Your search keyword '"Tetraspanin 30"' showing total 1,742 results

1. Aberrant TIMP-1 overexpression in tumor-associated fibroblasts drives tumor progression through CD63 in lung adenocarcinoma.

Author

Duch, Paula, Díaz-Valdivia, Natalia, Ikemori, Rafael, Gabasa, Marta, Radisky, Evette, Arshakyan, Marselina, Gea-Sorlí, Sabrina, Mateu-Bosch, Anna, Bragado, Paloma, Carrasco, Josep, Mori, Hidetoshi, Ramírez, Josep, Teixidó, Cristina, Reguart, Noemí, Fillat, Cristina, Radisky, Derek, and Alcaraz, Jordi

Subjects

CD63, Cancer-associated fibroblast, Fibrosis, SMAD3, TGF-β1, TIMP-1, Tumor microenvironment, Adenocarcinoma of Lung, Animals, Cancer-Associated Fibroblasts, Carcinoma, Squamous Cell, Fibroblasts, Humans, Lung Neoplasms, Mice, Tetraspanin 30, Tissue Inhibitor of Metalloproteinase-1, Transforming Growth Factor beta1, Tumor Microenvironment

Abstract

Tissue inhibitor of metalloproteinase-1 (TIMP-1) is an important regulator of extracellular matrix turnover that has been traditionally regarded as a potential tumor suppressor owing to its inhibitory effects of matrix metalloproteinases. Intriguingly, this interpretation has been challenged by the consistent observation that increased expression of TIMP-1 is associated with poor prognosis in virtually all cancer types including lung cancer, supporting a tumor-promoting function. However, how TIMP-1 is dysregulated within the tumor microenvironment and how it drives tumor progression in lung cancer is poorly understood. We analyzed the expression of TIMP-1 and its cell surface receptor CD63 in two major lung cancer subtypes: lung adenocarcinoma (ADC) and squamous cell carcinoma (SCC), and defined the tumor-promoting effects of their interaction. We found that TIMP-1 is aberrantly overexpressed in tumor-associated fibroblasts (TAFs) in ADC compared to SCC. Mechanistically, TIMP-1 overexpression was mediated by the selective hyperactivity of the pro-fibrotic TGF-β1/SMAD3 pathway in ADC-TAFs. Likewise, CD63 was upregulated in ADC compared to SCC cells. Genetic analyses revealed that TIMP-1 secreted by TGF-β1-activated ADC-TAFs is both necessary and sufficient to enhance growth and invasion of ADC cancer cells in culture, and that tumor cell expression of CD63 was required for these effects. Consistently, in vivo analyses revealed that ADC cells co-injected with fibroblasts with reduced SMAD3 or TIMP-1 expression into immunocompromised mice attenuated tumor aggressiveness compared to tumors bearing parental fibroblasts. We also found that high TIMP1 and CD63 mRNA levels combined define a stronger prognostic biomarker than TIMP1 alone. Our results identify an excessive stromal TIMP-1 within the tumor microenvironment selectively in lung ADC, and implicate it in a novel tumor-promoting TAF-carcinoma crosstalk, thereby pointing to TIMP-1/CD63 interaction as a novel therapeutic target in lung cancer.

Published

2022

2. Protein analysis of extracellular vesicles to monitor and predict therapeutic response in metastatic breast cancer.

Author

Tian, Fei, Zhang, Shaohua, Liu, Chao, Han, Ziwei, Liu, Yuan, Deng, Jinqi, Li, Yike, Wu, Xia, Cai, Lili, Qin, Lili, Chen, Qinghua, Yuan, Yang, Liu, Yi, Cong, Yulong, Ding, Baoquan, Jiang, Zefei, and Sun, Jiashu

Subjects

Biomarkers, Tumor, Breast Neoplasms, Cell Line, Tumor, Extracellular Vesicles, Female, Humans, Platelet Membrane Glycoprotein IIb, Prospective Studies, Survival Rate, Tetraspanin 30

Abstract

Molecular profiling of circulating extracellular vesicles (EVs) provides a promising noninvasive means to diagnose, monitor, and predict the course of metastatic breast cancer (MBC). However, the analysis of EV protein markers has been confounded by the presence of soluble protein counterparts in peripheral blood. Here we use a rapid, sensitive, and low-cost thermophoretic aptasensor (TAS) to profile cancer-associated protein profiles of plasma EVs without the interference of soluble proteins. We show that the EV signature (a weighted sum of eight EV protein markers) has a high accuracy (91.1 %) for discrimination of MBC, non-metastatic breast cancer (NMBC), and healthy donors (HD). For MBC patients undergoing therapies, the EV signature can accurately monitor the treatment response across the training, validation, and prospective cohorts, and serve as an independent prognostic factor for progression free survival in MBC patients. Together, this work highlights the potential clinical utility of EVs in management of MBC.

Published

2021

3. Sequential deletion of CD63 identifies topologically distinct scaffolds for surface engineering of exosomes in living human cells

Author

Curley, Natalie, Levy, Daniel, Do, Mai Anh, Brown, Annie, Stickney, Zachary, Marriott, Gerard, and Lu, Biao

Subjects

Biotechnology, Nanotechnology, Bioengineering, 5.2 Cellular and gene therapies, Development of treatments and therapeutic interventions, Generic health relevance, Exosomes, Extracellular Vesicles, HEK293 Cells, Humans, Protein Transport, Proteins, Tetraspanin 30, Physical Sciences, Chemical Sciences, Technology, Nanoscience & Nanotechnology

Abstract

Exosomes are cell-derived extracellular vesicles that have great potential in the field of nano-medicine. However, a fundamental challenge in the engineering of exosomes is the design of biocompatible molecular scaffolds on their surface to enable cell targeting and therapeutic functions. CD63 is a hallmark protein of natural exosomes that is highly enriched on the external surface of the membrane. We have previously described engineering of CD63 for use as a molecular scaffold in order to introduce cell-targeting features to the exosome surface. Despite this initial success, the restrictive M-shaped topology of full-length CD63 may hinder specific applications that require N- or C-terminal display of cell-targeting moieties on the outer surface of the exosome. In this study, we describe new and topologically distinct CD63 scaffolds that enable robust and flexible surface engineering of exosomes. In particular, we conducted sequential deletions of the transmembrane helix of CD63 to generate a series of CD63 truncates, each genetically-fused to a fluorescent protein. Molecular and cellular characterization studies showed truncates of CD63 harboring the transmembrane helix 3 (TM3) correctly targeted and anchored to the exosome membrane and exhibited distinct n-, N-, Ω-, or I-shaped membrane topologies in the exosomal membrane. We further established that these truncates retained robust membrane-anchoring and exosome-targeting activities when stably expressed in the HEK293 cells. Moreover, HEK293 cells produced engineered exosomes in similar quantities to cells expressing full-length CD63. Based on the results of our systematic sequential deletion studies, we propose a model to understand molecular mechanisms that underlie membrane-anchoring and exosome targeting features of CD63. In summary, we have established new and topologically distinct scaffolds based on engineering of CD63 that enables flexible engineering of the exosome surface for applications in disease-targeted drug delivery and therapy.

Published

2020

4. A cavity induced mode hybridization plasmonic sensor for portable detection of exosomes.

Author

Luo X, Yan S, Chen G, Wang Y, Zhang X, Lan J, Chen J, and Yao X

Subjects

Humans, Aptamers, Nucleotide chemistry, Epithelial Cell Adhesion Molecule, Tetraspanin 30, Hep G2 Cells, Biosensing Techniques methods, Biosensing Techniques instrumentation, Reproducibility of Results, Equipment Design, Nanospheres chemistry, Nucleic Acid Hybridization, Biomarkers, Tumor blood, Biomarkers, Tumor analysis, Exosomes chemistry, Surface Plasmon Resonance, Gold chemistry, Limit of Detection, Silicon Dioxide chemistry

Abstract

Exosomes have been considered as promising biomarkers for cancer diagnosis due to their abundant information from originating cells. However, sensitive and reliable detection of exosomes is still facing technically challenges due to the lack of a sensing platform with high sensitivity and reproducibility. To address the challenges, here we propose a portable surface plasmon resonance (SPR) sensing of exosomes with a three-layer Au mirror/SiO 2 spacer/Au nanohole sensor, fabricated by an economical polystyrene nanosphere self-assembly method. The SiO 2 spacer can act as an optical cavity and induce mode hybridization, leading to excellent optimization of both sensitivity and full width at half maximum compared with normal single layer Au nanohole sensors. When modified with CD63 or EpCAM aptamers, a detection of limit (LOD) of as low as 600 particles/μL was achieved. The sensors showed good capability to distinguish between non-tumor derived L02 exosomes and tumor derived HepG2 exosomes. Additionally, high reproducibility was also achieved in detection of artificial serum samples with RSD as low as 2%, making it feasible for clinical applications. This mode hybridization plasmonic sensor provides an effective approach to optimize the detection sensitivity of exosomes, pushing SPR sensing one step further towards cancer diagnosis., 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., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

5. CRISPR/Cas12a and aptamer-chemiluminescence based analysis for the relative abundance determination of tumor-related protein positive exosomes for breast cancer diagnosis.

Author

Guan X, Zhao J, Sha Z, Liang Y, Huang J, Zhang J, and Sun S

Subjects

Humans, Female, Luminescent Measurements methods, Tetraspanin 30, Limit of Detection, Breast Neoplasms diagnosis, Breast Neoplasms blood, Breast Neoplasms genetics, Exosomes chemistry, Exosomes genetics, Aptamers, Nucleotide chemistry, Biosensing Techniques methods, Mucin-1 blood, Mucin-1 genetics, Mucin-1 analysis, Biomarkers, Tumor blood, Biomarkers, Tumor genetics, Epithelial Cell Adhesion Molecule genetics, CRISPR-Cas Systems

Abstract

Exosomes, as novel biomarker for liquid biopsy, exhibit huge important potential value for cancer diagnosis. However, various proteins show different expression levels on exosomal membrane, and the absolute concentration of exosomes in clinical samples is easily influenced by a number of factors. Here, we developed a CRISPR/Cas12a and aptamer-chemiluminescence based analysis (CACBA) for the relative abundance determination of tumor-related protein positive exosomes in plasma for breast cancer diagnosis. The total concentration of exosomes was determined through captured CD63 using a CRISPR/Cas12a-based method with the LoD of 8.97 × 10 3 particles/μl. Meanwhile, EpCAM and MUC1 positive exosomes were quantitatively detected by aptamer-chemiluminescence (ACL) based method with the LoD of 1.45 × 10 2 and 3.73 × 10 2 particles/μl, respectively. It showed that the percentages of EpCAM and MUC1 positive exosomes offered an excellent capability to differentiate breast cancer patients and healthy donors. The high sensitivity, strong specificity, outstanding anti-interference capability, and steady recovery rate of this approach offered higher accuracy and robustness than the commercialized method in clinical trial. In addition with good stability, easy preparation and low cost, this method not only provides a new approach to rapid analysis of exosome proteins, it may be quickly extended to the diagnoses of various cancers., 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., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

6. Blocking Allergic Reaction through Targeting Surface-Bound IgE with Low-Affinity Anti-IgE Antibodies

Author

Zhang, Ke, Liu, Jeffrey, Truong, Thao, Zukin, Elyssa, Chen, Wendy, and Saxon, Andrew

Subjects

Biomedical and Clinical Sciences, Immunology, Food Allergies, Rare Diseases, Biotechnology, 2.1 Biological and endogenous factors, 5.1 Pharmaceuticals, Development of treatments and therapeutic interventions, Aetiology, Inflammatory and immune system, Anaphylaxis, Animals, Antibodies, Anti-Idiotypic, Antibodies, Monoclonal, Antibody Affinity, Basophils, Cell Degranulation, Cytokines, Humans, Hypersensitivity, Immunoglobulin E, Mice, Mice, Transgenic, Passive Cutaneous Anaphylaxis, Phosphoric Diester Hydrolases, Protein Binding, Pyrophosphatases, Tetraspanin 30, Biochemistry and cell biology

Abstract

Allergic disorders have now become a major worldwide public health issue, but the effective treatment options remain limited. We report a novel approach to block allergic reactivity by targeting the surface-bound IgE of the allergic effector cells via low-affinity anti-human IgE Abs with dissociation constants in the 10-6 to 10-8 M range. We demonstrated that these low-affinity anti-IgE mAbs bind to the cell surface-bound IgE without triggering anaphylactic degranulation even at high concentration, albeit they would weakly upregulate CD203c expression on basophils. This is in contrast to the high-affinity anti-IgE mAbs that trigger anaphylactic degranulation at low concentration. Instead, the low-affinity anti-IgE mAbs profoundly block human peanut- and cat-allergic IgE-mediated basophil CD63 induction indicative of anaphylactic degranulation; suppress peanut-, cat-, and dansyl-specific IgE-mediated passive cutaneous anaphylaxis; and attenuate dansyl IgE-mediated systemic anaphylaxis in human FcεRIα transgenic mouse model. Mechanistic studies reveal that the ability of allergic reaction blockade by the low-affinity anti-IgE mAbs was correlated with their capacity to downregulate the surface IgE and FcεRI level on human basophils and the human FcεRIα transgenic mouse bone marrow-derived mast cells via driving internalization of the IgE/FcεRI complex. Our studies demonstrate that targeting surface-bound IgE with low-affinity anti-IgE Abs is capable of suppressing allergic reactivity while displaying an excellent safety profile, indicating that use of low-affinity anti-IgE mAbs holds promise as a novel therapeutic approach for IgE-mediated allergic diseases.

Published

2017

7. An easy-operation aptasensor for simultaneous detection of multiple tumor-associated exosomal proteins based on multicolor fluorescent DNA nanoassemblies.

