Your search keyword '"Subcellular Fractions metabolism"' showing total 14,512 results

1. Nascent and Mature RNA Profiling by Subcellular Fractionation in Human Cells.

Author

Pinskaya M, Jarroux J, Cipolla R, and Morillon A

Subjects

Humans, RNA, Messenger genetics, RNA, Messenger metabolism, Gene Expression Profiling methods, RNA genetics, RNA metabolism, Subcellular Fractions metabolism, Chromatin metabolism, Chromatin genetics, Alpha-Amanitin pharmacology, Cell Nucleus metabolism, Cell Nucleus genetics, Cytoplasm metabolism, Transcription, Genetic, Transcriptome, RNA Polymerase II metabolism, RNA Stability, Cell Fractionation methods

Abstract

Transcription and RNA decay determine steady-state RNA levels in cells available for translation and RNA-mediated regulatory functions. Both processes can be assessed by various techniques, for majority, based on RNA labelling or chromatin immunoprecipitation, but require a high level of expertise. Here, we describe a cost-effective, fast, and simple protocol that enables the profiling of nascent and mature RNA in the cytoplasm, nucleoplasm, and chromatin through subcellular fractionation. The workflow can include α-amanitin inhibition of RNA Polymerase II to assess nascent RNAs as a proxy of transcriptional activity, or it can be used without this treatment to investigate distribution of partially processed or mature transcripts across distinct subcellular compartments. It is applicable for studying any of RNA biotypes, including small and long noncoding RNAs, mRNAs, and their splice variants, on both transcript-specific and transcriptome-wide scales. Nascent or mature RNAs isolated from each fraction can be further analyzed by any technique of choice (northern blot, reverse transcription, RNA sequencing)., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

2. REAP+: A single preparation for rapid isolation of nuclei, cytoplasm, and mitochondria.

Author

Dos Santos B, Bion MC, Goujon-Svrzic M, Maher P, and Dafre AL

Subjects

Humans, Mice, Animals, Cell Fractionation methods, Cytoplasm metabolism, Cytosol metabolism, Subcellular Fractions metabolism, Mitochondria metabolism, Cell Nucleus metabolism

Abstract

REAP+ is an enhanced version of the rapid, efficient, and practical (REAP) method designed for the isolation of nuclear fractions. This improved version, REAP+, enables fast and effective extraction of mitochondria, cytoplasm, and nuclei. The mechanical cell disruption process has been optimized to cerebral tissues, snap-frozen liver, and HT22 cells with remarkable fraction enrichment. REAP+ is well-suited for samples containing minimal protein quantities, such as mouse hippocampal slices. The method was validated by Western blot and marker enzyme activities, such as LDH and G6PDH for the cytoplasmic fraction and succinate dehydrogenase and cytochrome c oxidase for the mitochondrial fraction. One of the outstanding features of this method is its rapid execution, yielding fractions within 15 min, allowing for simultaneous preparation of multiple samples. In essence, REAP+ emerges as a swift, efficient, and practical technique for the concurrent isolation of nuclei, cytoplasm, and mitochondria from various cell types and tissues. The method would be suitable to study the multicompartment translocation of proteins, such as metabolic enzymes and transcription factors migrating from cytosol to the mitochondria and nuclei. Moreover, its compatibility with small samples, such as hippocampal slices, and its potential applicability to human biopsies, highlights the potential application in medical research., Competing Interests: Declaration of competing interest The authors declare no conflict of interests, (Copyright © 2024 Elsevier Inc. All rights reserved.)

Published

2024

3. Bafilomycin A1 Molecular Effect on ATPase Activity of Subcellular Fraction of Human Colorectal Cancer and Rat Liver.

Author

Bychkova S, Bychkov M, Dordevic D, Vítězová M, Rittmann SKR, and Kushkevych I

Subjects

Humans, Rats, Animals, Macrolides pharmacology, Subcellular Fractions metabolism, Liver metabolism, Calcium metabolism, Vacuolar Proton-Translocating ATPases metabolism, Colonic Neoplasms, Colorectal Neoplasms

Abstract

Bafilomycin A1 inhibits V-type H + ATPases on the molecular level, which acidifies endo-lysosomes. The main objective of the study was to assess the effect of bafilomycin A1 on Ca 2+ content, NAADP-induced Ca 2+ release, and ATPase activity in rat hepatocytes and human colon cancer samples. Chlortetracycline (CTC) was used for a quantitative measure of stored calcium in permeabilized rat hepatocytes. ATPase activity was determined by orthophosphate content released after ATP hydrolysis in subcellular post-mitochondrial fraction obtained from rat liver as well as from patients' samples of colon mucosa and colorectal cancer samples. In rat hepatocytes, bafilomycin A1 decreased stored Ca 2+ and prevented the effect of NAADP on stored Ca 2+ . This effect was dependent on EGTA-Ca 2+ buffers in the medium. Bafilomycin A1 significantly increased the activity of Ca 2+ ATPases of endoplasmic reticulum (EPR), but not plasma membrane (PM) Ca 2+ ATPases in rat liver. Bafilomycin A1 also prevented the effect of NAADP on these pumps. In addition, bafilomycin A1 reduced Na + /K + ATPase activity and increased basal Mg 2+ ATPase activity in the subcellular fraction of rat liver. Concomitant administration of bafilomycin A1 and NAADP enhanced these effects. Bafilomycin A1 increased the activity of the Ca 2+ ATPase of EPR in the subcellular fraction of normal human colon mucosa and also in colon cancer tissue samples. In contrast, it decreased Ca 2+ ATPase PM activity in samples of normal human colon mucosa and caused no changes in colon cancer. Bafilomycin A1 decreased Na + /K + ATPase activity and increased basal Mg 2+ ATPase activity in normal colon mucosa samples and in human colon cancer samples. It can be concluded that bafilomycin A1 targets NAADP-sensitive acidic Ca 2+ stores, effectively modulates ATPase activity, and assumes the link between acidic stores and EPR. Bafilomycin A1 may be useful for cancer therapy.

Published

2024

4. Subcellular fractionation by differential centrifugation for mitochondrial studies.

Author

Steiert C, Busto JV, Melchionda L, and Wiedemann N

Subjects

Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae chemistry, Mitochondria metabolism, Mitochondria chemistry, Cell Fractionation methods, Centrifugation methods, Subcellular Fractions metabolism, Subcellular Fractions chemistry

Abstract

In addition to fluorescence microscopy, the subcellular fractionation of eukaryotic cells remains one of the central methods for the basic characterization of proteins. Here we describe an optimized procedure for the subcellular fractionation of yeast cells, specifically for mitochondrial studies. Major recommendations are to separate the fractions immediately after each centrifugation step, to carefully discard a significant part of the supernatant fractions which is in the direct vicinity to the pellets and, in addition, to perform an extra homogenization step of the post nuclear supernatant fraction. These principles help to collect supernatant fractions with less cross-contaminations from the corresponding pellets. These approaches are scalable and adaptable for the fractionation of other cell types and are also useful for the characterization of other organelles., (Copyright © 2024. Published by Elsevier Inc.)

Published

2024

5. Detection of Stress-Induced Changes in Subcellular Protein Distribution.

Author

Seidel T

Subjects

Protein Transport, Proteins metabolism, Subcellular Fractions metabolism, Humans, Proteomics methods, Cell Nucleus metabolism, Stress, Physiological

Abstract

Proteins often show alterations in their subcellular localization with changing environmental conditions; transcription factors enter the nucleus or are actively removed from the nucleus; some even bind to endo-membranes by conditional membrane anchors; and other proteins and mRNA arrange in RNA granules. These are some examples of the complex regulation of subcellular localization, which often depends on posttranslational modifications and is triggered by environmental stressors. The challenge is the precise identification of the compartments, the quantitative analysis of proteins, which reside in multiple compartments, and their transport dynamics. Therefore, appropriate compartment markers and routines for a reproducible quantitative workflow are required., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

6. System-wide analysis of RNA and protein subcellular localization dynamics.

Author

Villanueva E, Smith T, Pizzinga M, Elzek M, Queiroz RML, Harvey RF, Breckels LM, Crook OM, Monti M, Dezi V, Willis AE, and Lilley KS

Subjects

Subcellular Fractions metabolism, Proteome analysis, RNA genetics, RNA metabolism, Endoplasmic Reticulum metabolism

Abstract

Although the subcellular dynamics of RNA and proteins are key determinants of cell homeostasis, their characterization is still challenging. Here we present an integrative framework to simultaneously interrogate the dynamics of the transcriptome and proteome at subcellular resolution by combining two methods: localization of RNA (LoRNA) and a streamlined density-based localization of proteins by isotope tagging (dLOPIT) to map RNA and protein to organelles (nucleus, endoplasmic reticulum and mitochondria) and membraneless compartments (cytosol, nucleolus and cytosolic granules). Interrogating all RNA subcellular locations at once enables system-wide quantification of the proportional distribution of RNA. We obtain a cell-wide overview of localization dynamics for 31,839 transcripts and 5,314 proteins during the unfolded protein response, revealing that endoplasmic reticulum-localized transcripts are more efficiently recruited to cytosolic granules than cytosolic RNAs, and that the translation initiation factor eIF3d is key to sustaining cytoskeletal function. Overall, we provide the most comprehensive overview so far of RNA and protein subcellular localization dynamics., (© 2023. The Author(s).)

Published

2024

7. Dual-Signal Feature Spaces Map Protein Subcellular Locations Based on Immunohistochemistry Image and Protein Sequence.

Author

Zou K, Wang S, Wang Z, Zou H, and Yang F

Subjects

Humans, Immunohistochemistry, Amino Acid Sequence, Databases, Protein, Subcellular Fractions chemistry, Subcellular Fractions metabolism, Proteins analysis, Cell Nucleus metabolism

Abstract

Protein is one of the primary biochemical macromolecular regulators in the compartmental cellular structure, and the subcellular locations of proteins can therefore provide information on the function of subcellular structures and physiological environments. Recently, data-driven systems have been developed to predict the subcellular location of proteins based on protein sequence, immunohistochemistry (IHC) images, or immunofluorescence (IF) images. However, the research on the fusion of multiple protein signals has received little attention. In this study, we developed a dual-signal computational protocol by incorporating IHC images into protein sequences to learn protein subcellular localization. Three major steps can be summarized as follows in this protocol: first, a benchmark database that includes 281 proteins sorted out from 4722 proteins of the Human Protein Atlas (HPA) and Swiss-Prot database, which is involved in the endoplasmic reticulum (ER), Golgi apparatus, cytosol, and nucleoplasm; second, discriminative feature operators were first employed to quantitate protein image-sequence samples that include IHC images and protein sequence; finally, the feature subspace of different protein signals is absorbed to construct multiple sub-classifiers via dimensionality reduction and binary relevance (BR), and multiple confidence derived from multiple sub-classifiers is adopted to decide subcellular location by the centralized voting mechanism at the decision layer. The experimental results indicated that the dual-signal model embedded IHC images and protein sequences outperformed the single-signal models with accuracy, precision, and recall of 75.41%, 80.38%, and 74.38%, respectively. It is enlightening for further research on protein subcellular location prediction under multi-signal fusion of protein.

