-uation of the proteomic data showed proteins with fluctuating serum protein levels induced by gravity unloading.

Dataset for serum proteome analysis of patients with osteoporosis and with osteopenia by data-independent acquisition mass spectrometry (DIA-MS)

We performed proteomic analysis of serum collected from two patient groups, one with osteoporosis but no fractures and the other with osteopenia and fragility fractures. Quantitative analysis showed serum proteins that changed in both patient groups compared with controls.

Dataset for serum proteome analysis of COVID-19 patients by data-independent acquisition mass spectrometry (DIA-MS)

The COVID-19 pandemic was an unprecedented threat to humanity that has provoked global health concerns. To identify the serum proteins that are closely associated with COVID-19 prognosis, we performed quantitative proteomic analysis of serum collected from COVID-19 patients using data-independent acquisition mass spectrometry (DIA-MS)¹. Quantitative analysis provided information on the characteristic serum protein differentially expressed between severely ill COVID-19 patients with adverse or favorable prognosis.

Data for LC-MS/MS analysis of peptides and proteins produced in the cell-free translation systems

Analysis of the peptides and proteins synthesized in a cell-free translation system containing either the natural tRNA extract, the hybrid-SL tRNA set, or the hybrid-SL tRNA set minus one chimeric tRNA using LC-MS/MS.

Dataset for proteomic analysis of secreted proteins from bovine periosteum and blood vessels with explant culture

A combination of mass spectrometry (MS) and immunohistochemistry was used to detect important proteins for bone regeneration. In a previous study, electrospray ionization quadrupole time-of-flight (ESI-Q-TOF) MS discovered candidate proteins from supernatants of bovine periosteum, then immunohistochemistry revealed protein expression in periosteum tissue. Using these methods, F-box and WD-40 domain-containing protein 2 (FBXW2) was found in elastic fibers in the periosteum and blood vessels. Osteocalcin was expressed around FBXW2 in the periosteum. However, the combination of ESI-Q-TOF MS and immunohistochemistry revealed expression of several proteins including FBXW2, uveal autoantigen with coiled-coil domains and ankyrin repeats (UACA), exosome complex component RRP45 (EXOSC9), thioredoxin-related transmembrane protein 2 (ΤΜX2), and F-box/leucine-rich repeat protein 14 (FBXL14). In the present study, proteins in supernatants of the periosteum were investigated using ESI-Q-Orbitrap MS and then compared with the results obtained from blood vessels. Tissue specific proteins were compared between the periosteum and blood vessels, especially components of elastic fibers. ESI-Q-Orbitrap MS detected over 890 similar proteins secreted from both the periosteum and blood vessel and other proteins secreted exclusively from only the periosteum or blood vessels. ESI-Q-TOF MS and ESI-Q-Orbitrap MS detected collagen types 1 and 3, but only ESI-Q-Orbitrap MS detected collagen type 4.

Data for Comprehensive characterization of the phosphoproteome of gastric cancer from endoscopic biopsy specimens

Cancer phosphoproteomics provides insights into actionable kinases for targeted therapies. Monitoring phosphoproteomics in cancer is crucial for optimizing treatments with kinase inhibitors. We have developed a highly sensitive method for analyzing phosphoproteomics in endoscopic biopsies. Our approach aims to enhance the accuracy of monitoring therapeutic kinase activities.

Generation of a human serum spectral library for data-independent acquisition mass spectrometry (DIA-MS)

We aimed to develop a spectral library for human serum proteome analysis using data-independent acquisition mass spectrometry (DIA-MS). Finally, we succeeded in constructing a customized spectral library containing information on 1,534 human serum proteins.