Your search keyword '"Endothelial Cells"' showing total 7,890 results

1. CircRNA_0003307 promoted brain microvascular endothelial cell angiogenesis, invasion, and migration in cerebral ischemia-reperfusion injury: Potential involvement of miRNA-191-5p/CDK6 pathway.

Author

Wu, Ying, Zheng, Zhi, Bai, Xue, Liu, Ping, Hu, Shanshan, Wang, Lingxue, and Yang, Sijing

Subjects

*ENDOTHELIAL cells, *REPERFUSION injury, *GENE transfection, *NEOVASCULARIZATION, *REPERFUSION, *CIRCULAR RNA

Abstract

• CircRNA_0003307 enhanced angiogenesis, invasion, and migration in BMECs under OGD. • CircRNA_0003307 acts as a sponge for miRNA-191-5p, preventing its binding to CDK6. • CircRNA_0003307 enhanced BMEC angiogenesis by targeting the miR-191-5p/CDK6. • CircRNA_0003307 ameliorated cerebral injury in the I/R-injured mice. The role of miR-191-5p in cerebral ischemia–reperfusion (I/R) injury has been established, with its expression in endothelial cells demonstrating anti-angiogenic effects. A potential circular RNA, circRNA_0003307, has been identified through bioinformatics analysis as a candidate for interaction with miR-191-5p, yet its functional significance in brain I/R injury remains unexplored. We aimed to investigate whether circRNA_0003307 regulates brain microvascular endothelial cell (BMEC) vascular tube formation, invasion, and migration by regulating the miR-191-5p cascade. Mouse BMECs (bEnd.3) were cultured and exposed to oxygen-glucose deprivation (OGD). The effects of circRNA_0003307 on vessel-like tube formation and cellular migration were examined. In addition, we investigated the protective effects of circRNA_0003307 on I/R injury in mice. The results showed the level of circRNA_0003307 was concentration-dependently increased in OGD-induced bEnd.3 cells. ODG-induction enhanced angiogenesis, migration, and invasion of bEnd.3 cells, which were further promoted by the transfection of pcDNA-0003307. Silencing circRNA_0003307 expression showed the opposite results. The dual luciferase assay demonstrated miRNA-191-5p interacted with circRNA_00033073′ UTR, and miRNA-191-5p could bind with CDK6. Meanwhile, circRNA_0003307 promoted the expression of CDK6 by sponging miRNA-191-5p. The overexpression of circRNA_0003307 activated the angiogenesis, migration, and invasion of OGD-induced bEnd.3 cells, which were hindered by miRNA-191-5p mimic or siRNA-CDK6. Thus, circRNA_0003307 promoted ODG-induced angiogenesis, migration, and invasion of bEnd.3 cells by targeting miR-191-5p/CDK6 axis. In vivo, circRNA_0003307 had protective effects on brain I/R injury, including neuroprotection, anti-apoptosis and angiogenesis. CircRNA_0003307 may be a promising therapeutic target for the treatment of cerebral I/R injury. [ABSTRACT FROM AUTHOR]

Published

2024

2. Endothelial metabolic control of insulin sensitivity through resident macrophages.

Author

Zhang, Jing, Sjøberg, Kim Anker, Gong, Songlin, Wang, Tongtong, Li, Fengqi, Kuo, Andrew, Durot, Stephan, Majcher, Adam, Ardicoglu, Raphaela, Desgeorges, Thibaut, Mann, Charlotte Greta, Soro Arnáiz, Ines, Fitzgerald, Gillian, Gilardoni, Paola, Abel, E. Dale, Kon, Shigeyuki, Olivares-Villagómez, Danyvid, Zamboni, Nicola, Wolfrum, Christian, and Hornemann, Thorsten

Abstract

Endothelial cells (ECs) not only form passive blood conduits but actively contribute to nutrient transport and organ homeostasis. The role of ECs in glucose homeostasis is, however, poorly understood. Here, we show that, in skeletal muscle, endothelial glucose transporter 1 (Glut1 /Slc2a1) controls glucose uptake via vascular metabolic control of muscle-resident macrophages without affecting transendothelial glucose transport. Lowering endothelial Glut1 via genetic depletion (Glut1 ΔEC) or upon a short-term high-fat diet increased angiocrine osteopontin (OPN/ Spp1) secretion. This promoted resident muscle macrophage activation and proliferation, which impaired muscle insulin sensitivity. Consequently, co-deleting Spp1 from ECs prevented macrophage accumulation and improved insulin sensitivity in Glut1 ΔEC mice. Mechanistically, Glut1- dependent endothelial glucose metabolic rewiring increased OPN in a serine metabolism-dependent fashion. Our data illustrate how the glycolytic endothelium creates a microenvironment that controls resident muscle macrophage phenotype and function and directly links resident muscle macrophages to the maintenance of muscle glucose homeostasis. [Display omitted] • EC-specific loss of Glut1 impairs insulin sensitivity in skeletal muscle • Angiocrine OPN controls resident macrophage phenotype and function • Resident macrophage accumulation and activation impair muscle insulin sensitivity • Endothelial glucose metabolic control of OPN is serine dependent Zhang et al. found that endothelial GLUT1 regulates muscle insulin sensitivity independently of transendothelial glucose transport. Lowering endothelial GLUT1 through genetic deletion or upon a short-term high-fat diet rewires endothelial glucose metabolism, thereby increasing angiocrine OPN secretion. This promotes resident macrophage accumulation and activation, which leads to muscle insulin resistance. [ABSTRACT FROM AUTHOR]

Published

2024

3. β-arrestin2 promotes angiogenesis of liver sinusoidal endothelial cells through the VEGF/VEGFR2 pathway to aggravate cirrhosis.

Author

Gao, Feng, Mu, Wei, Fan, Jiangbo, and Shen, Jing

Subjects

*GENE expression, *CIRRHOSIS of the liver, *ENDOTHELIAL cells, *EXTRACELLULAR matrix, *GENETIC code

Abstract

Excessive extracellular matrix deposition and increased intrahepatic angiogenesis are prominent features of cirrhosis. β-arrestin2 is thought to be involved in the pathological processes of various fibrotic diseases. This study aimed to investigate the role and possible mechanism of β-arrestin2 in the angiogenesis of cirrhosis. Firstly, β-arrestin2 expression in liver tissues of cirrhotic patients was detected, and the correlation between β-arrestin2 and α-SMA, CD-31, PDGF, and VEGF indexes was analyzed. Then, after liver cirrhosis induced by CCL 4 in Arrb2-KO mice (β-arrestin2 coding gene), liver histopathological changes were observed, and the expressions of α-SMA, CD-31, PDGF, VEGF, and VEGFR2 were detected. Finally, VEGF-A was used to treat human liver sinusoidal endothelial cells (LSECs) to simulate pathological conditions. After transfection with si-ARRB2, the cell activity, MDA and GSH-PX activities, cell invasion, angiogenesis, and the expressions of α-SMA, CD-31, and VEGF/VEGFR2 pathway were detected. Results showed that β-arrestin2 expression in the liver increased significantly during cirrhosis and was positively correlated with angiogenesis. In vivo , Arrb2-KO significantly inhibited fibrosis and angiogenesis in cirrhotic mice, and decreased the expressions of α-SMA, CD31, PDGF, VEGF, and VEGFR2. Studies using LSECs in vitro showed that after intervention of ARRB2, the activity of LSECs and the number of invasions and tubule formations were significantly reduced. Similarly, after transfection with si-ARRB2, the expressions of α-SMA, CD31, PDGF, VEGF, and VEGFR2 in LSECs were significantly decreased. Collectively, β-arrestin2 aggravated cirrhosis by promoting the angiogenesis of LSECs. Blocking β-arrestin2 may be an important target against angiogenesis and fibrosis in cirrhosis. [Display omitted] • β-arrestin2 expression was increased in cirrhosis and correlated with angiogenesis. • Knockout Arrb2 inhibited the progression of liver cirrhosis, reduce angiogenesis. • ARRB2 intervention inhibited the proliferation, invasion and angiogenesis of LSECs. • β-arrestin2 (Arrb2) promoted LSECs angiogenesis through the VEGF/VEGFR2 pathway. [ABSTRACT FROM AUTHOR]

Published

2024

4. Procoagulant phenotype of virus-infected pericytes is associated with portal thrombosis and intrapulmonary vascular dilations in fatal COVID-19.

Author

Cadamuro, Massimiliano, Lasagni, Alberto, Radu, Claudia Maria, Calistri, Arianna, Pilan, Matteo, Valle, Clarissa, Bonaffini, Pietro Andrea, Vitiello, Adriana, Toffanin, Serena, Venturin, Camilla, Friòn-Herrera, Yahima, Sironi, Sandro, Alessio, Maria Grazia, Previtali, Giulia, Seghezzi, Michela, Gianatti, Andrea, Strazzabosco, Mario, Strain, Alastair J., Campello, Elena, and Spiezia, Luca

Subjects

*COVID-19, *VON Willebrand factor, *ENDOTHELIAL cells, *VON Willebrand disease, *LIVER histology

Abstract

The underlying mechanisms and clinical impact of portal microthrombosis in severe COVID-19 are unknown. Intrapulmonary vascular dilation (IPVD)-related hypoxia has been described in severe liver diseases. We hypothesised that portal microthrombosis is associated with IPVD and fatal respiratory failure in COVID-19. Ninety-three patients who died from COVID-19 were analysed for portal microvascular damage (histology), IPVD (histology and chest-computed tomography, CT), and hypoxemia (arterial blood gas). Seventeen patients who died from COVID-19-unrelated pneumonia served as controls. Vascular lesions and microthrombi were phenotyped for endothelial (vWF) and pericyte (αSMA/PDGFR-β) markers, tissue factor (TF), viral spike protein and nucleoprotein (SP, NP), fibrinogen, and platelets (CD41a). Viral particles in vascular cells were assessed by transmission electron microscopy. Cultured pericytes were infected with SARS-CoV-2 to measure TF expression and tubulisation of human pulmonary microvascular endothelial cells was assessed upon vWF treatment. IPVD was present in 16/66 patients with COVID-19, with available liver and lung histology, and was associated with younger age (62 vs. 78 years-old), longer illness (25 vs. 14 days), worsening hypoxemia (PaO 2 /FiO 2 from 209 to 89), and an increased requirement for ventilatory support (63% vs. 22%) compared to COVID-19/Non-IPVD. IPVD, absent in controls, was confirmed by chest CT. COVID-19/IPVD liver histology showed portal microthrombosis in >82.5% of portal areas, with a thicker wall of αSMA/PDGFR-β+/SP+/NP+ pericytes compared with COVID-19/Non-IPVD. Thrombosed portal venules correlated with αSMA+ area, whereas infected SP+/NP+ pericytes expressed TF. SARS-CoV-2 viral particles were observed in portal pericytes. In vitro SARS-CoV-2 infection of pericytes upregulated TF and induced endothelial cells to overexpress vWF, which expanded human pulmonary microvascular endothelial cell tubules. SARS-CoV-2 infection of liver pericytes elicits a local procoagulant response associated with extensive portal microthrombosis, IPVD and worsening respiratory failure in fatal COVID-19. Vascular involvement of the liver represents a serious complication of COVID-19 infection that must be considered in the work-up of patients with long-lasting and progressively worsening respiratory failure, as it may associate with the development of intrapulmonary vascular dilations. This clinical picture is associated with a procoagulant phenotype of portal venule pericytes, which is induced by SARS-CoV-2 infection of pericytes. Both observations provide a model that may apply, at least in part, to other vascular disorders of the liver, featuring obliterative portal venopathy, similarly characterised at the clinical level by development of hypoxemia and at the histological level by phlebosclerosis and reduced calibre of the portal vein branches in the absence of cirrhosis. Moreover, our findings shed light on an overlooked player in the pathophysiology of thrombosis, i.e. pericytes, which may present a novel therapeutic target. [Display omitted] • Portal vein microthrombosis is associated with IPVD in fatal COVID-19-related hypoxia. • In thrombosed portal venules, pericytes are preponderantly infected by SARS-CoV-2. • Pericytes embedding the thrombosed portal vein radicles overexpress tissue factor. • SARS-CoV-2 induces infected pericytes to overexpress tissue factor. • Infected pericytes kindle endothelial cells to overexpress von Willebrand factor. [ABSTRACT FROM AUTHOR]

Published

2024

5. Matrix stiffness increases energy efficiency of endothelial cells.

Author

Schunk, Curtis T., Wang, Wenjun, Sabo, Lindsey N., Taufalele, Paul V., and Reinhart-King, Cynthia A.