Published

2023

8. Separation of Single Core and Multicore Lytic Granules by Subcellular Fractionation and Immunoisolation.

Author

Schirra C, Alawar N, Becherer U, and Chang HF

Subjects

Mice, Animals, Cell Fractionation methods, Cytological Techniques, Organelles, Centrifugation, Density Gradient methods, Cytoplasmic Granules, Subcellular Fractions metabolism, Vesicle-Associated Membrane Protein 2 analysis, Vesicle-Associated Membrane Protein 2 metabolism, Proteins metabolism

Abstract

Subcellular fractionation is an important tool used to separate intracellular organelles, structures or proteins. Here, we describe a stepwise protocol to isolate two types of lytic granules, multicore (MCG), and single core (SCG), from primary murine CTLs. We used cell disruption by nitrogen cavitation followed by separation of organelles via discontinuous sucrose density gradient centrifugation. Immunoisolation with a Synaptobrevin 2 antibody attached to magnetic beads was then used to harvest Synaptobrevin 2 positive granules for immunoblotting, mass spectrometry, electron, and light microscopy., (© 2023. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2023

9. LAFITE Reveals the Complexity of Transcript Isoforms in Subcellular Fractions.

Author

Zhang J, Lin X, Chen Y, Li TH, Lee AC, Chow EY, Cho WC, and Chan TF

Subjects

Reproducibility of Results, RNA, Messenger genetics, RNA, Messenger metabolism, Protein Isoforms genetics, Subcellular Fractions metabolism, Transcriptome genetics

Abstract

Characterization of the subcellular distribution of RNA is essential for understanding the molecular basis of biological processes. Here, the subcellular nanopore direct RNA-sequencing (DRS) of four lung cancer cell lines (A549, H1975, H358, and HCC4006) is performed, coupled with a computational pipeline, Low-abundance Aware Full-length Isoform clusTEr (LAFITE), to comprehensively analyze the full-length cytoplasmic and nuclear transcriptome. Using additional DRS and orthogonal data sets, it is shown that LAFITE outperforms current methods for detecting full-length transcripts, particularly for low-abundance isoforms that are usually overlooked due to poor read coverage. Experimental validation of six novel isoforms exclusively identified by LAFITE further confirms the reliability of this pipeline. By applying LAFITE to subcellular DRS data, the complexity of the nuclear transcriptome is revealed in terms of isoform diversity, 3'-UTR usage, m6A modification patterns, and intron retention. Overall, LAFITE provides enhanced full-length isoform identification and enables a high-resolution view of the RNA landscape at the isoform level., (© 2022 The Authors. Advanced Science published by Wiley-VCH GmbH.)

Published

2023

10. Subcellular partitioning of protein kinase activity revealed by functional kinome profiling.

Author

Wegman-Points L, Alganem K, Imami AS, Mathis V, Creeden JF, McCullumsmith R, and Yuan LL

Subjects

Animals, Phosphorylation, Rats, Serine metabolism, Subcellular Fractions metabolism, Threonine metabolism, Peptides metabolism, Protein Kinases metabolism

Abstract

Protein kinases and their substrates form signaling networks partitioned across subcellular compartments to facilitate critical biological processes. While the subcellular roles of many individual kinases have been elucidated, a comprehensive assessment of the synaptic subkinome is lacking. Further, most studies of kinases focus on transcript, protein, and/or phospho-protein expression levels, providing an indirect measure of protein kinase activity. Prior work suggests that gene expression levels are not a good predictor of protein function. Thus, we assessed global serine/threonine protein kinase activity profiles in synaptosomal, nuclear, and cytosolic fractions from rat frontal cortex homogenate using peptide arrays. Comparisons made between fractions demonstrated differences in overall protein kinase activity. Upstream kinase analysis revealed a list of cognate kinases that were enriched in the synaptosomal fraction compared to the nuclear fraction. We identified many kinases in the synaptic fraction previously implicated in this compartment, while also identifying other kinases with little or no evidence for synaptic localization. Our results show the feasibility of assessing subcellular fractions with peptide activity arrays, as well as suggesting compartment specific activity profiles associated with established and novel kinases., (© 2022. The Author(s).)

Published

2022

11. Inferring differential subcellular localisation in comparative spatial proteomics using BANDLE.

Author

Crook OM, Davies CTR, Breckels LM, Christopher JA, Gatto L, Kirk PDW, and Lilley KS

Subjects

Bayes Theorem, Mass Spectrometry methods, Subcellular Fractions metabolism, Proteome metabolism, Proteomics methods

Abstract

The steady-state localisation of proteins provides vital insight into their function. These localisations are context specific with proteins translocating between different subcellular niches upon perturbation of the subcellular environment. Differential localisation, that is a change in the steady-state subcellular location of a protein, provides a step towards mechanistic insight of subcellular protein dynamics. High-accuracy high-throughput mass spectrometry-based methods now exist to map the steady-state localisation and re-localisation of proteins. Here, we describe a principled Bayesian approach, BANDLE, that uses these data to compute the probability that a protein differentially localises upon cellular perturbation. Extensive simulation studies demonstrate that BANDLE reduces the number of both type I and type II errors compared to existing approaches. Application of BANDLE to several datasets recovers well-studied translocations. In an application to cytomegalovirus infection, we obtain insights into the rewiring of the host proteome. Integration of other high-throughput datasets allows us to provide the functional context of these data., (© 2022. The Author(s).)

Published

2022

12. Bioaccumulation, Detoxification, and Biological Macromolecular Damage of Benzo[a]pyrene in Exposure in Tissues and Subcellular Fractions of Scallop Chlamys farreri.

Author

Bi Y, Chen W, Miao J, Pan L, and Li D

Subjects

Animals, Benzo(a)pyrene metabolism, Benzo(a)pyrene toxicity, Bioaccumulation, Cytochrome P-450 CYP1A1 metabolism, Glutathione metabolism, Glutathione Transferase metabolism, Subcellular Fractions chemistry, Subcellular Fractions metabolism, Superoxide Dismutase metabolism, Bivalvia metabolism, Pectinidae metabolism, Polycyclic Aromatic Hydrocarbons toxicity, Water Pollutants, Chemical analysis

Abstract

Because of the persistence and high toxicity of benzo[a]pyrene (B[a]P), the bioaccumulation and detoxification mechanisms of B[a]P have been studied extensively at the tissue level; but the data at the subcellular level in bivalves have not been reported. The present study was conducted to investigate the effects of B[a]P exposure on bioaccumulation, detoxification, and biomacromolecular damage in gills, digestive glands, and their subcellular fractions of the scallop Chlamys farreri. The subcellular fraction contains cytoplasm, mitochondria, microsome, nucleus, cell membrane, and overall organelle. The results demonstrated that B[a]P accumulation showed a clear time-dose effect. Based on the time-dependent accumulation of B[a]P in subcellular fractions, we speculated that the intracellular migration order of B[a]P was cell membrane, organelle, and nucleus in turn. Considering the difference of B[a]P accumulation may be related to B[a]P metabolism, we have further confirmed that the activities of B[a]P metabolizing enzymes in scallop tissues and subcellular fractions were significantly tempted by B[a]P (p < 0.05), including 7-ethoxyresorufin O-deethylase (increased), glutathione-S-transferase (GST; decreased), and superoxide dismutase (increased). First, GST was detected in bivalve cytoplasm and microsome. Second, B[a]P exposure also caused biomacromolecules damage. The results demonstrated that mitochondria and microsome were more vulnerable to lipid peroxidation than cell membrane and nucleus. Taken together, the present study fills some of the gaps in our knowledge of the bioaccumulation and detoxification mechanisms of C. farreri exposed to B[a]P in subcellular fractions and deeply explores the transportation and the main metabolic and damage sites of polycyclic aromatic hydrocarbons (PAHs) in cells, which helped us to comprehensively understand the toxic mechanism of PAHs on bivalves. Environ Toxicol Chem 2022;41:2353-2364. © 2022 SETAC., (© 2022 SETAC.)

Published

2022

13. DeepLoc 2.0: multi-label subcellular localization prediction using protein language models.

Author

Thumuluri V, Almagro Armenteros JJ, Johansen AR, Nielsen H, and Winther O

Subjects

Humans, Eukaryota metabolism, Protein Transport, Language, Databases, Protein, Computational Biology, Subcellular Fractions metabolism, Proteins metabolism, Protein Sorting Signals

Abstract

The prediction of protein subcellular localization is of great relevance for proteomics research. Here, we propose an update to the popular tool DeepLoc with multi-localization prediction and improvements in both performance and interpretability. For training and validation, we curate eukaryotic and human multi-location protein datasets with stringent homology partitioning and enriched with sorting signal information compiled from the literature. We achieve state-of-the-art performance in DeepLoc 2.0 by using a pre-trained protein language model. It has the further advantage that it uses sequence input rather than relying on slower protein profiles. We provide two means of better interpretability: an attention output along the sequence and highly accurate prediction of nine different types of protein sorting signals. We find that the attention output correlates well with the position of sorting signals. The webserver is available at services.healthtech.dtu.dk/service.php?DeepLoc-2.0., (© The Author(s) 2022. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2022

14. Development of a UPLC-MRM-based targeted proteomic method to profile subcellular organelle marker proteins from human liver tissues.

Author

Qiu X, Doyle LM, and Wang MZ

Subjects

Biomarkers metabolism, Humans, Liver metabolism, Proteins metabolism, Reproducibility of Results, Subcellular Fractions metabolism, Organelles metabolism, Proteomics methods

Abstract

Subcellular organelles have long been an interest in biochemical research and drug development as the isolation of those organelles can help to probe protein functions and elucidate drug disposition within the cell. Usually, the purity of isolated subcellular organelle fractions was determined using immunoblot analysis of subcellular organelle marker proteins, which can be labor-intensive and lack reproducibility due to antibody batch-to-batch variability. As such, a higher throughput and more robust method is needed. Here, a UPLC-MRM-based targeted proteomic method was developed for a panel of human organelle marker proteins and used to profile a series of sucrose fractions isolated from the protein extract of human liver tissues. The method was validated by comparing to the traditional immunoblot and determining subcellular localization of three case study proteins (CYP3A4, FcRn, and β2M) pertaining to the disposition of small molecule and biologic drugs. All three case study proteins were co-enriched with their corresponding subcellular protein marker, and complete recoveries were achieved from isolated fractions. This newly developed MRM method for the panel of human organelle marker proteins can potentially accelerate future intracellular drug disposition analysis and facilitate subcellular organelle quality assessment., (© 2022. The Author(s).)

Published

2022

15. An endosome-associated actin network involved in directed apical plasma membrane growth.

Author

Ríos-Barrera LD and Leptin M

Subjects

Animals, Drosophila Proteins metabolism, Drosophila melanogaster embryology, Endocytosis, Green Fluorescent Proteins metabolism, Lasers, Subcellular Fractions metabolism, Time Factors, Actins metabolism, Cell Membrane metabolism, Drosophila melanogaster metabolism, Endosomes metabolism

Abstract

Membrane trafficking plays many roles in morphogenesis, from bulk membrane provision to targeted delivery of proteins and other cargos. In tracheal terminal cells of the Drosophila respiratory system, transport through late endosomes balances membrane delivery between the basal plasma membrane and the apical membrane, which forms a subcellular tube, but it has been unclear how the direction of growth of the subcellular tube with the overall cell growth is coordinated. We show here that endosomes also organize F-actin. Actin assembles around late endocytic vesicles in the growth cone of the cell, reaching from the tip of the subcellular tube to the leading filopodia of the basal membrane. Preventing nucleation of endosomal actin disturbs the directionality of tube growth, uncoupling it from the direction of cell elongation. Severing actin in this area affects tube integrity. Our findings show a new role for late endosomes in directing morphogenesis by organizing actin, in addition to their known role in membrane and protein trafficking., (© 2022 Ríos-Barrera and Leptin.)

