Your search keyword '"death receptor signaling"' showing total 26 results

1. Quantitative proteomics reveals stage-specific protein regulation of triple negative breast cancer.

Author

Lin, Yuxiang, Lin, Ling, Fu, Fangmeng, Wang, Chuan, Hu, Anqi, Xie, Juanjuan, Jiang, Meichen, Wang, Zhenxin, Yang, Lujie, Guo, Rongrong, Yang, Pengyuan, and Shen, Huali

Abstract

Backgrounds: Triple negative breast cancer (TNBC) is a heterogeneous disease with more aggressive clinical courses than other subtypes of breast cancer. In this study, we performed high-resolution mass spectrometry-based quantitative proteomics with TNBC clinical tissue specimens to explore the early and sensitive diagnostic signatures and potential therapeutic targets for TNBC patients. Methods: We performed an iTRAQ labeling coupled LC–MS/MS approach to explore the global proteome in tumor tissues and corresponding para-tumor tissues from 24 patients with grade I-II and grade III primary TNBC. Relative peptide quantification and protein identification were performed by Proteome Discoverer™ software with Mascot search engine. Differentially expressed proteins were analyzed by bioinformatic analyses, including GO function classification annotation and KEGG enrichment analysis. Pathway analyses for protein–protein interactions and upstream regulations of differentially expressed candidates were performed by Ingenuity Pathway Analysis (IPA) software. Results: Totally, 5401 unique proteins were identified and quantified in different stage of TNBCs. 845 proteins were changed in patients with grade I or II TNBC, among which 304 were up-regulated and 541 were down-regulated. Meanwhile, for patients with grade III TNBC, 358 proteins were increased and 651 proteins were decreased. Comparing to para-cancerous tissues, various signaling pathways and metabolic processes, including PPAR pathways, PI3K-Akt pathway, one-carbon metabolism, amino acid synthesis, and lipid metabolism were activated in TNBC cancer tissues. Death receptor signaling was significantly activated in grade I-II TNBCs, however, remarkably inhibited in grade III TNBCs. Western blot experiments were conducted to validate expression levels of CYCS, HMGA1 and XIAP with samples from individual patients. Conclusions: Overall, our proteomic data presented precise quantification of potential signatures, signaling pathways, regulatory networks, and characteristic differences in each clinicopathological subgroup. The proteome provides complementary information for TNBC accurate subtype classification and therapeutic targets research. [ABSTRACT FROM AUTHOR]

Published

2021

2. Auto Arginine-GlcNAcylation Is Crucial for Bacterial Pathogens in Regulating Host Cell Death

Author

Juan Xue, Xing Pan, Ting Peng, Meimei Duan, Lijie Du, Xiaohui Zhuang, Xiaobin Cai, Xueying Yi, Yang Fu, and Shan Li

Subjects

arginine-GlcNAcylation, auto-modification, T3SS effectors, bacterial pathogen, death receptor signaling, NleB, Microbiology, QR1-502

Abstract

Many Gram-negative bacterial pathogens utilize the type III secretion system (T3SS) to inject virulence factors, named effectors, into host cells. These T3SS effectors manipulate host cellular signaling pathways to facilitate bacterial pathogenesis. Death receptor signaling plays an important role in eukaryotic cell death pathways. NleB from enteropathogenic Escherichia coli (EPEC) and SseK1/3 from Salmonella enterica serovar Typhimurium (S. Typhimurium) are T3SS effectors. They are defined as a family of arginine GlcNAc transferase to modify a conserved arginine residue in the death domain (DD) of the death receptor TNFR and their corresponding adaptors to hijack death receptor signaling. Here we identified that these enzymes, NleB, SseK1, and SseK3 could catalyze auto-GlcNAcylation. Residues, including Arg13/53/159/293 in NleB, Arg30/158/339 in SseK1, and Arg153/184/305/335 in SseK3 were identified as the auto-GlcNAcylation sites by mass spectrometry. Mutation of the auto-modification sites of NleB, SseK1, and SseK3 abolished or attenuated the capability of enzyme activity toward their death domain targets during infection. Loss of this ability led to the increased susceptibility of the cells to TNF- or TRAIL-induced cell death during bacterial infection. Overall, our study reveals that the auto-GlcNAcylation of NleB, SseK1, and SseK3 is crucial for their biological activity during infection.

Published

2020

3. Bacteria-Catalyzed Arginine Glycosylation in Pathogens and Host

Author

Xing Pan, Jie Luo, and Shan Li

Subjects

arginine glycosylation, T3SS effectors, death receptor signaling, NleB, SseK, EarP, Microbiology, QR1-502

Abstract

In recent years, protein glycosylation in pathogenic bacteria has attracted more and more attention, and accumulating evidence indicated that this type of posttranslational modification is involved in many physiological processes. The NleB from several enteropathogenic bacteria species as well as SseK from Salmonella enterica are type III secretion system effectors, which have an atypical N-acetylglucosamine (N-GlcNAc) transferase activity that specifically modified a conserved arginine in TRADD, FADD, and RIPK1. NleB/SseKs GlcNAcylation of death domain proteins abrogates homotypic and heterotypic death receptors/adaptors interactions, thereby blocking an important antimicrobial host response. Interestingly, NleB/SseKs could also GlcNAcylate themselves, and self-GlcNAcylation of NleB, SseK1, and SseK3 are crucial for their biological activity during infection. In addition, EarP (EF-P specific arginine rhamnosyl transferase for Posttranslational activation) catalyzes arginine rhamnosylation of translation elongation factor P (EF-P). Importantly, this kind of N-linked protein glycosylation is not only important for EF-P dependent rescue of polyproline stalled ribosomes but also for pathogenicity in Pseudomonas aeruginosa and other clinically relevant bacteria. Glycosylation of arginine is unique because the guanidine group of arginine has a high acid dissociation constant value and representing an extremely poor nucleophile. Recently, the crystal structures of NleB, SseKs, EarP, arginine GlcNAcylated death domain-containing proteins, NleB/FADD-DD, and EarP/EF-P/dTDP-β-L-rhamnose were solved by our group and other groups, revealing the unique catalytic mechanisms. In this review, we provide detailed information about the currently known arginine glycosyltransferases and their potential catalytic mechanisms.