Subjects

*EXTRACELLULAR matrix, *CELL metabolism, *ENDOTHELIAL cells, *ENERGY consumption, *FORCE & energy

Abstract

• Cells increase traction forces and energy usage with substrate stiffness. • Cells on stiffer substrates convert energy into traction forces more efficiently. • Cell behaviors are regulated by both energy production and utilization efficiency. To form blood vessels, endothelial cells rearrange their cytoskeleton, generate traction stresses, migrate, and proliferate, all of which require energy. Despite these energetic costs, stiffening of the extracellular matrix promotes tumor angiogenesis and increases cell contractility. However, the interplay between extracellular matrix, cell contractility, and cellular energetics remains mechanistically unclear. Here, we utilized polyacrylamide substrates with various stiffnesses, a real-time biosensor of ATP, and traction force microscopy to show that endothelial cells exhibit increasing traction forces and energy usage trend as substrate stiffness increases. Inhibition of cytoskeleton reorganization via ROCK inhibition resulted in decreased cellular energy efficiency, and an opposite trend was found when cells were treated with manganese to promote integrin affinity. Altogether, our data reveal a link between matrix stiffness, cell contractility, and cell energetics, suggesting that endothelial cells on stiffer substrates can better convert intracellular energy into cellular traction forces. Given the critical role of cellular metabolism in cell function, our study also suggests that not only energy production but also the efficiency of its use plays a vital role in regulating cell behaviors and may help explain how increased matrix stiffness promotes angiogenesis. [ABSTRACT FROM AUTHOR]

Published

2024

6. Enhanced vascularity in gelatin scaffolds via copper-doped magnesium–calcium silicates incorporation: In-vitro and ex-ovo insights.

Author

Salahinejad, Erfan, Muralidharan, Avaneesh, Sayahpour, Forough Azam, Kianpour, Maryam, Akbarian, Mohsen, Vashaee, Daryoosh, and Tayebi, Lobat

Subjects

*CHICKEN embryos, *CHORIOALLANTOIS, *REGENERATIVE medicine, *UMBILICAL veins, *ENDOTHELIAL cells, *BONE regeneration, *TISSUE scaffolds

Abstract

Addressing a critical challenge in current tissue-engineering practices, this study aims to enhance vascularization in 3D porous scaffolds by incorporating bioceramics laden with pro-angiogenic ions. Specifically, freeze-dried gelatin-based scaffolds were infused with sol-gel-derived powders of Cu-doped akermanite (Ca 2 MgSi2O 7) and bredigite (Ca 7 MgSi 4 O 16) at various concentrations (10, 20, and 30 wt%). The scaffolds were initially characterized for their structural integrity, biodegradability, swelling behavior, impact on physiological pH, and cytocompatibility with human umbilical vein endothelial cells (HUVECs). The silicate incorporation effectiveness in promoting vascularity was then assessed through HUVEC attachment, capillary tube formation, and ex-ovo chick embryo chorioallantoic membrane assays. The findings revealed significant improvements in both in-vitro and ex-ovo vascularity of the gelatin scaffolds upon the addition of Cu-doped akermanite. The most effective concentrations were determined to be 10 and 20 %, which led to notable HUVEC metabolic activity, a well-spread morphology with extensive peripheral filopodia and lamellipodia at 10 % and a cobblestone phenotype indicative of in-vivo endothelium at 20 % during cell attachment, the formation of complex networks of tubular structures, and robust vascularization in chick embryo development. Moving forward, the incorporation of Cu-doped akermanite into tissue-engineering scaffolds shows great potential for addressing the limitations of vascularization, especially for critical-sized bone defects, by facilitating the controlled release of pro-angiogenic and pro-osteogenic ions. [ABSTRACT FROM AUTHOR]

Published

2024

7. Novel mechanism of cyclic nucleotide crosstalk mediated by PKG-dependent proteasomal degradation of the Hsp90 client protein phosphodiesterase 3A.

Author

Zemskov, Evgeny A., Zemskova, Marina A., Xiaomin Wu, Caceres, Santiago Moreno, Delgado, David Caraballo, Yegambaram, Manivannan, Qing Lu, Panfeng Fu, Ting Wang, and Black, Stephen M.

Subjects

*MOLECULAR chaperones, *MUTANT proteins, *PROTEIN stability, *PROTEIN kinases, *ENDOTHELIAL cells

Abstract

Endothelial cAMP-specific phosphodiesterase PDE3A is one of the major negative regulators of the endothelial barrier function in acute lung injury models. However, the mechanisms underlying its regulation still need to be fully resolved. We show here that the PDE3A is a newly described client of the molecular chaperone heat shock protein 90 (hsp90). In endothelial cells (ECs), hsp90 inhibition by geldanamycin (GA) led to a disruption of the hsp90/PDE3A complex, followed by a significant decrease in PDE3A protein levels. The decrease in PDE3A protein levels was ubiquitin-proteasome-dependent and required the activity of the E3 ubiquitin ligase C terminus of Hsc70-interacting protein. GA treatment also enhanced the association of PDE3A with hsp70, which partially prevented PDE3A degradation. GA-induced decreases in PDE3A protein levels correlated with decreased PDE3 activity and increased cAMP levels in EC. We also demonstrated that protein kinase G-dependent phosphorylation of PDE3A at Ser654 can signal the dissociation of PDE3A from hsp90 and PDE3A degradation. This was confirmed by endogenous PDE3A phosphorylation and degradation in 8-Br-cGMP-or 8-CPT-cGMP- and Bay 41-8543-stimulated EC and comparisons of WT- and phospho-mimic S654D mutant PDE3A protein stability in transiently transfected HEK293 cells. In conclusion, we have identified a new mechanism of PDE3A regulation mediated by the ubiquitin-proteasome system. Further, the degradation of PDE3A is controlled by the phosphorylation of S654 and the interaction with hsp90. We speculate that targeting the PDE3A/hsp90 complex could be a therapeutic approach for acute lung injury. [ABSTRACT FROM AUTHOR]

Published

2024

8. Feto-placental and coronary endothelial genes implicated in miscarriage, congenital heart disease and stillbirth, a systematic review and meta-analysis.

Author

Kalisch-Smith, Jacinta I., Ehtisham-Uddin, Nusaybah, and Rodriguez-Caro, Helena

Abstract

The first trimester placenta is very rarely investigated for placental vascular formation in developmental or diseased contexts. Defects in placental formation can cause heart defects in the fetus, and vice versa. Determining the causality is therefore difficult as both organs develop concurrently and express many of the same genes. Here, we performed a systematic review to determine feto-placental and coronary endothelial genes implicated in miscarriages, stillbirth and congenital heart defects (CHD) from human genome wide screening studies. 4 single cell RNAseq datasets from human first/early second trimester cardiac and placental samples were queried to generate a list of 1187 endothelial genes. This broad list was cross-referenced with genes implicated in the pregnancy disorders above. 39 papers reported feto-placental and cardiac coronary endothelial genes, totalling 612 variants. Vascular gene variants were attributed to the incidence of miscarriage (8 %), CHD (4 %) and stillbirth (3 %). The most common genes for CHD (NOTCH, DST, FBN1, JAG1, CHD4), miscarriage (COL1A1, HERC1), and stillbirth (AKAP9, MYLK), were involved in blood vessel and cardiac valve formation, with roles in endothelial differentiation, angiogenesis, extracellular matrix signaling, growth factor binding and cell adhesion. NOTCH1, AKAP12, CHD4, LAMC1 and SOS1 showed greater relative risk ratios with CHD. Many of the vascular genes identified were expressed highly in both placental and heart EC populations. Both feto-placental and cardiac vascular genes are likely to result in poor endothelial cell development and function during human pregnancy that leads to higher risk of miscarriage, congenital heart disease and stillbirth. • Placental and cardiac vascular endothelial genes are associated with pregnancy-associated conditions. • 39 studies reported significant vascular genes for congenital heart defects, miscarriage and stillbirth. • Many genes were expressed in both first trimester and early second trimester coronary and placental endothelial cells. • This data verifies known vascular genes with important roles in endothelial specification and function. • This provides new gene candidates to explore in the miscarriage, congenital heart disease and stillbirth fields. [ABSTRACT FROM AUTHOR]

Published

2024

9. Angiogenesis and full thickness wound repair in a cell sheet-based vascularized skin substitute.

Author

Mauroux, Adèle, Gofflo, Sandrine, Breugnot, Josselin, Malbouyres, Marilyne, Atlas, Yoann, Ardidie-Robouant, Corinne, Marchand, Laëtitia, Monnot, Catherine, Germain, Stéphane, Bordes, Sylvie, Closs, Brigitte, Ruggiero, Florence, and Muller, Laurent

Subjects

VASCULAR endothelial growth factors, TISSUE engineering, SKIN grafting, ENDOTHELIAL cells, NEOVASCULARIZATION, WOUND healing

Abstract

Skin tissue engineering is undergoing tremendous expansion as a result from clinical needs, mandatory replacement of animal models and development of new technologies. Many approaches have been used to produce vascularized skin substitutes for grafting purposes showing the presence of capillary-like structures but with limited analysis of their in vitro maturation and plasticity. Such knowledge is however important for the development of tissue substitutes with improved implantation success as well as for validation of vascularization in vitro models, including as a readout in pharmacological analyses. For optimal interactions of cells with microenvironment and vasculature, we here used a cell sheet approach consisting in the sole production of matrix by the cells. In this context, we limited the density of endothelial cells seeded for self-assembly and rather relied on the stimulation of angiogenesis for the development of an extensive connected microvascular-like network. After detailed characterization of this network, we challenged its plasticity both during and after establishment of the skin substitute. We show that fine tuning of VEGF concentration and time of application differentially affects formation of capillary-like structures and their perivascular coverage. Furthermore, we performed a deep wound assay that displayed tissue repair and angiogenesis with unique characteristics of the physiological process. These studies demonstrate the importance of cell-derived microenvironment for the establishment of mature yet dynamic vascularized skin models allowing a wide range of pharmacological and basic investigations. The significant advancements in organ-on-chips and tissue engineering call for more relevant models including microvascularization with remodeling potential. While vascularized skin substitutes have been developed for years, focus has primarily been on the impact of microvascularization on implantation rather than on its in vitro characterization. We here developed a cell sheet-based vascularized skin substitute relying on angiogenesis, i.e. growth of vessel-like structures within the 3D model, rather than solely on endothelial cell self-assembly. We then characterized :1/ vascularization after modulation of angiogenic factor VEGF during the substitute construction; -2/ angiogenesis associated to tissue repair after deep mechanical wounding. These studies establish a solid physiologically relevant model for further investigation of skin cell interactions and in vitro wound healing. [Display omitted] [ABSTRACT FROM AUTHOR]

Published

2024

10. The regulation of the expression of prokineticin 1 and its receptors and its mechanism of action in the porcine corpus luteum.