Published

2022

16. Subcellular regulation of glucose metabolism through multienzyme glucosome assemblies by EGF-ERK1/2 signaling pathways.

Author

Jeon M, Chauhan KM, Szeto GL, Kyoung M, and An S

Subjects

Humans, Phosphorylation, Serine metabolism, Subcellular Fractions metabolism, Epidermal Growth Factor metabolism, Glucose metabolism, MAP Kinase Signaling System, Multienzyme Complexes metabolism

Abstract

A multienzyme metabolic assembly for human glucose metabolism, namely the glucosome, has been previously demonstrated to partition glucose flux between glycolysis and building block biosynthesis in an assembly size-dependent manner. Among three different sizes of glucosome assemblies, we have shown that large-sized glucosomes are functionally associated with the promotion of serine biosynthesis in the presence of epidermal growth factor (EGF). However, due to multifunctional roles of EGF in signaling pathways, it is unclear which EGF-mediated signaling pathways promote these large glucosome assemblies in cancer cells. In this study, we used Luminex multiplexing assays and high-content single-cell imaging to demonstrate that EGF triggers temporal activation of extracellular signal-regulated kinases 1/2 (ERK1/2) in Hs578T cells. Subsequently, we found that treatments with a pharmacological inhibitor of ERK1/2, SCH772984, or short-hairpin RNAs targeting ERK1/2 promote the dissociation of large-sized assemblies to medium-sized assemblies in Hs578T cells. In addition, our Western blot analyses revealed that EGF treatment does not increase the expression levels of enzymes that are involved in both glucose metabolism and serine biosynthesis. The observed spatial transition of glucosome assemblies between large and medium sizes appears to be mediated by the degree of dynamic partitioning of glucosome enzymes without changing their expression levels. Collectively, our study demonstrates that EGF-ERK1/2 signaling pathways play an important role in the upregulation of large-sized glucosomes in cancer cells, thus functionally governing the promotion of glycolysis-derived serine biosynthesis., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2022 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2022

17. Discovery of an Amino Acid-Modified Near-Infrared Aza-BODIPY Photosensitizer as an Immune Initiator for Potent Photodynamic Therapy in Melanoma.

Author

Yu Z, Wang H, Chen Z, Dong X, Zhao W, Shi Y, and Zhu Q

Subjects

Animals, Aspartic Acid chemistry, Cell Line, Tumor, Drug Discovery, Female, Humans, Immunotherapy, Mice, Mice, Inbred C57BL, Reactive Oxygen Species, Structure-Activity Relationship, Subcellular Fractions metabolism, Xenograft Model Antitumor Assays, Amino Acids chemistry, Boron Compounds chemical synthesis, Boron Compounds pharmacology, Melanoma drug therapy, Photochemotherapy methods, Photosensitizing Agents chemical synthesis, Photosensitizing Agents pharmacology

Abstract

The discovery of novel photosensitizers with potent phototoxicity and desirable water solubility is an urgent task for photodynamic therapy. Herein, a series of amino acid-modified aza-BODIPY photosensitizers were synthesized and evaluated. These new PSs exhibited enhanced aqueous solubility, increased 1 O 2 generation efficiency, and an improved photo-dark toxicity ratio. Aspartic acid-modified PS of 1a , which possessed intense NIR absorption and high 1 O 2 quantum yield, demonstrated the most potent efficacy toward the investigated tumor cell lines without using an emulsifier. Subcellular localization, cell-based ROS production, and cell death pathway of 1a were studied. In vivo fluorescence imaging and ex vivo organ distribution assays manifested that 1a possessed reasonable distribution and clearance. In vivo PDT studies indicated that 1a revealed advantages over Ce6 and our previously optimized PS of BDP-4 . It not only afforded an excellent PDT effect with a low drug dose under only single-time photoirradiation but also induced an antitumor immunological response.

Published

2022

18. Tau interactome maps synaptic and mitochondrial processes associated with neurodegeneration.

Author

Tracy TE, Madero-Pérez J, Swaney DL, Chang TS, Moritz M, Konrad C, Ward ME, Stevenson E, Hüttenhain R, Kauwe G, Mercedes M, Sweetland-Martin L, Chen X, Mok SA, Wong MY, Telpoukhovskaia M, Min SW, Wang C, Sohn PD, Martin J, Zhou Y, Luo W, Trojanowski JQ, Lee VMY, Gong S, Manfredi G, Coppola G, Krogan NJ, Geschwind DH, and Gan L

Subjects

Alzheimer Disease genetics, Amino Acids metabolism, Biotinylation, Brain metabolism, Brain pathology, Cell Nucleus metabolism, Disease Progression, Energy Metabolism, Frontotemporal Dementia genetics, Humans, Induced Pluripotent Stem Cells metabolism, Mutant Proteins metabolism, Mutation genetics, Nerve Degeneration pathology, Neurons metabolism, Protein Binding, Protein Domains, Proteomics, Severity of Illness Index, Subcellular Fractions metabolism, Tauopathies genetics, tau Proteins chemistry, Mitochondria metabolism, Nerve Degeneration metabolism, Protein Interaction Maps, Synapses metabolism, tau Proteins metabolism

Abstract

Tau (MAPT) drives neuronal dysfunction in Alzheimer disease (AD) and other tauopathies. To dissect the underlying mechanisms, we combined an engineered ascorbic acid peroxidase (APEX) approach with quantitative affinity purification mass spectrometry (AP-MS) followed by proximity ligation assay (PLA) to characterize Tau interactomes modified by neuronal activity and mutations that cause frontotemporal dementia (FTD) in human induced pluripotent stem cell (iPSC)-derived neurons. We established interactions of Tau with presynaptic vesicle proteins during activity-dependent Tau secretion and mapped the Tau-binding sites to the cytosolic domains of integral synaptic vesicle proteins. We showed that FTD mutations impair bioenergetics and markedly diminished Tau's interaction with mitochondria proteins, which were downregulated in AD brains of multiple cohorts and correlated with disease severity. These multimodal and dynamic Tau interactomes with exquisite spatial resolution shed light on Tau's role in neuronal function and disease and highlight potential therapeutic targets to block Tau-mediated pathogenesis., Competing Interests: Declaration of interests L.G. is a founder of Aeton Therapeutics. N.J.K. received research support from Vir Biotechnology and F. Hoffmann-La Roche; has consulting agreements with the Icahn School of Medicine at Mount Sinai, New York, Maze Therapeutics, and Interline Therapeutics; is a shareholder in Tenaya Therapeutics, Maze Therapeutics, and Interline Therapeutics; and is a financially compensated Scientific Advisory Board Member for GEn1E Life sciences., (Copyright © 2021 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2022

19. GLUT4 On the move.

Author

Fazakerley DJ, Koumanov F, and Holman GD

Subjects

Adipocytes metabolism, Animals, Cell Membrane metabolism, Glucose metabolism, Humans, Insulin metabolism, Insulin pharmacology, Models, Biological, Muscle Cells metabolism, Phosphorylation, Protein Processing, Post-Translational, Protein Transport drug effects, Signal Transduction, Subcellular Fractions metabolism, Glucose Transporter Type 4 physiology

Abstract

Insulin rapidly stimulates GLUT4 translocation and glucose transport in fat and muscle cells. Signals from the occupied insulin receptor are translated into downstream signalling changes in serine/threonine kinases within timescales of seconds, and this is followed by delivery and accumulation of the glucose transporter GLUT4 at the plasma membrane. Kinetic studies have led to realisation that there are distinct phases of this stimulation by insulin. There is a rapid initial burst of GLUT4 delivered to the cell surface from a subcellular reservoir compartment and this is followed by a steady-state level of continuing stimulation in which GLUT4 recycles through a large itinerary of subcellular locations. Here, we provide an overview of the phases of insulin stimulation of GLUT4 translocation and the molecules that are currently considered to activate these trafficking steps. Furthermore, we suggest how use of new experimental approaches together with phospho-proteomic data may help to further identify mechanisms for activation of these trafficking processes., (© 2022 The Author(s).)

Published

2022

20. Two novel STAT1 mutations cause Mendelian susceptibility to mycobacterial disease.

Author

Liu Z, Zhou M, Yuan C, Ni Z, Liu W, Tan Y, Zhang D, Zhou X, Zou T, Wang J, Hou M, Peng X, and Zhang X

Subjects

Amino Acid Sequence, Base Sequence, Cell Nucleus metabolism, DNA metabolism, Female, HEK293 Cells, HeLa Cells, Humans, Male, Mutant Proteins chemistry, Mutant Proteins genetics, Pedigree, Protein Binding, Protein Domains, Protein Transport, STAT1 Transcription Factor chemistry, STAT1 Transcription Factor metabolism, Subcellular Fractions metabolism, Genetic Predisposition to Disease, Mutation genetics, Mycobacterium Infections genetics, Mycobacterium Infections microbiology, STAT1 Transcription Factor genetics

Abstract

Mendelian susceptibility to mycobacterial disease (MSMD) is a rare monogenetic disease, which is characterized by susceptibility to some weakly virulent mycobacteria. Here, we explored the pathogenic genes and molecular mechanisms of MSMD patients. We recruited three patients diagnosed with MSMD from two families. Two novel mutations (c.1228A > G, p.K410E and c.2071A > G, p.M691V) in STAT1 gene were identified from two families. The translocation of K410E mutant STAT1 protein into nucleus was not affected. The binding ability between gamma-activating sequence (GAS) and K410E mutant STAT1 protein was significantly reduced, which will reduce the interaction between STAT1 protein with the promoters of target genes. The M691V mutant STAT1 protein cannot translocate into the nucleus after IFN-γ stimulation, which will affect the STAT1 protein form gamma-activating factors (GAF) and bind the GAS in the promoter region of downstream target genes. Taken together, our results showed that the mutation of K410E led to impaired binding of STAT1 to target DNA, and the mutation of M691V prevented the transport of STAT1 into the nucleus, which led to MSMD. Together, we identified two novel mutations (c.1228A > G, p.K410E and c.2071A > G, p.M691V) in STAT1 gene in MSMD patients, and deciphered the molecular mechanism of MSMD caused by STAT1 mutations., Competing Interests: Declaration of competing interest The authors declare no conflict of interest., (Copyright © 2021 Elsevier Inc. All rights reserved.)