Author

Li C, Jia H, Wei R, Liu J, Wang H, Zhou M, Yan C, and Huang L

Subjects

Humans, Fluorescent Dyes chemistry, Tetraspanin 30, Biomarkers, Tumor analysis, Neoplasms diagnosis, Neoplasms diagnostic imaging, Limit of Detection, Fluorescence, Exosomes chemistry, Aptamers, Nucleotide chemistry, Biosensing Techniques methods, Quantum Dots chemistry, DNA chemistry

Abstract

As a promising liquid biopsy biomarker, exosomes have demonstrated great potential and advantages in the noninvasive tumor diagnosis. However, an accurate and sensitive method for tumors-associated exosomes detection is scarce. Herein, we presented an easy-operation aptasensor which simultaneously detect multiple exosomal proteins by using multicolor fluorescent DNA nanoassemblies (FDNs) and CD63 aptamer-modified magnetic beads (MNPs-Apt CD63 ). In this system, the FDNs were firstly constructed by encapsulating different quantum dots (QDs) into rolling circle amplification (RCA) products that contained different aptamer sequences. Thus, the FDNs could selectively recognize the different exosomal proteins captured by the MNPs-Apt CD63 , and achieve the multiplex and sensitive detection according to the fluorescence of QDs. Benefiting from the signal amplification capacity and high selectivity of FDNs, this aptasensor not only could detect exosomes as low as 650 particles/μL, but also showed accurate analysis in clinical samples. In addition, we can also achieve point-of-care testing (POCT) due to the simple analysis steps and naked-eye observable fluorescence of QDs under the ultraviolet irradiation. We believe that our aptasensor could provide a promising platform for exosomes-based personalized diagnosis and precise monitoring of human health., 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., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2025

8. IRTIDP: A simple integrated real-time isolation and detection platform for small extracellular vesicles Glypican-1 in pancreatic cancer patients.

Author

Xi Y, Zhao Z, Wang F, Zhang D, and Guo Y

Subjects

Humans, Spectrum Analysis, Raman methods, Silver chemistry, Metal-Organic Frameworks chemistry, Biomarkers, Tumor blood, Biomarkers, Tumor analysis, Limit of Detection, Tetraspanin 30, Glypicans blood, Glypicans immunology, Pancreatic Neoplasms diagnosis, Pancreatic Neoplasms blood, Extracellular Vesicles chemistry, Metal Nanoparticles chemistry

Abstract

Glypican-1 (GPC-1) protein-positive small extracellular vesicles (GPC-1 + -sEV) have been proposed as potential biomarkers for early diagnosis of pancreatic cancer. In this study, we present an integrated real-time isolation and detection platform (IRTIDP) to capture and analyze GPC-1 + -sEV directly from sera of pancreatic cancer patients. First, CD63 antibody-modified metal-organic framework (MOF) materials were utilized to enrich sEVs with a capture efficiency of 93.93 %. Second, a SERS probe was constructed by Raman reporter 4-MBA and GPC-1 antibody modified SERS active silver nanoparticles (AgNPs), which formed a sandwich complex structure of "MOFs@GPC-1 + -sEV@AgNPs-4-MBA" with MOFs-enriched sEVs. The IRTSDP can complete the capture and detection process within 35 min, with a detection limit for 1 GPC-1 + -sEV/μL, and linear range between 10 5 ∼10 9 GPC-1 + -sEV/mL. Furthermore, this approach has been applied to quantify serum sEV GPC-1 in clinical pancreatic cancer patients. Based on the SERS intensity analysis, pancreatic cancer patients can be distinguished from pancreatic cystadenoma patients and healthy individuals effectively using this innovative platform that provides highly specific and sensitive means for early diagnosis of pancreatic cancer as well as other tumor types., Competing Interests: Declaration of competing interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests:Yongcan Guo reports article publishing charges and equipment, drugs, or supplies were provided by Sichuan Provincial Science and Technology Department. Yongcan Guo reports article publishing charges and equipment, drugs, or supplies were provided by Health Commission of Sichuan Province. Yongcan Guo reports article publishing charges and equipment, drugs, or supplies were provided by Sichuan Medical Association. If there are other authors, they declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

9. Y-box protein 1 is required to sort microRNAs into exosomes in cells and in a cell-free reaction.

Author

Shurtleff, Matthew J, Temoche-Diaz, Morayma M, Karfilis, Kate V, Ri, Sayaka, and Schekman, Randy

Subjects

Cell-Free System, Humans, Luciferases, Immunoglobulin G, MicroRNAs, Centrifugation, Density Gradient, Gene Expression Profiling, Cell Movement, Gene Expression Regulation, Genes, Reporter, Y-Box-Binding Protein 1, Exosomes, HEK293 Cells, Tetraspanin 30, Y-box, YBX1, biochemistry, cancer biology, exosome, extracellular vesicles, human, microRNA, Centrifugation, Density Gradient, Genes, Reporter, Biochemistry and Cell Biology

Abstract

Exosomes are small vesicles that are secreted from metazoan cells and may convey selected membrane proteins and small RNAs to target cells for the control of cell migration, development and metastasis. To study the mechanisms of RNA packaging into exosomes, we devised a purification scheme based on the membrane marker CD63 to isolate a single exosome species secreted from HEK293T cells. Using immunoisolated CD63-containing exosomes we identified a set of miRNAs that are highly enriched with respect to their cellular levels. To explore the biochemical requirements for exosome biogenesis and RNA packaging, we devised a cell-free reaction that recapitulates the species-selective enclosure of miR-223 in isolated membranes supplemented with cytosol. We found that the RNA-binding protein Y-box protein I (YBX1) binds to and is required for the sorting of miR-223 in the cell-free reaction. Furthermore, YBX1 serves an important role in the secretion of miRNAs in exosomes by HEK293T cells.

Published

2016

10. Detection of exosomal biomarker by electric field-induced release and measurement (EFIRM).

Author

Tu, Michael, Wei, Fang, Yang, Jieping, and Wong, David

Subjects

Biotechnology, Animals, Biomarkers, Biomarkers, Tumor, Blood Chemical Analysis, Cell Line, Tumor, Electrochemical Techniques, Electromagnetic Fields, Exosomes, Heterografts, Humans, Lung Neoplasms, Mice, Proteins, RNA, Saliva, Tetraspanin 30, Bioengineering, Issue 95, Exosome, Electrochemical sensors, Tumor biomarkers, Lung cancer, Salivary diagnostics, Biochemistry and Cell Biology, Psychology, Cognitive Sciences

Abstract

Exosomes are microvesicular structures that play a mediating role in intercellular communication. It is of interest to study the internal cargo of exosomes to determine if they carry disease discriminatory biomarkers. For performing exosomal analysis, it is necessary to develop a method for extracting and analyzing exosomes from target biofluids without damaging the internal content. Electric field-induced release and measurement (EFIRM) is a method for specifically extracting exosomes from biofluids, unloading their cargo, and testing their internal RNA/protein content. Using an anti-human CD63 specific antibody magnetic microparticle, exosomes are first precipitated from biofluids. Following extraction, low-voltage electric cyclic square waves (CSW) are applied to disrupt the vesicular membrane and cause cargo unloading. The content of the exosome is hybridized to DNA primers or antibodies immobilized on an electrode surface for quantification of molecular content. The EFIRM method is advantageous for extraction of exosomes and unloading cargo for analysis without lysis buffer. This method is capable of performing specific detection of both RNA and protein biomarker targets in the exosome. EFIRM extracts exosomes specifically based on their surface markers as opposed to size-based techniques. Transmission electron microscopy (TEM) and assay demonstrate the functionality of the method for exosome capture and analysis. The EFIRM method was applied to exosomal analysis of 9 mice injected with human lung cancer H640 cells (a cell line transfected to express the exosome marker human CD63-GFP) in order to test their exosome profile against 11 mice receiving saline controls. Elevated levels of exosomal biomarkers (reference gene GAPDH and protein surface marker human CD63-GFP) were found for the H640 injected mice in both serum and saliva samples. Furthermore, saliva and serum samples were demonstrated to have linearity (R = 0.79). These results are suggestive for the viability of salivary exosome biomarkers for detection of distal diseases.

Published

2015

11. Detection of Tumor Cell-Specific mRNA and Protein in Exosome-Like Microvesicles from Blood and Saliva

Author

Yang, Jieping, Wei, Fang, Schafer, Christopher, and Wong, David TW

Subjects

Lung, Lung Cancer, Cancer, Biotechnology, Genetics, 2.1 Biological and endogenous factors, Aetiology, Animals, Exosomes, Green Fluorescent Proteins, Humans, Lung Neoplasms, Male, Mice, Nude, Neoplasm Proteins, RNA, Messenger, Recombinant Fusion Proteins, Saliva, Tetraspanin 30, Xenograft Model Antitumor Assays, General Science & Technology

Abstract

The discovery of disease-specific biomarkers in oral fluids has revealed a new dimension in molecular diagnostics. Recent studies have reported the mechanistic involvement of tumor cells derived mediators, such as exosomes, in the development of saliva-based mRNA biomarkers. To further our understanding of the origins of disease-induced salivary biomarkers, we here evaluated the hypothesis that tumor-shed secretory lipidic vesicles called exosome-like microvesicles (ELMs) that serve as protective carriers of tissue-specific information, mRNAs, and proteins, throughout the vasculature and bodily fluids. RNA content was analyzed in cell free-saliva and ELM-enriched fractions of saliva. Our data confirmed that the majority of extracellular RNAs (exRNAs) in saliva were encapsulated within ELMs. Nude mice implanted with human lung cancer H460 cells expressing hCD63-GFP were used to follow the circulation of tumor cell specific protein and mRNA in the form of ELMs in vivo. We were able to identify human GAPDH mRNA in ELMs of blood and saliva of tumor bearing mice using nested RT-qPCR. ELMs positive for hCD63-GFP were detected in the saliva and blood of tumor bearing mice as well as using electric field-induced release and measurement (EFIRM). Altogether, our results demonstrate that ELMs carry tumor cell-specific mRNA and protein from blood to saliva in a xenografted mouse model of human lung cancer. These results therefore strengthen the link between distal tumor progression and the biomarker discovery of saliva through the ELMs.

Published

2014

12. APPROACH: Sensitive Detection of Exosomal Biomarkers by Aptamer-Mediated Proximity Ligation Assay and Time-Resolved Förster Resonance Energy Transfer.

Author

Li Y, Qian M, Liu Y, and Qiu X

Subjects

Humans, Biomarkers, Nucleic Acid Amplification Techniques methods, Tetraspanin 30, Fluorescence Resonance Energy Transfer methods, Aptamers, Nucleotide, Exosomes, Biosensing Techniques

Abstract

Exosomal biomarker detection holds great importance in the field of in vitro diagnostics, offering a non-invasive and highly sensitive approach for early disease detection and personalized treatment. Here, we proposed an "APPROACH" strategy, combining aptamer-mediated proximity ligation assay (PLA) with rolling circle amplification (RCA) and time-resolved Förster resonance energy transfer (TR-FRET) for the sensitive and semi-homogenous detection of exosomal biomarkers. PLA probes consisted of a cholesterol-conjugated oligonucleotide, which anchored to the membrane of an exosome, and a specific aptamer oligonucleotide that recognized a target protein of the exosome; the proximal binding of pairs of PLA probes to the same exosome positioned the oligonucleotides in the vicinity of each other, guiding the hybridization and ligation of two subsequently added backbone and connector oligonucleotides to form a circular DNA molecule. Circular DNA formed from PLA underwent rolling circle amplification (RCA) for signal amplification, and the resulting RCA products were subsequently quantified by TR-FRET. The limits of detection provided by APPROACH for the exosomal biomarkers CD63, PD-L1, and HER2 were 0.46 ng∙μL -1 , 0.77 ng∙μL -1 , and 1.1 ng∙μL -1 , respectively, demonstrating excellent analytical performance with high sensitivity and quantification accuracy. Furthermore, the strategy afforded sensitive detection of exosomal CD63 with a LOD of 1.56 ng∙μL -1 in complex biological matrices, which underscored its anti-interference capability and potential for in vitro detection. The proposed strategy demonstrates wide-ranging applicability in quantifying diverse exosomal biomarkers while exhibiting robust analytical characteristics, including high sensitivity and accuracy.

Published

2024

13. Infiltration analysis of eosinophils and basophils and co-expression of CD69, CD63, IL-31 and IgE in patients with bullous and non-bullous pemphigoid.

Author

Kotnik N, Langner A, Meyer NH, Pas HH, Gibbs BF, Meijer JM, Diercks GFH, Horváth B, and Raap U

Subjects

Humans, Basophils, Immunoglobulin E, Collagen Type XVII, Autoantibodies, Tetraspanin 30, Eosinophils, Pemphigoid, Bullous

Published

2024

14. The metabolic activity of Mycobacterium tuberculosis, assessed by use of a novel inducible GFP expression system, correlates with its capacity to inhibit phagosomal maturation and acidification in human macrophages

Author

Lee, Bai‐Yu, Clemens, Daniel L, and Horwitz, Marcus A

Subjects

Biochemistry and Cell Biology, Biological Sciences, Rare Diseases, Infectious Diseases, Tuberculosis, Infection, Good Health and Well Being, Acids, Antigens, CD, Cell Line, Genes, Reporter, Green Fluorescent Proteins, Humans, Hydrogen-Ion Concentration, Isopropyl Thiogalactoside, Macrophages, Mycobacterium tuberculosis, Phagosomes, Plasmids, Platelet Membrane Glycoproteins, Recombinant Proteins, Tetraspanin 30, Xanthenes, Agricultural and Veterinary Sciences, Medical and Health Sciences, Microbiology, Biological sciences

Abstract

Mycobacterium tuberculosis generally reside in phagosomes within human macrophages that resist maturation and acidification, but exhibit significant heterogeneity. In this study we have constructed an IPTG-inducible GFP expression system in M. tuberculosis to assess the relationship between the metabolic status of M. tuberculosis and the degree of phagosomal maturation. Using these recombinant bacteria, we have found that, in human macrophages, M. tuberculosis that respond to IPTG with expression of GFP fluorescence, and hence are metabolically active, reside in non-acidified phagosomes that have not fused with Texas red dextran pre-labelled lysosomes. In contrast, M. tuberculosis that fail to express GFP in response to IPTG, and hence are metabolically inactive, reside within acidified phagosomes that have fused with Texas red dextran labelled lysosomes. These studies demonstrate that metabolic activity of M. tuberculosis correlates strongly with phagosomal maturation and that the inducible GFP expression system is useful for assessing metabolic activity of intracellular M. tuberculosis.

