Yeast Interspecies Comparative Proteomics Reveals Divergence in Expression Profiles and Provides Insights into Proteome Resource Allocation and Evolutionary Roles of Gene Duplication

Kito, Keiji; Ito, Haruka; Nohara, Takehiro; Ohnishi, Mihoko; Ishibashi, Yuko; Takeda, Daisuke

doi:10.1074/mcp.m115.051854

Cited by 15 publications

(9 citation statements)

References 81 publications

(97 reference statements)

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“…Protein extraction from yeast cells, digestion of proteins into tryptic peptides and their fractionation via isoelectronic focusing were performed according to our previous report (Kito et al 2016). Fractionated peptides were analyzed with a LC-MS/MS system consisting of a LTQ-Orbitrap mass spectrometer (Thermo Fisher Scientific) and a DiNa nano LC (KYA Technologies, Tokyo, Japan).…”

Section: Mass Spectrometric Analysis For Extracted Proteins From Yeasmentioning

confidence: 99%

Proteomics analysis for asymmetric inheritance of preexisting proteins between mother and daughter cells in budding yeast

et al. 2017

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In budding yeast, a mother cell can produce a finite number of daughter cells over its life. The accumulation of a variety of types of damaged components has an impact on the aging process. Asymmetrical inheritance during cell division causes these aberrant intracellular constituents to be retained in mother cells and prevents them from segregating to daughter cells. However, the understanding of asymmetrical inheritance of individual proteins that are damaged or old age, and their relevance to the aging process, has been limited. The aim of this study is to propose a proteomics strategy for asymmetrical inheritance of preexisting proteins between mother and daughter cells. During synchronous culture for one generation, newly synthesized proteins were labeled with stable isotope amino acids to discriminate preexisting proteins originally expressed in mother cells, followed by separation of mother and daughter cells using a conventional method based on biotin labeling. Isotope incorporation ratios for individual proteins were quantified using mass spectrometry. We successfully identified 21 proteins whose preexisting versions were asymmetrically inherited in mother cells, including plasma membrane transporter involved in the aging process and organelle-anchoring proteins related to the stress response to misfolded proteins. Thus, our approach would be useful for making catalog of asymmetrically inherited proteins.

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Section: Mass Spectrometric Analysis For Extracted Proteins From Yeasmentioning

confidence: 99%

Proteomics analysis for asymmetric inheritance of preexisting proteins between mother and daughter cells in budding yeast

et al. 2017

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“…The absolute abundances measured by our strategy in which multiple PCSs are hierarchically used were compared to protein abundances provided by label‐free methods using mass spectrometric analyses. Relative copy numbers of expressed proteins calculated by identification frequency of peptide ions (PSM counts) in our large‐scale mass spectrometric analysis (see also Supporting Materials and methods) for budding yeast, which was cultured in our laboratory in identical conditions, showed significantly overall high correlation with the absolute abundances determined by the strategy used here (Spearman correlation coefficient = 0.79∼0.80, Fig. A and Supporting Information Fig.…”

Section: Resultsmentioning

confidence: 91%

“…(A) Comparison to the relative copy number calculated by the label‐free method. The relative copy numbers (ppm, fraction in total protein copy number) determined in our large‐scale analysis based on the identification frequency of peptide ions (PSM counts) (see also Supporting Materials and methods) was plotted against the absolute protein abundances determined by PCS in this study. (B) Comparison to the protein abundance in a public database (PaxDB ) integrated from many quantitative datasets mainly determined by label‐free methods.…”

Section: Resultsmentioning

confidence: 99%

“…For the design of artificial sequences suited for ID‐tag peptides, we explored the amino acid residues that affect spectral peak intensities in a large‐scale proteomic dataset, including 24 LC‐MS/MS analyses for 24 fractions of tryptic peptides separated by isoelectric focusing using the OFFGEL fractionator system (see also Supporting Materials and methods). As the numbers of identified peptides and their detected frequencies were relatively high for peptide ions with double‐charged state and within a range of peptide length from ten to 15 (Supporting Information Fig.…”

Section: Methodsmentioning

confidence: 99%

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A strategy for absolute proteome quantification with mass spectrometry by hierarchical use of peptide‐concatenated standards

et al. 2016

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The accurate and precise absolute abundance of proteins can be determined using mass spectrometry by spiking the sample with stable isotope-labeled standards. In this study, we developed a strategy of hierarchical use of peptide-concatenated standards (PCSs) to quantify more proteins over a wider dynamic range. Multiple primary PCSs were used for quantification of many target proteins. Unique "ID-tag peptides" were introduced into individual primary PCSs, allowing us to monitor the exact amounts of individual PCSs using a "secondary PCS" in which all "ID-tag peptides" were concatenated. Furthermore, we varied the copy number of the "ID-tag peptide" in each PCS according to a range of expression levels of target proteins. This strategy accomplished absolute quantification over a wider range than that of the measured ratios. The quantified abundance of budding yeast proteins showed a high reproducibility for replicate analyses and similar copy numbers per cell for ribosomal proteins, demonstrating the accuracy and precision of this strategy. A comparison with the absolute abundance of transcripts clearly indicated different post-transcriptional regulation of expression for specific functional groups. Thus, the approach presented here is a faithful method for the absolute quantification of proteomes and provides insights into biological mechanisms, including the regulation of expressed protein abundance.

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“…Proteins of interest were excised from the gels and digested using trypsin. The tryptic peptides were analyzed by LC-MS/MS consisting of an LTQ-Orbitrap mass spectrometer (ThermoFisher) and a DiNa nano LC (KYA Technologies) system according to the method described previously ( Kito et al, 2016 ). The peptide mixture was separated with reverse-phase chromatography.…”

Section: Methodsmentioning

confidence: 99%

Estimating the protein burden limit of yeast cells by measuring the expression limits of glycolytic proteins

Eguchi

Makanae

Hasunuma

et al. 2018

eLife

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The ultimate overexpression of a protein could cause growth defects, which are known as the protein burden. However, the expression limit at which the protein-burden effect is triggered is still unclear. To estimate this limit, we systematically measured the overexpression limits of glycolytic proteins in Saccharomyces cerevisiae. The limits of some glycolytic proteins were up to 15% of the total cellular protein. These limits were independent of the proteins’ catalytic activities, a finding that was supported by an in silico analysis. Some proteins had low expression limits that were explained by their localization and metabolic perturbations. The codon usage should be highly optimized to trigger the protein-burden effect, even under strong transcriptional induction. The S–S-bond-connected aggregation mediated by the cysteine residues of a protein might affect its expression limit. Theoretically, only non-harmful proteins could be expressed up to the protein-burden limit. Therefore, we established a framework to distinguish proteins that are harmful and non-harmful upon overexpression.

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Yeast Interspecies Comparative Proteomics Reveals Divergence in Expression Profiles and Provides Insights into Proteome Resource Allocation and Evolutionary Roles of Gene Duplication

Cited by 15 publications

References 81 publications

Proteomics analysis for asymmetric inheritance of preexisting proteins between mother and daughter cells in budding yeast

Proteomics analysis for asymmetric inheritance of preexisting proteins between mother and daughter cells in budding yeast

A strategy for absolute proteome quantification with mass spectrometry by hierarchical use of peptide‐concatenated standards

Estimating the protein burden limit of yeast cells by measuring the expression limits of glycolytic proteins

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