Published

2022

21. PSL-LCCL: a resource for subcellular protein localization in liver cancer cell line SK&#95;HEP1.

Author

Huang F, Tang X, Ye B, Wu S, and Ding K

Subjects

Cell Line, Humans, Organelles, Proteomics methods, Subcellular Fractions metabolism, Liver Neoplasms genetics, Liver Neoplasms metabolism, Proteome genetics, Proteome metabolism

Abstract

The characterization of subcellular protein localization provides a basis for further understanding cellular behaviors. A delineation of subcellular localization of proteins on cytosolic membrane-bound organelles in human liver cancer cell lines (hLCCLs) has yet to be performed. To obtain its proteome-wide view, we isolated and enriched six cytosolic membrane-bound organelles in one of the hLCCLs (SK&#95;HEP1) and quantified their proteins using mass spectrometry. The vigorous selection of marker proteins and a machine-learning-based algorithm were implemented to localize proteins at cluster and neighborhood levels. We validated the performance of the proposed method by comparing the predicted subcellular protein localization with publicly available resources. The profiles enabled investigating the correlation of protein domains with their subcellular localization and colocalization of protein complex members. A subcellular proteome database for SK&#95;HEP1, including (i) the subcellular protein localization and (ii) the subcellular locations of protein complex members and their interactions, was constructed. Our research provides resources for further research on hLCCLs proteomics. Database URL:  http://www.igenetics.org.cn/project/PSL-LCCL/., (© The Author(s) 2022. Published by Oxford University Press.)

Published

2022

22. Drought-Responsive NAC Transcription Factor RcNAC72 Is Recognized by RcABF4 , Interacts with RcDREB2A to Enhance Drought Tolerance in Arabidopsis.

Author

Jia X, Zeng Z, Lyu Y, and Zhao S

Subjects

Abscisic Acid pharmacology, Arabidopsis drug effects, Arabidopsis genetics, Gene Expression Profiling, Gene Expression Regulation, Plant drug effects, Gene Silencing, Models, Biological, Phenotype, Plant Roots anatomy & histology, Plant Roots drug effects, Plants, Genetically Modified, Promoter Regions, Genetic, Protein Binding drug effects, Seeds drug effects, Seeds growth & development, Stress, Physiological drug effects, Stress, Physiological genetics, Subcellular Fractions metabolism, Adaptation, Physiological, Arabidopsis physiology, Droughts, Plant Proteins metabolism, Rosa metabolism, Transcription Factors metabolism

Abstract

RcNAC72 , a key transcription factor that may respond to drought stress in Rosa chinensis 'Old Blush', was selected in our previous study. In the present study, we found that RcNAC72 is localized in the nucleus and is a transcriptional activator. RcNAC72 expression could be significantly induced by drought, low temperature, salt as well as abscisic acid (ABA) treatment. Analysis of the promoter revealed that multiple abiotic stress and hormone response elements were located in the promoter region. The promoter could respond to drought, low temperature, salt and ABA treatments to activate GUS gene expression. Overexpressing RcNAC72 in Arabidopsis thaliana enhanced sensitivity to ABA and tolerance to drought stress. Silencing of RcNAC72 by virus-induced gene silencing (VIGS) in rose leaves significantly reduced leaf water loss tolerance and leaf extension capacity. Physical interaction of RcNAC72 with RcDREB2A was shown by means of the yeast two-hybrid (Y2H) and bimolecular fluorescence complementation (BiFC) assays. RcABF4 was demonstrated to be able to bind to the promoter of RcNAC72 by means of the yeast one-hybrid (Y1H) assay. These results provide new insights into the regulatory network of RcNAC72 response to drought stress in roses.

Published

2022

23. Non-TZF Transcriptional Activator AtC3H12 Negatively Affects Seed Germination and Seedling Development in Arabidopsis.

Author

Seok HY, Kim T, Lee SY, and Moon YH

Subjects

Amino Acid Sequence, Cell Nucleus metabolism, Gene Expression Regulation, Plant, Models, Biological, Mutation genetics, Promoter Regions, Genetic genetics, Protein Domains, Protein Transport, Protoplasts metabolism, Saccharomyces cerevisiae metabolism, Subcellular Fractions metabolism, Time Factors, Transcriptional Activation genetics, Zinc Fingers, Arabidopsis genetics, Arabidopsis growth & development, Arabidopsis metabolism, Arabidopsis Proteins chemistry, Arabidopsis Proteins genetics, Arabidopsis Proteins metabolism, Germination, Seedlings growth & development, Seedlings metabolism, Seeds growth & development, Seeds metabolism, Trans-Activators chemistry, Trans-Activators metabolism

Abstract

CCCH zinc finger proteins are a large protein family and are classified as either tandem CCCH zinc finger (TZF) or non-TZF proteins. The roles of TZF genes in several plants have been well determined, whereas the functions of many non-TZF genes in plants remain uncharacterized. Herein, we describe biological and molecular functions of AtC3H12, an Arabidopsis non-TZF protein containing three CCCH zinc finger motifs. AtC3H12 has orthologs in several plant species but has no paralog in Arabidopsis. AtC3H12 -overexpressing transgenic plants (OXs) germinated slower than wild-type (WT) plants, whereas atc3h12 mutants germinated faster than WT plants. The fresh weight (FW) and primary root lengths of AtC3H12 OX seedlings were lighter and shorter than those of WT seedlings, respectively. In contrast, FW and primary root lengths of atc3h12 seedlings were heavier and longer than those of WT seedlings, respectively. AtC3H12 was localized in the nucleus and displayed transactivation activity in both yeast and Arabidopsis. We found that the 97-197 aa region of AtC3H12 is an important part for its transactivation activity. Detection of expression levels and analysis of Arabidopsis transgenic plants harboring a P AtC3H12 :: GUS construct showed that AtC3H12 expression increases as the Arabidopsis seedlings develop. Taken together, our results demonstrate that AtC3H12 negatively affects seed germination and seedling development as a nuclear transcriptional activator in Arabidopsis. To our knowledge, this is the first report to show that non-TZF proteins negatively affect plant development as nuclear transcriptional activators.

Published

2022

24. Usher Syndrome Belongs to the Genetic Diseases Associated with Radiosensitivity: Influence of the ATM Protein Kinase.

Author

Al-Choboq J, Ferlazzo ML, Sonzogni L, Granzotto A, El-Nachef L, Maalouf M, Berthel E, and Foray N

Subjects

Cell Survival drug effects, Cell Survival radiation effects, Clone Cells, Diphosphonates pharmacology, Fibroblasts drug effects, Fibroblasts pathology, Fibroblasts radiation effects, Histones metabolism, Humans, Kinetics, MRE11 Homologue Protein metabolism, Micronuclei, Chromosome-Defective radiation effects, Models, Biological, Phosphorylation drug effects, Phosphorylation radiation effects, Radiation Tolerance drug effects, Radiation Tolerance radiation effects, Subcellular Fractions drug effects, Subcellular Fractions metabolism, Subcellular Fractions radiation effects, Ataxia Telangiectasia Mutated Proteins metabolism, Radiation Tolerance genetics, Usher Syndromes enzymology, Usher Syndromes genetics

Abstract

Usher syndrome (USH) is a rare autosomal recessive disease characterized by the combination of hearing loss, visual impairment due to retinitis pigmentosa, and in some cases vestibular dysfunctions. Studies published in the 1980s reported that USH is associated with cellular radiosensitivity. However, the molecular basis of this particular phenotype has not yet been documented. The aim of this study was therefore to document the radiosensitivity of USH1-a subset of USH-by examining the radiation-induced nucleo-shuttling of ATM (RIANS), as well as the functionality of the repair and signaling pathways of the DNA double-strand breaks (DSBs) in three skin fibroblasts derived from USH1 patients. The clonogenic cell survival, the micronuclei, the nuclear foci formed by the phosphorylated forms of the X variant of the H2A histone (ɣH2AX), the phosphorylated forms of the ATM protein (pATM), and the meiotic recombination 11 nuclease (MRE11) were used as cellular and molecular endpoints. The interaction between the ATM and USH1 proteins was also examined by proximity ligation assay. The results showed that USH1 fibroblasts were associated with moderate but significant radiosensitivity, high yield of micronuclei, and impaired DSB recognition but normal DSB repair, likely caused by a delayed RIANS, suggesting a possible sequestration of ATM by some USH1 proteins overexpressed in the cytoplasm. To our knowledge, this report is the first radiobiological characterization of cells from USH1 patients at both molecular and cellular scales.

Published

2022

25. Secondary Structures of Proteins Follow Menzerath-Altmann Law.

Author

Matlach V, Dostál D, and Novotný M

Subjects

Algorithms, Databases, Protein, Protein Structure, Secondary, Statistics as Topic, Subcellular Fractions metabolism, Models, Molecular, Proteins chemistry

Abstract

This article examines the presence of the empirical tendency known as the Menzerath-Altmann Law (MAL) on protein secondary structures. MAL is related to optimization principles observed in natural languages and in genetic information on chromosomes or protein domains. The presence of MAL is examined on a non-redundant dataset of 4728 proteins by verifying significant, negative correlations and testing classical and newly proposed formulas by fitting the observed trend. We conclude that the lengths of secondary structures are specifically dependent on their number inside the protein sequence, while possibly reflecting the formula proposed in this paper. This behavior is observed on average but is individually avoidable and possibly driven by a latent cost function. The data suggest that MAL could provide a useful guiding principle in protein design.

Published

2022

26. Molecular characterization of a novel His333Arg variant of human protoporphyrinogen oxidase IX.

Author

Novakova Z, Mikesova J, Ondrakova M, Kutil Z, Vesela K, Martasek P, and Barinka C

Subjects

Amino Acid Sequence, Biophysical Phenomena, Cell Line, Enzyme Stability, Flavoproteins chemistry, Flavoproteins isolation & purification, Humans, Kinetics, Mitochondrial Proteins chemistry, Mitochondrial Proteins isolation & purification, Models, Molecular, Protein Multimerization, Protoporphyrinogen Oxidase chemistry, Protoporphyrinogen Oxidase isolation & purification, Subcellular Fractions metabolism, Temperature, Flavoproteins genetics, Mitochondrial Proteins genetics, Mutation genetics, Protoporphyrinogen Oxidase genetics

Abstract

Variegate porphyria is caused by mutations in the protoporphyrinogen oxidase IX (PPOX, EC 1.3.3.4) gene, resulting in reduced overall enzymatic activity of PPOX in human tissues. Recently, we have identified the His333Arg mutation in the PPOX protein (PPOX(H333R)) as a putative founder mutation in the Moroccan Jewish population. Herein we report the molecular characterization of PPOX(H333R) in vitro and in cells. Purified recombinant PPOX(H333R) did not show any appreciable enzymatic activity in vitro, corroborating the clinical findings. Biophysical experiments and molecular modeling revealed that PPOX(H333R) is not folded properly and fails to adopt its native functional three-dimensional conformation due to steric clashes in the vicinity of the active site of the enzyme. On the other hand, PPOX(H333R) subcellular distribution, as evaluated by live-cell confocal microscopy, is unimpaired suggesting that the functional three-dimensional fold is not required for efficient transport of the polypeptide chain into mitochondria. Overall, the data presented here provide molecular underpinnings of the pathogenicity of PPOX(H333R) and might serve as a blueprint for deciphering whether a given PPOX variant represents a disease-causing mutation., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper. The authors declare the following financial interests/personal relationships which may be considered as potential competing interests:, (Copyright © 2021 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2022

27. Evolutionary Origin of Insulin-Degrading Enzyme and Its Subcellular Localization and Secretion Mechanism: A Study in Microglial Cells.