Published

2008

15. Tetraspanin heterogeneity of small extracellular vesicles in human biofluids and brain tissue

Author

Mami Okada-Tsuchioka, Naoto Kajitani, Wataru Omori, Takashi Kurashige, Shuken Boku, and Minoru Takebayashi

Subjects

Extracellular Vesicles, Tetraspanin 30, Tetraspanins, Biophysics, Brain, Humans, Cell Biology, Exosomes, Molecular Biology, Biochemistry, Biomarkers, Tetraspanin 28

Abstract

Extracellular vesicles (EVs) are particles released from most cell types delimited by a lipid bilayer. Small EVs (sEVs) are nanosized (200 nm) and include exosomes. Brain-derived sEVs may provide a source for new biomarkers of brain status. CD9, CD63, and CD81 are major members of the tetraspanin family frequently used as sEV markers. However, according to a recent report, tetraspanins were not equally expressed in all sEVs, but rather show heterogeneity that reflects the expression levels in their secretory cells. We therefore investigated tetraspanin heterogeneity of sEVs in biofluids commonly used for clinical laboratory tests, and those in the brain. Expression levels and distributions of CD9, CD63 and CD81 on sEVs were determined in serum, plasma, and cerebrospinal fluid (CSF) samples collected from each healthy donor, and in post-mortem brain tissue samples. We found heterogeneous mixes of sEVs with various tetraspanin combinations among sEVs, and the predominant types and heterogeneous patterns of tetraspanins were specific to sample type. Hierarchical clustering revealed that brain sEVs were similar to those in the CSF, but different from those in peripheral blood. Our findings both provide basic information and contribute to the development of biomarkers for neurological and psychiatric disorders.

Published

2022

16. Virulent and Avirulent Strains of Francisella tularensis Prevent Acidification and Maturation of Their Phagosomes and Escape into the Cytoplasm in Human Macrophages

Author

Clemens, Daniel L, Lee, Bai-Yu, and Horwitz, Marcus A

Subjects

Rare Diseases, Biodefense, Vaccine Related, Emerging Infectious Diseases, Prevention, Immunization, Infectious Diseases, Infection, Antigens, CD, Cathepsin D, Cell Line, Cytoplasm, Francisella tularensis, Humans, Hydrogen-Ion Concentration, Lysosomal-Associated Membrane Protein 1, Lysosome-Associated Membrane Glycoproteins, Macrophages, Microscopy, Immunoelectron, Phagosomes, Platelet Membrane Glycoproteins, Tetraspanin 30, Tularemia, Virulence, Biological Sciences, Agricultural and Veterinary Sciences, Medical and Health Sciences, Microbiology

Abstract

Francisella tularensis, the agent of tularemia, is an intracellular pathogen, but little is known about the compartment in which it resides in human macrophages. We have examined the interaction of a recent virulent clinical isolate of F. tularensis subsp. tularensis and the live vaccine strain with human macrophages by immunoelectron and confocal immunofluorescence microscopy. We assessed the maturation of the F. tularensis phagosome by examining its acquisition of the lysosome-associated membrane glycoproteins (LAMPs) CD63 and LAMP1 and the acid hydrolase cathepsin D. Two to four hours after infection, vacuoles containing live F. tularensis cells acquired abundant staining for LAMPs but little or no staining for cathepsin D. However, after 4 h, the colocalization of LAMPs with live F. tularensis organisms declined dramatically. In contrast, vacuoles containing formalin-killed bacteria exhibited intense staining for all of these late endosomal/lysosomal markers at all time points examined (1 to 16 h). We examined the pH of the vacuoles 3 to 4 h after infection by quantitative immunogold staining and by fluorescence staining for lysosomotropic agents. Whereas phagosomes containing killed bacteria stained intensely for these agents, indicating a marked acidification of the phagosomes (pH 5.5), phagosomes containing live F. tularensis did not concentrate these markers and thus were not appreciably acidified (pH 6.7). An ultrastructural analysis of the F. tularensis compartment revealed that during the first 4 h after uptake, the majority of F. tularensis bacteria reside within phagosomes with identifiable membranes. The cytoplasmic side of the membranes of approximately 50% of these phagosomes was coated with densely staining fibrils of approximately 30 nm in length. In many cases, these coated phagosomal membranes appeared to bud, vesiculate, and fragment. By 8 h after infection, the majority of live F. tularensis bacteria lacked any ultrastructurally discernible membrane separating them from the host cell cytoplasm. These results indicate that F. tularensis initially enters a nonacidified phagosome with LAMPs but without cathepsin D and that the phagosomal membrane subsequently becomes morphologically disrupted, allowing the bacteria to gain direct access to the macrophagic cytoplasm. The capacity of F. tularensis to alter the maturation of its phagosome and to enter the cytoplasm is likely an important element of its capacity to parasitize macrophages and has major implications for vaccine development.

Published

2004

17. Aberrant TIMP-1 overexpression in tumor-associated fibroblasts drives tumor progression through CD63 in lung adenocarcinoma

Author

Paula Duch, Natalia Díaz-Valdivia, Rafael Ikemori, Marta Gabasa, Evette S. Radisky, Marselina Arshakyan, Sabrina Gea-Sorlí, Anna Mateu-Bosch, Paloma Bragado, Josep Lluís Carrasco, Hidetoshi Mori, Josep Ramírez, Cristina Teixidó, Noemí Reguart, Cristina Fillat, Derek C. Radisky, and Jordi Alcaraz

Subjects

Drug targeting, Lung Neoplasms, Tissue Inhibitor of Metalloproteinase-1, Tetraspanin 30, Proteins, Adenocarcinoma of Lung, Fibrosi pulmonar, Fibroblasts, Pulmonary fibrosis, Transforming Growth Factor beta1, Mice, Dianes farmacològiques, Cancer-Associated Fibroblasts, Carcinoma, Squamous Cell, Tumor Microenvironment, Càncer de pulmó, Animals, Humans, Lung cancer, Proteïnes, Molecular Biology

Abstract

Tissue inhibitor of metalloproteinase-1 (TIMP-1) is an important regulator of extracellular matrix turnover that has been traditionally regarded as a potential tumor suppressor owing to its inhibitory effects of matrix metalloproteinases. Intriguingly, this interpretation has been challenged by the consistent observation that increased expression of TIMP-1 is associated with poor prognosis in virtually all cancer types including lung cancer, supporting a tumor-promoting function. However, how TIMP-1 is dysregulated within the tumor microenvironment and how it drives tumor progression in lung cancer is poorly understood. We analyzed the expression of TIMP-1 and its cell surface receptor CD63 in two major lung cancer subtypes: lung adenocarcinoma (ADC) and squamous cell carcinoma (SCC), and defined the tumor-promoting effects of their interaction. We found that TIMP-1 is aberrantly overexpressed in tumor-associated fibroblasts (TAFs) in ADC compared to SCC. Mechanistically, TIMP-1 overexpression was mediated by the selective hyperactivity of the pro-fibrotic TGF-β1/SMAD3 pathway in ADC-TAFs. Likewise, CD63 was upregulated in ADC compared to SCC cells. Genetic analyses revealed that TIMP-1 secreted by TGF-β1-activated ADC-TAFs is both necessary and sufficient to enhance growth and invasion of ADC cancer cells in culture, and that tumor cell expression of CD63 was required for these effects. Consistently, in vivo analyses revealed that ADC cells co-injected with fibroblasts with reduced SMAD3 or TIMP-1 expression into immunocompromised mice attenuated tumor aggressiveness compared to tumors bearing parental fibroblasts. We also found that high TIMP1 and CD63 mRNA levels combined define a stronger prognostic biomarker than TIMP1 alone. Our results identify an excessive stromal TIMP-1 within the tumor microenvironment selectively in lung ADC, and implicate it in a novel tumor-promoting TAF-carcinoma crosstalk, thereby pointing to TIMP-1/CD63 interaction as a novel therapeutic target in lung cancer.

Published

2022

18. Adenotonsillar pathology in mucopolysaccharidoses - lysosomal storage predominates in paracortical CD63+ cells.

Author

Murgasova L, Hulkova H, Baresova V, Jurovcik M, Stritesky J, Jurickova K, Magner M, and Sikora J

Subjects

Humans, Lymphoid Tissue pathology, Lysosomes, Enzyme Replacement Therapy, Tetraspanin 30, Mucopolysaccharidoses diagnosis, Mucopolysaccharidoses drug therapy, Mucopolysaccharidoses genetics

Abstract

Despite the adenoids are regularly removed in patients with mucopolysaccharidoses (MPS), the underlying tissue and cellular pathologies remain understudied. We characterized an (immuno)histopathologic and ultrastructural phenotype dominated by lysosomal storage changes in a specific subset of adenotonsillar paracortical cells in 8 MPS patients (3 MPS I, 3 MPS II, and 2 MPS IIIA). These abnormal cells were effectively detected by an antibody targeting the lysosomal membrane tetraspanin CD63. Important, CD63+ storage vacuoles in these cells lacked the monocytes/macrophages lysosomal marker CD68. Such a distinct patterning of CD63 and CD68 was not present in a patient with infantile neurovisceral variant of acid sphingomyelinase deficiency. The CD63+ storage pathology was absent in two MPS I patients who either received enzyme-replacement therapy or underwent hematopoietic stem cells transplantation prior the adenoidectomy. Our study demonstrates novel features of lysosomal storage patterning and suggests diagnostic utility of CD63 detection in adenotonsillar lymphoid tissue of MPS patients., (© 2023. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published

2024

19. Characterization of the Mycobacterium tuberculosis phagosome and evidence that phagosomal maturation is inhibited.

Author

Clemens, DL and Horwitz, MA

Subjects

Biomedical and Clinical Sciences, Health Sciences, Vaccine Related, Tuberculosis, Prevention, Biodefense, Rare Diseases, Orphan Drug, Infectious Diseases, Emerging Infectious Diseases, Infection, Good Health and Well Being, Antigens, CD, Cell Compartmentation, HLA-DR Antigens, Histocompatibility Antigens Class I, Humans, Immunohistochemistry, In Vitro Techniques, Intracellular Membranes, Legionella pneumophila, Lysosome-Associated Membrane Glycoproteins, Lysosomes, Membrane Fusion, Membrane Glycoproteins, Monocytes, Mycobacterium tuberculosis, Phagocytosis, Phagosomes, Platelet Membrane Glycoproteins, Receptors, Transferrin, Tetraspanin 30, beta 2-Microglobulin, Medical and Health Sciences, Immunology, Biomedical and clinical sciences, Health sciences

Abstract

We have used the cryosection immunogold technique to study the composition of the Mycobacterium tuberculosis phagosome. We have used quantitative immunogold staining to determine the distribution of several known markers of the endosomal-lysosomal pathway in human monocytes after ingestion of either M. tuberculosis, Legionella pneumophila, or polystyrene beads. Compared with the other phagocytic particles studied, the M. tuberculosis phagosome exhibits delayed clearance of major histocompatibility complex (MHC) class I molecules, relatively intense staining for MHC class II molecules and the endosomal marker transferrin receptor, and relatively weak staining for the lysosomal membrane glycoproteins, CD63, LAMP-1, and LAMP-2 and the lysosomal acid protease, cathepsin D. In contrast to M. tuberculosis, the L. pneumophila phagosome rapidly clears MHC class I molecules and excludes all endosomal-lysosomal markers studied. In contrast to both live M. tuberculosis and L. pneumophila phagosomes, phagosomes containing either polystyrene beads or heat-killed M. tuberculosis stain intensely for lysosomal membrane glycoproteins and cathepsin D. These findings suggest that (a) M. tuberculosis retards the maturation of its phagosome along the endosomal-lysosomal pathway and resides in a compartment with endosomal, as opposed to lysosomal, characteristics; and (b) the intraphagosomal pathway, i.e., the pathway followed by several intracellular parasites that inhibit phagosome-lysosome fusion, is heterogeneous.

Published

1995

20. Correspondence to "Diagnosis of immediate reactions to amoxicillin: Comparison of basophil activation markers CD63 and CD203c in a prospective study".

Author

Elst J, van der Poorten MM, Toscano A, Van Gasse AL, Mertens C, Beyens M, Hagendorens MM, Ebo DG, and Sabato V

Subjects

Humans, Prospective Studies, Basophil Degranulation Test, Antigens, CD, Flow Cytometry, Tetraspanin 30, Phosphoric Diester Hydrolases, Pyrophosphatases, Basophils, Amoxicillin adverse effects

Published

2023

21. Reply to correspondence to 'Diagnosis of immediate reactions to amoxicillin: Comparison of basophil activation markers CD63 and CD203c in a prospective study'.