Author

Baryla, Monika, Kaczynski, Piotr, Goryszewska-Szczurek, Ewelina, and Waclawik, Agnieszka

Subjects

*CORPUS luteum, *GENE expression, *ESTRUS, *ESTROGEN receptors, *ENDOTHELIAL cells

Abstract

Prokineticin 1 (PROK1) is an important factor in pregnancy establishment in pigs, acting at the embryo–maternal interface and the corpus luteum (CL). Estradiol-17β (E2) is the primary pregnancy recognition signal in pigs, and its effects are augmented by luteotropic prostaglandin E2 (PGE2). On the contrary, prostaglandin F2α (PGF2α) exerts mainly a luteolytic effect. The present study aimed to elucidate whether E2, PGE2, and PGF2α regulate the expression of PROK1 and its receptors in the porcine CL and to determine the PROK1 effect on luteal endothelial cells and pathways that may be involved in this regulation. The effects of E2, PGE2, and PGF2α on the expressions of PROK1 and its receptors in the CL were studied using an in vitro model of ultrathin luteal tissue explants model. Additionally, the effects of E2 and PGE2 on the PROK1 system were determined using an in vivo approach, in which the hormones were administered into the uterine lumen to imitate their secretion by embryos. Endothelial cell proliferation was measured using the colorimetric method. E2 acting via estrogen receptors simulated the mRNA and protein expressions of PROK1 and PROKR1 in CL explants in vitro (p < 0.05). The simultaneous action of E2 with PGE2 enhanced the expression of luteal PROK1 mRNA in vitro (p < 0.05). Estradiol-17β acting alone significantly increased PROK1 mRNA levels in vivo, whereas E2 simultaneously administered with PGE2 significantly elevated the PROK1 mRNA expression and PROKR1 mRNA and protein contents in CLs adjacent to uterine horns receiving hormonal infusion compared with CLs adjacent to placebo-treated uterine horns (p < 0.01). The PROK1 protein expression was significantly higher in the CLs of pigs treated with E2, PGE2, and E2 together with PGE2 than in the control group. PGF2α increased the PROK1 mRNA content in CLs on days 12 and 14 of the estrous cycle (p < 0.05). The expression of PROKR2 at the mRNA and protein levels remained unchanged in response to in vitro and in vivo treatments. PROK1 stimulated the proliferation of luteal endothelial cells by activating the MAPK, AKT, and mTOR pathways (p < 0.05). In summary, the luteal expressions of PROK1 and PROKR1 in early pregnancy are regulated by E2 and PGE2. PROK1 stimulates luteal angiogenesis by activating the MAPK, AKT, and mTOR pathways. The regulation of luteal PROK1 expression by PGF2α indicates PROK1's putative role during luteolysis. We conclude that PROK1-PROKR1 signaling supports luteal function during CL rescue in pregnancy in pigs. [Display omitted] • Luteal expressions of prokineticin 1 and PROKR1 are regulated by primary embryonic signal (estradiol) and prostaglandin E2. • Luteolytic factor (prostaglandin F2α) is a putative regulator of luteal gene PROK1 expression during luteolysis. • Prokineticin 1 contributes to angiogenesis in the porcine CL by activation of MAPK, AKT and mTOR intracellular pathways. [ABSTRACT FROM AUTHOR]

Published

2024

11. Dexmedetomidine improves mitophagy and pyroptosis through the ALKBH5/FUNDC1 axis during epidural-related maternal fever.

Author

Xiao, Fei, Yao, Hanqing, Qian, Jing, Huang, Jiayue, and Xia, Guangfa

Subjects

*PYROPTOSIS, *UMBILICAL veins, *EPIDURAL analgesia, *ENDOTHELIAL cells, *ELECTRON microscopy

Abstract

Epidural analgesia has emerged as a commonly used method for relieving labor pain. However, epidural-related maternal fever (ERMF) is characterized by a high occurrence rate and can have detrimental consequences for the well-being of both the mother and the fetus. This study aimed to investigate the functional role and underlying mechanism of dexmedetomidine (DEX) in ERMF. Ropivacaine (ROP)-induced human umbilical vein endothelial cells (HUVECs) were treated with DEX and/or transfected with ALKBH5 or FUNDC1 overexpression plasmid. qPCR and Western blot were adopted for mitophagy and pyroptosis marker protein detection. Autophagosomes were observed through electron microscopy, Caspase-1/PI double-positive cells were determined using flow cytometry. Inflammation-related factors were quantified using ELISA. The N6-methyladenosine (m6A) modification of FUNDC1 mRNA was examined using methylated RNA immunoprecipitation (MeRIP) and the binding between ALKBH5 and FUNDC1 mRNA was confirmed by RNA immunoprecipitation (RIP). In ROP-induced HUVECs, there was a significant upregulation in ALKBH5 and FUNDC1, resulting in a notable increase in inflammation, pyroptosis, and mitophagy. The administration of DEX demonstrated the ability to alleviate ROP-induced pyroptosis and promote protective mitophagy. Interestingly, DEX treatment significantly reduced the interaction between ALKBH5 and FUNDC1 mRNA, while simultaneously increasing the m6A level of FUNDC1 mRNA in ROP-treated cells. Moreover, the overexpression of FUNDC1 partially reversed the effects of ALKBH5 overexpression on mitophagy and pyroptosis in HUVECs. DEX can promote mitophagy and inhibit pyroptosis through the ALKBH5/FUNDC1 axis in ERMF, indicating its potential as a therapeutic strategy for clinical ERMF treatment. • Dexmedetomidine (DEX) enhances mitophagy and alleviates pyroptosis in ropivacaine-induced HUVECs. • DEX regulates ALKBH5-mediated m6A modification of FUNDC1 mRNA. • DEX inhibits pyroptosis through ALKBH5/FUNDC1-mediated mitophagy. [ABSTRACT FROM AUTHOR]

Published

2024

12. HuMSC-EVs Protect Endothelial Cells Against Hypoxia/Reoxygenation Injury by Inhibiting the Pannexin 1/p38-MAPK Pathway.

Author

Ma, Qian, Cai, Liwei, Zhou, Yu, and Zhang, Changyi

Subjects

*VASCULAR endothelial cells, *MITOGEN-activated protein kinases, *UMBILICAL veins, *ENDOTHELIAL cells, *UMBILICAL cord

Abstract

Vascular endothelial cell dysfunction plays an important role in myocardial ischemia–reperfusion (I/R) injury, and pannexin 1 (Panx1), an ATP-permeable channel, is closely associated with the pathophysiological processes of I/R injury. The purpose of this study was to investigate the protective effects of human umbilical cord mesenchymal stromal cell-derived extracellular vesicles (HuMSC-EVs) and the underlying mechanism in a model of I/R injury. For the cellular model of I/R injury, human umbilical vein endothelial cells (HuVECs) were exposed to hypoxia/reoxygenation (H/R) conditions. The model cells were then treated with HuMSC-EVs, and the effects on cell survival and specific signaling activities were observed. The results showed that after H/R exposure, Panx1 expression and other markers of cellular damage were increased in HuVECs. However, treatment with HuMSC-EVs inhibited the H/R-induced increase in Panx1 expression and improved HuVEC survival. Mechanistically, HuMSC-EVs were found to inhibit the p38 mitogen-activated protein kinase (MAPK)-dependent apoptosis pathway, as evidenced by increased Bcl2 expression and reductions in p38 MAPK phosphorylation, Bax expression, and cleaved-caspase 3 expression. Together our data suggest that HuMSC-EVs alleviate H/R-induced apoptosis among HuVECs by inhibiting activity of the Panx1/p38-MAPK-dependent apoptosis pathway. [ABSTRACT FROM AUTHOR]

Published

2024

13. Mitochondria-containing extracellular vesicles from mouse vs. human brain endothelial cells for ischemic stroke therapy.

Author

Dave, Kandarp M., Venna, Venugopal R., Rao, Krithika S., Stolz, Donna B., Brady, Bodhi, Quaicoe, Victoria A., Maniskas, Michael E., Hildebrand, Ella E., Green, Dawson, Chen, Mingxi, Milosevic, Jadranka, Zheng, Si-yang, Shiva, Sruti S., McCullough, Louise D., and S Manickam, Devika

Subjects

*EXTRACELLULAR vesicles, *ISCHEMIC stroke, *ENDOTHELIAL cells, *INTRAVENOUS therapy, *ARTERIAL occlusions, *OXYGEN consumption

Abstract

Ischemic stroke-induced mitochondrial dysfunction in the blood-brain barrier-forming brain endothelial cells (BECs) results in long-term neurological dysfunction post-stroke. We previously reported data from a pilot study where intravenous administration of human BEC (hBEC)-derived mitochondria-containing extracellular vesicles (EVs) showed a potential efficacy signal in a mouse middle cerebral artery occlusion (MCAo) model of stroke. We hypothesized that EVs harvested from donor species homologous to the recipient species (e.g. , mouse) may improve therapeutic efficacy, and therefore, use of mouse BEC (mBEC)-derived EVs may improve post-stroke outcomes in MCAo mice. We investigated potential differences in the mitochondria transfer of EVs derived from the same species as the recipient cell (mBEC-EVs and recipient mBECs or hBECs-EVs and recipient hBECs) vs. cross-species EVs and recipient cells (mBEC-EVs and recipient hBECs or vice versa). Our results showed that while both hBEC- and mBEC-EVs transferred EV mitochondria, mBEC-EVs outperformed hBEC-EVs in increasing ATP levels and improved recipient mBEC mitochondrial function via increasing oxygen consumption rates. mBEC-EVs significantly reduced brain infarct volume and neurological deficit scores compared to vehicle-injected MCAo mice. The superior therapeutic efficacy of mBEC-EVs in MCAo mice support the continued use of mBEC-EVs to optimize the therapeutic potential of mitochondria-containing EVs in preclinical mouse models. [Display omitted] [ABSTRACT FROM AUTHOR]

Published

2024

14. Inhibition of GBP1 alleviates pyroptosis of human pulmonary microvascular endothelial cells through STAT1/NLRP3/GSDMD pathway.

Author

Hao, Yingting, Fu, Hongxue, Li, Kaili, Zou, Xuan, Zhou, Xin, Tang, Xiyue, Liu, Chang, and Zhou, Fachun

Subjects

*ADULT respiratory distress syndrome, *CELL migration, *ENDOTHELIAL cells, *PYROPTOSIS, *CARRIER proteins

Abstract

Restoring and maintaining the function of endothelial cells is critical for acute respiratory distress syndrome (ARDS). Guanylate binding protein 1(GBP1) is proved to elevated in ARDS patients, but its role and mechanism remains unclear. The objective of this study is to investigate the internal mechanism of GBP1 in lung injury. Our study showed that when the LPS and IFN-γ induced human Pulmonary Microvascular Endothelial Cells (HPMECs) injury model was established, cell viability was significantly reduced, and the levels of GBP1 levels and inflammatory factors were significantly increased. When transfection with si-GBP1, low expression of GBP1 promoted cell proliferation and migration, and decreased the expression of downstream inflammatory factors. Furthermore, the inhibition of GBP1 significantly reduced the occurrence of cell pyroptosis and the expression of NLRP3 and STAT1. Our study indicated that GBP1 alleviates endothelial pyroptosis and inflammation through STAT1 / NLRP3/GSDMD signaling pathway, and GBP1 may be a new target in the treatment of lung injury in the future. • GBP1 was increased in Inflammation induced HPMECs. • GBP1 is the key to regulate the proliferation and migration of HPMECs. • GBP1 regulate the inflammatory response of HPMECs. • GBP1 may regulate the pyroptosis of HPMECs through regulating STAT1 and NLRP3. [ABSTRACT FROM AUTHOR]

Published

2024

15. Assessment of the Predictive Ability of Theranostics for Corneal Cross-linking in Treating Keratoconus: A Randomized Clinical Trial.