Published

2020

4. Auto Arginine-GlcNAcylation Is Crucial for Bacterial Pathogens in Regulating Host Cell Death.

Author

Xue, Juan, Pan, Xing, Peng, Ting, Duan, Meimei, Du, Lijie, Zhuang, Xiaohui, Cai, Xiaobin, Yi, Xueying, Fu, Yang, and Li, Shan

Subjects

CELL death, SECRETION, SALMONELLA enterica serovar typhimurium, DEATH receptors, EUKARYOTIC cells

Abstract

Many Gram-negative bacterial pathogens utilize the type III secretion system (T3SS) to inject virulence factors, named effectors, into host cells. These T3SS effectors manipulate host cellular signaling pathways to facilitate bacterial pathogenesis. Death receptor signaling plays an important role in eukaryotic cell death pathways. NleB from enteropathogenic Escherichia coli (EPEC) and SseK1/3 from Salmonella enterica serovar Typhimurium (S. Typhimurium) are T3SS effectors. They are defined as a family of arginine GlcNAc transferase to modify a conserved arginine residue in the death domain (DD) of the death receptor TNFR and their corresponding adaptors to hijack death receptor signaling. Here we identified that these enzymes, NleB, SseK1, and SseK3 could catalyze auto-GlcNAcylation. Residues, including Arg13/53/159/293 in NleB, Arg30/158/339 in SseK1, and Arg153/184/305/335 in SseK3 were identified as the auto-GlcNAcylation sites by mass spectrometry. Mutation of the auto-modification sites of NleB, SseK1, and SseK3 abolished or attenuated the capability of enzyme activity toward their death domain targets during infection. Loss of this ability led to the increased susceptibility of the cells to TNF- or TRAIL-induced cell death during bacterial infection. Overall, our study reveals that the auto-GlcNAcylation of NleB, SseK1, and SseK3 is crucial for their biological activity during infection. [ABSTRACT FROM AUTHOR]

Published

2020

5. Bacteria-Catalyzed Arginine Glycosylation in Pathogens and Host.

Author

Pan, Xing, Luo, Jie, and Li, Shan

Subjects

ARGININE, PSEUDOMONAS aeruginosa, GLYCOSYLATION, POST-translational modification, DEATH receptors, GLYCANS, SALMONELLA enterica, PROLINE

Abstract

In recent years, protein glycosylation in pathogenic bacteria has attracted more and more attention, and accumulating evidence indicated that this type of posttranslational modification is involved in many physiological processes. The NleB from several enteropathogenic bacteria species as well as SseK from Salmonella enterica are type III secretion system effectors, which have an atypical N-acetylglucosamine (N-GlcNAc) transferase activity that specifically modified a conserved arginine in TRADD, FADD, and RIPK1. NleB/SseKs GlcNAcylation of death domain proteins abrogates homotypic and heterotypic death receptors/adaptors interactions, thereby blocking an important antimicrobial host response. Interestingly, NleB/SseKs could also GlcNAcylate themselves, and self-GlcNAcylation of NleB, SseK1, and SseK3 are crucial for their biological activity during infection. In addition, EarP (E F-P specific a rginine r hamnosyl transferase for P osttranslational activation) catalyzes arginine rhamnosylation of translation elongation factor P (EF-P). Importantly, this kind of N-linked protein glycosylation is not only important for EF-P dependent rescue of polyproline stalled ribosomes but also for pathogenicity in Pseudomonas aeruginosa and other clinically relevant bacteria. Glycosylation of arginine is unique because the guanidine group of arginine has a high acid dissociation constant value and representing an extremely poor nucleophile. Recently, the crystal structures of NleB, SseKs, EarP, arginine GlcNAcylated death domain-containing proteins, NleB/FADD-DD, and EarP/EF-P/dTDP-β-L-rhamnose were solved by our group and other groups, revealing the unique catalytic mechanisms. In this review, we provide detailed information about the currently known arginine glycosyltransferases and their potential catalytic mechanisms. [ABSTRACT FROM AUTHOR]

Published

2020

6. TP53INP2 at the crossroad of apoptosis and autophagy in death receptor signaling

Author

Saška Ivanova and Antonio Zorzano

Subjects

tp53inp2, death receptor signaling, apoptosis, autophagy, trail, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

The binding of ligands to death receptors elicits distinct outcomes, such as apoptosis, inflammation and necroptosis, depending on the cellular context. We have recently described that the autophagic protein TP53INP2 favors apoptosis upon death receptor signaling and is a potential biomarker of responsiveness to TRAIL treatment.

Published

2019

7. Workshop Summary: Cell Death Mechanisms Controlled by the TNF Family

Author

Eriksson, John E., Vandenabeele, Peter, Wallach, David, editor, Kovalenko, Andrew, editor, and Feldmann, Marc, editor

Published

2011

8. Exploring Crimean-Congo Hemorrhagic Fever Virus-Induced Hepatic Injury Using Antibody-Mediated Type I Interferon Blockade in Mice.

Author

Lindquist, Michael E., Xiankun Zeng, Altamura, Louis A., Daye, Sharon P., Delp, Korey L., Blancett, Candace, Coffin, Kayla M., Koehler, Jeffrey W., Coyne, Susan, Shoemaker, Charles J., Garrison, Aura R., and Goldena, Joseph W.