Author

Fernández TD, Mayorga C, and Torres MJ

Subjects

Humans, Prospective Studies, Basophil Degranulation Test, Antigens, CD, Tetraspanin 30, Basophils, Amoxicillin adverse effects

Published

2023

22. Diagnosis of immediate reactions to amoxicillin: Comparison of basophil activation markers CD63 and CD203c in a prospective study.

Author

Céspedes JA, Fernández-Santamaría R, Ariza A, Bogas G, Doña I, Rondón C, Salas M, Labella M, Frecha C, Mayorga C, Torres MJ, and Fernández TD

Subjects

Humans, Amoxicillin adverse effects, Prospective Studies, Basophils, Basophil Degranulation Test methods, Clavulanic Acid, Tetraspanin 30, Hypersensitivity, Immediate diagnosis, Anaphylaxis diagnosis, Anaphylaxis etiology

Abstract

Background: Amoxicillin (AX) combined or not with clavulanic acid (CLV) is frequently involved in IgE-mediated reactions. Drug provocation test (DPT) is considered as the gold standard for diagnosis, although contraindicated in high-risk patients. Basophil activation test (BAT) can help diagnose immediate reactions to beta-lactams, although controversy exists regarding the best activation marker. We have performed a real-life study in a prospective cohort to analyze the real value of BAT as diagnostic tool and the best activation marker, CD63 and CD203c, for the evaluation of immediate reactions to these drugs., Methods: We prospectively evaluated patients with a clinical suspicion of immediate reactions after AX or AX-CLV administration during a 6-year period. The allergological work-up was done following the EAACI recommendations. BAT was performed in all patients using CD63 and CD203c as activation markers., Results: In AX-allergic patients, both activation markers, CD63 and CD203c, showed similar SE values (48.6% and 46.7%, respectively); however, specificity was of 81.1% and 94.6%, respectively, with CD203c showing good positive predictive value and like-hood ratio. In CLV-allergic patients, CD203c showed higher SE (50%) than CD63 (42.9%), maintaining the same value of SP (80%). Combining the results of both markers can slightly increase the sensitivity (51.4% for AX and 54.8% for CLV), although decreasing the specificity (79.7% and 73%, respectively). Interestingly, all patients with an anaphylactic shock showed a positive BAT to CLV using CD203c., Conclusions: BAT using CD203c showed a good confirmatory power, especially for AX allergy. Placing BAT as a first step in the diagnostic procedure can help reduce the need of performing a complete allergological work-up in 46.6% of patients, diminishing the risk of reinducing allergic reactions., (© 2022 The Authors. Allergy published by European Academy of Allergy and Clinical Immunology and John Wiley & Sons Ltd.)

Published

2023

23. Transmembrane proteins tetraspanin 4 and CD9 sense membrane curvature

Author

Raviv Dharan, Shahar Goren, Sudheer Kumar Cheppali, Petr Shendrik, Guy Brand, Alisa Vaknin, Li Yu, Michael M. Kozlov, and Raya Sorkin

Subjects

Multidisciplinary, Microvilli, Tetraspanin 30, Tetraspanins, Cell Membrane, Oocytes, Tetraspanin 29, Tetraspanin 28

Abstract

Multiple membrane-shaping and remodeling processes are associated with tetraspanin proteins by yet unknown mechanisms. Tetraspanins constitute a family of proteins with four transmembrane domains present in every cell type. Prominent examples are tetraspanin4 and CD9, which are required for the fundamental cellular processes of migrasome formation and fertilization, respectively. These proteins are enriched in curved membrane structures, such as cellular retraction fibers and oocyte microvilli. The factors driving this enrichment are, however, unknown. Here, we revealed that tetraspanin4 and CD9 are curvature sensors with a preference for positive membrane curvature. To this end, we used a biomimetic system emulating membranes of cell retraction fibers and oocyte microvilli by membrane tubes pulled out of giant plasma membrane vesicles with controllable membrane tension and curvature. We developed a simple thermodynamic model for the partitioning of curvature sensors between flat and tubular membranes, which allowed us to estimate the individual intrinsic curvatures of the two proteins. Overall, our findings illuminate the process of migrasome formation and oocyte microvilli shaping and provide insight into the role of tetraspanin proteins in membrane remodeling processes.

Published

2022

24. Designed Co-DNA-Locker and Ratiometric SERS Sensing for Accurate Detection of Exosomes Based on Gold Nanorod Arrays

Author

Hongyang Xie, Caifeng Ding, and Jing Wang

Subjects

Gold nanorod, Materials science, Receptor, ErbB-2, Aptamer, Nanotechnology, Biosensing Techniques, Exosomes, Spectrum Analysis, Raman, Rhodamine 6G, chemistry.chemical_compound, Limit of Detection, Cell Line, Tumor, Humans, General Materials Science, Fluorescent Dyes, Detection limit, Nanotubes, Rhodamines, Tetraspanin 30, Hexagonal crystal system, Nucleic Acid Hybridization, DNA, Aptamers, Nucleotide, Carbocyanines, Microvesicles, HEK293 Cells, chemistry, Gold, Signal amplification

Abstract

Exosomes, which can transfer and deliver information about the original cell, are considered to be ideal candidates for early cancer diagnosis and evaluation of therapeutic efficacy due to their high abundance and stability. However, the highly expressed proteins on the surface of exosomes are usually associated with a variety of cancers; it is difficult to distinguish them by a single marker. Herein, a controlled self-assembly of gold nanorod (AuNR) arrays was prepared to construct a surface-enhanced Raman spectroscopy (SERS) sensor for the specific detection of exosomes secreted by SK-Br-3 cells based on a designed colocalization-dependent system (Co-DNA-Locker) and ratiometric strategy. After the exosomes are captured in the sensing array by the EpCAM aptamer modified on the surface of AuNRs, the DNA logic process occurs because the other two proteins, CD63 and HER2, are expressed simultaneously on the surface of exosomes secreted by SK-Br-3 cells, and the SERS signal intensity of the Rhodamine 6G (R6G) tagged on the terminal of DNA TE increased with an increase in the concentration of the exosomes, while the SERS signal intensity of Cy5 linked on the terminal of the EpCAM aptamer, which acts as an internal standard, remains stable. The AuNRs are uniformly arranged in a hexagonal shape, and the dense "hot spots" produce "hot surfaces," which greatly improve the sensitivity and uniformity of detection. In the presence of target exosomes, the DNA colocalization three-signal input switch and the ratiometric strategy realize the specific and accurate detection of exosomes. This sensing strategy achieves a wide detection range (1.0 × 104-5.0 × 106 particles/mL) and a lower detection limit (5.3 × 103 particles/mL), without using any signal amplification mechanism, demonstrating promising applications in health care monitoring and clinical diagnostics.

Published

2021

25. Activated steady status and distinctive FcεRI-mediated responsiveness in basophils of atopic dermatitis

Author

Shinya Imamura, Chikako Nishigori, Yoshiko Oda, Atsushi Fukunaga, Ken Washio, and Mayuko Mizuno

Subjects

Adult, Male, FcεRI, Cell, Stimulation, Inflammation, chemical and pharmacologic phenomena, Basophil, Immunoglobulin E, Dermatitis, Atopic, Young Adult, parasitic diseases, medicine, Immunology and Allergy, Humans, Pyrophosphatases, Atopic dermatitis, biology, CD63, business.industry, Phosphoric Diester Hydrolases, Receptors, IgE, Tetraspanin 30, hemic and immune systems, General Medicine, RC581-607, Middle Aged, medicine.disease, Surface-bound IgE, Basophils, medicine.anatomical_structure, Case-Control Studies, Immunology, biology.protein, Female, Total serum IgE, Immunologic diseases. Allergy, medicine.symptom, Antibody, business

Abstract

Background Although basophils are considered to play an important role for maintenance of type 2 inflammation in atopic dermatitis (AD), studies on basophils in AD patients are limited. Some studies have reported the activation status, including CD203c and CD63, of peripheral blood basophils in AD patients. Methods We examined the features of circulating basophils in AD patients, assessed cell surface marker expressions and total serum IgE, and compared basophil responsiveness to stimulation between AD patients and healthy controls (HCs). In addition, the correlations among AD severity, laboratory factors, and features of basophils were examined. Blood samples from 38 AD patients and 21 HCs were analyzed. Basophil response markers CD203c and CD63, and expression of surface-bound IgE and FceRI on basophils were measured. CD203c and CD63 expressions induced by stimulation with anti-IgE and anti-FceRI antibodies were measured. Clinical/laboratory factors including total serum IgE were examined for correlations with these basophil parameters. Results Baseline CD203c and CD63 expression on basophils were significantly higher in AD patients compared with HCs. The CD203c/CD63 response ratio to anti-FceRI stimulation was higher than that to anti-IgE stimulation in AD patients, but not HCs. FceRI expression on basophils was higher in AD patients than in HCs, although surface-bound IgE on basophils was equivalent. Total serum IgE had negative correlations with surface-bound IgE and CD63 responsiveness to anti-IgE stimulation. Conclusions Basophils were spontaneously activated under steady-state conditions in AD patients and responsiveness to anti-IgE stimulation was lower than in HCs. Despite high serum IgE and high basophil FceRI expression, surface-bound IgE on basophils remained relatively low. Basophils might be suppressed or exhausted regarding FceRI signaling via IgE in severe AD.

Published

2021

26. Extracellular vesicles and exosomes generated from cystic renal epithelial cells promote cyst growth in autosomal dominant polycystic kidney disease

Author

Peter C. Harris, Hao Ding, Linda Xiaoyan Li, Xiaogang Li, and Junwei Yang

Subjects

0301 basic medicine, Nephrology, General Physics and Astronomy, urologic and male genital diseases, Exosomes, Kidney, Mice, 0302 clinical medicine, Polycystic kidney disease, Cyst, Cystic kidney, Multidisciplinary, Aniline Compounds, Cysts, Polycystic Kidney, Autosomal Dominant, female genital diseases and pregnancy complications, medicine.anatomical_structure, 030220 oncology & carcinogenesis, Collagen, Signal Transduction, medicine.medical_specialty, Cell biology, TRPP Cation Channels, Science, Autosomal dominant polycystic kidney disease, Biology, Exosome, Benzylidene Compounds, Models, Biological, General Biochemistry, Genetics and Molecular Biology, Article, Exocytosis, Cell Line, 03 medical and health sciences, Internal medicine, medicine, Animals, Cell Proliferation, PKD1, urogenital system, Tetraspanin 30, Epithelial Cells, General Chemistry, medicine.disease, Fibrosis, Rats, MicroRNAs, 030104 developmental biology, Gene Expression Regulation, Mutation, Cancer research

Abstract

Autosomal dominant polycystic kidney disease (ADPKD) is caused by germline mutations of PKD1 or PKD2 on one allele and a somatic mutation inactivating the remaining normal allele. However, if and how null ADPKD gene renal epithelial cells affect the biology and function of neighboring cells, including heterozygous renal epithelial cells, fibroblasts and macrophages during cyst initiation and expansion remains unknown. Here we address this question with a “cystic extracellular vesicles/exosomes theory”. We show that cystic cell derived extracellular vesicles and urinary exosomes derived from ADPKD patients promote cyst growth in Pkd1 mutant kidneys and in 3D cultures. This is achieved by: 1) downregulation of Pkd1 gene expression and upregulation of specific miRNAs, resulting in the activation of PKD associated signaling pathways in recipient renal epithelial cells and tissues; 2) the activation of fibroblasts; and 3) the induction of cytokine expression and the recruitment of macrophages to increase renal inflammation in cystic kidneys. Inhibition of exosome biogenesis/release with GW4869 significantly delays cyst growth in aggressive and milder ADPKD mouse models, suggesting that targeting exosome secretion has therapeutic potential for ADPKD., Autosomal dominant polycystic kidney disease is characterized by the formation of cysts in the kidney. Here the authors show that cystic extracellular vesicles/exosomes play a critical role in regulating the biology and function of adjacent cells, including renal epithelial cells, fibroblasts and macrophages, and contribute to renal cyst growth.

Published

2021

27. Detailed Characterization of Small Extracellular Vesicles from Different Cell Types Based on Tetraspanin Composition by ExoView R100 Platform

Author

Kai, Breitwieser, Leon F, Koch, Tobias, Tertel, Eva, Proestler, Luisa D, Burgers, Christoph, Lipps, James, Adjaye, Robert, Fürst, Bernd, Giebel, and Meike J, Saul

Subjects

Extracellular Vesicles, Tetraspanin 30, Tetraspanins, Mesenchymal Stem Cells, Biomarkers

Abstract

Small extracellular vesicles (sEV) hold enormous potential as biomarkers, drug carriers, and therapeutic agents. However, due to previous limitations in the phenotypic characterization of sEV at the single vesicle level, knowledge of cell type-specific sEV signatures remains sparse. With the introduction of next-generation sEV analysis devices, such as the single-particle interferometric reflectance imaging sensor (SP-IRIS)-based ExoView R100 platform, single sEV analyses are now possible. While the tetraspanins CD9, CD63, and CD81 were generally considered pan-sEV markers, it became clear that sEV of different cell types contain several combinations and amounts of these proteins on their surfaces. To gain better insight into the complexity and heterogeneity of sEV, we used the ExoView R100 platform to analyze the CD9/CD63/CD81 phenotype of sEV released by different cell types at a single sEV level. We demonstrated that these surface markers are sufficient to distinguish cell-type-specific sEV phenotypes. Furthermore, we recognized that tetraspanin composition in some sEV populations does not follow a random pattern. Notably, the tetraspanin distribution of sEV derived from mesenchymal stem cells (MSCs) alters depending on cell culture conditions. Overall, our data provide an overview of the cell-specific characteristics of sEV populations, which will increase the understanding of sEV physiology and improve the development of new sEV-based therapeutic approaches.