Author

Roszkowska, Anna Maria, Scorcia, Vincenzo, Mencucci, Rita, Giannaccare, Giuseppe, Lombardo, Giuseppe, Alunni Fegatelli, Danilo, Vestri, Annarita, Bifezzi, Luca, Bernava, Giuseppe Massimo, Serrao, Sebastiano, and Lombardo, Marco

Subjects

*CORNEAL cross-linking, *VISUAL acuity, *CLINICAL trials, *VITAMIN B2, *ENDOTHELIAL cells, *PHOTOREFRACTIVE keratectomy, *CORNEAL transplantation

Abstract

To validate the ability of theranostic imaging biomarkers in assessing corneal cross-linking (CXL) efficacy in flattening the maximum keratometry (K max) index. Prospective, randomized, multicenter, masked clinical trial (ClinicalTrails.gov identifier, NCT05457647). Fifty patients with progressive keratoconus. Participants were stratified to undergo epithelium-off (25 eyes) and epithelium-on (25 eyes) CXL protocols using an ultraviolet A (UV-A) medical device with theranostic software. The device controlled UV-A light both for performing CXL and assessing the corneal riboflavin concentration (riboflavin score) and treatment effect (theranostic score). A 0.22% riboflavin formulation was applied onto the cornea for 15 minutes and 20 minutes in epithelium-off and epithelium-on protocols, respectively. All eyes underwent 9 minutes of UV-A irradiance at 10 mW/cm2. The primary outcome measure was validation of the combined use of theranostic imaging biomarkers through measurement of their accuracy (proportion of correctly classified eyes) and precision (positive predictive value) to classify eyes correctly and predict a K max flattening at 1 year after CXL. Other outcome measures included change in K max , endothelial cell density, uncorrected and corrected distance visual acuity, manifest spherical equivalent refraction and central corneal thickness 1 year after CXL. Accuracy and precision of the theranostic imaging biomarkers in predicting eyes that had >0.1 diopter (D) of K max flattening at 1 year were 91% and 95%, respectively. The K max value significantly flattened by a median of –1.3 D (IQR, –2.11 to –0.49 D; P < 0.001); both the uncorrected and corrected distance visual acuity improved by a median of –0.1 logarithm of the minimum angle of resolution (logMAR; IQR, –0.3 to 0.0 logMAR [ P < 0.001] and –0.2 to 0.0 logMAR [ P < 0.001], respectively). No significant changes in endothelial cell density (P = 0.33) or central corneal thickness (P = 0.07) were noted 1 year after surgery. The study demonstrated the efficacy of integrating theranostics in a UV-A medical device for the precise and predictive treatment of keratoconus with epithelium-off and epithelium-on CXL protocols. Concentration of riboflavin and its UV-A light mediated photoactivation in the cornea are the primary factors determining CXL efficacy. Proprietary or commercial disclosure may be found in the Footnotes and Disclosures at the end of this article. [ABSTRACT FROM AUTHOR]

Published

2024

16. Ultrasound Induces Similar Temporal Endothelial Expression Patterns of eNOS and KLF2 as Normal Flow.

Author

Sahni, Jaideep, McCue, Ian S., Johnson, Adam R., Schake, Morgan A., Sotelo, Luz D., Turner, Joseph A., and Pedrigi, Ryan M.

Subjects

*VASCULAR endothelial cells, *GENE expression, *SOUND pressure, *KRUPPEL-like factors, *NITRIC-oxide synthases

Abstract

To determine the sensitivity of vascular endothelial cells to long durations of low-intensity pulsed ultrasound (LIPUS) compared to normal flow and identify the duration that maximizes expression of two mechanosensitive genes related to healthy endothelial function, endothelial nitric oxide synthase (eNOS) and Krüppel-like factor 2 (KLF2). Custom ultrasound exposure tanks were developed and the acoustic field was characterized. Human umbilical vein endothelial cells were seeded into culture plates and exposed to LIPUS at a frequency of 1 MHz and acoustic pressure of 217 kPa for 20 min, 1 h, 6 h, 9 h, or 24 h. As a comparator, other cells were exposed to normal flow. RT-qPCR was used to assess mRNA expression of eNOS and KLF2. Maximum eNOS and KLF2 expression occurred at 6 h and was localized to the beam path. Both genes exhibited qualitatively similar patterns of expression under LIPUS compared to normal flow. LIPUS induced a more rapid beneficial response compared to normal flow, but flow induced higher expression of both genes. eNOS expression after 6 h of LIPUS was dependent on RNA yield and culture duration prior to experiments. Endothelial cells exposed to longer durations of LIPUS than typically employed exhibited greater expression of beneficial genes. The temporal gene expression patterns resulting from LIPUS and normal flow suggest activation of similar signaling pathways. However, LIPUS also caused increased RNA yield that may be linked to proliferation, which would suggest more of a wound healing than atheroprotective phenotype. [ABSTRACT FROM AUTHOR]

Published

2024

17. Siglec-5 as a novel receptor mediates endothelial cells oxLDL transcytosis to promote atherosclerosis.

Author

Jia, Xiong, Bai, Xiangli, Yin, Zhiqiang, Zheng, Qijun, Zhao, Yin, Lu, Yajing, Shu, Yan, Wang, Yayu, Zhang, Yifei, and Jin, Si

Abstract

Excessive subendothelial retention of oxidized low-density lipoprotein (oxLDL) and subsequent oxLDL engulfment by macrophages leads to the formation of foam cells and the development of atherosclerosis. Our previous study showed that the plasma level of sialic acid-binding immunoglobulin-like lectin 5 (Siglec-5) was a novel biomarker for the prognosis of atherosclerosis in diabetic patients. However, the role and underlying mechanisms of Siglec-5 in atherosclerosis have not been elucidated. The interaction between oxLDL and Siglec-5 was detected by fluorescence colocalization and coimmunoprecipitation. The effect of oxLDL on Siglec-5 expression was detected in endothelial cells and macrophages, and the effect of Siglec-5 on oxLDL transcytosis and uptake was investigated. Siglec-5 was overexpressed in mice using recombinant adeno-associated virus vector serotype 9 (rAAV9-Siglec-5) to evaluate the effect of Siglec-5 on oxLDL uptake and atherogenesis in vivo. In addition, the effects of Siglec-5 antibodies and soluble Siglec-5 proteins on oxLDL transcytosis and uptake and their role in atherogenesis were investigated in vivo and in vitro. We found that oxLDL interacted with Siglec-5 and that oxLDL stimulated the expression of Siglec-5. Siglec-5 promotes the transcytosis and uptake of oxLDL, while both anti-Siglec-5 antibodies and soluble Siglec-5 protein attenuated oxLDL transcytosis and uptake. Interestingly, overexpression of Siglec-5 by recombinant adeno-associated viral vector serotype 9 (rAAV9-Siglec-5) promoted the retention of oxLDL in the aorta of C57BL/6 mice. Moreover, overexpression of Siglec-5 significantly accelerated the formation of atherosclerotic lesions in Apoe−/− mice. Moreover, both anti-Siglec-5 antibodies and soluble Siglec-5 protein significantly alleviated the retention of oxLDL in the aorta of rAAV9-Siglec-5-transfected C57BL/6 mice and the formation of atherosclerotic plaques in rAAV9-Siglec-5-transfected Apoe−/− mice. Our results suggested that Siglec-5 was a novel receptor that mediated oxLDL transcytosis and promoted the formation of foam cells. Interventions that inhibit the interaction between oxLDL and Siglec-5, including anti-Siglec-5 antibody or soluble Siglec-5 protein treatment, may provide novel therapeutic strategies in treating atherosclerosis. [ABSTRACT FROM AUTHOR]

Published

2024

18. Oligomeric Tau-induced oxidative damage and functional alterations in cerebral endothelial cells: Role of RhoA/ROCK signaling pathway.

Author

Hossen, Faruk, Sun, Grace Y., and Lee, James C.

Subjects

*OCCLUDINS, *ENDOTHELIAL cells, *MONONUCLEAR leukocytes, *CELLULAR signal transduction, *ALZHEIMER'S disease, *TIGHT junctions

Abstract

Despite of yet unknown mechanism, microvascular deposition of oligomeric Tau (oTau) has been implicated in alteration of the Blood-Brain Barrier (BBB) function in Alzheimer's disease (AD) brains. In this study, we employed an in vitro BBB model using primary mouse cerebral endothelial cells (CECs) to investigate the mechanism underlying the effects of oTau on BBB function. We found that exposing CECs to oTau induced oxidative stress through NADPH oxidase, increased oxidative damage to proteins, decreased proteasome activity, and expressions of tight junction (TJ) proteins including occludin, zonula occludens-1 (ZO-1) and claudin-5. These effects were suppressed by the pretreatment with Fasudil, a RhoA/ROCK signaling inhibitor. Consistent with the biochemical alterations, we found that exposing the basolateral side of CECs to oTau in the BBB model disrupted the integrity of the BBB, as indicated by an increase in FITC-dextran transport across the model, and a decrease in trans endothelial electrical resistance (TEER). oTau also increased the transmigration of peripheral blood mononuclear cells (PBMCs) in the BBB model. These functional alterations in the BBB induced by oTau were also suppressed by Fasudil. Taken together, our findings suggest that targeting the RhoA/ROCK pathway can be a potential therapeutic strategy to maintain BBB function in AD. [Display omitted] • Oligomeric Tau (oTau) induces oxidative stress and impairs function in cerebral endothelial cells. • Inhibition of the RhoA/ROCK pathway mitigates the effects of oTau on CECs. • Targeting the Rho/ROCK pathway can be therapeutic strategy to maintain blood-brain barrier function in Alzheimer's disease. [ABSTRACT FROM AUTHOR]

Published

2024

19. Inflammatory lung injury is associated with endothelial cell mitochondrial fission and requires the nitration of RhoA and cytoskeletal remodeling.

Author

Pokharel, Marissa D., Fu, Panfeng, Garcia-Flores, Alejandro, Yegambaram, Manivannan, Lu, Qing, Sun, Xutong, Unwalla, Hoshang, Aggarwal, Saurabh, Fineman, Jeffrey R., Wang, Ting, and Black, Stephen M.

Subjects

*MITOCHONDRIAL dynamics, *LUNG injuries, *ENDOTHELIAL cells, *NITRATION, *CYTOSKELETON, *NICOTINAMIDE

Abstract

Higher levels of extracellular nicotinamide phosphoribosyltransferase (eNAMPT), a TLR4 agonist, are associated with poor clinical outcomes in sepsis-induced acute lung injury (ALI). Little is known regarding the mechanisms by which eNAMPT is involved in ALI. Our recent work has identified a crucial role for mitochondrial dysfunction in ALI. Thus, this study aimed to determine if eNAMPT-mediated inflammatory injury is associated with the loss of mitochondrial function. Our data show that eNAMPT disrupted mitochondrial bioenergetics. This was associated with cytoskeleton remodeling and the loss of endothelial barrier integrity. These changes were associated with enhanced mitochondrial fission and blocked when Rho-kinase (ROCK) was inhibited. The increases in mitochondrial fission were also associated with the nitration-mediated activation of the small GTPase activator of ROCK, RhoA. Blocking RhoA nitration decreased eNAMPT-mediated mitochondrial fission and endothelial barrier dysfunction. The increase in fission was linked to a RhoA-ROCK mediated increase in Drp1 (dynamin-related protein 1) at serine(S)616. Another TLR4 agonist, lipopolysaccharide (LPS), also increased mitochondrial fission in a Drp1 and RhoA-ROCK-dependent manner. To validate our findings in vivo , we challenged C57BL/6 mice with eNAMPT in the presence and absence of the Drp1 inhibitor, Mdivi-1. Mdivi-1 treatment protected against eNAMPT-induced lung inflammation, edema, and lung injury. These studies demonstrate that mitochondrial fission-dependent disruption of mitochondrial function is essential in TLR4-mediated inflammatory lung injury and identify a key role for RhoA-ROCK signaling. Reducing mitochondrial fission could be a potential therapeutic strategy to improve ARDS outcomes. [Display omitted] • eNAMPT disrupts endothelial barrier integrity and mitochondrial function in pulmonary endothelial cells. • Mitochondrial fission induced by eNAMPT depends on actin cytoskeleton remodeling via Rho-kinase (ROCK). • eNAMPT increases superoxide generation, subsequently activating the small GTPase activator of ROCK (RhoA) via nitration. • Activation of RhoA contributes to the effects of eNAMPT on mitochondrial network dynamics through the activation of Drp1. • Drp1 inhibition is protective against eNAMPT-induced inflammatory lung injury in mice. [ABSTRACT FROM AUTHOR]

Published

2024

20. Visualizing hydrogen peroxide and nitric oxide dynamics in endothelial cells using multispectral imaging under controlled oxygen conditions.