Subjects

*LIVER injuries, *CYTOKINE genetics, *HEMORRHAGIC diseases, *KUPFFER cells, *CYTOTOXIC T cells

Abstract

Crimean-Congo hemorrhagic fever virus (CCHFV) can cause severe hepatic injury in humans. However, the mechanism(s) causing this damage is poorly characterized. CCHFV produces an acute disease, including liver damage, in mice lacking type I interferon (IFN-I) signaling due to either STAT-1 gene deletion or disruption of the IFN-I receptor 1 gene. Here, we explored CCHFV-induced liver pathogenesis in mice using an antibody to disrupt IFN-I signaling. When IFN-I blockade was induced within 24 h postexposure to CCHFV, mice developed severe disease with greater than 95% mortality by 6 days postexposure. In addition, we observed increased proinflammatory cytokines, chemoattractants, and liver enzymes in these mice. Extensive liver damage was evident by 4 days postexposure and was characterized by hepatocyte necrosis and the loss of CLEC4F-positive Kupffer cells. Similar experiments in CCHFV-exposed NOD-SCID-γ (NSG), Rag2-deficient, and perforin-deficient mice also demonstrated liver injury, suggesting that cytotoxic immune cells are dispensable for hepatic damage. Some apoptotic liver cells contained viral RNA, while other apoptotic liver cells were negative, suggesting that cell death occurred by both intrinsic and extrinsic mechanisms. Protein and transcriptional analysis of livers revealed that activation of tumor necrosis factor superfamily members occurred by day 4 postexposure, implicating these molecules as factors in liver cell death. These data provide insights into CCHFV-induced hepatic injury and demonstrate the utility of antibody-mediated IFN-I blockade in the study of CCHFV pathogenesis in mice. IMPORTANCE CCHFV is an important human pathogen that is both endemic and emerging throughout Asia, Africa, and Europe. A common feature of acute disease is liver injury ranging from mild to fulminant hepatic failure. The processes through which CCHFV induces severe liver injury are unclear, mostly due to the limitations of existing small-animal systems. The only small-animal model in which CCHFV consistently produces severe liver damage is mice lacking IFN-I signaling. In this study, we used antibody-mediated blockade of IFN-I signaling in mice to study CCHFV liver pathogenesis in various transgenic mouse systems. We found that liver injury did not depend on cytotoxic immune cells and observed extensive activation of death receptor signaling pathways in the liver during acute disease. Furthermore, acute CCHFV infection resulted in a nearly complete loss of Kupffer cells. Our model system provides insight into both the molecular and the cellular features of CCHFV hepatic injury. [ABSTRACT FROM AUTHOR]

Published

2018

9. Caspase-8

Author

Schomburg, Dietmar, editor, Schomburg, Ida, editor, and Chang, Antje, editor

Published

2009

10. Sensitizing Tumor Cells by Targeting Death Receptor Signaling Inhibitors

Author

Voelkel-Johnson, Christina, Teicher, Beverly A., editor, and El-Deiry, Wafik S., editor

Published

2005

11. TP53INP2 at the crossroad of apoptosis and autophagy in death receptor signaling.

Author

Ivanova, Saška and Zorzano, Antonio

Subjects

*APOPTOSIS, *AUTOPHAGY, *DEATH receptors, *LIGANDS (Biochemistry), *BIOLOGICAL tags

Abstract

The binding of ligands to death receptors elicits distinct outcomes, such as apoptosis, inflammation and necroptosis, depending on the cellular context. We have recently described that the autophagic protein TP53INP2 favors apoptosis upon death receptor signaling and is a potential biomarker of responsiveness to TRAIL treatment. [ABSTRACT FROM AUTHOR]

Published

2019

12. Differential changes in gene expression in human neutrophils following TNF-α stimulation: Up-regulation of anti-apoptotic proteins and down-regulation of proteins involved in death receptor signaling.

Author

Chiewchengchol, Direkrit, Wright, Helen L., Thomas, Huw B., Lam, Connie W., Roberts, Kate J., Hirankarn, Nattiya, Beresford, Michael W., Moots, Robert J., and Edwards, Steven W.

Subjects

*GENE expression, *MOLECULAR genetics, *DEVELOPMENTAL stability (Genetics), *NEUTROPHILS, *GRANULOCYTES

Abstract

Responses of human neutrophils to TNF-α are complex and multifactorial. Exposure of human neutrophils to TNF-α in vitro primes the respiratory burst, delays apoptosis and induces the expression of several genes including chemokines, and TNF-α itself. This study aimed to determine the impact of TNF-α exposure on the expression of neutrophil genes and proteins that regulate apoptosis. Quantitative PCR and RNA-Seq, identified changes in expression of several apoptosis regulating genes in response to TNF-α exposure. Up-regulated genes included TNF-α itself, and several anti-apoptotic genes, including BCL2A1, CFLAR (cFLIP) and TNFAIP3, whose mRNA levels increased above control values by between 4-20 fold ( n = 3, P < 0.05). In contrast, the expression of pro-apoptotic genes, including CASP8, FADD and TNFRSF1A and TNFRSF1B, were significantly down-regulated following TNF-α treatment. These changes in mRNA levels were paralleled by decreases in protein levels of caspases 8 and 10, TRADD, FADD, TNFRSF1A and TNFRSF1B, and increased cFLIP protein levels, as detected by western blotting. These data indicate that when neutrophils are triggered by TNF-α exposure, they undergo molecular changes in transcriptional expression to up-regulate expression of specific anti-apoptotic proteins and concomitantly decrease expression of specific proteins involved in death receptor signaling which will alter their function in TNF-α rich environments. [ABSTRACT FROM AUTHOR]

