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Proteomes

Proteomes is an international, peer-reviewed, open access journal on all aspects of proteomics published quarterly online by MDPI.

Indexed in PubMed | Quartile Ranking JCR - Q2 (Biochemistry and Molecular Biology)

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All Articles (531)

The liver is a central metabolic organ that integrates nutrient sensing, lipid handling, and detoxification to maintain systemic homeostasis. In metabolic dysfunction–associated steatotic liver disease (MASLD), chronic metabolic overload accelerates hepatocyte senescence, impairing regenerative capacity and promoting progression toward fibrosis and hepatocellular carcinoma. While transcriptomic studies have provided important insights into stress-responsive pathways, they incompletely capture the proteome remodeling and proteoform-level alterations that govern hepatocyte function during aging and disease. Recent mass spectrometry–based proteomics studies have revealed that disruption of autophagy-dependent proteome homeostasis is a defining feature of senescent hepatocytes. Quantitative analyses demonstrate coordinated alterations in selective autophagy pathways—including lipophagy, mitophagy, ferritinophagy, ER-phagy, and pexophagy—accompanied by organelle-specific protein abundance signatures and remodeling of autophagy-related proteoforms. These findings position proteomics as an essential tool for resolving the spatial and functional reorganization of hepatocyte proteomes that cannot be inferred from transcript abundance alone. In this review, we synthesize proteomics-driven evidence defining selective autophagy dysfunction in aging and MASLD livers, critically evaluate methodological limitations, and propose a conceptual framework in which impaired selective autophagy acts as a proteome-level driver of hepatocyte senescence. We further outline future directions for proteoform-resolved and spatial proteomics approaches aimed at identifying actionable targets for therapeutic intervention in liver disease.

27 May 2026

Diverse Factors Inducing Cellular Senescence, subsequent telomere impairment activate a signaling cascade known as the DNA Damage Response (DDR). This signaling is transmitted from ATM and ATR to CHK2 and CHK1, ultimately leading to activation of the tumor suppressor protein p53, induction of cell cycle arrest, and, upon prolonged DDR activation, the onset of senescence. Furthermore, the activation of oncogenes promotes hyperproliferation and alterations in DNA replication patterns through the generation of reactive oxygen species (ROS), leading to DNA replication stress and the accumulation of genomic damage. In addition, mitochondrial dysfunction, characterized by low mitochondrial membrane potential (MMP), induces ROS production, which sustains persistent DDR signaling and facilitates the progression of cellular senescence. DDR; DNA damage response, ATM; Ataxia Telangiectasia Mutated, ATR; Ataxia Telangiectasia and Rad3-related, CHK1; Checkpoint Kinase 1, CHK2; Checkpoint Kinase 2, ROS; Reactive Oxygen Species.

Quantitative Metaproteomic Characterization of Acetic Acid Bacteria Reveals Functional Dynamics During Verdejo Wine Acetification

  • Cristina Campos-Vázquez,
  • Juan C. García-García and
  • Juan Carlos Mauricio
  • + 6 authors

Background: Acetification is a complex process driven by acetic acid bacteria (AAB), in which high ethanol and acidity levels require strong microbial metabolic adaptation. Although the microbiota involved in vinegar production has been described, the functional mechanisms that enable these bacteria to maintain metabolic activity remain poorly understood. In this study, the functional dynamics of AAB during Verdejo vinegar acetification were analyzed using a quantitative metaproteomic approach. Methods: Acetification was performed in submerged culture under semi-continuous conditions, and samples were collected at four stages of the cycle (S1–S4). Results: LC-MS/MS analysis led to the identification of 1626 proteins, of which 1409 were assigned to the Acetobacteraceae family. Komagataeibacter europaeus was the dominant species (73.7%). Hierarchical clustering revealed four protein abundance patterns, and differential analysis identified 350 proteins with increased abundance and 169 with decreased abundance, with the greatest changes observed between S1 and S4. Functional annotation and protein–protein interaction analyses indicated that the main metabolic adaptations involve pathways related to energy metabolism, amino acid biosynthesis, membrane-associated functions, cellular homeostasis, and acid stress response. Conclusions: Overall, the results show that K. europaeus concentrates most of the metabolic activity during acetification and that proteome reorganization reflects key molecular strategies for adaptation and survival under high-acidity conditions.

20 May 2026

Main system variables throughout the acetification profile of Verdejo wine, including both the variables continuously monitored and those measured exclusively at sampling times: (A) working volume, (B) acetic acid concentration, (C) ethanol concentration, and (D) total cell count. Green shaded areas indicate the sampling stages (S1–S4). The average values of these variables in each sample are presented together with their corresponding standard deviations (SD).
  • Perspective
  • Open Access

Single-cell proteomics (SCP) is an exciting new field of study with developments in the areas of sample preparation, instrumentation and informatics. SCP has captured the imagination of biologists and clinicians and the critical interest of both academic and commercial mass-spectrometry groups. Currently (i.e., at the time this manuscript was written), SCP is still difficult and slow relative to competing single-cell technologies. What SCP may lose in relative throughput, it trades for direct analysis of protein and proteoforms, albeit with biases toward those of the highest relative concentration in each cell. These strengths may not make SCP the technology of choice for every study. This perspective is intended to identify current and future biological or clinical areas where SCP has or could have the greatest potential to advance human health and knowledge. I will also discuss applications where SCP would be less impactful than other technologies and where SCP, when mature, could play a true role in clinical diagnostics.

18 May 2026

A summary of applications of single-cell proteomics that will be discussed in this Perspective article.

Background: Maize is a vital crop, supporting 19.5% of global calorie intake. However, maize is vulnerable to even brief periods of drought which substantially reduces seed set and therefore yield. Methods: To identify proteins involved in responses of maize to drought, soluble proteins were extracted from leaf and silk tissues of Zea mays and protein abundance and phosphorylation status were quantified relative to well-watered controls. Label-free quantification and phosphopeptide enrichment were applied to the same biological samples and over 300 proteins were identified with significantly different changes. Results: Proteins known to be involved in drought responses were identified, such as the abscisic acid pathway and transcription factors. Of particular interest is a group of dehydrins quantified at both total protein and phosphopeptide levels, permitting insight into stoichiometry. The biological function of dehydrins in the model plant Arabidopsis thaliana is known to be regulated by phosphorylation. Conclusions: Translation of protein function from model plant to crops remains highly challenging because genome duplication has created complex sets of orthologous and homologous proteins. By focusing on proteomic changes during crop stress responses, this work enables the identification of known and novel proteins, substantially aiding the transfer of knowledge from model plants to crops.

9 May 2026

The impact of drought on maize yield for the samples analysed. (A). Schematic diagram showing maize growth and drought treatment. (B) Typical cobs from well-watered and drought-treated plants. (C) Changes to cob weight and (D) seed weight and numbers. Well-watered control in blue and droughted samples in red, N = 3. * represents p value of <0.05 in the Student’s t-test.

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Neuroproteomics
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Neuroproteomics

Editors: Angus C. Nairn, Kenneth R. Williams
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Proteomes - ISSN 2227-7382