Author

Altun, Hamza Yusuf, Secilmis, Melike, Yang, Fan, Akgul Caglar, Tuba, Vatandaslar, Emre, Toy, Muhammed Fatih, Vilain, Sven, Mann, Giovanni E., Öztürk, Gürkan, and Eroglu, Emrah

Subjects

*ENDOTHELIAL cells, *NITRIC oxide, *MULTISPECTRAL imaging, *HYDROGEN peroxide, *TEMPERATURE control, *OXYGEN, *DRUG therapy

Abstract

The complex interplay between hydrogen peroxide (H 2 O 2) and nitric oxide (NO) in endothelial cells presents challenges due to technical limitations in simultaneous measurement, hindering the elucidation of their direct relationship. Previous studies have yielded conflicting findings regarding the impact of H 2 O 2 on NO production. To address this problem, we employed genetically encoded biosensors, HyPer7 for H 2 O 2 and geNOps for NO, allowing simultaneous imaging in single endothelial cells. Optimization strategies were implemented to enhance biosensor performance, including camera binning, temperature regulation, and environmental adjustments to mimic physiological normoxia. Our results demonstrate that under ambient oxygen conditions, H 2 O 2 exhibited no significant influence on NO production. Subsequent exploration under physiological normoxia (5 kPa O 2) revealed distinct oxidative stress levels characterized by reduced basal HyPer7 signals, enhanced H 2 O 2 scavenging kinetics, and altered responses to pharmacological treatment. Investigation of the relationship between H 2 O 2 and NO under varying oxygen conditions revealed a lack of NO response to H 2 O 2 under hyperoxia (18 kPa O 2) but a modest NO response under physiological normoxia (5 kPa O 2). Importantly, the NO response was attenuated by l -NAME, suggesting activation of eNOS by endogenous H 2 O 2 generation upon auranofin treatment. Our study highlights the intricate interplay between H 2 O 2 and NO within the endothelial EA.hy926 cell line, emphasizing the necessity for additional research within physiological contexts due to differential response observed under physiological normoxia (5 kPa O 2). This further investigation is essential for a comprehensive understanding of the H 2 O 2 and NO signaling considering the physiological effects of ambient O 2 levels involved. [Display omitted] • Co-expressing HyPer7 and O-geNOps enable multichromatic imaging of H 2 O 2 and NO in endothelial cells. • Exogenous H 2 O 2 does not affect NO levels under hyperoxic and normoxic conditions. • Endogenous H 2 O 2 generation has minimal NO impact under normoxic conditions. [ABSTRACT FROM AUTHOR]

Published

2024

21. Endothelial and macrophage interactions in the angiogenic niche.

Author

Shah, Fahad Hassan and Lee, Heon-Woo

Subjects

*CELL communication, *HEMATOPOIESIS, *GENETIC engineering, *THERAPEUTICS, *ENGINEERING models

Abstract

The interactions between vascular cells, especially endothelial cells, and macrophages play a pivotal role in maintaining the subtle balance of vascular biology, which is crucial for angiogenesis in both healthy and diseased states. These cells are central to ensuring a harmonious balance between tissue repair and preventing excessive angiogenic activity, which could lead to pathological conditions. Recent advances in sophisticated genetic engineering vivo models and novel sequencing approaches, such as single-cell RNA-sequencing, in immunobiology have significantly enhanced our understanding of the gene expression and behavior of macrophages. These insights offer new perspectives on the role macrophages play not only in development but also across various health conditions. In this review, we explore the complex interactions between multiple types of macrophages and endothelium, focusing on their impact on new blood vessel formation. By understanding these intricate interactions, we aim to provide insights into new methods for managing angiogenesis in various diseases, thereby offering hope for the development of novel therapeutic approaches. [Display omitted] • Endothelial cells (ECs) and macrophages are crucial in maintaining vascular biology's balance. • Macrophages are involved in the initiation, extension, pruning, and maturation of angiogenesis. • Venous ECs are progenitors for ECs in angiogenesis; perivascular macrophages reside selectively around venous vessels. • Macrophages represent an attractive therapeutic target for the treatment of vascular-associated diseases. [ABSTRACT FROM AUTHOR]

Published

2024

22. DNA methyltransferase isoforms regulate endothelial cell exosome proteome composition.

Author

Vasishta, Sampara, Ammankallu, Shruthi, Umakanth, Shashikiran, Keshava Prasad, Thottethodi Subrahmanya, and Joshi, Manjunath B.

Subjects

*ENDOTHELIAL cells, *EXOSOMES, *CELL physiology, *METHYLTRANSFERASES, *GENE expression, *DEOXYRIBOZYMES, *PROTEIN-protein interactions, *DNA methyltransferases

Abstract

Extrinsic and intrinsic pathological stimuli in vascular disorders induce DNA methylation based epigenetic reprogramming in endothelial cells, which leads to perturbed gene expression and subsequently results in endothelial dysfunction (ED). ED is also characterized by release of exosomes with altered proteome leading to paracrine interactions in vasculature and subsequently contributing to manifestation, progression and severity of vascular complications. However, epigenetic regulation of exosome proteome is not known. Hence, our present study aimed to understand influence of DNA methylation on exosome proteome composition and their influence on endothelial cell (EC) function. DNMT isoforms (DNMT1, DNMT3A, and DNMT3B) were overexpressed using lentivirus in ECs. Exosomes were isolated and characterized from ECs overexpressing DNMT isoforms and C57BL/6 mice plasma treated with 5-aza-2′-deoxycytidine. 3D spheroid assay was performed to understand the influence of exosomes derived from cells overexpressing DNMTs on EC functions. Further, the exosomes were subjected to TMT labelled proteomics analysis followed by validation. 3D spheroid assay showed increase in the pro-angiogenic activity in response to exosomes derived from DNMT overexpressing cells which was impeded by inclusion of 5-aza-2′-deoxycytidine. Our results showed that exosome proteome and PTMs were significantly modulated and were associated with dysregulation of vascular homeostasis, metabolism, inflammation and endothelial cell functions. In vitro and in vivo validation showed elevated DNMT1 and TGF-β1 exosome proteins due to DNMT1 and DNMT3A overexpression, but not DNMT3B which was mitigated by 5-aza-2′-deoxycytidine indicating epigenetic regulation. Further, exosomes induced ED as evidenced by reduced expression of phospho-eNOSser1177. Our study unveils epigenetically regulated exosome proteins, aiding management of vascular complications. [Display omitted] • Exosomes derived from endothelial cells overexpressing DNMT isoforms induce endothelial dysfunction. • DNMT isoform overexpression leads to altered endothelial exosome proteome. • Gene ontology analysis showed dysregulation of pathways linked with EC functions. • PTM changes in the exosome proteome are associated with pan vascular pathologies. • Increase in exosome protein content of DNMT1 and TGF-β1 are associated with ED. [ABSTRACT FROM AUTHOR]

Published

2024

23. Fine-tuning of liposome integrity for differentiated transcytosis and enhanced antitumor efficacy.

Author

Su, Jiajia, Wu, Chenchen, Zou, Jiahui, Wang, Xinqiuyue, Yang, Kaiyun, Liu, Jianping, Wu, Zimei, and Zhang, Wenli

Subjects

*BIOLOGICAL transport, *TRANSCYTOSIS, *FLUORESCENCE resonance energy transfer, *LIPOSOMES, *ACTIVE biological transport, *ENDOCYTOSIS, *ENDOTHELIAL cells

Abstract

Transcytosis-inducing nanomedicines have been developed to improve tumor extravasation. However, the fate during transcytosis across multicell layers and the structural integrity of the nanomedicines before reaching tumor cells could impact antitumor therapy. Here, a BAY 87–2243 (a hypoxia-inducible factor-1 inhibitor)-loaded liposomal system (HA-P-L BAY) modified by low molecular weight protamine (LMWP) and crosslinked by hyaluronic acid (HA) was constructed. This system could accomplish differentiate cellular transport in endothelial and tumor cells by fine-tuning its structural integrity, i.e. transcytosis across the endothelial cells while preserving structural integrity, facilitating subsequent retention and drug release within tumor cells via degradation-induced aggregation. In vitro cellular uptake and transwell studies demonstrated that HA-P-L BAY were internalized by endothelial cells (bEnd.3) via an active, caveolin and heparin sulfate proteoglycan (HSPG)-mediated endocytosis, and subsequently achieved transcytosis mainly through the ER/Golgi pathway. Moreover, the fluorescence resonance energy transfer (FRET) study showed that HA-crosslinking maintained higher integrity of HA-P-L BAY after transcytosis, more efficiently than electrostatic coating of HA (HA/P-L BAY). In addition, more HA-P-L BAY was retained in tumor cells (4T1) compared to HA/P-L BAY corresponding to its enhanced in vitro cytotoxicity. This may be attributed to better integrity of HA-P-L BAY post endothelial transcytosis and more degradation of HA in tumor cells, leading to more liposome aggregation and inhibition of their transcytosis, which was inferred by both TEM images and the HAase responsiveness assay proved by FRET. In vivo, HA-P-L BAY exhibited more potency in tumor suppression than the other formulations in both low and high permeability tumor models. This highlighted that fine-tuning of structural integrity of nanocarriers played a key role no matter whether the transcytosis of nanocarriers contributed to cellular transport. Collectively, this study provides a promising strategy for antitumor therapies by fine-tuning liposome integrity to achieve active trans-endothelial transport with structural integrity and selective aggregation for prolonged tumor retention. [Display omitted] • Fine-tuning the structural integrity of liposomes by HA wrapping and degradation. • Transcytosis across endothelial cells with integrity mainly via ER/Golgi pathway. • Intracellular retention in tumor by HAase-responsive degradation and aggregation. • HA-P-L BAY exhibited potent efficacy in low and high permeability tumor models. [ABSTRACT FROM AUTHOR]

Published

2024

24. Ailanthone ameliorates pulmonary fibrosis by suppressing JUN-dependent MEOX1 activation.

Author

Zhao, Lixin, Zhu, Yuguang, Tao, Hua, Chen, Xiying, Yin, Feng, Zhang, Yingyi, Qin, Jianfeng, Huang, Yongyin, Cai, Bikun, Lin, Yonghao, Wu, Jiaxiang, Zhang, Yu, Liang, Lu, Shen, Ao, and Yu, Xi-Yong

Subjects

PULMONARY fibrosis, CHEMICAL libraries, HIGH throughput screening (Drug development), SMALL molecules, ENDOTHELIAL cells

Abstract

Pulmonary fibrosis poses a significant health threat with very limited therapeutic options available. In this study, we reported the enhanced expression of mesenchymal homobox 1 (MEOX1) in pulmonary fibrosis patients, especially in their fibroblasts and endothelial cells, and confirmed MEOX1 as a central orchestrator in the activation of profibrotic genes. By high-throughput screening, we identified Ailanthone (AIL) from a natural compound library as the first small molecule capable of directly targeting and suppressing MEOX1. AIL demonstrated the ability to inhibit both the activation of fibroblasts and endothelial-to-mesenchymal transition of endothelial cells when challenged by transforming growth factor- β 1 (TGF- β 1). In an animal model of bleomycin-induced pulmonary fibrosis, AIL effectively mitigated the fibrotic process and restored respiratory functions. Mechanistically, AIL acted as a suppressor of MEOX1 by disrupting the interaction between the transcription factor JUN and the promoter of MEOX1, thereby inhibiting MEOX1 expression and activity. In summary, our findings pinpointed MEOX1 as a cell-specific and clinically translatable target in fibrosis. Moreover, we demonstrated the potent anti-fibrotic effect of AIL in pulmonary fibrosis, specifically through the suppression of JUN-dependent MEOX1 activation. MEOX1 is a central orchestrator during pulmonary fibrosis and promotes fibroblasts activation and EndMT. High-throughput screening identifies Ailanthone as the first direct suppressor of MEOX1 by disrupting the interaction between JUN and MEOX1 promoter. [Display omitted] [ABSTRACT FROM AUTHOR]

Published

2024

25. USP11 Exacerbates Radiation-Induced Pneumonitis by Activating Endothelial Cell Inflammatory Response via OTUD5-STING Signaling.