Published

2016

13. How do viruses control mitochondria-mediated apoptosis?

Author

Neumann, Simon, El Maadidi, Souhayla, Faletti, Laura, Haun, Florian, Labib, Shirin, Schejtman, Andrea, Maurer, Ulrich, and Borner, Christoph

Subjects

*MITOCHONDRIA, *APOPTOSIS, *EUKARYOTIC cells, *VIRAL replication, *VIRUS diseases, *VIRAL proteins, *VIRAL antigens, *VIRUSES, *CELLULAR signal transduction

Abstract

There is no doubt that viruses require cells to successfully reproduce and effectively infect the next host. The question is what is the fate of the infected cells? All eukaryotic cells can “sense” viral infections and exhibit defence strategies to oppose viral replication and spread. This often leads to the elimination of the infected cells by programmed cell death or apoptosis. This “sacrifice” of infected cells represents the most primordial response of multicellular organisms to viruses. Subverting host cell apoptosis, at least for some time, is therefore a crucial strategy of viruses to ensure their replication, the production of essential viral proteins, virus assembly and the spreading to new hosts. For that reason many viruses harbor apoptosis inhibitory genes, which once inside infected cells are expressed to circumvent apoptosis induction during the virus reproduction phase. On the other hand, viruses can take advantage of stimulating apoptosis to (i) facilitate shedding and hence dissemination, (ii) to prevent infected cells from presenting viral antigens to the immune system or (iii) to kill non-infected bystander and immune cells which would limit viral propagation. Hence the decision whether an infected host cell undergoes apoptosis or not depends on virus type and pathogenicity, its capacity to oppose antiviral responses of the infected cells and/or to evade any attack from immune cells. Viral genomes have therefore been adapted throughout evolution to satisfy the need of a particular virus to induce or inhibit apoptosis during its life cycle. Here we review the different strategies used by viruses to interfere with the two major apoptosis as well as with the innate immune signaling pathways in mammalian cells. We will focus on the intrinsic mitochondrial pathway and discuss new ideas about how particular viruses could activately engage mitochondria to induce apoptosis of their host. [ABSTRACT FROM AUTHOR]

Published

2015

14. Aquaporin 1 suppresses apoptosis and affects prognosis in esophageal squamous cell carcinoma

Author

Tomohiro Arita, Hitoshi Fujiwara, Daisuke Ichikawa, Eigo Otsuji, Katsutoshi Shoda, Yuzo Yamazato, Hirotaka Konishi, Yoshinori Marunaka, Kazuma Okamoto, Toshiyuki Kosuga, Shuhei Komatsu, Eiichi Konishi, Takeshi Kubota, Atsushi Shiozaki, and Mitsuo Kishimoto

Subjects

0301 basic medicine, Cell physiology, cellular physiology, medicine.disease_cause, 03 medical and health sciences, death receptor signaling, 0302 clinical medicine, medicine, Carcinoma, AQP1(aquaporin 1), Survival rate, business.industry, apoptosis, medicine.disease, Primary tumor, esophageal squamous cell carcinoma, 030104 developmental biology, Oncology, Apoptosis, Tumor progression, 030220 oncology & carcinogenesis, Aquaporin 1, Cancer research, business, Carcinogenesis, Research Paper

Abstract

// Yuzo Yamazato 1, * , Atsushi Shiozaki 1, * , Daisuke Ichikawa 1, 2 , Toshiyuki Kosuga 1 , Katsutoshi Shoda 1 , Tomohiro Arita 1 , Hirotaka Konishi 1 , Shuhei Komatsu 1 , Takeshi Kubota 1 , Hitoshi Fujiwara 1 , Kazuma Okamoto 1 , Mitsuo Kishimoto 3 , Eiichi Konishi 3 , Yoshinori Marunaka 4, 5 and Eigo Otsuji 1 1 Division of Digestive Surgery, Department of Surgery, Kyoto Prefectural University of Medicine, Kyoto, 602-8566, Japan 2 Department of Gastrointestinal, Breast & Endocrine Surgery, Faculty of Medicine, University of Yamanashi, Chuo, 409-3898, Japan 3 Department of Pathology, Kyoto Prefectural University of Medicine, Kyoto, 602-8566, Japan 4 Departments of Molecular Cell Physiology and Bio-Ionomics, Graduate School of Medical Science, Kyoto Prefectural University of Medicine, Kyoto, 602-8566, Japan 5 Japan Institute for Food Education and Health, St. Agnes’ University, Kyoto, 602-8013, Japan * These authors have contributed equally to this work Correspondence to: Atsushi Shiozaki, email: shiozaki@koto.kpu-m.ac.jp Keywords: AQP1(aquaporin 1); esophageal squamous cell carcinoma; apoptosis; death receptor signaling; cellular physiology Received: January 22, 2018 Accepted: June 19, 2018 Published: July 06, 2018 ABSTRACT Aquaporin 1 (AQP1) is a membrane protein whose main function is to transfer water across cellular membranes. Recent studies have described important roles for AQP1 in epithelial carcinogenesis and tumor behavior. The objectives of the present study were to investigate the role of AQP1 in the regulation of genes involved in tumor progression and the clinicopathological significance of its expression in esophageal squamous cell carcinoma (ESCC). An immunohistochemical analysis was performed on 50 primary tumor samples underwent esophagectomy. AQP1 was primarily located in the cytoplasm and/or the nuclear membrane of carcinoma cells. The 5-year survival rate of patients with the “cytoplasm dominant” expression of AQP1 (47.1%) was significantly lower than other patients (83.2%). The depletion of AQP1 using siRNA induced apoptosis in TE5 and TE15 cells. The results of microarray analysis revealed that Death receptor signaling pathway-related genes were changed in AQP1-depleted TE5 cells. In conclusion, the results of the present study suggested that the cytoplasm dominant expression of AQP1 is related to a poor prognosis in patients with ESCC, and that it activates tumor progression by affecting Death receptor signaling pathway. These results provide insights into the role of AQP1 as a mediator of and/or a biomarker for ESCC.