Published

2022

28. The large extracellular loop of CD63 interacts with gp41 of HIV-1 and is essential for establishing the virological synapse

Author

Norbert Bannert, Joachim Denner, Daniel Ivanusic, and Kazimierz Madela

Subjects

0301 basic medicine, Cell biology, Science, Immunology, HIV Infections, Biology, Gp41, Article, Green fluorescent protein, Pathogenesis, 03 medical and health sciences, 0302 clinical medicine, Immune system, Tetraspanin, Extracellular, Humans, Binding site, Human immunodeficiency virus type 1 (HIV-1), Multidisciplinary, Tetraspanin 30, FOS: Clinical medicine, 500 Naturwissenschaften und Mathematik::570 Biowissenschaften, Biologie::570 Biowissenschaften, Biologie, Transmembrane protein, HIV Envelope Protein gp41, 030104 developmental biology, HEK293 Cells, 030220 oncology & carcinogenesis, HIV-1, Medicine

Abstract

Human immunodeficiency virus type 1 (HIV-1) persists lifelong in infected individuals and has evolved unique strategies in order to evade the immune system. One of these strategies is the direct cell-to-cell spread of HIV-1. The formation of a virological synapse (VS) between donor and target cell is important for this process. Tetraspanins are cellular proteins that are actively involved in the formation of a VS. However, the molecular mechanisms of recruiting host proteins for the cell-cell transfer of particles to the VS remains unclear. Our study has mapped the binding site for the transmembrane envelope protein gp41 of HIV-1 within the large extracellular loop (LEL) of CD63 and showed that this interaction occurs predominantly at the VS between T cells where viral particles are transferred. Mutations within the highly conserved CCG motif of the tetraspanin superfamily abrogated recruiting of expressed HIV-1 GFP fused Gag core protein and CD63 to the VS. This demonstrates the biological significance of CD63 for enhanced formation of a VS. Since cell-cell spread of HIV-1 is a major route of persistent infection, these results highlight the central role of CD63 as a member of the tetraspanin superfamily during HIV-1 infection and pathogenesis.

Published

2021

29. Generation of cd63-deficient zebrafish to analyze the role of cd63 in viral infection

Author

Sarithaa Sellaththurai, Jehee Lee, Sumi Jung, Suna Kim, Seongdo Lee, and Myoung-Jin Kim

Subjects

Fish Proteins, 0301 basic medicine, Cell signaling, Cellular differentiation, Aquatic Science, Novirhabdovirus, Fish Diseases, 03 medical and health sciences, Tetraspanin, Rhabdoviridae Infections, Animals, Environmental Chemistry, CRISPR, Amino Acid Sequence, Gene, Zebrafish, Phylogeny, biology, Tetraspanin 30, Gene Expression Profiling, Immunity, 04 agricultural and veterinary sciences, General Medicine, biology.organism_classification, Transmembrane protein, Cell biology, 030104 developmental biology, Gene Expression Regulation, embryonic structures, 040102 fisheries, 0401 agriculture, forestry, and fisheries, Signal transduction, Sequence Alignment

Abstract

The tetraspanin superfamily proteins are transmembrane proteins identified in a diverse range of eukaryotic organisms. Tetraspanins are involved in a variety of essential biological functions, including cell differentiation, adhesion, migration, signal transduction, intracellular trafficking, and immune responses. For an infection to occur, viruses must interact with various cell surface components, including receptors and signaling molecules. Tetraspanin CD63 is involved in the organization of the cell membrane and trafficking of cellular transmembrane proteins that interact with many viruses. In this study, the cd63 gene was characterized by studying its expression and function in a zebrafish model. The functional domains and structural features of Cd63, such as the Cys-Cys-Gly (CCG) motif in the large extracellular loop and cysteine residues, are conserved in zebrafish. We confirmed that cd63 was expressed in immune system organs, such as the axial vein and pronephric duct, during the embryonic development of zebrafish. To better understand the role of cd63 in the zebrafish immune system, we established cd63-deficient zebrafish lines using the clustered regularly interspaced short palindromic repeats/CRISPR-associated protein 9 (CRISPR/Cas9) system. A 19 bp insertion mutation was generated in single guide RNA (sgRNA) target sequence of exon 3 of the cd63 gene, to create a pre-mature stop codon. We then analyzed the expression of cd63-related genes cxcr4a and cxcr4b in wild type (WT) and cd63-deficient zebrafish. We believe our study provides an important model that could be used to investigate the roles of cd63 in viral infection in vivo.

Published

2021

30. CD63 orchestrates ferritin export

Author

Suzy V. Torti and Frank M. Torti

Subjects

medicine.medical_specialty, Iron, Immunology, Platelet Membrane Glycoproteins, Biochemistry, Cell Line, Extracellular Vesicles, Red Cells, Iron, and Erythropoiesis, Internal medicine, medicine, Humans, Gene Silencing, Iron Regulatory Protein 1, RNA, Messenger, Iron Regulatory Protein 2, biology, Tetraspanin 30, Chemistry, Cell Biology, Hematology, Up-Regulation, Ferritin, Protein Transport, Endocrinology, Apoferritins, Ferritins, biology.protein, Oxidoreductases

Abstract

The interplay between intracellular and extracellular ferritin is not well understood despite the recognition 3 years ago that cellular ferritin can be exported into plasma by the exosome pathway. Yanatori et al report new insights into the triggers for ferritin secretion and how this is coordinated with iron metabolism. They demonstrate that CD63, a tetraspanin protein and constituent of extracellular vesicles, is induced by iron and in turn that this increases the secretion by various cells of CD63- positive extracellular vesicles containing iron-loaded ferritin., Key Points CD63 is involved in EV secretion from cells and is shown herein to be regulated by iron via the IRE-IRP system.Iron-loading increased secretion of CD63+ EVs containing iron-loaded ferritin., Visual Abstract, Extracellular vesicles (EVs) transfer functional molecules between cells. CD63 is a widely recognized EV marker that contributes to EV secretion from cells. However, the regulation of its expression remains largely unknown. Ferritin is a cellular iron storage protein that can also be secreted by the exosome pathway, and serum ferritin levels classically reflect body iron stores. Iron metabolism–associated proteins such as ferritin are intricately regulated by cellular iron levels via the iron responsive element-iron regulatory protein (IRE-IRP) system. Herein, we present a novel mechanism demonstrating that the expression of the EV-associated protein CD63 is under the regulation of the IRE-IRP system. We discovered a canonical IRE in the 5′ untranslated region of CD63 messenger RNA that is responsible for regulating its expression in response to increased iron. Cellular iron loading caused a marked increase in CD63 expression and the secretion of CD63+ EVs from cells, which were shown to contain ferritin-H and ferritin-L. Our results demonstrate that under iron loading, intracellular ferritin is transferred via nuclear receptor coactivator 4 (NCOA4) to CD63+ EVs that are then secreted. Such iron-regulated secretion of the major iron storage protein ferritin via CD63+ EVs, is significant for understanding the local cell-to-cell exchange of ferritin and iron.

Published

2021

31. Basophil activation test: Mechanisms and considerations for use in clinical trials and clinical practice

Author

Oral Alpan, Alexandra F. Santos, and Hans Jürgen Hoffmann

Subjects

Allergy, diagnosis, Immunology, Basophil Degranulation Test, Basophil, Immunoglobulin E, medicine.disease_cause, Allergen, CD63, medicine, Humans, Immunology and Allergy, Sensitization, biology, Tetraspanin 30, business.industry, Reproducibility of Results, Allergens, allergy, Flow Cytometry, medicine.disease, Basophils, Clinical trial, Basophil activation, medicine.anatomical_structure, basophil activation test, biology.protein, immunotherapy, business, Food Hypersensitivity

Abstract

The basophil activation test (BAT) is a functional assay that measures the degree of degranulation following stimulation with allergen or controls by flow cytometry. It correlates directly with histamine release. From the dose-response curve resulting from BAT in allergic patients, basophil reactivity (%CD63(+) basophils) and basophil sensitivity (EC50 or similar) are the main outcomes of the test. BAT takes into account all characteristics of IgE and allergen and thus can be more specific than sensitization tests in the diagnosis of allergic disease. BAT reduces the need for in vivo procedures, such as intradermal tests and allergen challenges, which can cause allergic reactions of unpredictable severity. As it closely reflects the patients' phenotype in most cases, it may be used to support the diagnosis of food, venom and drug allergies and chronic urticaria, to monitor the natural resolution of food allergies and to predict and monitor clinical the response to immunomodulatory treatments, such as allergen-specific immunotherapy and biologicals. Clinical application of BAT requires analytical validation, clinical validation, standardization of procedures and quality assurance to ensure reproducibility and reliability of results. Currently, efforts are ongoing to establish a platform that could be used by laboratories in Europe and in the USA for quality assurance and certification.

Published

2021

32. Targeting the TXNIP‐NLRP3 interaction with PSSM1443 to suppress inflammation in sepsis‐induced myocardial dysfunction

Author

Huifen Xu, Qingyun Peng, Xiangxin Liu, Mingbing Xiao, Xinlong Chen, Linhua Wang, and Hongsheng Zhao

Subjects

0301 basic medicine, Heart Diseases, Inflammasomes, Physiology, Interleukin-1beta, Clinical Biochemistry, Anti-Inflammatory Agents, Inflammation, Exosomes, Systemic inflammation, Exosome, Pyrin domain, Monocytes, Proinflammatory cytokine, Pathogenesis, Mice, 03 medical and health sciences, Thioredoxins, 0302 clinical medicine, Sepsis, NLR Family, Pyrin Domain-Containing 3 Protein, medicine, Animals, Tetraspanin 30, Chemistry, Macrophages, Interleukin-18, Cell Biology, Macrophage Activation, Coculture Techniques, Microvesicles, Mice, Inbred C57BL, Disease Models, Animal, Oxidative Stress, RAW 264.7 Cells, 030104 developmental biology, 030220 oncology & carcinogenesis, Cancer research, Inflammation Mediators, medicine.symptom, Carrier Proteins, TXNIP

Abstract

Sepsis-induced myocardial dysfunction (SIMD), a deadly symptom in sepsis patients, is mainly caused by cardiovascular inflammation. However, it remains unclear how systemic inflammation triggers and aggravates cardiovascular inflammation in the pathogenesis of SIMD. This study found that proinflammatory cytokines and H2 O2 concentrations were significantly induced in SIMD-mice. In particular, a microarray analysis of CD63+ exosomes isolated from sham- and SIMD-monocytes revealed a significant induction of thioredoxin-interacting protein (TXNIP) and NLR family pyrin domain-containing 3 (NLRP3). We proved that oxidative stress caused the disassociation of the TXNIP-TRX2 (thioredoxin 2) complex and the assembly of the TXNIP-NLRP3 complex. In addition, this finding showed that the latter complex could be embedded into CD63+ exosomes and traffic from monocytes to the resident heart macrophages, where it activated caspase-1 and cleaved inactive interleukin 1β (IL-1β) and IL-18. Furthermore, using an amplified luminescent proximity homogeneous assay (Alpha) with GST-TXNIP and His-NLRP3, we obtained a small molecule named PSSM1443 that could disrupt the TXNIP-NLRP3 interaction in vitro, impairing NLRP3 downstream events. Of note, after administering PSSM1443 to the SIMD-mice, we found the small molecule could significantly suppress the activation of caspase-1 and the cleavage of pro-IL-1β and pro-IL-18, reducing inflammation in the SIMD-mice. Collectively, our results reveal that monocyte-derived exosomes harbor the overexpressed TXNIP-NLRP3 complex, which traffics from circulating monocytes to local macrophages and promotes the cleavage of inactive IL-1β and IL-18 in the macrophages, aggravating cardiovascular inflammation. PSSM1443 functions as an inhibitor of the TXNIP-NLRP3 complex and its administration can decrease inflammation in SIMD-mice.

Published

2021

33. A light-up fluorescence resonance energy transfer magnetic aptamer-sensor for ultra-sensitive lung cancer exosome detection

Author

Yao Wu, Binwu Ying, Yujia Zhang, Juan Zhou, Ke Kang, Guohao Li, Qiangying Yi, and Nanhang Zhu

Subjects

DNA, Complementary, Lung Neoplasms, Aptamer, Biomedical Engineering, Metal Nanoparticles, Nanoparticle, Biosensing Techniques, 02 engineering and technology, Exosomes, 010402 general chemistry, Sensitivity and Specificity, 01 natural sciences, Exosome, Magnetics, chemistry.chemical_compound, Quantum Dots, Fluorescence Resonance Energy Transfer, Humans, General Materials Science, Tetraspanin 30, Chemistry, Liquid Biopsy, Epithelial cell adhesion molecule, General Chemistry, General Medicine, Aptamers, Nucleotide, Epithelial Cell Adhesion Molecule, equipment and supplies, 021001 nanoscience & nanotechnology, Fluorescence, 0104 chemical sciences, Förster resonance energy transfer, Quantum dot, Biophysics, Magnetic nanoparticles, Gold, 0210 nano-technology

Abstract

In vitro liquid biopsy based on exosomes offers promising opportunities for fast and reliable detection of lung cancers. In this work, we present a fluorescence resonance energy transfer (FRET) magnetic aptamer-sensor for magnetic enrichment of exosomes with aptamers and detection of cancerous-surface proteins based on a light-up FRET strategy. Fluorescent quantum dots (QDs) and aptamers were introduced onto magnetic nanoparticles and the fluorescence emission turned down when the aptamers were paired with their complementary DNA on the surface of Au nanoparticles. Later, competitive binding of exosomes with the aptamers expelled the Au nanoparticles resulting in an exosome concentration-dependent linear increase of QD fluorescence intensity in a broad exosome concentration range (5 × 102-5 × 109 particles per mL). As found in our work, this system behaved ultra-sensitively and the calculated detection limit of this FRET magnetic aptamer-sensor was as low as 13 particles per mL. Furthermore, taking epithelial cancer-specific antigen (epithelial cell adhesion molecule, EpCAM) screening as a typical example, our built FRET magnetic aptamer-sensor allowed a rapid and efficient distinction of all the epithelial cancer cases (7 lung cancers and 5 other cancers) from health volunteers with 100% accuracy.