Author

Tang, Yiting, Wang, Tingya, Gu, Liming, Xu, Ying, Yang, Zhao, Zhu, Wei, Zhang, Qi, Luo, Judong, Cao, Jianping, and Jiao, Yang

Subjects

*RADIATION pneumonitis, *ENDOTHELIAL cells, *PROTEOMICS, *INFLAMMATION, *DEUBIQUITINATING enzymes, *ENDOTHELIUM diseases, *HEPATOCELLULAR carcinoma

Abstract

Radiation-induced pneumonitis (RIP) seriously limits the application of radiation therapy in the treatment of thoracic tumors, and its etiology and pathogenesis remain elusive. This study aimed to elucidate the role of ubiquitin-specific peptidase 11 (USP11) in the progression of RIP and the associated underlying mechanisms. Changes in cytokines and infiltrated immune cells were detected by enzyme-linked immunosorbent assays and immunohistochemistry after exposure to 20 Gy x-ray with whole-thorax irradiation. The effects of USP11 expression on endothelial cell proliferation and apoptosis were analyzed by costaining of CD31/Ki67 and CD31/caspase-3 in vivo, and the production of cytokines and reactive oxygen species was confirmed by reverse-transcription polymerase chain reaction and flow cytometry in vitro. Comprehensive proteome and ubiquitinome analyses were used for USP11 substrate screening after radiation. Results were verified by Western blotting and coimmunoprecipitation experiments. Recombinant adeno-associated virus lung vectors expressing OTUD5 were used for localized overexpression of OTUD5 in mouse pulmonary tissue, and immunohistochemistry was conducted to analyze cytokine expression. The progression of RIP was significantly alleviated by reduced expression of proinflammatory cytokines in both Usp11-knockout (Usp11−/−) mice and in mice treated with the USP11 inhibitor mitoxantrone. Likewise, the absence of USP11 resulted in decreased permeability of pulmonary vessels and neutrophils and macrophage infiltration. The proliferation rates of endothelial cells were prominently increased in the Usp11−/− lung, whereas apoptosis in Usp11−/− lungs decreased after irradiation compared with that observed in Usp11+/+ lungs. Conversely, USP11 overexpression increased proinflammatory cytokine expression and reactive oxygen species production in endothelial cells after radiation. Comprehensive proteome and ubiquitinome analyses indicated that USP11 overexpression upregulates the expression of several deubiquitinating enzymes, including USP22, USP33, and OTUD5. We demonstrate that USP11 deubiquitinates OTUD5 and implicates the OTUD5-STING signaling pathway in the progression of the inflammatory response in endothelial cells. USP11 exacerbates RIP by triggering an inflammatory response in endothelial cells both in vitro and in vivo, and the OTUD5-STING pathway is involved in the USP11-dependent promotion of RIP. This study provides experimental support for the development of precision intervention strategies targeting USP11 to mitigate RIP. [ABSTRACT FROM AUTHOR]

Published

2024

26. In vitro throughput screening of anticancer drugs using patient-derived cell lines cultured on vascularized three-dimensional stromal tissues.

Author

Takahashi, Yuki, Morimura, Rii, Tsukamoto, Kei, Gomi, Sayaka, Yamada, Asuka, Mizukami, Miki, Naito, Yasuyuki, Irie, Shinji, Nagayama, Satoshi, Shinozaki, Eiji, Yamaguchi, Kensei, Fujita, Naoya, Kitano, Shiro, Katayama, Ryohei, and Matsusaki, Michiya

Subjects

ENDOTHELIAL cells, TISSUE culture, VASCULAR endothelial growth factors, VASCULAR endothelial cells, CELL culture, CELL lines

Abstract

The development of high-throughput anticancer drug screening methods using patient-derived cancer cell (PDC) lines that maintain their original characteristics in an in vitro three-dimensional (3D) culture system poses a significant challenge to achieving personalized cancer medicine. Because stromal tissue plays a critical role in the composition and maintenance of the cancer microenvironment, in vitro 3D-culture using reconstructed stromal tissues has attracted considerable attention. Here, a simple and unique in vitro 3D-culture method using heparin and collagen together with fibroblasts and endothelial cells to fabricate vascularized 3D-stromal tissues for in vitro culture of PDCs is reported. Whereas co-treatment with bevacizumab, a monoclonal antibody against vascular endothelial growth factor, and 5-fluorouracil significantly reduced the survival rate of 3D-cultured PDCs to 30%, separate addition of each drug did not induce comparable strong cytotoxicity, suggesting the possibility of evaluating the combined effect of anticancer drugs and angiogenesis inhibitors. Surprisingly, drug evaluation using eight PDC lines with the 3D-culture method resulted in a drug efficacy concordance rate of 75% with clinical outcomes. The model is expected to be applicable to in vitro throughput drug screening for the development of personalized cancer medicine. To replicate the cancer microenvironment, we constructed a cancer-stromal tissue model in which cancer cells are placed above and inside stromal tissue with vascular network structures derived from vascular endothelial cells in fibroblast tissue using CAViTs method. Using this method, we were able to reproduce the invasion and metastasis processes of cancer cells observed in vivo. Using patient-derived cancer cells, we assessed the possibility of evaluating the combined effect with an angiogenesis inhibitor. Further, primary cancer cells also grew on the stromal tissues with the normal medium. These data suggest that the model may be useful for new in vitro drug screening and personalized cancer medicine. [Display omitted] [ABSTRACT FROM AUTHOR]

Published

2024

27. Reprint of: Fibrinolytic and Non-fibrinolytic Roles of Tissue-type Plasminogen Activator in the Ischemic Brain.

Author

Yepes, Manuel

Subjects

*TISSUE plasminogen activator, *FIBRINOLYTIC agents, *BASAL lamina, *CELL anatomy, *ENDOTHELIAL cells, *PLASMINOGEN

Abstract

• Tissue-type plasminogen activator (tPA) is a serine proteinase that catalyzes the conversion of plasminogen into plasmin. • The neurovascular unit is assembled by endothelial cells, pericytes, the perivascular basement membrane, astrocytes, neurons and microglia. • TPA is abundantly the cellular components of the NVU where it regulates its function under physiologic and pathologic conditions. The neurovascular unit (NVU) is assembled by endothelial cells (ECs) and pericytes, and encased by a basement membrane (BM) surveilled by microglia and surrounded by perivascular astrocytes (PVA), which in turn are in contact with synapses. Cerebral ischemia induces the rapid release of the serine proteinase tissue-type plasminogen activator (tPA) from endothelial cells, perivascular astrocytes, microglia and neurons. Owning to its ability to catalyze the conversion of plasminogen into plasmin, in the intravascular space tPA functions as a fibrinolytic enzyme. In contrast, the release of astrocytic, microglial and neuronal tPA have a plethora of effects that not always require the generation of plasmin. In the ischemic brain tPA increases the permeability of the NVU, induces microglial activation, participates in the recycling of glutamate, and has various effects on neuronal survival. These effects are mediated by different receptors, notably subunits of the N-methyl-D-aspartate receptor (NMDAR) and the low-density lipoprotein receptor-related protein-1 (LRP-1). Here we review data on the role of tPA in the NVU under non-ischemic and ischemic conditions, and analyze how this knowledge may lead to the development of potential strategies for the treatment of acute ischemic stroke patients. [ABSTRACT FROM AUTHOR]

Published

2024

28. TRPC4 aggravates hypoxic pulmonary hypertension by promoting pulmonary endothelial cell apoptosis.

Author

Yang, Liu, Peng, Zeyu, Gong, Fanpeng, Yan, WenXin, Shi, Yi, Li, Hanyi, Zhou, Chang, Yao, Hong, Yuan, Menglu, Yu, Fan, Feng, Lei, Wan, Naifu, and Liu, Guizhu

Subjects

*TRP channels, *PULMONARY hypertension, *ENDOTHELIAL cells, *VASCULAR remodeling, *APOPTOSIS, *PULMONARY arterial hypertension

Abstract

Pulmonary hypertension (PH) is a devastating disease that lacks effective treatment options and is characterized by severe pulmonary vascular remodeling. Pulmonary arterial endothelial cell (PAEC) dysfunction drives the initiation and pathogenesis of pulmonary arterial hypertension. Canonical transient receptor potential (TRPC) channels, a family of Ca2+-permeable channels, play an important role in various diseases. However, the effect and mechanism of TRPCs on PH development have not been fully elucidated. Among the TRPC family members, TRPC4 expression was markedly upregulated in PAECs from hypoxia combined with SU5416 (HySu)-induced PH mice and monocrotaline (MCT)-treated PH rats, as well as in hypoxia-exposed PAECs, suggesting that TRPC4 in PAECs may participate in the occurrence and development of PH. In this study, we aimed to investigate whether TRPC4 in PAECs has an aggravating effect on PH and elucidate the molecular mechanisms. We observed that hypoxia treatment promoted PAEC apoptosis through a caspase-12/endoplasmic reticulum stress (ERS)-dependent pathway. Knockdown of TRPC4 attenuated hypoxia-induced apoptosis and caspase-3/caspase-12 activity in PAECs. Accordingly, adeno-associated virus (AAV) serotype 6-mediated pulmonary endothelial TRPC4 silencing (AAV6-Tie-shRNA-TRPC4) or TRPC4 antagonist suppressed PH progression as evidenced by reduced right ventricular systolic pressure (RVSP), pulmonary vascular remodeling, PAEC apoptosis and reactive oxygen species (ROS) production. Mechanistically, unbiased RNA sequencing (RNA-seq) suggested that TRPC4 deficiency suppressed the expression of the proapoptotic protein sushi domain containing 2 (Susd2) in hypoxia-exposed mouse PAECs. Moreover, TRPC4 activated hypoxia-induced PAEC apoptosis by promoting Susd2 expression. Therefore, inhibiting TRPC4 ameliorated PAEC apoptosis and hypoxic PH in animals by repressing Susd2 signaling, which may serve as a therapeutic target for the management of PH. [Display omitted] • TRPC4 activates PAEC apoptosis in a caspase-12/ERS-dependent manner. • Susd2 acts as a key regulator of TRPC4-mediated PAEC apoptosis during PH. • TRPC4 is an endogenous pathogenic factor of PH. TRPC4 inhibition attenuates PAEC apoptosis and PH in rodent models. [ABSTRACT FROM AUTHOR]

Published

2024

29. Modeling blood vessel dynamics: Effects of glucose variations on HUVECs in a hollow fiber bioreactor under laminar shear stress.

Author

Ladyzynski, Piotr, Ciechanowska, Anna, Sabalinska, Stanislawa, Foltynski, Piotr, Wencel, Agnieszka, Wojciechowski, Cezary, Pluta, Krzysztof, and Chwojnowski, Andrzej

Subjects

HOLLOW fibers, SHEARING force, BLOOD vessels, UMBILICAL veins, ENDOTHELIAL cells

Abstract

This study aimed to establish a blood vessel model within a hollow fiber bioreactor to evaluate the impact of high and fluctuating glucose levels on human umbilical vein endothelial cells (HUVECs) under laminar shear stress (LSS). HUVECs were cultured for 48 h in normal (5 mM), high (20 mM), and variable (20 mM / 5 mM alternating every 24 h) glucose concentrations under LSS of 0.66 Pa. An automated medium replacement system was developed. The control cultures remained static. The analysis included cell viability via cytometric analysis, glucose consumption, lactate production via electroenzymatic methods, and the expression of 21 genes via qPCR. The percentage of apoptotic cells did not significantly differ across glucose concentrations under LSS. HUVECs favor glycolysis for energy regardless of LSS. Under LSS, the IL1B , CCL2 , and SELE genes were upregulated under high-glucose conditions and downregulated under variable-glucose conditions. A few other genes related to inflammation, oxidative stress, cell adhesion and apoptosis were upregulated under high-glucose conditions. In conclusion, using the blood vessel model we effectively examined the impact of glucose profiles on HUVECs under LSS in a device replicating the cylindrical geometry of blood vessels. LSS and tubular cell arrangement might mitigate the adverse effects of variable glucose on endothelial cells. [ABSTRACT FROM AUTHOR]

Published

2024

30. The hybrid CL-SP-D molecule has the potential to regulate xenogeneic rejection by human neutrophils more efficiently than CD47.