Published

2018

15. Regulation of death receptor signaling by the autophagy protein TP53INP2

Author

Ivanova, Saška, Polajnar, Mira, Narbona‐Perez, Alvaro Jesus, Hernandez‐Alvarez, Maria Isabel, Frager, Petra, Slobodnyuk, Konstantin, Plana, Natalia, Nebreda, Angel R, Palacin, Manuel, Gomis, Roger R, Behrends, Christian, and Zorzano, Antonio

Published

2019

16. The SseK effector proteins of Salmonella Typhimurium target host cell signaling proteins

Author

Newson, Joshua Patrick Mark and Newson, Joshua Patrick Mark

Abstract

Pathogenic serovars of Salmonella are the causative agents of a variety of disease states, including typhoid fever, self-limiting gastroenteritis, and invasive bacteremia. To achieve infection, Salmonella relies on two type-three secretion systems (T3SS) to deliver distinct cohorts of effector proteins into host cells. These effector proteins interact with specific human proteins to subvert normal cellular processes, thus impairing the ability of host cells to respond to the invading bacteria. To date, more than 40 different effector proteins have been identified, though many remain poorly characterised. This thesis focused on the SseK family of effector proteins, which had a largely unknown molecular mechanism and role in Salmonella infection. The aim of this thesis was to identify the host proteins that are targeted by the SseK effectors in order to determine how these effectors contribute to Salmonella virulence. The SseK effectors show strong sequence similarity to NleB1, a unique T3SS effector of enteropathogenic E. coli, which functions as an arginine glycosyltransferase and catalyses the addition of N-acetylglucosamine (GlcNAc) to arginine residues of the mammalian signaling adaptors FADD and TRADD. Based on strong sequence homology to NleB1, we predicted that the SseK effectors would similarly catalyse arginine glycosylation. Here, we determined that SseK1 and SseK3, but not SseK2, also function as arginine glycosyltransferases. We showed that these effectors catalyse arginine glycosylation of different host proteins and appear to play different roles during infection. We developed a mass spectrometry-based strategy to enrich for arginine glycosylated peptides from host cells infected with Salmonella Typhimurium (S. Typhimurium). Using this approach, we identified the preferred substrate of SseK1 as the signaling adaptor TRADD, which participates in a range of innate immune signaling pathways. We also showed that overexpression of SseK1 broadens the range of

Published

2019

17. Triggering of death receptor apoptotic signaling by human papillomavirus 16 E2 protein in cervical cancer cell lines is mediated by interaction with c-FLIP.

Author

Wang, Wei, Fang, Yong, Sima, Ni, Li, Yan, Li, Wei, Li, Li, Han, Linfei, Liao, Shujie, Han, Zhiqiang, Gao, Qinglei, Li, Kezhen, Deng, Dongrui, Meng, Li, Zhou, Jianfeng, Wang, Shixuan, and Ma, Ding

Abstract

Human papillomavirus (HPV) E2 gene disruption is one of the key features of HPV-induced cervical malignant transformation. Though it is thought to prevent progression of carcinogenesis, the pro-apoptotic function of E2 protein remains poorly understood. This study shows that expression of HPV16 E2 induces apoptosis both in HPV-positive and -negative cervical cancer cell lines and leads to hyperactivation of caspase-8 and caspase-3. Activation of these signaling factors is responsible for the observed sensitivity to apoptosis upon treatment with anti-Fas antibody or TNF-α. In addition, immunoprecipitation experiments clearly show an interaction between HPV16 E2 and c-FLIP, a key regulator of apoptotic cell death mediated by death receptor signaling. Moreover, c-FLIP and a caspase-8 inhibitor protect cells from HPV16 E2-mediated apoptosis. Overexpression of c-FLIP rescues cervical cancer cells from apoptosis induced by HPV16 E2 protein expression. The data suggest that HPV16 E2 abrogates the apoptosis-inhibitory function of c-FLIP and renders the cell hypersensitive to the Fas/FasL apoptotic signal even below threshold concentration. This suggests a novel mechanism for deregulation of cervical epithelial cell growth upon HPV-induced transformation, which is of great significance in developing therapeutic strategies for intervention of cervical carcinogenesis. [ABSTRACT FROM AUTHOR]

Published

2011

18. Death à la carte The 8th European Workshop on Cell Death; June 3—8, 2012 Monêtier-les-Bains, Serre Chevalier Valley, France.

Author

Jackson, Thomas R., Larkin, Samantha E. T., Pickard, Olubukunola A., and Townsend, Paul A.

Subjects

*CONFERENCES & conventions, *CELL death

Abstract

Information on the 8th European Workshop on Cell Death (EWCD) that was held in Monêtier-les-Bains, Serre Chevalier Valley, France on June 3-8, 2012 is presented. The sessions in this bi-annual conference focused on topics such as death receptor signaling, inflammation, pattern-recognition receptors and tumor therapy. The event also featured several researchers including Conor Kearney, Stephen Tait and Sarah Pensa.

Published

2012

19. Structural and Functional Insights into Host Death Domains Inactivation by the Bacterial Arginine GlcNAcyltransferase Effector.