Author

Corraliza-Gómez M, Lillo C, Cózar-Castellano I, Arranz E, Sanchez D, and Ganfornina MD

Subjects

Animals, Cell Line, Cells, Cultured, Conserved Sequence, Cytosol metabolism, Extracellular Vesicles metabolism, Insulysin ultrastructure, Membrane Microdomains metabolism, Metalloendopeptidases metabolism, Mice, Inbred C57BL, Mice, Knockout, Microglia ultrastructure, Multivesicular Bodies metabolism, Phylogeny, Subcellular Fractions metabolism, Mice, Evolution, Molecular, Insulysin metabolism, Microglia enzymology

Abstract

The insulin-degrading enzyme (IDE) is a zinc-dependent metalloendopeptidase that belongs to the M16A metalloprotease family. IDE is markedly expressed in the brain, where it is particularly relevant due to its in vitro amyloid beta (Aβ)-degrading activity. The subcellular localization of IDE, a paramount aspect to understand how this enzyme can perform its proteolytic functions in vivo, remains highly controversial. In this work, we addressed IDE subcellular localization from an evolutionary perspective. Phylogenetic analyses based on protein sequence and gene and protein structure were performed. An in silico analysis of IDE signal peptide suggests an evolutionary shift in IDE exportation at the prokaryote/eukaryote divide. Subcellular localization experiments in microglia revealed that IDE is mostly cytosolic. Furthermore, IDE associates to membranes by their cytoplasmatic side and further partitions between raft and non-raft domains. When stimulated, microglia change into a secretory active state, produces numerous multivesicular bodies and IDE associates with their membranes. The subsequent inward budding of such membranes internalizes IDE in intraluminal vesicles, which later allows IDE to be exported outside the cells in small extracellular vesicles. We further demonstrate that such an IDE exportation mechanism is regulated by stimuli relevant for microglia in physiological conditions and upon aging and neurodegeneration.

Published

2022

28. RNALocate v2.0: an updated resource for RNA subcellular localization with increased coverage and annotation.

Author

Cui T, Dou Y, Tan P, Ni Z, Liu T, Wang D, Huang Y, Cai K, Zhao X, Xu D, Lin H, and Wang D

Subjects

Animals, Base Sequence, Cell Compartmentation, Datasets as Topic, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, Eukaryotic Cells cytology, Eukaryotic Cells metabolism, Gene Expression Regulation, Gene Ontology, Humans, Internet, Mice, Molecular Sequence Annotation, RNA, Untranslated classification, RNA, Untranslated metabolism, Rats, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Sequence Alignment, Sequence Homology, Nucleic Acid, Subcellular Fractions chemistry, Subcellular Fractions metabolism, Zebrafish genetics, Zebrafish metabolism, Databases, Nucleic Acid, RNA, Untranslated genetics, Software, Transcriptome

Abstract

Resolving the spatial distribution of the transcriptome at a subcellular level can increase our understanding of biology and diseases. To facilitate studies of biological functions and molecular mechanisms in the transcriptome, we updated RNALocate, a resource for RNA subcellular localization analysis that is freely accessible at http://www.rnalocate.org/ or http://www.rna-society.org/rnalocate/. Compared to RNALocate v1.0, the new features in version 2.0 include (i) expansion of the data sources and the coverage of species; (ii) incorporation and integration of RNA-seq datasets containing information about subcellular localization; (iii) addition and reorganization of RNA information (RNA subcellular localization conditions and descriptive figures for method, RNA homology information, RNA interaction and ncRNA disease information) and (iv) three additional prediction tools: DM3Loc, iLoc-lncRNA and iLoc-mRNA. Overall, RNALocate v2.0 provides a comprehensive RNA subcellular localization resource for researchers to deconvolute the highly complex architecture of the cell., (© The Author(s) 2021. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2022

29. Genome-Wide Identification and Characterization of the RCI2 Gene Family in Allotetraploid Brassica napus Compared with Its Diploid Progenitors.

Author

Sun W, Li M, and Wang J

Subjects

Base Sequence, Chromosomes, Plant genetics, Exons genetics, Gene Duplication genetics, Gene Expression Regulation, Plant, Genes, Plant, Introns genetics, Phylogeny, Plant Proteins genetics, Plant Proteins metabolism, Promoter Regions, Genetic, Subcellular Fractions metabolism, Synteny genetics, Brassica napus genetics, Diploidy, Genome, Plant, Multigene Family, Polyploidy

Abstract

Brassica napus and its diploid progenitors ( B. rapa and B. oleracea ) are suitable for studying the problems associated with polyploidization. As an important anti-stress protein, RCI2 proteins widely exist in various tissues of plants, and are crucial to plant growth, development, and stress response. In this study, the RCI2 gene family was comprehensively identified and analyzed, and 9, 9, and 24 RCI2 genes were identified in B. rapa , B. oleracea , and B. napus , respectively. Phylogenetic analysis showed that all of the identified RCI2 genes were divided into two groups, and further divided into three subgroups. Ka/Ks analysis showed that most of the identified RCI2 genes underwent a purifying selection after the duplication events. Moreover, gene structure analysis showed that the structure of RCI2 genes is largely conserved during polyploidization. The promoters of the RCI2 genes in B. napus contained more cis -acting elements, which were mainly involved in plant development and growth, plant hormone response, and stress responses. Thus, B. napus might have potential advantages in some biological aspects. In addition, the changes of RCI2 genes during polyploidization were also discussed from the aspects of gene number, gene structure, gene relative location, and gene expression, which can provide reference for future polyploidization analysis.

Published

2022

30. Sympathetic Stimulation Upregulates the Ca 2+ Channel Subunit, Ca V α2δ1, via the β1 and ERK 1/2 Pathway in Neonatal Ventricular Cardiomyocytes.

Author

Al Katat A, Zhao J, Calderone A, and Parent L

Subjects

Animals, Animals, Newborn, Calcium metabolism, Hypertrophy, Myocytes, Cardiac drug effects, Norepinephrine pharmacology, Phosphorylation drug effects, Rats, Sprague-Dawley, Subcellular Fractions metabolism, Rats, Calcium Channels, L-Type metabolism, Heart Ventricles cytology, MAP Kinase Signaling System drug effects, Myocytes, Cardiac metabolism, Protein Subunits metabolism, Receptors, Adrenergic, beta-1 metabolism, Sympathetic Nervous System metabolism, Up-Regulation drug effects

Abstract

Intracellular Ca 2+ overload secondary to chronic hemodynamic stimuli promotes the recruitment of Ca 2+ -dependent signaling implicated in cardiomyocyte hypertrophy. The present study tested the hypothesis that sympathetic-mediated hypertrophy of neonatal rat ventricular cardiomyocytes (NRVMs) translated to an increase in calcium influx secondary to the upregulation of Ca V 1.2 channel subunits. Confocal imaging of norepinephrine (NE)-treated NRVMs revealed a hypertrophic response compared to untreated NRVMs. L-type Ca V 1.2 peak current density was increased 4-fold following a 24-h stimulation with NE. NE-treated NRVMs exhibited a significant upregulation of Ca V α2δ1 and Ca V β3 protein levels without significant changes of Ca V α1C and Ca V β2 protein levels. Pre-treatment with the β 1 -blocker metoprolol failed to inhibit hypertrophy or Ca V β3 upregulation whereas Ca V α2δ1 protein levels were significantly reduced. NE promoted the phosphorylation of ERK 1/2, and the response was attenuated by the β 1 -blocker. U0126 pre-treatment suppressed NE-induced ERK1/2 phosphorylation but failed to attenuate hypertrophy. U0126 inhibition of ERK1/2 phosphorylation prevented NE-mediated upregulation of Ca V α2δ1, whereas Ca V β3 protein levels remained elevated. Thus, β 1 -adrenergic receptor-mediated recruitment of the ERK1/2 plays a seminal role in the upregulation of Ca V α2δ1 in NRVMs independent of the concomitant hypertrophic response. However, the upregulation of Ca V β3 protein levels may be directly dependent on the hypertrophic response of NRVMs.

Published

2022

31. Application of RNA subcellular fraction estimation method to explore RNA localization regulation.

Author

Dai X, Li Y, Liu W, Pan X, Guo C, Zhao X, Lv J, Lei H, and Zhang L

Subjects

Protein Isoforms metabolism, Subcellular Fractions metabolism, Biological Phenomena, RNA metabolism

Abstract

RNA localization is involved in multiple biological processes. Recent advances in subcellular fractionation-based sequencing approaches uncovered localization pattern on a global scale. Most of existing methods adopt relative localization ratios (such as ratios of separately normalized transcripts per millions of different subcellular fractions without considering the difference in total RNA abundances in different fractions), however, absolute ratios may yield different results on the preference to different cellular compartment. Experimentally, adding external Spike-in RNAs to different fractionation can be used to obtain absolute ratios. In addition, a spike-in independent computational approach based on multiple linear regression model can also be used. However, currently, no custom tool is available. To solve this problem, we developed a method called subcellular fraction abundance estimator to correctly estimate relative RNA abundances of different subcellular fractionations. The ratios estimated by our method were consistent with existing reports. By applying the estimated ratios for different fractions, we explored the RNA localization pattern in cell lines and also predicted RBP motifs that were associated with different localization patterns. In addition, we showed that different isoforms of same genes could exhibit distinct localization patterns. To conclude, we believed our tool will facilitate future subcellular fractionation-related sequencing study to explore the function of RNA localization in various biological problems., (© The Author(s) 2021. Published by Oxford University Press on behalf of Genetics Society of America.)

Published

2022

32. Subcellular fractionation of brain tumor stem cells.

Author

Sharanek A, Raco L, Soleimani VD, and Jahani-Asl A

Subjects

Animals, Brain metabolism, Cell Fractionation methods, Cell Nucleus metabolism, Mammals metabolism, Proteome metabolism, Subcellular Fractions metabolism, Neoplastic Stem Cells pathology, Proteomics methods

Abstract

Brain tumor stem cells (BTSCs) are a rare population of self-renewing stem cells that are cultured as spheres and are often slow growing compared to other mammalian cell lines. Analysis of BTSC proteome requires careful handling as well as techniques that can be applied to small quantities of cell material. Subcellular fractionation is a widely used technique to assess protein localization. Although proteins are often destined to a defined cell compartment via a signal peptide such as mitochondrial or nuclear localization signals, the recruitment of a protein from one compartment to another can occur as a result of post-translational modification and/or structural variations in response to intracellular and extracellular stimuli. These events assign different functions to a protein making the study of protein localization a useful approach for better understanding of its role in disease progression. Sequential centrifugation remains a simple and versatile fractionation method for proteomic analysis. It can also be applied for diverse downstream applications such as multi-omics using pure nuclear fractions or metabolomic studies on isolated mitochondria. In this chapter, we describe our optimized protocol for subcellular fractionation of BTSC spheres in which we use a commercially available kit with additional centrifugation steps. We provide details on BTSC maintenance and handling, fractionation protocol and evaluation of fraction purity., (Copyright © 2022 Elsevier Inc. All rights reserved.)