Author

Keigo Iemitsu, Rieko Sakai, Akira Maeda, Katarzyna Gadomska, Shuhei Kogata, Daiki Yasufuku, Jun Matsui, Kazunori Masahata, Masafumi Kamiyama, Hiroshi Eguchi, Soichi Matsumura, Yoichi Kakuta, Hiroshi Nagashima, Hiroomi Okuyam, and Shuji Miyagawa

Subjects

*NATURAL immunity, *CD47 antigen, *CYTOTOXINS, *NEUTROPHILS, *ENDOTHELIAL cells

Abstract

Objective: Innate immunity plays a vital role in xenotransplantation. A CD47 molecule, binding to the SIRPa expressed on monocyte/macrophage cells, can suppress cytotoxicity. Particularly, the SIRPa contains ITIM, which delivers a negative signal. Our previous study demonstrated that the binding between CL-P1 and surfactant protein-D hybrid (CL-SP-D) with SIRPa regulates macrophages' phagocytic activity. In this study, we examined the effects of human CD47 and CL-SP-D expression on the inhibition of xenograft rejection by neutrophils in swine endothelial cells (SECs). Methods: We first examined SIRPa expression on HL-60 cells, a neutrophil-like cell line, and neutrophils isolated from peripheral blood. CD47-expressing SECs or CL-SP-D-expressing SECs were generated through plasmid transfection. Subsequently, these SECs were co-cultured with HL-60 cells or neutrophils. After co-culture, the degree of cytotoxicity was calculated using the WST-8 assay. The suppressive function of CL-SP-D on neutrophils was subsequently examined, and the results were compared with those of CD47 using naïve SECs as controls. Additionally, we assessed ROS production and neutrophil NETosis. Results: In initial experiments, the expression of SIRPa on HL-60 and neutrophils was confirmed. Exposure to CLSP-D significantly suppressed the cytotoxicity in HL-60 (p = 0.0038) and neutrophils (p = 0.00003). Furthermore, engagement with CD47 showed a suppressive effect on neutrophils obtained from peripheral blood (p = 0.0236) but not on HL-60 (p = 0.4244). The results of the ROS assays also indicated a significant downregulation of SEC by CD47 (p = 0.0077) or CL-SP-D (p = 0.0018). Additionally, the suppression of NETosis was confirmed (p = 0.0125) in neutrophils co-cultured with S/CL-SP-D. Conclusion: These results indicate that CL-SP-D is highly effective on neutrophils in xenogeneic rejection. Furthermore, CL-SP-D was more effective than CD47 at inhibiting neutrophil-mediated xenograft rejection. [ABSTRACT FROM AUTHOR]

Published

2024

31. Peroxiredoxin 6 suppresses ferroptosis in lung endothelial cells.

Author

Torres-Velarde, Julia María, Allen, Kaitlin N., Salvador-Pascual, Andrea, Leija, Roberto G., Luong, Diamond, Moreno-Santillán, Diana Daniela, Ensminger, David C., and Vázquez-Medina, José Pablo

Subjects

*LUNGS, *ENDOTHELIAL cells, *GLUTATHIONE peroxidase, *SELENOPROTEINS, *ACYL group, *CELL death, *EPITHELIAL cells, *CELL analysis

Abstract

Peroxiredoxin 6 (Prdx6) repairs peroxidized membranes by reducing oxidized phospholipids, and by replacing oxidized sn-2 fatty acyl groups through hydrolysis/reacylation by its phospholipase A 2 (aiPLA 2) and lysophosphatidylcholine acyltransferase activities. Prdx6 is highly expressed in the lung, and intact lungs and cells null for Prdx6 or with single-point mutations that inactivate either Prdx6-peroxidase or aiPLA 2 activity alone exhibit decreased viability, increased lipid peroxidation, and incomplete repair when exposed to paraquat, hyperoxia, or organic peroxides. Ferroptosis is form of cell death driven by the accumulation of phospholipid hydroperoxides. We studied the role of Prdx6 as a ferroptosis suppressor in the lung. We first compared the expression Prdx6 and glutathione peroxidase 4 (GPx4) and visualized Prdx6 and GPx4 within the lung. Lung Prdx6 mRNA levels were five times higher than GPx4 levels. Both Prdx6 and GPx4 localized to epithelial and endothelial cells. Prdx6 knockout or knockdown sensitized lung endothelial cells to erastin-induced ferroptosis. Cells with genetic inactivation of either aiPLA 2 or Prdx6-peroxidase were more sensitive to ferroptosis than WT cells, but less sensitive than KO cells. We then conducted RNA-seq analyses in Prdx6-depleted cells to further explore how the loss of Prdx6 sensitizes lung endothelial cells to ferroptosis. Prdx6 KD upregulated transcriptional signatures associated with selenoamino acid metabolism and mitochondrial function. Accordingly, Prdx6 deficiency blunted mitochondrial function and increased GPx4 abundance whereas GPx4 KD had the opposite effect on Prdx6. Moreover, we detected Prdx6 and GPx4 interactions in intact cells, suggesting that both enzymes cooperate to suppress lipid peroxidation. Notably, Prdx6-depleted cells remained sensitive to erastin-induced ferroptosis despite the compensatory increase in GPx4. These results show that Prdx6 suppresses ferroptosis in lung endothelial cells and that both aiPLA 2 and Prdx6-peroxidase contribute to this effect. These results also show that Prdx6 supports mitochondrial function and modulates several coordinated cytoprotective pathways in the pulmonary endothelium. [Display omitted] • Ferroptosis is a form of cell death driven by the accumulation of phospholipid hydroperoxides. • Prdx6 limits lipid peroxidation in the lung via its peroxidase, PLA 2 , and LPCAT activities. • Prdx6 KO, KD, or KI pulmonary cells without Prdx6-peroxidase or PLA 2 are sensitized to ferroptosis. • Prdx6 deficiency blunts mitochondrial function and upregulates GPx4, which interacts with Prdx6. • Prdx6 is a cytoprotective protein that guards the pulmonary endothelium against ferroptosis. [ABSTRACT FROM AUTHOR]

Published

2024

32. Macrophage migration inhibitor factor (MIF): Potential role in cognitive impairment disorders.

Author

Zeng, Lian, Hu, Pengchao, Zhang, Yu, Li, Mingyue, Zhao, Yilin, Li, Shiyong, and Luo, Ailin

Subjects

*COGNITION disorders, *MACROPHAGE migration inhibitory factor, *ENTORHINAL cortex, *ENDOTHELIAL cells, *ACUTE kidney failure, *MACROPHAGES, *CELL death

Abstract

Macrophage migration inhibitory factor (MIF) is a cytokine in the immune system, participated in both innate and adaptive immune responses. Except from immune cells, MIF is also secreted by a variety of non-immune cells, including hematopoietic cells, endothelial cells (ECs), and neurons. MIF plays a crucial role in various diseases, such as sepsis, rheumatoid arthritis, acute kidney injury, and neurodegenerative diseases. The role of MIF in the neuropathogenesis of cognitive impairment disorders is emphasized, as it recruits multiple inflammatory mediators, leading to activating microglia or astrocyte-derived neuroinflammation. Furthermore, it contributes to the cell death of neurons and ECs with the binding of apoptosis-inducing factor (AIF) through parthanatos-associated apoptosis-inducing factor nuclease (PAAN) / MIF pathway. This review comprehensively delves into the relationship between MIF and the neuropathogenesis of cognitive impairment disorders, providing a series of emerging MIF-targeted pharmaceuticals as potential treatments for cognitive impairment disorders. [Display omitted] • MIF modulates neuronal and glial function in brain. • MIF-induced neuroinflammation and cell death contributed to cognitive impairment. • MIF inhibitors are promising to prevent cognitive impairment disorders. [ABSTRACT FROM AUTHOR]

Published

2024

33. Mucopolysaccharide polysulfate increases local skin blood volume through nitric oxide production.

Author

Kurachi, Tam, Ishimaru, Hironobu, Tadakuma, Ryo, Okaue, Miu, Koda, Akira, Ueda, Yuhki, and Doi, Takaaki

Subjects

*BLOOD volume, *NITRIC-oxide synthases, *TOPICAL drug administration, *BLOOD flow, *NITRIC oxide, *ENDOTHELIAL cells, *TRANEXAMIC acid

Abstract

Mucopolysaccharide polysulfate (MPS) is widely used as an active ingredient in topical preparations for the treatment of asteatosis and blood flow disorders. Although topical MPS products can increase cutaneous blood flow (CBF), the underlying mechanism remains unclear. In this study, we aimed to elucidate how MPS increases CBF. We investigated the association of nitric oxide (NO), a powerful mediator associated with increased local blood volume, with the blood flow-accelerating action of MPS in mice. In addition, we verified the effects of MPS on NO production in different skin cell types, such as keratinocytes (KCs), endothelial cells (ECs), and dermal fibroblasts (DFs). We used raster-scanning optoacoustic imaging mesoscopy to observe in vivo changes in the skin blood volume. NO production was determined in each cell using an NO indicator. An enzyme-linked immunoassay was used to measure the phosphorylated nitric oxide synthase (NOS) levels in ECs, DFs, and KCs in the presence or absence of MPS. Topical application of MPS increased the skin blood volume in mice, and this increase was abolished through the addition of NOS inhibitors. MPS promoted the dose-dependent production of NO in various cells, which caused alterations in the phosphorylation state of NOS. Our findings demonstrate that MPS promotes an increase in skin blood volume and NO production in various skin cell types. These results suggest that MPS can potentially accelerate CBF through the NO biosynthesis pathway in different skin cell types. • Topical MPS cream increased local skin blood volume in mice. • NOS inhibitor attenuated MPS-induced increase in local skin blood volume. • MPS enhanced intracellular or extracellular NO production in ECs, DFs, and KCs. • MPS-induced NO production is blocked by cNOS inhibition. • MPS promoted eNOS Ser1177 phosphorylation and nNOS Ser852 dephosphorylation. [ABSTRACT FROM AUTHOR]

Published

2024

34. Neutrophil-derived nanovesicles deliver IL-37 to mitigate renal ischemia-reperfusion injury via endothelial cell targeting.

Author

Ma, Wenjie, Wu, Di, Long, Chengcheng, Liu, Jingyu, Xu, Luwei, Zhou, Liuhua, Dou, Quanliang, Ge, Yuzheng, Zhou, Changcheng, and Jia, Ruipeng

Subjects

*INTERLEUKIN-37, *ENDOTHELIAL cells, *REPERFUSION injury, *P-selectin glycoprotein ligand-1, *ACUTE kidney failure, *NEOVASCULARIZATION, *NEUTROPHILS

Abstract

Renal ischemia-reperfusion injury (IRI) is one of the most important causes of acute kidney injury (AKI). Interleukin (IL)-37 has been suggested as a novel anti-inflammatory factor for the treatment of IRI, but its application is still limited by its low stability and delivery efficiency. In this study, we reported a novel engineered method to efficiently and easily prepare neutrophil membrane-derived vesicles (N-MVs), which could be utilized as a promising vehicle to deliver IL-37 and avoid the potential side effects of neutrophil-derived natural extracellular vesicles. N-MVs could enhance the stability of IL-37 and targetedly deliver IL-37 to damaged endothelial cells of IRI kidneys via P-selectin glycoprotein ligand-1 (PSGL-1). In vitro and in vivo evidence revealed that N-MVs encapsulated with IL-37 (N-MV@IL-37) could inhibit endothelial cell apoptosis, promote endothelial cell proliferation and angiogenesis, and decrease inflammatory factor production and leukocyte infiltration, thereby ameliorating renal IRI. Our study establishes a promising delivery vehicle for the treatment of renal IRI and other endothelial damage-related diseases. [Display omitted] • Engineered method yields abundant, pure neutrophil membrane nanovesicles efficiently. • N-MVs target injured endothelial cells, avoiding neutrophil vesicle potential side effects. • N-MV@IL-37 enable targeted kidney delivery of IL-37 to counteract IRI. • N-MV@IL-37 mitigate renal IRI by reducing endothelial apoptosis and inflammation. [ABSTRACT FROM AUTHOR]

Published

2024

35. Quantitative proteomics reveals CLR interactome in primary human cells.

Author

Manolis, Dimitrios, Hasan, Shirin, Maraveyas, Anthony, O’Brien, Darragh P., Kessler, Benedikt M., Kramer, Holger, and Nikitenko, Leonid L.