Author

Ding, Jingjin, Pan, Xing, Du, Lijie, Yao, Qing, Xue, Juan, Yao, Hongwei, Wang, Da-Cheng, Li, Shan, and Shao, Feng

Subjects

*BACTERIAL inactivation, *ARGININE, *CRYSTAL structure, *DEATH, *DEATH receptors

Abstract

Enteropathogenic E. coli NleB and related type III effectors catalyze arginine GlcNAcylation of death domain (DD) proteins to block host defense, but the underlying mechanism is unknown. Here we solve crystal structures of NleB alone and in complex with FADD-DD, UDP, and Mn2+ as well as NleB-GlcNAcylated DDs of TRADD and RIPK1. NleB adopts a GT-A fold with a unique helix-pair insertion to hold FADD-DD; the interface contacts explain the selectivity of NleB for certain DDs. The acceptor arginine is fixed into a cleft, in which Glu253 serves as a base to activate the guanidinium. Analyses of the enzyme-substrate complex and the product structures reveal an inverting sugar-transfer reaction and a detailed catalytic mechanism. These structural insights are validated by mutagenesis analyses of NleB-mediated GlcNAcylation in vitro and its function in mouse infection. Our study builds a structural framework for understanding of NleB-catalyzed arginine GlcNAcylation of host death domain. • Crystal structures of arginine-GlcNAcylated death domains of TRADD and RIPK1 • Crystal structures of NleB alone and in complex with FADD-DD and the ligand • Structural basis for the death-domain substrate specificity of NleB • An inverting sugar-transfer reaction and mechanisms for inactivating the arginine The NleB family of bacterial effectors blocks host inflammation by catalyzing arginine GlcNAcylation of host death-domain (DD) proteins. Ding et al. determines crystal structures of NleB, NleB in complex with FADD-DD, and NleB-GlcNAcylated TRADD-DD and RIPK1-DD. The study uncovers the mechanism for NleB substrate selectivity and an inverting sugar-transfer reaction. [ABSTRACT FROM AUTHOR]

Published

2019

20. Differential changes in gene expression in human neutrophils following TNF-α stimulation: Up-regulation of anti-apoptotic proteins and down-regulation of proteins involved in death receptor signaling

Author

Direkrit, Chiewchengchol, Helen L, Wright, Huw B, Thomas, Connie W, Lam, Kate J, Roberts, Nattiya, Hirankarn, Michael W, Beresford, Robert J, Moots, and Steven W, Edwards

Subjects

Death receptor signaling, neutrophils, TNF receptors, Original Research

Abstract

Responses of human neutrophils to TNF‐α are complex and multifactorial. Exposure of human neutrophils to TNF‐α in vitro primes the respiratory burst, delays apoptosis and induces the expression of several genes including chemokines, and TNF‐α itself. This study aimed to determine the impact of TNF‐α exposure on the expression of neutrophil genes and proteins that regulate apoptosis. Quantitative PCR and RNA‐Seq, identified changes in expression of several apoptosis regulating genes in response to TNF‐α exposure. Up‐regulated genes included TNF‐α itself, and several anti‐apoptotic genes, including BCL2A1, CFLAR (cFLIP) and TNFAIP3, whose mRNA levels increased above control values by between 4‐20 fold (n = 3, P

Published

2015

21. How do viruses control mitochondria-mediated apoptosis?

Author

Florian Haun, Shirin Labib, Ulrich Maurer, Souhayla El Maadidi, Christoph Borner, Simon Neumann, Andrea Schejtman, and Laura Faletti

Subjects

RNA viruses, Cancer Research, Programmed cell death, Death receptor signaling, Viral pathogenesis, viruses, Apoptosis, Biology, Virus Replication, Virus, Article, Immune system, Bcl-2 family, Virology, Humans, Innate immune signaling, Viral shedding, Innate immune system, fungi, Intrinsic mitochondrial signaling, food and beverages, Immunity, Innate, Cell biology, Mitochondria, Infectious Diseases, Viral replication, Host-Pathogen Interactions, Viruses

Abstract

Highlights • Viruses can block extrinsic and intrinsic apoptosis signaling of host cells. • Type I interferon response is used to either eliminate virus or induce host apoptosis. • Viruses can actively engage the apoptotic cell death machinery. • Virally infected cells are killed by CTL and NK cells., There is no doubt that viruses require cells to successfully reproduce and effectively infect the next host. The question is what is the fate of the infected cells? All eukaryotic cells can “sense” viral infections and exhibit defence strategies to oppose viral replication and spread. This often leads to the elimination of the infected cells by programmed cell death or apoptosis. This “sacrifice” of infected cells represents the most primordial response of multicellular organisms to viruses. Subverting host cell apoptosis, at least for some time, is therefore a crucial strategy of viruses to ensure their replication, the production of essential viral proteins, virus assembly and the spreading to new hosts. For that reason many viruses harbor apoptosis inhibitory genes, which once inside infected cells are expressed to circumvent apoptosis induction during the virus reproduction phase. On the other hand, viruses can take advantage of stimulating apoptosis to (i) facilitate shedding and hence dissemination, (ii) to prevent infected cells from presenting viral antigens to the immune system or (iii) to kill non-infected bystander and immune cells which would limit viral propagation. Hence the decision whether an infected host cell undergoes apoptosis or not depends on virus type and pathogenicity, its capacity to oppose antiviral responses of the infected cells and/or to evade any attack from immune cells. Viral genomes have therefore been adapted throughout evolution to satisfy the need of a particular virus to induce or inhibit apoptosis during its life cycle. Here we review the different strategies used by viruses to interfere with the two major apoptosis as well as with the innate immune signaling pathways in mammalian cells. We will focus on the intrinsic mitochondrial pathway and discuss new ideas about how particular viruses could activately engage mitochondria to induce apoptosis of their host.