Published

2022

33. Overexpression of the Aldehyde Dehydrogenase Gene ZmALDH Confers Aluminum Tolerance in Arabidopsis thaliana .

Author

Du HM, Liu C, Jin XW, Du CF, Yu Y, Luo S, He WZ, and Zhang SZ

Subjects

Adaptation, Physiological drug effects, Aldehyde Dehydrogenase chemistry, Aldehyde Dehydrogenase metabolism, Amino Acid Sequence, Antioxidants metabolism, Arabidopsis drug effects, Ascorbate Peroxidases metabolism, Ascorbic Acid metabolism, Cloning, Molecular, Gene Expression Regulation, Plant drug effects, Glutathione metabolism, Glutathione Reductase metabolism, Hydrogen Peroxide metabolism, Lipid Peroxidation drug effects, Oxidative Stress drug effects, Phylogeny, Plant Leaves drug effects, Plant Leaves metabolism, Plant Roots drug effects, Plant Roots metabolism, Plants, Genetically Modified, Proline metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Subcellular Fractions metabolism, Superoxides metabolism, Nicotiana metabolism, Adaptation, Physiological genetics, Aldehyde Dehydrogenase genetics, Aluminum toxicity, Arabidopsis genetics, Arabidopsis physiology, Genes, Plant, Zea mays genetics

Abstract

Aluminum (Al) toxicity is the main factor limiting plant growth and the yield of cereal crops in acidic soils. Al-induced oxidative stress could lead to the excessive accumulation of reactive oxygen species (ROS) and aldehydes in plants. Aldehyde dehydrogenase ( ALDH ) genes, which play an important role in detoxification of aldehydes when exposed to abiotic stress, have been identified in most species. However, little is known about the function of this gene family in the response to Al stress. Here, we identified an ALDH gene in maize, ZmALDH , involved in protection against Al-induced oxidative stress. Al stress up-regulated ZmALDH expression in both the roots and leaves. The expression of ZmALDH only responded to Al toxicity but not to other stresses including low pH and other metals. The heterologous overexpression of ZmALDH in Arabidopsis increased Al tolerance by promoting the ascorbate-glutathione cycle, increasing the transcript levels of antioxidant enzyme genes as well as the activities of their products, reducing MDA, and increasing free proline synthesis. The overexpression of ZmALDH also reduced Al accumulation in roots. Taken together, these findings suggest that ZmALDH participates in Al-induced oxidative stress and Al accumulation in roots, conferring Al tolerance in transgenic Arabidopsis .

Published

2022

34. Dynamic Distribution of HIG2A between the Mitochondria and the Nucleus in Response to Hypoxia and Oxidative Stress.

Author

Salazar C, Barros M, Elorza AA, and Ruiz LM

Subjects

Animals, Cell Hypoxia, HEK293 Cells, Humans, Mice, Models, Biological, Protein Transport, Subcellular Fractions metabolism, Cell Nucleus metabolism, Membrane Proteins metabolism, Mitochondria metabolism, Mitochondrial Proteins metabolism, Oxidative Stress

Abstract

Mitochondrial respiratory supercomplex formation requires HIG2A protein, which also has been associated with cell proliferation and cell survival under hypoxia. HIG2A protein localizes in mitochondria and nucleus. DNA methylation and mRNA expression of the HIGD2A gene show significant alterations in several cancers, suggesting a role for HIG2A in cancer biology. The present work aims to understand the dynamics of the HIG2A subcellular localization under cellular stress. We found that HIG2A protein levels increase under oxidative stress. H 2 O 2 shifts HIG2A localization to the mitochondria, while rotenone shifts it to the nucleus. HIG2A protein colocalized at a higher level in the nucleus concerning the mitochondrial network under normoxia and hypoxia (2% O 2 ). Hypoxia (2% O 2 ) significantly increases HIG2A nuclear colocalization in C2C12 cells. In HEK293 cells, chemical hypoxia with CoCl 2 (>1% O 2 ) and FCCP mitochondrial uncoupling, the HIG2A protein decreased its nuclear localization and shifted to the mitochondria. This suggests that the HIG2A distribution pattern between the mitochondria and the nucleus depends on stress and cell type. HIG2A protein expression levels increase under cellular stresses such as hypoxia and oxidative stress. Its dynamic distribution between mitochondria and the nucleus in response to stress factors suggests a new communication system between the mitochondria and the nucleus.

Published

2021

35. Introgression of SbERD4 Gene Encodes an Early-Responsive Dehydration-Stress Protein That Confers Tolerance against Different Types of Abiotic Stresses in Transgenic Tobacco.

Author

Jha RK and Mishra A

Subjects

Dehydration, Gene Expression Regulation, Plant, Homeostasis, Ions, Membrane Proteins metabolism, Osmosis, Plant Development genetics, Plants, Genetically Modified, Reactive Oxygen Species metabolism, Subcellular Fractions metabolism, Transformation, Genetic, Adaptation, Physiological genetics, Chenopodiaceae genetics, Heat-Shock Proteins genetics, Plant Proteins genetics, Stress, Physiological genetics, Nicotiana genetics, Nicotiana physiology

Abstract

Salicornia brachiata is an extreme halophyte that commonly grows on marsh conditions and is also considered a promising resource for drought and salt-responsive genes. To unveil a glimpse of stress endurance by plants, it is of the utmost importance to develop an understanding of stress tolerance mechanisms. 'Early Responsive to Dehydration' (ERD) genes are defined as a group of genes involved in stress tolerance and the development of plants. To increase this understanding, parallel to this expedited thought, a novel SbERD4 gene was cloned from S. brachiata , characterized, and functionally validated in the model plant tobacco. The study showed that SbERD4 is a plasma-membrane bound protein, and its overexpression in tobacco plants improved salinity and osmotic stress tolerance. Transgenic plants showed high relative water, chlorophylls, sugars, starch, polyphenols, proline, free amino acids, and low electrolyte leakage and H 2 O 2 content compared to control plants (wild type and vector control) under different abiotic stress conditions. Furthermore, the transcript expression of antioxidant enzyme encoding genes NtCAT , NtSOD , NtGR , and NtAPX showed higher expression in transgenic compared to wild-type and vector controls under varying stress conditions. Overall, the overexpression of a novel early responsive to dehydration stress protein 4-encoding gene ( SbERD4 ) enhanced the tolerance of the plant against multiple abiotic stresses. In conclusion, the overexpression of the SbERD4 gene mitigates plant physiology by enduring stress tolerance and might be considered as a promising key gene for engineering salinity and drought stress tolerance in crops.

Published

2021

36. Mitochondria-Targeted Photoactivatable Real-Time Monitoring of a Controlled Drug Delivery Platform.

Author

Singh N, Gupta A, Prasad P, Sah RK, Singh A, Kumar S, Singh S, Gupta S, and Sasmal PK

Subjects

Antibiotics, Antineoplastic administration & dosage, Antibiotics, Antineoplastic pharmacokinetics, Doxorubicin administration & dosage, Doxorubicin pharmacokinetics, Drug Liberation, HeLa Cells, Humans, Mitochondria metabolism, Subcellular Fractions metabolism, Drug Delivery Systems, Infrared Rays, Mitochondria drug effects, Ultraviolet Rays

Abstract

The current anticancer therapies are limited by their lack of controlled spatiotemporal release at the target site of action. We report a novel drug delivery platform that provides on-demand, real-time, organelle-specific drug release and monitoring upon photoactivation. The system is comprised of a model anticancer drug doxorubicin, an alkyltriphenylphosphonium moiety to target mitochondria in cancer cells, and a hydroxycinnamate photoactivatable linker that is covalently attached to the drug and mitochondria-targeting moieties such that it can be phototriggered by either UV (one-photon) or NIR (two-photon) light to form a fluorescent coumarin product and facilitate the release of drug payload. The extent of drug release is quantified by the fluorescence intensity of the coumarin formed. Further, the photoactivatable prodrug accumulates in the mitochondria and shows light-triggered temporally controlled cell death. In the future, our platform can be tuned for any biological application of interest, offering immense value in biomedicine.

Published

2021

37. Genome-Wide Identification and Characterization of HSP70 Gene Family in Aquilaria sinensis (Lour.) Gilg.

Author

Yu C, Rong M, Liu Y, Sun P, Xu Y, and Wei J

Subjects

Gene Expression Profiling, HSP70 Heat-Shock Proteins classification, Heat-Shock Response, Phylogeny, Subcellular Fractions metabolism, Genes, Plant, HSP70 Heat-Shock Proteins genetics, Thymelaeaceae genetics

Abstract

The heat shock protein 70 ( HSP70 ) gene family perform a fundamental role in protecting plants against biotic and abiotic stresses. Aquilaria sinensis is a classic stress-induced medicinal plant, producing a valuable dark resin in a wood matrix, known as agarwood, in response to environmental stresses. The HSP70 gene family has been systematic identified in many plants, but there is no comprehensive analysis at the genomic level in A. sinensis . In this study, 15 putative HSP70 genes were identified in A. sinensis through genome-wide bioinformatics analysis. Based on their phylogenetic relationships, the 15 AsHSP70 were grouped into six sub-families that with the conserved motifs and gene structures, and the genes were mapped onto six separate linkage groups. A qRT-PCR analysis showed that the relative expression levels of all the AsHSP70 genes were up-regulated by heat stress. Subcellular localization of all HSP70s was predicted, and three were verified by transiently expressed in Arabidopsis protoplasts. Based on the expression profiles in different tissues and different layers treated with Agar-Wit, we predict AsHSP70 genes are involved in different stages of agarwood formation. The systematic identification and expression analysis of HSP70s gene family imply some of them may play important roles in the formation of agarwood. Our findings not only provide a foundation for further study their biological function in the later research in A. sinensis , but also provides a reference for the analysis of HSPs in other species.

Published

2021

38. PHOrming the inflammasome: phosphorylation is a critical switch in inflammasome signalling.

Author

McKee CM, Fischer FA, Bezbradica JS, and Coll RC

Subjects

Animals, Humans, Phosphorylation, Protein Processing, Post-Translational, Subcellular Fractions metabolism, Inflammasomes metabolism, Signal Transduction

Abstract

Inflammasomes are protein complexes in the innate immune system that regulate the production of pro-inflammatory cytokines and inflammatory cell death. Inflammasome activation and subsequent cell death often occur within minutes to an hour, so the pathway must be dynamically controlled to prevent excessive inflammation and the development of inflammatory diseases. Phosphorylation is a fundamental post-translational modification that allows rapid control over protein function and the phosphorylation of inflammasome proteins has emerged as a key regulatory step in inflammasome activation. Phosphorylation of inflammasome sensor and adapter proteins regulates their inter- and intra-molecular interactions, subcellular localisation, and function. The control of inflammasome phosphorylation may thus provide a new strategy for the development of anti-inflammatory therapeutics. Herein we describe the current knowledge of how phosphorylation operates as a critical switch for inflammasome signalling., (© 2021 The Author(s).)

Published

2021

39. Protein Kinase A (PRKA) Activity Is Regulated by the Proteasome at the Onset of Human Sperm Capacitation.

Author

Zapata-Carmona H, Barón L, Kong M, and Morales P

Subjects

A Kinase Anchor Proteins metabolism, Adult, Humans, Phosphorylation drug effects, Proteasome Inhibitors pharmacology, Proteolysis drug effects, Signal Transduction drug effects, Sperm Capacitation drug effects, Subcellular Fractions metabolism, Substrate Specificity drug effects, Young Adult, Cyclic AMP-Dependent Protein Kinases metabolism, Proteasome Endopeptidase Complex metabolism, Sperm Capacitation physiology

Abstract

The proteasome increases its activity at the onset of sperm capacitation due to the action of the SACY/PRKACA pathway; this increase is required for capacitation to progress. PRKA activity also increases and remains high during capacitation. However, intracellular levels of cAMP decrease in this process. Our goal was to evaluate the role of the proteasome in regulating PRKA activity once capacitation has started. Viable human sperm were incubated in the presence and absence of epoxomicin or with 0.1% DMSO. The activity of PRKA; the phosphorylation pattern of PRKA substrates (pPRKAs); and the expression of PRKAR1, PRKAR2, and AKAP3 were evaluated by Western blot. The localization of pPRKAs, PRKAR1, PRKAR2, and AKAP3 was evaluated by immunofluorescence. Treatment with epoxomicin changed the localization and phosphorylation pattern and decreased the percentage of pPRKAs-positive sperm. PRKA activity significantly increased at 1 min of capacitation and remained high throughout the incubation. However, epoxomicin treatment significantly decreased PRKA activity after 30 min. In addition, PRKAR1 and AKAP3 were degraded by the proteasome but with a different temporal kinetic. Our results suggest that PRKAR1 is the target of PRKA regulation by the proteasome.