Published

2021

34. CD63 negatively regulates hepatocellular carcinoma development through suppression of inflammatory cytokine‐induced STAT3 activation

Author

Shijun Yu, Li Li, Jingde Chen, Yandong Li, Ming Quan, and Yong Gao

Subjects

Male, STAT3 Transcription Factor, 0301 basic medicine, Carcinoma, Hepatocellular, Carcinogenesis, proliferation, medicine.medical_treatment, Mice, Nude, Biology, migration, medicine.disease_cause, Metastasis, STAT3, 03 medical and health sciences, 0302 clinical medicine, Tetraspanin, Cell Movement, Cell Line, Tumor, CD63, medicine, Animals, Humans, Cell Proliferation, Inflammation, Mice, Inbred BALB C, Gene knockdown, Tetraspanin 30, Cell growth, Liver Neoplasms, Original Articles, hepatocellular carcinoma, Cell Biology, Middle Aged, medicine.disease, digestive system diseases, Disease Models, Animal, 030104 developmental biology, Cytokine, 030220 oncology & carcinogenesis, Hepatocellular carcinoma, Cancer research, Cytokines, Molecular Medicine, Immunohistochemistry, Female, Original Article, Inflammation Mediators, Signal Transduction

Abstract

Tetraspanin CD63 has been widely implicated in tumour progression of human malignancies. However, its role in the tumorigenesis and metastasis of hepatocellular carcinoma (HCC) remains unclear yet. In the present study, we aimed to investigate the specific function and underlying mechanisms of CD63 in HCC progression. CD63 expression in HCC tissues was detected using immunohistochemistry and quantitative real‐time PCR analyses; effects of CD63 on HCC cell proliferation and migration were investigated by CCK‐8 assay, colony formation assay, transwell assay and a xenograft model of nude mice. RNA‐sequencing, bioinformatics analysis, dual‐luciferase reporter assay and Western blot analysis were performed to explore the underlying molecular mechanisms. Results of our experiments showed that CD63 expression was frequently reduced in HCC tissues compared with adjacent normal tissues, and decreased CD63 expression was significantly associated with larger tumour size, distant site metastasis and higher tumour stages of HCC. Overexpression of CD63 inhibited HCC cell proliferation and migration, whereas knockdown of CD63 promoted these phenotypes. IL‐6, IL‐27 and STAT3 activity was regulated by CD63, and blockade of STAT3 activation impaired the promotive effects of CD63 knockdown on HCC cell growth and migration. Our findings identified a novel CD63‐IL‐6/IL‐27‐STAT3 axis in the development of HCC and provided a potential target for the diagnosis and treatment of this disease.

Published

2020

35. Positive MITF and NKI/C3 Expression in Cellular Neurothekeoma and Dermatofibroma

Author

Maram Abdaljaleel and Jeffrey P. North

Subjects

Adult, Male, Pathology, medicine.medical_specialty, Skin Neoplasms, Histology, Adolescent, Carcinogenesis, Cellular differentiation, Microphthalmia, Dermatofibroma, Neurothekeoma, Pathology and Forensic Medicine, Young Adult, stomatognathic system, Biomarkers, Tumor, Humans, Medicine, Child, Myofibroblasts, Aged, Aged, 80 and over, Microphthalmia-Associated Transcription Factor, Histiocytoma, Benign Fibrous, Tetraspanin 30, business.industry, Cell Differentiation, Middle Aged, medicine.disease, Microphthalmia-associated transcription factor, Immunohistochemistry, Myofibroblastic Differentiation, Cellular neurothekeoma, Medical Laboratory Technology, Female, business, Immunostaining

Abstract

Background Cellular neurothekeoma (CNT) is a benign mesenchymal tumor with uncertain cellular differentiation. Studies have found evidence of myofibroblastic differentiation and possible relation to dermatofibromas (DFs). As microphthalmia transcription factor (MITF) and NKI/C3 stains are routinely positive in CNT, we compared expression patterns of both markers in CNT and DF to assess their relationship. Materials and methods We assessed cases of CNT (n=25) and DFs (n=35) for histopathologic characteristics and MITF and NKI/C3 expression. Immunostaining results were classified as negative, focally positive ( 50%). At least 1 additional melanocytic marker was assessed in each case of CNT. Results Both DFs and CNTs showed a female predilection and a wide age range. Immunostaining in CNTs for MITF was positive in the vast majority (focal 68%, diffuse 24%), as was NKI/C3 (focal 72%, diffuse 24%). All DFs were MITF positive (diffuse 74%, focal 26%), and most DFs were NKI/C3 positive (focal 57%, diffuse 3%). Conclusion CNT and DF share demographic, histopathologic, and immunohistochemical features, including shared expression of MITF and NKI/C3, especially cellular DF.

Published

2020

36. Visualization of extracellular vesicles in the regenerating caudal fin blastema of zebrafish using in vivo electroporation

Author

Sachihiro Matsunaga, Takuya Sakamoto, Wataru Nakajima, Naoyuki Wada, and Shiro Ohgo

Subjects

0301 basic medicine, Biophysics, Biology, Biochemistry, Animals, Genetically Modified, Fin regeneration, Extracellular Vesicles, 03 medical and health sciences, 0302 clinical medicine, In vivo, Animals, Regeneration, Molecular Biology, Zebrafish, Tetraspanin 30, Electroporation, Regeneration (biology), Gene Transfer Techniques, Fish fin, Cell Biology, Extracellular vesicle, Zebrafish Proteins, biology.organism_classification, Cell biology, 030104 developmental biology, Microscopy, Fluorescence, 030220 oncology & carcinogenesis, Animal Fins, Blastema, Plasmids

Abstract

Zebrafish have high regenerative ability in several organs including the fin. Although various mechanisms underlying fin regeneration have been revealed, some mechanisms remain to be elucidated. Recently, extracellular vesicles (EVs) have been the focus of research with regard to their role in cell-to-cell communication. It has been suggested that cells in regenerating tissues communicate using EVs. In this study, we examined the involvement of EVs in the caudal fin regeneration of zebrafish using an in vivo electroporation method. The process of regeneration appeared normal after in vivo electroporation, and the transferred plasmid showed mosaic expression in the blastema. We took advantage of this mosaic expression to observe the distribution of exosomal markers in the blastema. We transferred exosomal markers by in vivo electroporation and identified EVs in the regenerating caudal fin. The results suggest that blastemal cells communicate with other cells via EVs during caudal fin regeneration.

Published

2020

37. CD63/81 Small Extracellular Vesicles in the Aqueous Humor are Retinoblastoma Associated.

Author

Pike S, Peng CC, Neviani P, Berry JL, and Xu L

Subjects

Humans, Aqueous Humor, Biomarkers, Tetraspanin 30, Retinoblastoma diagnosis, Extracellular Vesicles, Retinal Neoplasms diagnosis

Abstract

Purpose: Although biopsy is contraindicated in retinoblastoma (RB), the aqueous humor (AH) is a robust liquid biopsy source of molecular tumor information, facilitating biomarker discovery. Small extracellular vesicles (sEVs), promising biomarker candidates across multiple cancers, were recently identified in RB AH, but relationships between sEVs and RB clinical features are unknown., Methods: We analyzed sEVs in 37 AH samples from 18 RB eyes of varying International Intraocular Retinoblastoma Classification (IIRC) groups and explored clinical correlations. Ten samples were collected at diagnosis (DX) and 27 during treatment (Tx). Unprocessed AH underwent Single Particle-Interferometric Reflectance Imaging Sensor (SP-IRIS) analysis for fluorescent particle count and tetraspanin immunophenotyping; counts were subsequentially converted to percentages for analysis., Results: Comparing DX and Tx samples, a higher percentage of CD63/81+ sEVs was found in DX AH (16.3 ± 11.6% vs. 5.49 ± 3.67% P = 0.0009), with a more homogenous mono-CD63+ sEV population seen in Tx AH (43.5 ± 14.7% vs. 28.8 ± 9.38%, P = 0.0073). Among DX samples, CD63/81+ sEVs were most abundant in group E eyes (n = 2) compared to group D (n = 6) by count (2.75 × 105 ± 3.40 × 105 vs. 5.95 × 103 ± 8.16 × 103, P = 0.0006), and to group A + B (n = 2) by count (2.75 × 105 ± 3.40 × 105 vs. 2.73 × 102 ± 2.59 × 102, P = 0.0096) and percentage (32.1 ± 7.98% vs. 7.79 ± 0.02%, P = 0.0187)., Conclusions: CD63/81+ sEVs enrich AH from RB eyes before treatment and those with more significant tumor burden, suggesting they are tumor-derived. Future research into their cargo may reveal mechanisms of cellular communication via sEVs in RB and novel biomarkers.

Published

2023

38. A fusion of CD63–BCAR4 identified in lung adenocarcinoma promotes tumorigenicity and metastasis

Author

Jin Soo Lee, June Koo Lee, H.-G. Jung, Jin Hee Kim, Kyong-Ah Yoon, Yang-Kyu Choi, Sun-Young Kong, Kieun Bae, Young Seok Ju, Sunshin Kim, Geon Kook Lee, and Yun-Hee Kim

Subjects

Cancer Research, Lung Neoplasms, Oncogene Proteins, Fusion, Carcinogenesis, Adenocarcinoma of Lung, Biology, medicine.disease_cause, Article, Metastasis, Fusion gene, 03 medical and health sciences, Mice, 0302 clinical medicine, Cyclin D1, Cell Movement, medicine, Animals, Humans, Oncogene Fusion, 030304 developmental biology, 0303 health sciences, Gene knockdown, Oncogene, Tetraspanin 30, Oncogenes, medicine.disease, Oncology, Fusion transcript, 030220 oncology & carcinogenesis, Cancer research, Adenocarcinoma, Heterografts, RNA, Long Noncoding, KRAS, Non-small-cell lung cancer

Abstract

Background Recently, fusion variants of the breast cancer anti-oestrogen-resistance 4 (BCAR4) gene were recurrently discovered in lung adenocarcinoma from the genome-wide studies. However, the functional characterisation of BCAR4 fusion has not been investigated. Methods Based on the analysis of RNA-sequencing data, we identified a fusion transcript of CD63–BCAR4 in a Korean patient with lung adenocarcinoma who did not harbour any known activating mutations in EGFR and KRAS genes. To investigate the oncogenic effect of CD63–BCAR4, in vitro and in vivo animal experiments were performed. Results In vitro experiments showed strongly enhanced cell migration and proliferation by the exogenous expression of CD63–BCAR4 protein in bronchial epithelial cells. Cell migration was notably reduced after knockdown of BCAR4 fusion by small-interfering RNA. The tumorigenic and metastatic capability of the CD63–BCAR4 fusion was confirmed by using the mouse xenograft model. Fusion-overexpressed cells result in metastasis to the liver and lung as well as the primary tumours after subcutaneous injection into mice. Cyclin D1, MMP1, Slug and mesenchymal markers were significantly increased after CD63–BCAR4 overexpression in the in vitro and in vivo experiments. Conclusions Taken together, our results suggest a newly identified fusion gene, CD63–BCAR4 as a potential novel oncogene in lung adenocarcinoma.

Published

2020

39. Adhesion molecule cross‐linking and cytokine exposure modulate IgE‐ and non‐IgE‐dependent basophil activation

Author

Joachim Lundahl, Frida Kalm, Aman Russom, Ladan Mansouri, and Anna Nopp

Subjects

Adult, 0301 basic medicine, Adolescent, Immunology, chemical and pharmacologic phenomena, Adaptive Immunity, Basophil, Immunoglobulin E, Allergic inflammation, Young Adult, 03 medical and health sciences, 0302 clinical medicine, Immune system, Antigens, CD, parasitic diseases, Cell Adhesion, Hypersensitivity, medicine, Humans, CD62L, Immunology and Allergy, Aged, degranulation, Innate immune system, biology, Tetraspanin 30, Cell adhesion molecule, Chemistry, Endothelial Cells, hemic and immune systems, Original Articles, Middle Aged, Flow Cytometry, Acquired immune system, Immunity, Innate, miBAT, Basophils, Extracellular Matrix, Up-Regulation, Cell biology, Basophil activation, 030104 developmental biology, medicine.anatomical_structure, biology.protein, Cytokines, Original Article, CD203c, 030215 immunology

Abstract

Summary Basophils are known for their role in allergic inflammation, which makes them suitable targets in allergy diagnostics such as the basophil activation test (BAT) and the microfluidic immunoaffinity basophil activation test (miBAT). Beside their role in allergy, basophils have an immune modulatory role in both innate immunity and adaptive immunity. To accomplish this mission, basophils depend on the capability to migrate from blood to extravascular tissues, which includes interactions with endothelial cells, extracellular matrix and soluble mediators. Their receptor repertoire is well known, but less is known how these receptor–ligand interactions impact the degranulation process and the responsiveness to subsequent activation. As the consequences of these interactions are crucial to fully appreciate the role of basophils in immune modulation and to enable optimization of the miBAT, we explored how basophil activation status is regulated by cytokines and cross‐linking of adhesion molecules. The expression of adhesion molecules and activation markers on basophils from healthy blood donors was analysed by flow cytometry. Cross‐linking of CD203c, CD62L, CD11b and CD49d induced a significant upregulation of CD63 and CD203c. To mimic in vivo conditions, valid also for miBAT, CD62L and CD49d were cross‐linked followed by IgE‐dependent activation (anti‐IgE), which caused a reduced CD63 expression compared with anti‐IgE activation only. IL‐3 and IL‐33 priming caused increased CD63 expression after IgE‐independent activation (fMLP). Together, our data suggest that mechanisms operational both in the microfluidic chip and in vivo during basophil adhesion may impact basophil anaphylactic and piecemeal degranulation procedures and hence their immune regulatory function., Basophil adhesion and activation are important steps for the basophil immune modulatory functions and can be investigated with flow cytometry and microfluidics (miBAT). Cross‐linking of CD203c and the adhesion molecule CD62L, which mimics both adhesion in vivo and capture in miBAT, has a regulator effect on IgE‐mediated (anti‐IgE) basophil degranulation, by reducing the CD63 expression compared with anti‐IgE activation only. In addition, IL‐3 and IL‐33 enhance the CD63 expression on basophils after IgE‐independent (fMLP) activation compared with fMLP activation only.