Published

2014

22. Salmonella Effectors SseK1 and SseK3 Target Death Domain Proteins in the TNF and TRAIL Signaling Pathways.

Author

Newson JPM, Scott NE, Yeuk Wah Chung I, Wong Fok Lung T, Giogha C, Gan J, Wang N, Strugnell RA, Brown NF, Cygler M, Pearson JS, and Hartland EL

Subjects

Acetylglucosamine metabolism, Animals, Bacterial Proteins chemistry, Conserved Sequence, Glutamic Acid metabolism, Glycosylation, HEK293 Cells, HeLa Cells, Humans, Mice, Mice, Inbred C57BL, Mutagenesis, Mutation genetics, Protein Domains, RAW 264.7 Cells, Receptors, TNF-Related Apoptosis-Inducing Ligand metabolism, Receptors, Tumor Necrosis Factor, Type I metabolism, Substrate Specificity, TNF Receptor-Associated Death Domain Protein chemistry, TNF Receptor-Associated Death Domain Protein metabolism, Bacterial Proteins metabolism, Salmonella metabolism, Signal Transduction, TNF-Related Apoptosis-Inducing Ligand metabolism, Tumor Necrosis Factor-alpha metabolism

Abstract

Strains of Salmonella utilize two distinct type three secretion systems to deliver effector proteins directly into host cells. The Salmonella effectors SseK1 and SseK3 are arginine glycosyltransferases that modify mammalian death domain containing proteins with N -acetyl glucosamine (GlcNAc) when overexpressed ectopically or as recombinant protein fusions. Here, we combined Arg-GlcNAc glycopeptide immunoprecipitation and mass spectrometry to identify host proteins GlcNAcylated by endogenous levels of SseK1 and SseK3 during Salmonella infection. We observed that SseK1 modified the mammalian signaling protein TRADD, but not FADD as previously reported. Overexpression of SseK1 greatly broadened substrate specificity, whereas ectopic co-expression of SseK1 and TRADD increased the range of modified arginine residues within the death domain of TRADD. In contrast, endogenous levels of SseK3 resulted in modification of the death domains of receptors of the mammalian TNF superfamily, TNFR1 and TRAILR, at residues Arg 376 and Arg 293 respectively. Structural studies on SseK3 showed that the enzyme displays a classic GT-A glycosyltransferase fold and binds UDP-GlcNAc in a narrow and deep cleft with the GlcNAc facing the surface. Together our data suggest that salmonellae carrying sseK1 and sseK3 employ the glycosyltransferase effectors to antagonise different components of death receptor signaling., (© 2019 Newson et al.)

Published

2019

23. PS02.155: THE ROLE OF AQUAPORIN 1 IN ESOPHAGEAL SQUAMOUS CELL CARCINOMA.

Author

Yamazato, Yuzo, Shiozaki, Atsushi, Kosuga, Toshiyuki, Shoda, Katsutoshi, Arita, Tomohiro, Konishi, Hirotaka, Morimura, Ryo, Murayama, Yasutoshi, Kuriu, Yoshiaki, Ikoma, Hisashi, Kubota, Takeshi, Nakanishi, Masayoshi, Fujiwara, Hitoshi, Okamoto, Kazuma, Kishimoto, Mitsuo, and Otsuji, Eigo

Subjects

*SQUAMOUS cell carcinoma, *EPITHELIAL tumors, *GENETIC regulation, *CELL membranes, *CYTOPLASM

Abstract

Background Aquaporin 1 (AQP1) is a membrane protein whose main function is to transfer water via cellular membranes. Recent studies have described important roles for AQP1 in epithelial carcinogenesis and tumor behavior. The objectives of the present study were to investigate the role of AQP1 in the regulation of genes involved in tumor progression and the clinicopathological significance of its expression in esophageal squamous cell carcinoma (ESCC). Methods Immunohistochemistry for the AQP1 protein was performed to investigate the expression of AQP1 in primary tumor tissues of 50 human ESCC samples underwent curative esophagectomy. Samples were categorized into two groups according to the expression of AQP1 in each of cytoplasm and nuclear membrane, and relationships with the clinicopathological features and prognosis of ESCC patients were investigated. Next, the location of AQP1 protein in TE5, TE15, and KYSE70 cells was investigated using immunofluorescence analysis. In addition, apoptosis assay was performed in these ESCC cells and the gene expression profiles of AQP1-depleted TE5 cells was analyzed using microarray and bioinformatic studies. Results In an immunohistochemical analysis, AQP1 was primarily located in the cytoplasm and/or the nuclear membrane of carcinoma cells. The 5-year survival rate of patients with the 'cytoplasm dominant' expression of AQP1 (46.8%) was significantly lower than other patients (77.6%). A multivariate analysis of the 5-year overall survival rate showed that the pT categories and cytoplasm dominance groups of AQP1 were independent prognostic factors (P = 0.042 and 0.036, respectively). Immunofluorescence analysis revealed that AQP1 protein mainly existed in the cytoplasm in TE5 and TE15 cells. On the other hand, the expression of AQP1 in KYSE170 cells was confirmed on the nuclear membrane. The depletion of AQP1 using siRNA induced apoptosis in TE5 and TE15 cells. The results of microarray analysis revealed that Death receptor signaling pathway-related genes were changed in AQP1-depleted TE5 cells. Conclusion The results of the present study suggested that the cytoplasm dominant expression of AQP1 is related to a poor prognosis in patients with ESCC, and that it regulates tumor progression by affecting Death receptor signaling pathway. These results provide insights into the role of AQP1 as a biomarker for ESCC. Disclosure All authors have declared no conflicts of interest. [ABSTRACT FROM AUTHOR]

Published

2018

24. Role of TRAIL and the pro-apoptotic Bcl-2 homolog Bim in acetaminophen-induced liver damage

Author

Philippe Bouillet, Anastasia Badmann, Adrian Keough, Thomas Brunner, Thomas Kaufmann, and Nadia Corazza