Published

2021

40. Spatial-proteomics reveals phospho-signaling dynamics at subcellular resolution.

Author

Martinez-Val A, Bekker-Jensen DB, Steigerwald S, Koenig C, Østergaard O, Mehta A, Tran T, Sikorski K, Torres-Vega E, Kwasniewicz E, Brynjólfsdóttir SH, Frankel LB, Kjøbsted R, Krogh N, Lundby A, Bekker-Jensen S, Lund-Johansen F, and Olsen JV

Subjects

Animals, Biological Phenomena, Cell Fractionation, HeLa Cells, Humans, Male, Mass Spectrometry, Mice, Mice, Inbred C57BL, Osmotic Pressure, Phosphorylation, Subcellular Fractions metabolism, Workflow, Proteome metabolism, Proteomics, Signal Transduction

Abstract

Dynamic change in subcellular localization of signaling proteins is a general concept that eukaryotic cells evolved for eliciting a coordinated response to stimuli. Mass spectrometry-based proteomics in combination with subcellular fractionation can provide comprehensive maps of spatio-temporal regulation of protein networks in cells, but involves laborious workflows that does not cover the phospho-proteome level. Here we present a high-throughput workflow based on sequential cell fractionation to profile the global proteome and phospho-proteome dynamics across six distinct subcellular fractions. We benchmark the workflow by studying spatio-temporal EGFR phospho-signaling dynamics in vitro in HeLa cells and in vivo in mouse tissues. Finally, we investigate the spatio-temporal stress signaling, revealing cellular relocation of ribosomal proteins in response to hypertonicity and muscle contraction. Proteomics data generated in this study can be explored through https://SpatialProteoDynamics.github.io ., (© 2021. The Author(s).)

Published

2021

41. Construction of lncRNA-related ceRNA regulatory network in diabetic subdermal endothelial cells.

Author

Wan J and Liu B

Subjects

Gene Expression Profiling, Gene Expression Regulation, Humans, RNA, Long Noncoding metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Subcellular Fractions metabolism, Dermis pathology, Diabetes Mellitus genetics, Diabetes Mellitus pathology, Endothelial Cells metabolism, Gene Regulatory Networks, RNA, Long Noncoding genetics

Abstract

Long non-coding RNAs (lncRNAs) were considered to be involved in vascular complications in diabetes mellitus, but still only limited knowledge in this regard has been obtained. Herein, we further explored the roles of lncRNAs and mRNAs in diabetic vasculopathy (DV) through conducting bioinformatics analysis using data set downloaded from GEO database. The differentially expressed lncRNAs and mRNAs were identified by edge package. GO enrichment analysis and KEGG pathway analysis were performed based on clusterprofiler package. The relationship between lncRNA and miRNA was predicted using starBase database, and the potential mRNAs targeted by miRNAs were predicted by TargetScan, miRTarbase and miRDB database. The string database was used to analyze the protein-protein interaction (PPI). As a result, a total of 12 lncRNAs and 711 mRNAs were found to be differentially expressed in the diabetic subdermal endothelial cells compared with normal controls. A ceRNA network was established, which was composed of seven lncRNA nodes, 49 miRNA nodes, 58 mRNA nodes and 183 edges, and MSC-AS1 and LINC01550 may serve as key nodes. GO function enrichment analysis showed enrichments of epithelial cell proliferation, intercellular junction, and cell adhesion molecule binding. KEGG pathway analysis revealed 33 enriched pathways. PPI protein interaction analysis identified 57 potential ceRNA-related proteins. Overall, this study suggests that multiple lncRNAs, specifically MSC-AS1 and LINC01550, may play an important role in DV development and they are like to be developed as the therapeutic targets for DV. However, further experiments in vitro and in vivo should be conducted to validate our results.

Published

2021

42. Physicochemical and structural characterization, epitope mapping and vaccine potential investigation of a new protein containing Tetratrico Peptide Repeats of Acinetobacter baumannii: An in-silico and in-vivo approach.

Author

Abdollahi S, Raoufi Z, and Fakoor MH

Subjects

Amino Acid Sequence, Animals, Antigens, Bacterial immunology, Epitopes, B-Lymphocyte immunology, Epitopes, T-Lymphocyte immunology, Mice, Inbred BALB C, Models, Molecular, Peptides chemistry, Peptides immunology, Protein Domains, Protein Structure, Secondary, Sequence Homology, Amino Acid, Subcellular Fractions metabolism, Survival Analysis, Virulence, Mice, Acinetobacter baumannii immunology, Bacterial Proteins chemistry, Bacterial Proteins immunology, Bacterial Vaccines immunology, Chemical Phenomena, Computer Simulation, Epitope Mapping, Tetratricopeptide Repeat

Abstract

Acinetobacter baumannii is an opportunistic multidrug-resistant pathogen that causes a significant mortality rate. The proteins containing Tetratrico Peptide Repeats (TPRs) are involved in the pathogenicity and virulence of bacteria and have different roles such as transfer of bacterial virulence factors to host cells, binding to the host cells and inhibition of phagolysosomal maturation. So, in this study, physicochemical properties of a new protein containing TPRs in A. baumannii which was named PcTPRs1 by this study were characterized and its 3D structure was predicted by in-silico tools. The protein B and T cell epitopes were mapped and its vaccine potential was in-silico and in-vivo investigated. Domain analysis indicated that the protein contains the Flp pilus assembly protein TadD domain which has three TPRs. The helix is dominant in the protein structure, and this protein is an outer membrane antigen which, is extremely conserved among A. baumannii strains; thus, has good properties to be applied as a recombinant vaccine. The best-predicted and refined model was applied in ligand-binding sites and conformational epitopes prediction. Based on epitope mapping results, several epitopes were characterized which could stimulate both immune systems. BLAST results showed the introduced epitopes are completely conserved among A. baumannii strains. The in-vivo analysis indicates that a 101 amino acid fragment of the protein which contains the best selected epitope, can produce a good protectivity against A. baumannii as well as the whole TPR protein and thus could be investigated as an effective subunit and potential vaccines., (Copyright © 2021 Elsevier Ltd. All rights reserved.)

Published

2021

43. Label-free multiplexed microtomography of endogenous subcellular dynamics using generalizable deep learning.

Author

Jo Y, Cho H, Park WS, Kim G, Ryu D, Kim YS, Lee M, Park S, Lee MJ, Joo H, Jo H, Lee S, Lee S, Min HS, Heo WD, and Park Y

Subjects

3T3 Cells, Actins metabolism, Animals, COS Cells, Cell Line, Tumor, Cell Membrane metabolism, Cell Nucleolus metabolism, Cell Nucleus metabolism, Chlorocebus aethiops, HEK293 Cells, HeLa Cells, Humans, Lipid Droplets metabolism, Mice, Mitochondria metabolism, Optical Imaging methods, Refractometry, Deep Learning, Electron Microscope Tomography methods, Imaging, Three-Dimensional methods, Single-Cell Analysis methods, Subcellular Fractions metabolism

Abstract

Simultaneous imaging of various facets of intact biological systems across multiple spatiotemporal scales is a long-standing goal in biology and medicine, for which progress is hindered by limits of conventional imaging modalities. Here we propose using the refractive index (RI), an intrinsic quantity governing light-matter interaction, as a means for such measurement. We show that major endogenous subcellular structures, which are conventionally accessed via exogenous fluorescence labelling, are encoded in three-dimensional (3D) RI tomograms. We decode this information in a data-driven manner, with a deep learning-based model that infers multiple 3D fluorescence tomograms from RI measurements of the corresponding subcellular targets, thereby achieving multiplexed microtomography. This approach, called RI2FL for refractive index to fluorescence, inherits the advantages of both high-specificity fluorescence imaging and label-free RI imaging. Importantly, full 3D modelling of absolute and unbiased RI improves generalization, such that the approach is applicable to a broad range of new samples without retraining to facilitate immediate applicability. The performance, reliability and scalability of this technology are extensively characterized, and its various applications within single-cell profiling at unprecedented scales (which can generate new experimentally testable hypotheses) are demonstrated., (© 2021. The Author(s), under exclusive licence to Springer Nature Limited.)

Published

2021

44. Compartment-specific metabolome labeling enables the identification of subcellular fluxes that may serve as promising metabolic engineering targets in CHO cells.

Author

Wijaya AW, Ulmer A, Hundsdorfer L, Verhagen N, Teleki A, and Takors R

Subjects

Animals, CHO Cells, Cricetulus, Metabolic Engineering, Metabolome, Subcellular Fractions metabolism

Abstract

13 C labeling data are used to calculate quantitative intracellular flux patterns reflecting in vivo conditions. Given that approaches for compartment-specific metabolomics exist, the benefits they offer compared to conventional non-compartmented 13 C flux studies remain to be determined. Using compartment-specific labeling information of IgG1-producing Chinese hamster ovary cells, this study investigated differences of flux patterns exploiting and ignoring metabolic labeling data of cytosol and mitochondria. Although cellular analysis provided good estimates for the majority of intracellular fluxes, half of the mitochondrial transporters, and NADH and ATP balances, severe differences were found for some reactions. Accurate flux estimations of almost all iso-enzymes heavily depended on the sub-cellular labeling information. Furthermore, key discrepancies were found for the mitochondrial carriers v AGC1 (Aspartate/Glutamate antiporter), v DIC (Malate/H + symporter), and v OGC (α-ketoglutarate/malate antiporter). Special emphasis is given to the flux of cytosolic malic enzyme (v ME ): it could not be estimated without the compartment-specific malate labeling information. Interesting enough, cytosolic malic enzyme is an important metabolic engineering target for improving cell-specific IgG1 productivity. Hence, compartment-specific 13 C labeling analysis serves as prerequisite for related metabolic engineering studies., (© 2021. The Author(s).)

Published

2021

45. Hsa-circ&#95;0058106 induces EMT and metastasis in laryngeal cancer via sponging miR-153 and inducing Twist1 nuclear translocation.