Published

2020

40. Ischaemic preconditioning‐induced serum exosomes protect against myocardial ischaemia/reperfusion injury in rats by activating the <scp>PI3K</scp> / <scp>AKT</scp> signalling pathway

Author

Jie Zhang and Xijiang Zhang

Subjects

Male, 0301 basic medicine, Necrosis, Clinical Biochemistry, Apoptosis, Pharmacology, Exosomes, Biochemistry, Ventricular Function, Left, Rats, Sprague-Dawley, Phosphatidylinositol 3-Kinases, chemistry.chemical_compound, 0302 clinical medicine, Creatine Kinase, MB Form, Ischemic Preconditioning, TUNEL assay, biology, Caspase 3, General Medicine, Proto-Oncogene Proteins c-bcl-2, 030220 oncology & carcinogenesis, medicine.symptom, Signal Transduction, Morpholines, Aspartate transaminase, Myocardial Reperfusion Injury, 03 medical and health sciences, Lactate dehydrogenase, parasitic diseases, medicine, Animals, cardiovascular diseases, Protein kinase B, PI3K/AKT/mTOR pathway, Tetraspanin 30, Tumor Necrosis Factor-alpha, business.industry, Myocardium, Hemodynamics, Cell Biology, medicine.disease, Rats, 030104 developmental biology, chemistry, Chromones, biology.protein, Creatine kinase, business, Proto-Oncogene Proteins c-akt, Reperfusion injury

Abstract

Ischaemia/reperfusion (I/R) injury can lead to severe arrhythmia and aggravate myocardial damage. Exosomes are small-membrane vesicles that play a protective role in myocardial I/R injury. This study aimed to explore the protective effects of ischaemic preconditioning (IPC)-induced serum exosomes (IPC-Exo) on myocardial I/R injury in rats and its underlying mechanism. Serum exosomes were extracted from IPC rats and quantified using a bicinchoninic acid assay kit. IPC-Exo (50 μg) was injected into the infarcted myocardium immediately after ligation. Rats were randomly divided into Sham, I/R, IPC-Exo + I/R, I/R + LY294002, and I/R + IPC-Exo + LY294002 groups. Haemodynamic parameters were measured by physiological recording. Transthoracic echocardiography was used to detect cardiac function. The serum levels of creatine kinase isomer-MB, lactate dehydrogenase, aspartate transaminase, tumour necrosis factor-alpha, interleukin (IL)-1β, and IL-10 were detected by enzyme-linked immunosorbent assay. Triphenyl tetrazolium chloride staining was used to measure the myocardial infarct size. Apoptosis in myocardial tissues was detected by TUNEL staining. Western blotting was used to detect the levels of PI3K/AKT and apoptosis-related proteins. Our results showed that treatment with IPC-Exo ameliorated cardiac function and reduced inflammatory factor production, cardiomyocyte apoptosis, and myocardial infarct size. Moreover, IPC-Exo treatment promoted the protein expression of Bcl-2, p-PI3K, and p-AKT but inhibited that of caspase-3 and Bax. However, treatment with LY294002 significantly reversed that IPC-Exo-induced increase in p-PI3K and p-AKT levels, improvement of haemodynamics, and decrease of inflammatory factor production and apoptosis in the I/R + IPC-Exo group. Taken together, our results suggest that IPC-Exo may alleviate I/R injury via activating the PI3K/AKT signalling pathway.

Published

2020

41. Novel Electrochemically Switchable, Flexible, Microporous Cloth that Selectively Captures, Releases, and Concentrates Intact Extracellular Vesicles

Author

Cherie Blenkiron, Lawrence W. Chamley, Clive W. Evans, David E. Williams, Diane Brewster, Yohanes Nursalim, Valentina Lucarelli, David Barker, Alireza Akbarinejad, Saman Sabet, Colin L. Hisey, Vanessa Chang, Jadranka Travas-Sejdic, and Jesna Ashraf

Subjects

Materials science, Polymers, Tetraspanin 30, Aptamer, 010401 analytical chemistry, Electrochemical Techniques, Microporous material, Aptamers, Nucleotide, Bridged Bicyclo Compounds, Heterocyclic, 01 natural sciences, Extracellular vesicles, Electrospinning, Cell Line, 0104 chemical sciences, Extracellular Vesicles, Chemical engineering, PEDOT:PSS, MCF-7 Cells, Humans, General Materials Science, Gold, Porosity, Sulfur

Abstract

There is a significant and growing research interest in the isolation of extracellular vesicles (EVs) from large volumes of biological samples and their subsequent concentration into clean and small volumes of buffers, especially for applications in medical diagnostics. Materials that are easily incorporated into simple sampling devices and which allow the release of EVs without the need for auxiliary and hence contaminating reagents are particularly in demand. Herein, we report on the design and fabrication of a flexible, microporous, electrochemically switchable cloth that addresses the key challenges in diagnostic applications of EVs. We demonstrate the utility of our electrochemically switchable substrate for the fast, selective, nondestructive, and efficient capture and subsequent release of EVs. The substrate consists of an electrospun cloth, infused with a conducting polymer and decorated with gold particles. Utilizing gold-sulfur covalent bonding, the electrospun substrates may be functionalized with SH-terminated aptamer probes selective to EV surface proteins. We demonstrate that EVs derived from primary human dermal fibroblast (HDFa) and breast cancer (MCF-7) cell lines are selectively captured with low nonspecific adsorption using an aptamer specific to the CD63 protein expressed on the EV membranes. The specific aptamer-EV interactions enable easy removal of the nonspecifically bound material through washing steps. The conducting polymer component of the cloth provides a means for efficient (92%) and fast (5 min) electrochemical release of clean and intact captured EVs by cathodic cleavage of the Au-S bond. We demonstrate successful capture of diluted EVs from a large volume sample and their release into a small volume of clean phosphate-buffered saline buffer. The developed cloth can easily be incorporated into different designs for separation systems and would be adaptable to other biological entities including cells and other EVs. Furthermore, the capture/release capability holds great promise for liquid biopsies if used to targeted disease-specific markers.

Published

2020

42. Exosome‐mediated delivery of miR‐204‐5p inhibits tumor growth and chemoresistance

Author

Yuhang Liu, Guoying Jin, Jia Zhang, Yong Mao, Zhaohui Huang, Yaling Hu, Zhimeng Wu, Min Li, Surui Yao, Xue Wang, Yuan Yin, Dan Li, Yuyang Feng, and Zehua Bian

Subjects

Male, 0301 basic medicine, Cancer Research, Apoptosis, Cell Communication, Exosomes, Mice, 0302 clinical medicine, Genes, Tumor Suppressor, Tumor Stem Cell Assay, Original Research, Cancer Biology, Mice, Inbred BALB C, medicine.diagnostic_test, Chemistry, chemoresistance, Flow Cytometry, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, Up-Regulation, Blot, Proto-Oncogene Proteins c-bcl-2, Oncology, 030220 oncology & carcinogenesis, Heterografts, cancer therapy, Mice, Nude, colorectal cancer, Real-Time Polymerase Chain Reaction, Exosome, lcsh:RC254-282, Flow cytometry, 03 medical and health sciences, Cell Line, Tumor, medicine, Animals, Humans, exosome, Radiology, Nuclear Medicine and imaging, miR‐204‐5p, Cell Proliferation, Tetraspanin 30, Cell growth, Membrane Proteins, Microvesicles, MicroRNAs, HEK293 Cells, 030104 developmental biology, Drug Resistance, Neoplasm, rab GTP-Binding Proteins, Cell culture, Culture Media, Conditioned, Cancer cell, drug delivery, Cancer research, Receptors, Cholecystokinin

Abstract

Background Nano‐sized extracellular vesicles secreted by cells play key roles in intercellular crosstalk, and appear to be an excellent biocompatible material as therapeutic cargoes in vivo. Previously, we have demonstrated that miR‐204‐5p is a key tumor suppressor that could inhibit tumor growth, metastasis and chemoresistance. Methods A HEK293T cell line stably expressing miR‐204‐5p (293T‐miR‐204) was constructed by lentivirus transduction. Fluorescence real‐time quantitative PCR (qPCR) was applied to measure the expression of miR‐204‐5p. CCK‐8 and colony formation assays were used to evaluate the in vitro anticancer effects, and the flow cytometry was used to detect apoptosis. The in vivo therapeutic effects of exosomal miR‐204‐5p were evaluated using a xenograft mouse model. Western blots were used to detect the protein levels of CD63, Flotillin‐2, RAB22A and Bcl2. The protein levels of RAB22A and Bcl2 in tumor tissues were measured by immunohistochemistry staining. Results MiR‐204‐5p was clearly upregulated in CRC cells after coculturing with 293T‐miR‐204 cell‐derived conditioned medium (CM) or exosomes. CCK‐8 and colony formation assays showed that the cell proliferation ability of CRC cells was clearly inhibited by 293T‐miR‐204 cell‐derived CM or exosomes. The inhibitory effects of exosomal miR‐204‐5p on cell proliferation were further confirmed in other types of cancers. Exosomal miR‐204‐5p could induce apoptosis and increase the sensitivity of cancer cells to the chemotherapeutic drug—5‐fluorourcil. In addition, exosomal miR‐204‐5p inhibited the tumor growth in mice. Western blot assay and IHC staining showed that the protein levels of miR‐204‐5p targets were clearly decreased in cancer cells or xenograft tissues treated with exosomal miR‐204‐5p. Conclusions In this study, we confirmed that exosomal miR‐204‐5p could efficiently inhibit cancer cell proliferation, induce apoptosis and increase chemosensitivity by specifically suppressing the target genes of miR‐204‐5p in human cancer cells., In this study, we confirmed that exosomal miR‐204‐5p could efficiently inhibit cancer cell proliferation, induce apoptosis, and increase chemosensitivity by specifically suppressing the target genes of miR‐204‐5p in human cancer cells.

Published

2020

43. Reconstruction of cell spatial organization from single-cell RNA sequencing data based on ligand-receptor mediated self-assembly

Author

Lei Zhang, Zemin Zhang, Guojie Zhong, Xianwen Ren, Yujie Sun, and Qiming Zhang

Subjects

Cell type, Cell signaling, Bioinformatics, Pulmonary Fibrosis, T-Lymphocytes, Cell, Receptors, Cell Surface, Cell Communication, Computational biology, Biology, Ligands, T-Lymphocytes, Regulatory, Article, Transcriptome, Single-cell analysis, Neoplasms, Databases, Genetic, medicine, Humans, Pancreas, Molecular Biology, Gene, Tumor microenvironment, Tissue Inhibitor of Metalloproteinase-1, Cell Death, Sequence Analysis, RNA, Tetraspanin 30, Immunity, Reproducibility of Results, Correction, RNA, Cell Biology, Adoptive Transfer, Pulmonary Alveoli, Phenotype, medicine.anatomical_structure, Tumour immunology, Single-Cell Analysis

Abstract

Single-cell RNA sequencing (scRNA-seq) has revolutionized transcriptomic studies by providing unprecedented cellular and molecular throughputs, but spatial information of individual cells is lost during tissue dissociation. While imaging-based technologies such as in situ sequencing show great promise, technical difficulties currently limit their wide usage. Here we hypothesize that cellular spatial organization is inherently encoded by cell identity and can be reconstructed, at least in part, by ligand-receptor interactions, and we present CSOmap, a computational tool to infer cellular interaction de novo from scRNA-seq. We show that CSOmap can successfully recapitulate the spatial organization of multiple organs of human and mouse including tumor microenvironments for multiple cancers in pseudo-space, and reveal molecular determinants of cellular interactions. Further, CSOmap readily simulates perturbation of genes or cell types to gain novel biological insights, especially into how immune cells interact in the tumor microenvironment. CSOmap can be a widely applicable tool to interrogate cellular organizations based on scRNA-seq data for various tissues in diverse systems.