Subjects

Cancer Research, Death receptor signaling, Liver cytology, paracetamol, TNF-Related Apoptosis-Inducing Ligand, Mice, 0302 clinical medicine, Tumor Cells, Cultured, Jun kinase, Mice, Knockout, 0303 health sciences, Bcl-2-Like Protein 11, Cell Death, Kinase, digestive, oral, and skin physiology, 3. Good health, medicine.anatomical_structure, Paracetamol, Liver, 030220 oncology & carcinogenesis, Hepatocyte, Original Article, Chemical and Drug Induced Liver Injury, medicine.drug, Programmed cell death, medicine.medical_specialty, Immunology, 610 Medicine & health, Biology, 03 medical and health sciences, Cellular and Molecular Neuroscience, death receptor signaling, Bcl-2 family, Internal medicine, Proto-Oncogene Proteins, ddc:570, medicine, Animals, Humans, Antipyretic, 030304 developmental biology, Acetaminophen, Membrane Proteins, Cell Biology, Mice, Inbred C57BL, Endocrinology, Apoptosis, Cancer research, Hepatocytes, Apoptosis Regulatory Proteins

Abstract

Acetaminophen (N-acetyl-para-aminophenol (APAP), paracetamol) is a commonly used analgesic and antipyretic agent. Although considered safe at therapeutic doses, accidental or intentional overdose causes acute liver failure characterized by centrilobular hepatic necrosis with high morbidity and mortality. Although many molecular aspects of APAP-induced cell death have been described, no conclusive mechanism has been proposed. We recently identified TNF-related apoptosis-inducing ligand (TRAIL) and c-Jun kinase(JNK)-dependent activation of the pro-apoptotic Bcl-2 homolog Bim as an important apoptosis amplification pathway in hepatocytes. In this study, we, thus, investigated the role of TRAIL, c-JNK and Bim in APAP-induced liver damage. Our results demonstrate that TRAIL strongly synergizes with APAP in inducing cell death in hepatocyte-like cells lines and primary hepatocyte. Furthermore, we found that APAP strongly induces the expression of Bim in a c-JNK-dependent manner. Consequently, TRAIL- or Bim-deficient mice were substantially protected from APAP-induced liver damage. This studyidentifies the TRAIL-JNK-Bim axis as a novel target in the treatment of APAP-induced liver damage and substantiates its general role in hepatocyte death.

Published

2011

25. Aquaporin 1 suppresses apoptosis and affects prognosis in esophageal squamous cell carcinoma.

Author

Yamazato Y, Shiozaki A, Ichikawa D, Kosuga T, Shoda K, Arita T, Konishi H, Komatsu S, Kubota T, Fujiwara H, Okamoto K, Kishimoto M, Konishi E, Marunaka Y, and Otsuji E

Abstract

Aquaporin 1 (AQP1) is a membrane protein whose main function is to transfer water across cellular membranes. Recent studies have described important roles for AQP1 in epithelial carcinogenesis and tumor behavior. The objectives of the present study were to investigate the role of AQP1 in the regulation of genes involved in tumor progression and the clinicopathological significance of its expression in esophageal squamous cell carcinoma (ESCC). An immunohistochemical analysis was performed on 50 primary tumor samples underwent esophagectomy. AQP1 was primarily located in the cytoplasm and/or the nuclear membrane of carcinoma cells. The 5-year survival rate of patients with the "cytoplasm dominant" expression of AQP1 (47.1%) was significantly lower than other patients (83.2%). The depletion of AQP1 using siRNA induced apoptosis in TE5 and TE15 cells. The results of microarray analysis revealed that Death receptor signaling pathway-related genes were changed in AQP1-depleted TE5 cells. In conclusion, the results of the present study suggested that the cytoplasm dominant expression of AQP1 is related to a poor prognosis in patients with ESCC, and that it activates tumor progression by affecting Death receptor signaling pathway. These results provide insights into the role of AQP1 as a mediator of and/or a biomarker for ESCC., Competing Interests: CONFLICTS OF INTEREST None of the authors have any conflicts of interest or financial ties to disclose.

Published

2018

26. Differential changes in gene expression in human neutrophils following TNF-α stimulation: Up-regulation of anti-apoptotic proteins and down-regulation of proteins involved in death receptor signaling.

Author

Chiewchengchol D, Wright HL, Thomas HB, Lam CW, Roberts KJ, Hirankarn N, Beresford MW, Moots RJ, and Edwards SW

Abstract

Responses of human neutrophils to TNF-α are complex and multifactorial. Exposure of human neutrophils to TNF-α in vitro primes the respiratory burst, delays apoptosis and induces the expression of several genes including chemokines, and TNF-α itself. This study aimed to determine the impact of TNF-α exposure on the expression of neutrophil genes and proteins that regulate apoptosis. Quantitative PCR and RNA-Seq, identified changes in expression of several apoptosis regulating genes in response to TNF-α exposure. Up-regulated genes included TNF-α itself, and several anti-apoptotic genes, including BCL2A1, CFLAR (cFLIP) and TNFAIP3, whose mRNA levels increased above control values by between 4-20 fold (n = 3, P < 0.05). In contrast, the expression of pro-apoptotic genes, including CASP8, FADD and TNFRSF1A and TNFRSF1B, were significantly down-regulated following TNF-α treatment. These changes in mRNA levels were paralleled by decreases in protein levels of caspases 8 and 10, TRADD, FADD, TNFRSF1A and TNFRSF1B, and increased cFLIP protein levels, as detected by western blotting. These data indicate that when neutrophils are triggered by TNF-α exposure, they undergo molecular changes in transcriptional expression to up-regulate expression of specific anti-apoptotic proteins and concomitantly decrease expression of specific proteins involved in death receptor signaling which will alter their function in TNF-α rich environments.

Published

2015