Author

Zhang X, Wu N, and Wang J

Subjects

Animals, Base Sequence, Cell Line, Tumor, Cell Movement genetics, Down-Regulation genetics, Gene Expression Regulation, Neoplastic, Gene Silencing, Humans, Laryngeal Neoplasms pathology, Male, Mice, Inbred BALB C, Mice, Nude, MicroRNAs genetics, Models, Biological, Neoplasm Invasiveness, Neoplasm Metastasis, Protein Transport, RNA, Circular genetics, Snail Family Transcription Factors metabolism, Subcellular Fractions metabolism, Up-Regulation genetics, Mice, Cell Nucleus metabolism, Epithelial-Mesenchymal Transition genetics, Laryngeal Neoplasms genetics, MicroRNAs metabolism, Nuclear Proteins metabolism, RNA, Circular metabolism, Twist-Related Protein 1 metabolism

Abstract

Purpose: A new circular RNA (hsa-circ&#95;0058106) has been found to be upregulated in laryngeal cancer, but its function remains unknown. Here, we explored its role in the metastasis of laryngeal cancer., Methods: The level of hsa-circ&#95;0058106 in laryngeal cancer was detected by qRT-PCR. The effect of hsa-circ&#95;0058106 silencing on the metastasis of laryngeal cancer was assessed using scratch wound healing and transwell assays, as well as nude mouse lung metastasis models. Fluorescence in situ hybridization was employed to analyze the cellular localization of hsa-circ&#95;0058106. A luciferase activity assay was used to assess binding between hsa-circ&#95;0058106 and miR-153. Interaction between hsa-circ&#95;0058106 and Twist1 was confirmed using RNA pull-down and RNA immunoprecipitation assays., Results: A high level of hsa-circ&#95;0058106 was found to be associated with lymph node metastasis and advanced clinical stages. Stable knockdown of hsa-circ&#95;0058106 inhibited the migration and invasion of laryngeal cancer cells in vitro and in vivo. Moreover, we found that downregulation of hsa-circ&#95;0058106 suppressed epithelial-mesenchymal transition (EMT), which was underscored by the observation that hsa-circ&#95;0058106 silencing led to decreases in the expression of N-cadherin and Vimentin, and an increase in the expression of E-cadherin. Mechanistically, we found that hsa-circ&#95;0058106 can specifically bind to miR-153 and regulate Snail1 expression by acting as a miR-153 sponge. In addition, we found that knockdown of hsa-circ&#95;0058106 blocked the nuclear translocation of Twist1., Conclusions: Our results indicate that hsa-circ&#95;0058106 induces EMT and metastasis in laryngeal cancer by sponging miR-153 and inducing Twist1 nuclear translocation. These observations provide new insights into the regulatory effects of circRNAs in laryngeal cancer metastasis., (© 2021. Springer Nature Switzerland AG.)

Published

2021

46. Inactivity of Peptidase ClpP Causes Primary Accumulation of Mitochondrial Disaggregase ClpX with Its Interacting Nucleoid Proteins, and of mtDNA.

Author

Key J, Torres-Odio S, Bach NC, Gispert S, Koepf G, Reichlmeir M, West AP, Prokisch H, Freisinger P, Newman WG, Shalev S, Sieber SA, Wittig I, and Auburger G

Subjects

Adult, Amino Acids metabolism, Brain metabolism, Computational Biology, Conserved Sequence, Fibroblasts metabolism, Humans, Male, Mitochondrial Proteins metabolism, Models, Biological, Protein Binding, Protein Interaction Maps, Proteome metabolism, Skin pathology, Subcellular Fractions metabolism, Transcription, Genetic, Cell Nucleus metabolism, DNA, Mitochondrial metabolism, Endopeptidase Clp metabolism, Mitochondria metabolism

Abstract

Biallelic pathogenic variants in CLPP , encoding mitochondrial matrix peptidase ClpP, cause a rare autosomal recessive condition, Perrault syndrome type 3 (PRLTS3). It is characterized by primary ovarian insufficiency and early sensorineural hearing loss, often associated with progressive neurological deficits. Mouse models showed that accumulations of (i) its main protein interactor, the substrate-selecting AAA+ ATPase ClpX, (ii) mitoribosomes, and (iii) mtDNA nucleoids are the main cellular consequences of ClpP absence. However, the sequence of these events and their validity in human remain unclear. Here, we studied global proteome profiles to define ClpP substrates among mitochondrial ClpX interactors, which accumulated consistently in ClpP-null mouse embryonal fibroblasts and brains. Validation work included novel ClpP-mutant patient fibroblast proteomics. ClpX co-accumulated in mitochondria with the nucleoid component POLDIP2, the mitochondrial poly(A) mRNA granule element LRPPRC, and tRNA processing factor GFM1 (in mouse, also GRSF1). Only in mouse did accumulated ClpX, GFM1, and GRSF1 appear in nuclear fractions. Mitoribosomal accumulation was minor. Consistent accumulations in murine and human fibroblasts also affected multimerizing factors not known as ClpX interactors, namely, OAT, ASS1, ACADVL, STOM, PRDX3, PC, MUT, ALDH2, PMPCB, UQCRC2, and ACADSB, but the impact on downstream metabolites was marginal. Our data demonstrate the primary impact of ClpXP on the assembly of proteins with nucleic acids and show nucleoid enlargement in human as a key consequence.

Published

2021

47. Transmission Electron Microscopy as a Powerful Tool to Investigate the Interaction of Nanoparticles with Subcellular Structures.

Author

Malatesta M

Subjects

Animals, Humans, Nanoparticles chemistry, Subcellular Fractions chemistry, Tissue Distribution, Microscopy, Electron, Transmission methods, Nanomedicine methods, Nanoparticles metabolism, Subcellular Fractions metabolism

Abstract

Nanomedical research necessarily involves the study of the interactions between nanoparticulates and the biological environment. Transmission electron microscopy has proven to be a powerful tool in providing information about nanoparticle uptake, biodistribution and relationships with cell and tissue components, thanks to its high resolution. This article aims to overview the transmission electron microscopy techniques used to explore the impact of nanoconstructs on biological systems, highlighting the functional value of ultrastructural morphology, histochemistry and microanalysis as well as their fundamental contribution to the advancement of nanomedicine.

Published

2021

48. Nuclear dengue virus NS5 antagonizes expression of PAF1-dependent immune response genes.

Author

Petit MJ, Kenaston MW, Pham OH, Nagainis AA, Fishburn AT, and Shah PS

Subjects

A549 Cells, CRISPR-Cas Systems, Dengue genetics, Dengue metabolism, Dengue Virus physiology, Humans, RNA-Seq, STAT2 Transcription Factor antagonists & inhibitors, STAT2 Transcription Factor genetics, Transcription Factors antagonists & inhibitors, Transcription Factors genetics, Viral Nonstructural Proteins genetics, Dengue virology, Mutation, Protein Interaction Domains and Motifs, STAT2 Transcription Factor metabolism, Subcellular Fractions metabolism, Transcription Factors metabolism, Viral Nonstructural Proteins metabolism

Abstract

Dengue virus (DENV) disruption of the innate immune response is critical to establish infection. DENV non-structural protein 5 (NS5) plays a central role in this disruption, such as antagonism of STAT2. We recently found that DENV serotype 2 (DENV2) NS5 interacts with Polymerase associated factor 1 complex (PAF1C). The primary members of PAF1C are PAF1, LEO1, CTR9, and CDC73. This nuclear complex is an emerging player in the immune response. It promotes the expression of many genes, including genes related to the antiviral, antimicrobial and inflammatory responses, through close association with the chromatin of these genes. Our previous work demonstrated that NS5 antagonizes PAF1C recruitment to immune response genes. However, it remains unknown if NS5 antagonism of PAF1C is complementary to its antagonism of STAT2. Here, we show that knockout of PAF1 enhances DENV2 infectious virion production. By comparing gene expression profiles in PAF1 and STAT2 knockout cells, we find that PAF1 is necessary to express immune response genes that are STAT2-independent. Finally, we mapped the viral determinants for the NS5-PAF1C protein interaction. We found that NS5 nuclear localization and the C-terminal region of the methyltransferase domain are required for its interaction with PAF1C. Mutation of these regions rescued the expression of PAF1-dependent immune response genes that are antagonized by NS5. In sum, our results support a role for PAF1C in restricting DENV2 replication that NS5 antagonizes through its protein interaction with PAF1C., Competing Interests: The authors have declared that no competing interests exist.

Published

2021

49. Blue Light Activated Rapamycin for Optical Control of Protein Dimerization in Cells and Zebrafish Embryos.

Author

Courtney TM, Darrah KE, Horst TJ, Tsang M, and Deiters A

Subjects

Animals, Dimerization, Embryo, Nonmammalian metabolism, Green Fluorescent Proteins metabolism, HeLa Cells, Humans, Sirolimus radiation effects, Subcellular Fractions metabolism, Light, Proteins metabolism, Sirolimus analogs & derivatives, Zebrafish embryology

Abstract

Rapamycin-induced dimerization of FKBP and FRB is the most commonly utilized chemically induced protein dimerization system. It has been extensively used to conditionally control protein localization, split-enzyme activity, and protein-protein interactions in general by simply fusing FKBP and FRB to proteins of interest. We have developed a new aminonitrobiphenylethyl caging group and applied it to the generation of a caged rapamycin analog that can be photoactivated using blue light. Importantly, the caged rapamycin analog shows minimal background activity with regard to protein dimerization and can be directly interfaced with a wide range of established (and often commercially available) FKBP/FRB systems. We have successfully demonstrated its applicability to the optical control of enzymatic function, protein stability, and protein subcellular localization. Further, we also showcased its applicability toward optical regulation of cell signaling, specifically mTOR signaling, in cells and aquatic embryos.

Published

2021

50. Zn 2+ -Dependent Nuclease Is Involved in Nuclear Degradation during the Programmed Cell Death of Secretory Cavity Formation in Citrus grandis 'Tomentosa' Fruits.

Author

Liang M, Bai M, and Wu H

Subjects

Cell Nucleus ultrastructure, Citrus genetics, Citrus ultrastructure, DNA Fragmentation, Deoxyribonucleases metabolism, Fruit ultrastructure, Gene Expression Regulation, Plant, Models, Biological, Subcellular Fractions metabolism, Apoptosis, Cell Nucleus metabolism, Citrus cytology, Endonucleases metabolism, Fruit cytology, Plant Proteins metabolism, Zinc metabolism

Abstract

Zn2+- and Ca2+-dependent nucleases exhibit activity toward dsDNA in the four classes of cation-dependent nucleases in plants. Programmed cell death (PCD) is involved in the degradation of cells during schizolysigenous secretory cavity formation in Citrus fruits. Recently, the Ca2+-dependent DNase CgCAN was proven to play a key role in nuclear DNA degradation during the PCD of secretory cavity formation in Citrus grandis ‘Tomentosa’ fruits. However, whether Zn2+-dependent nuclease plays a role in the PCD of secretory cells remains poorly understood. Here, we identified a Zn2+-dependent nuclease gene, CgENDO1, from Citrus grandis ‘Tomentosa’, the function of which was studied using Zn2+ ions cytochemical localization, DNase activity assays, in situ hybridization, and protein immunolocalization. The full-length cDNA of CgENDO1 contains an open reading frame of 906 bp that encodes a protein 301 amino acids in length with a S1/P1-like functional domain. CgENDO1 degrades linear double-stranded DNA at acidic and neutral pH. CgENDO1 is mainly expressed in the late stage of nuclear degradation of secretory cells. Further spatiotemporal expression patterns of CgENDO1 showed that CgENDO1 is initially located on the endoplasmic reticulum and then moves into intracellular vesicles and nuclei. During the late stage of nuclear degradation, it was concentrated in the area of nuclear degradation involved in nuclear DNA degradation. Our results suggest that the Zn2+-dependent nuclease CgENDO1 plays a direct role in the late degradation stage of the nuclear DNA in the PCD of secretory cavity cells of Citrus grandis ‘Tomentosa’ fruits.

Published

2021