Published

2020

44. HPV caught in the tetraspanin web?

Author

Jérôme Finke, Lisa Hitschler, Klaus Boller, Thorsten Lang, and Luise Florin

Subjects

0301 basic medicine, Microbiology (medical), Microdomains, Immunology, Endocytic cycle, Protein nanoclustering, CD63, Papillomavirus, Virusinfektion, Pathogen endocytosis, Actin, CD151, OBSL1, Tetraspanin 24, Filamentous actin, Cell membrane, 03 medical and health sciences, 0302 clinical medicine, Tetraspanin, Viral entry, medicine, HaCaT Cells, Humans, Immunology and Allergy, Cytoskeleton, Original Investigation, Human papillomavirus 16, Microscopy, Confocal, Tetraspanin 30, Chemistry, Papillomavirus Infections, Plakins, Virion, Signal transducing adaptor protein, Hep G2 Cells, General Medicine, Virus Internalization, Actins, Endocytosis, Cell biology, Cytoskeletal Proteins, Microscopy, Electron, 030104 developmental biology, medicine.anatomical_structure, 030220 oncology & carcinogenesis, embryonic structures, HeLa Cells

Abstract

Tetraspanins are master organizers of the cell membrane. Recent evidence suggests that tetraspanins themselves may become crowded by virus particles and that these crowds/aggregates co-internalize with the viral particles. Using microscopy, we studied human papillomavirus (HPV) type 16-dependent aggregates on the cell surface of tetraspanin overexpressing keratinocytes. We find that aggregates are (1) rich in at least two different tetraspanins, (2) three-dimensional architectures extending up to several micrometers into the cell, and (3) decorated intracellularly by filamentous actin. Moreover, in cells not overexpressing tetraspanins, we note that obscurin-like protein 1 (OBSL1), which is thought to be a cytoskeletal adaptor, associates with filamentous actin. We speculate that HPV contact with the cell membrane could trigger the formation of a large tetraspanin web. This web may couple the virus contact site to the intracellular endocytic actin machinery, possibly involving the cytoskeletal adaptor protein OBSL1. Functionally, such a tetraspanin web could serve as a virus entry platform, which is co-internalized with the virus particle. Electronic supplementary material The online version of this article (10.1007/s00430-020-00683-1) contains supplementary material, which is available to authorized users.

Published

2020

45. Levels of Extracellular Vesicles in Pulmonary and Peripheral Blood Correlate with Stages of Lung Cancer Patients

Author

Young Ho Choi, Kook Nam Han, Sunghoi Hong, Hyun Koo Kim, Yu Hua Quan, Yeonho Choi, Jiyun Rho, Byeong Hyeon Choi, Ji-Ho Park, Hwan Seok Yong, and Yong Park

Subjects

Adult, Male, medicine.medical_specialty, Lung Neoplasms, Gastroenterology, Pulmonary vein, Extracellular Vesicles, 03 medical and health sciences, 0302 clinical medicine, Internal medicine, medicine, Animals, Humans, Vein, Lung cancer, Lung, Aged, Neoplasm Staging, CD63, Tetraspanin 30, business.industry, Cancer, Extracellular vesicle, Middle Aged, medicine.disease, Peripheral, Cardiac surgery, medicine.anatomical_structure, 030220 oncology & carcinogenesis, Female, 030211 gastroenterology & hepatology, Surgery, Rabbits, business

Abstract

The extracellular vesicle (EV) concentration is known to be higher in cancer patients than in healthy individuals. Herein, we report that EV levels differ in the tumor-draining pulmonary vein blood and the peripheral blood of animal models and human subjects at different pathological stages of lung cancer. Ten rabbits and 40 humans formed the study cohorts. Blood was collected from the peripheral vein of members of all groups. Pulmonary blood was collected intraoperatively from all groups except for the healthy human controls. Quantitative analysis of EV levels was performed using a nanoparticle tracking assay, a CD63 enzyme-linked immunosorbent assay, and western blotting. The EV levels in the peripheral blood of animals and patients with lung cancer were higher than those in the peripheral blood of healthy controls (p

Published

2020

46. In vitro cultured human endometrial cells release extracellular vesicles that can be uptaken by spermatozoa

Author

Sofia Makieva, Valentina Murdica, Natasa Zarovni, Elisa Giacomini, Riccardo Vago, Massimo Candiani, Andrea Salonia, Paola Viganò, Murdica, V., Giacomini, E., Makieva, S., Zarovni, N., Candiani, M., Salonia, A., Vago, R., and Vigano, P.

Subjects

Male, Cell biology, media_common.quotation_subject, Acrosome reaction, lcsh:Medicine, Filipin, Exosome, Article, chemistry.chemical_compound, Endometrium, Extracellular Vesicles, Membrane Microdomains, Medical research, Capacitation, Humans, Particle Size, Phosphorylation, Internalization, lcsh:Science, Cells, Cultured, media_common, Multidisciplinary, Endosomal Sorting Complexes Required for Transport, Tetraspanin 30, Vesicle, lcsh:R, Tyrosine phosphorylation, Sperm, Spermatozoa, Endocytosis, Cold Temperature, DNA-Binding Proteins, Calcium Ionophores, chemistry, Female, lcsh:Q, Transcription Factors

Abstract

Extracellular vesicles (EVs) derived from different parts of the male reproductive tract can be internalized by human spermatozoa affecting their maturation and regulating their functions. Here we demonstrate that EVs derived from the female tract can be uptaken by sperm and affect their competence. Primary endometrial cells release EVs with a diameter between 50 and 350 nm and bear the standard vesicle and exosome marker proteins CD63, CD9, TSG101 and ALIX. The uptake of dye-labelled endometrial cell-derived EVs by spermatozoa, quantified as fluorescence intensity, was significantly higher when EVs were derived from cells in the proliferative phase. Vital, motile fluorescent sperm could be appreciated after a 48-hour co-incubation with endometrial cells previously labelled with the Vybrant™ DiO dye. EV internalization by sperm was blocked at 4 °C and by incubation with filipin, suggesting an energy-dependent process probably attributable to the lipid-raft domain mediated-endocytosis. Sperm ability to undergo capacitation and acrosome reaction was stimulated by endometrial cell-derived EVs as manifested by the increased protein tyrosine phosphorylation and evident reactivity when stimulated with a calcium ionophore. Based on these findings, EVs exchange may be suggested as an emerging way through which female reproductive tract cells can interact with the passing spermatozoa.

Published

2020

47. A role for tetraspanin proteins in regulating fusion induced by Burkholderia thailandensis

Author

Atiga Elgawidi, Mark S. Thomas, Peter N. Monk, Amyleigh Watts, Lynda J. Partridge, Muslim Idan Mohsin, and Fawwaz Ali

Subjects

0301 basic medicine, Microbiology (medical), Burkholderia pseudomallei, Tetraspanins, Burkholderia, 030106 microbiology, Immunology, Cell, Giant Cells, Tetraspanin 29, Cell Line, Tetraspanin 28, Microbiology, Cell Fusion, Mice, 03 medical and health sciences, Tetraspanin, medicine, Animals, Immunology and Allergy, Multinucleated giant cell, Original Investigation, Mice, Knockout, Cell fusion, Burkholderia thailandensis, biology, Cell:cell fusion, Tetraspanin 30, Macrophages, Correction, General Medicine, CD9, biology.organism_classification, Recombinant Proteins, Mice, Inbred C57BL, 030104 developmental biology, medicine.anatomical_structure, Membrane protein, Melioidosis, embryonic structures, CD81

Abstract

Burkholderia pseudomallei is the causative agent of melioidosis, a disease with high morbidity that is endemic in South East Asia and northern Australia. An unusual feature of the bacterium is its ability to induce multinucleated giant cell formation (MNGC), which appears to be related to bacterial pathogenicity. The mechanism of MNGC formation is not fully understood, but host cell factors as well as known bacterial virulence determinants are likely to contribute. Since members of the tetraspanin family of membrane proteins are involved in various types of cell:cell fusion, their role in MNGC formation induced by Burkholderia thailandensis, a mildly pathogenic species closely related to B. pseudomallei, was investigated. The effect of antibodies to tetraspanins CD9, CD81, and CD63 in MNGC formation induced by B. thailandensis in infected mouse J774.2 and RAW macrophage cell lines was assessed along with that of recombinant proteins corresponding to the large extracellular domain (EC2) of the tetraspanins. B. thailandensis-induced fusion was also examined in macrophages derived from CD9 null and corresponding WT mice, and in J774.2 macrophages over-expressing CD9. Antibodies to CD9 and CD81 promoted MNGC formation induced by B. thailandensis, whereas EC2 proteins of CD9, CD81, and CD63 inhibited MNGC formation. Enhanced MNGC formation was observed in CD9 null macrophages, whereas a decrease in MNGC formation was associated with overexpression of CD9. Overall our findings show that tetraspanins are involved in MNGC formation induced by B. thailandensis and by implication, B. pseudomallei, with CD9 and CD81 acting as negative regulators of this process.

Published

2020

48. A live cell reporter of exosome secretion and uptake reveals pathfinding behavior of migrating cells

Author

Jose M. Guerrero, Roxanne Pelletier, David R. Inman, Ariana von Lersner, Suzanne M. Ponik, Evan S. Krystofiak, Bong Hwan Sung, Alissa M. Weaver, and Andries Zijlstra

Subjects

0301 basic medicine, Time Factors, Endosome, Cell Survival, Science, Green Fluorescent Proteins, General Physics and Astronomy, Membrane trafficking, Exosomes, Exosome, General Biochemistry, Genetics and Molecular Biology, Article, Fluorescence imaging, 03 medical and health sciences, Paracrine signalling, 0302 clinical medicine, Live cell imaging, Cell Movement, Cell Line, Tumor, Humans, Secretion, Cell migration, Amino Acid Sequence, Autocrine signalling, lcsh:Science, Multidisciplinary, Chemistry, Tetraspanin 30, Multivesicular Bodies, General Chemistry, Microvesicles, Cell biology, 030104 developmental biology, Cell culture, 030220 oncology & carcinogenesis, Nanoparticles, lcsh:Q, Extracellular Space

Abstract

Small extracellular vesicles called exosomes affect multiple autocrine and paracrine cellular phenotypes. Understanding the function of exosomes requires a variety of tools, including live imaging. Our previous live-cell reporter, pHluorin-CD63, allows dynamic subcellular monitoring of exosome secretion in migrating and spreading cells. However, dim fluorescence and the inability to make stably-expressing cell lines limit its use. We incorporated a stabilizing mutation in the pHluorin moiety, M153R, which now exhibits higher, stable expression in cells and superior monitoring of exosome secretion. Using this improved construct, we visualize secreted exosomes in 3D culture and in vivo and identify a role for exosomes in promoting leader–follower behavior in 2D and 3D migration. Incorporating an additional non-pH-sensitive red fluorescent tag allows visualization of the exosome lifecycle, including multivesicular body (MVB) trafficking, MVB fusion, exosome uptake and endosome acidification. This reporter will be a useful tool for understanding both autocrine and paracrine roles of exosomes., A prior live-cell exosome reporter showed dim fluorescence and could not be expressed stably, limiting its usefulness. Here the authors stabilise the reporter to allow long-term tracking of exosomes, and incorporate a second fluorophore to visualise the entire exosome lifecycle.

Published

2020

49. Spatial and temporal tracking of cardiac exosomes in mouse using a nano-luciferase-CD63 fusion protein

Author

Jiang Chang, Weijia Luo, Xiaojing Yue, Kelsey C. Andrade-Powell, Zhishi Chen, and Yuan Dai

Subjects

0301 basic medicine, Genetically modified mouse, Male, Cell biology, RNA, Untranslated, Time Factors, Recombinant Fusion Proteins, Medicine (miscellaneous), Endogeny, 030204 cardiovascular system & hematology, Biology, Exosomes, Exosome, General Biochemistry, Genetics and Molecular Biology, Article, Animals, Genetically Modified, 03 medical and health sciences, 0302 clinical medicine, Live cell imaging, Bioluminescence, Animals, Luciferase, Myocytes, Cardiac, Tissue Distribution, Luciferases, Promoter Regions, Genetic, lcsh:QH301-705.5, Cells, Cultured, Biological models, Integrases, Myosin Heavy Chains, Tetraspanin 30, Fibroblasts, Fusion protein, Microvesicles, Cardiovascular biology, Mice, Inbred C57BL, 030104 developmental biology, lcsh:Biology (General), Luminescent Measurements, Extracellular signalling molecules, General Agricultural and Biological Sciences

Abstract

Exosomes are secreted extracellular vesicles with lipid bilayer membranes. They are emerging as a new category of messengers that facilitate cross-talk between cells, tissues, and organs. Thus, a critical demand arises for the development of a sensitive and non-invasive tracking system for endogenous exosomes. We have generated a genetic mouse model that meets this goal. The Nano-luciferase (NanoLuc) reporter was fused with the exosome surface marker CD63 for exosome labeling. The cardiomyocyte-specific αMHC promoter followed by the loxP-STOP-loxP cassette was engineered for temporal and spatial labeling of exosomes originated from cardiomyocytes. The transgenic mouse was bred with a tamoxifen-inducible Cre mouse (Rosa26Cre-ERT2) to achieve inducible expression of CD63NanoLuc reporter. The specific labeling and tissue distribution of endogenous exosomes released from cardiomyocytes were demonstrated by luciferase assay and non-invasive bioluminescent live imaging. This endogenous exosome tracking mouse provides a useful tool for a range of research applications., Using nano-luciferase-CD63, Weijia Luo et al. develop transgenic mice where cardiac exosomes can be tracked with non-invasive bioluminescent live imaging in a tamoxifen-inducible manner. These mice serve as a valuable tool that allow researchers to track cardiac exosomes in a defined time window.

Published

2020

50. Fluorescent labeling of major honeybee allergens Api m 1 and Api m 2 with quantum dots and the development of a multiplex basophil activation test

Author

Rudolf Valenta, Ana Koren, Mojca Lunder, Pia Gattinger, Peter Korošec, Peter Kopač, Peter Molek, Irene Mittermann, and Abida Zahirović

Subjects

Tetraspanin 30, Chemistry, Immunology, Basophil Degranulation Test, Allergens, Bees, Immunoglobulin E, Molecular biology, Basophils, Bee Venoms, Fluorescent labelling, Basophil activation, Quantum dot, Quantum Dots, Hypersensitivity, Animals, Humans, Immunology and Allergy, Multiplex

Published

2020