Subjects

*PROTEOMICS, *G protein coupled receptors, *CALCITONIN receptors, *ENDOTHELIAL cells, *SUMATRIPTAN

Abstract

The G protein–coupled receptor (GPCR) calcitonin receptor–like receptor (CLR) mediates essential functions in several cell types and is implicated in cardiovascular pathologies, skin diseases, migraine, and cancer. To date, the network of proteins interacting with CLR (“CLR interactome”) in primary cells, where this GPCR is expressed at endogenous (physiologically relevant) levels, remains unknown. To address this knowledge gap, we established a novel integrative methodological workflow/approach for conducting a comprehensive/proteome-wide analysis of Homo sapiens CLR interactome. We used primary human dermal lymphatic endothelial cells and combined immunoprecipitation utilizing anti-human CLR antibody with label-free quantitative nano LC-MS/MS and quantitative in situ proximity ligation assay. By using this workflow, we identified 37 proteins interacting with endogenously expressed CLR amongst 4902 detected members of the cellular proteome (by quantitative nano LC-MS/MS) and revealed direct interactions of two kinases and two transporters with this GPCR (by in situ proximity ligation assay). All identified interactors have not been previously reported as members of CLR interactome. Our approach and findings uncover the hitherto unrecognized compositional complexity of the interactome of endogenously expressed CLR and contribute to fundamental understanding of the biology of this GPCR. Collectively, our study provides a first-of-its-kind integrative methodological approach and datasets as valuable resources and robust platform/springboard for advancing the discovery and comprehensive characterization of physiologically relevant CLR interactome at a proteome-wide level in a range of cell types and diseases in future studies. [ABSTRACT FROM AUTHOR]

Published

2024

36. Magnetically assembled endothelial cell-coated spheroid for vascularization.

Author

Seok, Hodong, Roo, Dayeon, Cho, Sungwoo, Song, Wonmoon, Kim, Jeong-Uk, Park, Tai Hyun, So, Kyoung-Ha, and Hwang, Nathaniel S.

Subjects

VASCULAR endothelial cells, MAGNETISM, ENDOTHELIAL cells, MAGNETIC control, MAGNETIC nanoparticles

Abstract

[Display omitted] 3D spheroids are used as a therapeutic strategy and transplanted in vivo owing to their ability to better mimic the microphysiological environment that is crucial for the transplants to be able to engraft and vascularize for their long-term survival and functionalization in the host tissue. Among various methods of fabricating spheroids, the utilization of magnetic force enables rapid cell aggregation and spatial regulation. Encapsulating a magnetic spheroid with endothelial cells paves the way toward vascularization. Here, we magnetically bioprinted vascular assembly by coating magnetic spheroids with the magnetic nanoparticles (MNPs)-internalized vascular endothelial cells. MNPs-internalized mouse myoblasts cells (C2C12) were magnetically aggregated by placing a neodymium magnet under a well plate and then encapsulated by MNPs-internalized human umbilical vein endothelial cells (HUVECs). Internalization of MNPs did not hinder cell viability and vascularization-related gene expression, and the transplant of the vascular assemblies could sprout and be engrafted into the host tissue within three days. As these vascular assemblies are easily fabricated by coating spheroids with MNPs-internalized endothelial cells and controlled by a magnetic force, they may be used for engraftment and vascularization in various applications with spheroids with different functions. [ABSTRACT FROM AUTHOR]

Published

2024

37. Fundamental considerations for designing endothelialized in vitro models of thrombosis.

Author

Lemmens, Titus P., Bröker, Vanessa, Rijpkema, Minke, Hughes, Christopher C.W., Schurgers, Leon J., and Cosemans, Judith M.E.M.

Subjects

*THROMBOSIS, *ENDOTHELIAL cells, *EXTRACELLULAR matrix, *CONCENTRATION gradient, *RESEARCH questions

Abstract

Endothelialized in vitro models for cardiovascular disease have contributed greatly to our current understanding of the complex molecular mechanisms underlying thrombosis. To further elucidate these mechanisms, it is important to consider which fundamental aspects to incorporate into an in vitro model. In this review, we will focus on the design of in vitro endothelialized models of thrombosis. Expanding our understanding of the relation and interplay between the different pathways involved will rely in part on complex models that incorporate endothelial cells, blood, the extracellular matrix, and flow. Importantly, the use of tissue-specific endothelial cells will help in understanding the heterogeneity in thrombotic responses between different vascular beds. The dynamic and complex responses of endothelial cells to different shear rates underlines the importance of incorporating appropriate shear in in vitro models. Alterations in vascular extracellular matrix composition, availability of bioactive molecules, and gradients in concentration and composition of these molecules can all regulate the function of both endothelial cells and perivascular cells. Factors modulating these elements in in vitro models should therefore be considered carefully depending on the research question at hand. As the complexity of in vitro models increases, so can the variability. A bottom-up approach to designing such models will remain an important tool for researchers studying thrombosis. As new techniques are continuously being developed and new pathways are brought to light, research question-dependent considerations will have to be made regarding what aspects of thrombosis to include in in vitro models. • The interplay of endothelial cells, blood, extracellular matrix, and flow is crucial for understanding thrombosis pathways. • Incorporating fundamental aspects of thrombosis into in vitro endothelial models are vital in increasing translatability. • Designing endothelialized models for thrombosis requires a balance between reproducibility, accessibility, and complexity. [ABSTRACT FROM AUTHOR]

Published

2024

38. Hydrogen sulfide improves endothelial barrier function by modulating the ubiquitination degradation of KLF4 through TRAF7 S-sulfhydration in diabetic aorta.

Author

Li, Qianzhu, Kang, Jiaxin, Liu, Ning, Huang, Jiayi, Zhang, Xueya, Pang, Kemiao, Zhang, Shiwu, Wang, Mengyi, Zhao, Yajun, Dong, Shiyun, Li, Hongxia, Zhao, Dechao, Lu, Fanghao, and Zhang, Weihua

Subjects

*ENDOTHELIUM, *HYDROGEN sulfide, *KRUPPEL-like factors, *UBIQUITINATION, *ENDOTHELIAL cells, *TUMOR necrosis factors, *VASCULAR endothelium, *UBIQUITIN ligases

Abstract

Anomalous vascular endothelium significantly contributes to various cardiovascular diseases. VE-cadherin plays a vital role in governing the endothelial barrier. Krüppel-like factor 4(KLF4), as a transcription factor, which binds the VE-cadherin promoter and enhances its transcription. Tumor necrosis factor receptor-associated factor 7 (TRAF7) is an E3 ubiquitin ligase that has been shown to modulate the degradation of KLF4. H 2 S can covalently modify cysteine residues on proteins through S-sulfhydration, thereby influencing the structure and functionality of the target protein. However, the role of S-sulfhydration on endothelial barrier integrity remains to be comprehensively elucidated. This study aims to investigate whether protein S-sulfhydration in the endothelium regulates endothelial integrity and its underlying mechanism. In this study, we observed that protein S-sulfhydration was reduced in the endothelium during diabetes and TRAF7 was the main target. Overexpression of TRAF7-Cys327 mutant could mitigate the endothelial barrier damage by weakening TRAF7 interaction with KLF4 and reducing ubiquitination degradation of KLF4. In conclusion, our research demonstrates that H 2 S plays a pivotal role in regulating S-sulfhydration of TRAF7 at Cys327. This regulation effectively inhibits the ubiquitin-mediated degradation of KLF4, resulting in an upregulation of VE-cadherin levels. This molecular mechanism contributes to the prevention of endothelial barrier damage. [Display omitted] • H 2 S plays a pivotal role in regulating S-sulfhydration of TRAF7 at Cys327. • Transfection with TRAF7-Cys327, the S-sulfhydration level of TRAF7 significantly decreased with NaHS treatment. • S-sulfhydration of TRAF7 at Cys327 prevents KLF4 degradation. • S-sulfhydration of TRAF7 at Cys327 maintains endothelial permeability. [ABSTRACT FROM AUTHOR]

Published

2024

39. Fibrinolytic and Non-fibrinolytic Roles of Tissue-type Plasminogen Activator in the Ischemic Brain.

Author

Yepes, Manuel

Subjects

*TISSUE plasminogen activator, *STROKE patients, *FIBRINOLYTIC agents, *BASAL lamina, *CELL anatomy, *ENDOTHELIAL cells

Abstract

• Tissue-type plasminogen activator (tPA) is a serine proteinase that catalyzes the conversion of plasminogen into plasmin. • The neurovascular unit is assembled by endothelial cells, pericytes, the perivascular basement membrane, astrocytes, neurons and microglia. • TPA is abundantly the cellular components of the NVU where it regulates its function under physiologic and pathologic conditions. The neurovascular unit (NVU) is assembled by endothelial cells (ECs) and pericytes, and encased by a basement membrane (BM) surveilled by microglia and surrounded by perivascular astrocytes (PVA), which in turn are in contact with synapses. Cerebral ischemia induces the rapid release of the serine proteinase tissue-type plasminogen activator (tPA) from endothelial cells, perivascular astrocytes, microglia and neurons. Owning to its ability to catalyze the conversion of plasminogen into plasmin, in the intravascular space tPA functions as a fibrinolytic enzyme. In contrast, the release of astrocytic, microglial and neuronal tPA have a plethora of effects that not always require the generation of plasmin. In the ischemic brain tPA increases the permeability of the NVU, induces microglial activation, participates in the recycling of glutamate, and has various effects on neuronal survival. These effects are mediated by different receptors, notably subunits of the N-methyl-D-aspartate receptor (NMDAR) and the low-density lipoprotein receptor-related protein-1 (LRP-1). Here we review data on the role of tPA in the NVU under non-ischemic and ischemic conditions, and analyze how this knowledge may lead to the development of potential strategies for the treatment of acute ischemic stroke patients. [ABSTRACT FROM AUTHOR]

Published

2024

40. Neurological impairment is crucial for tire rubber-derived contaminant 6PPDQ-induced acute toxicity to rainbow trout.

Author

Liao, Xiao-Liang, Chen, Zhi-Feng, Ou, Shi-Ping, Liu, Qian-Yi, Lin, Shan-Hong, Zhou, Jia-Ming, Wang, Yujie, and Cai, Zongwei

Subjects

*RAINBOW trout, *BLOOD-brain barrier, *ENDOTHELIAL cells, *TROUT, *GENE expression, *PHENYLENEDIAMINES, *ELASTOMERS, *TIRES

Abstract

[Display omitted] N -(1,3-dimethylbutyl)- N ′-phenyl- p -phenylenediamine quinone (6PPDQ) has attracted significant attention due to its highly acute lethality to sensitive salmonids. However, studies investigating the mechanisms underlying its acute toxicity have been lacking. In this work, we demonstrated the sensitivity of rainbow trout to 6PPDQ-induced mortality. Moribund trout exhibited significantly higher brain concentrations of 6PPDQ compared to surviving trout. In an in vitro model using human brain microvascular endothelial cells, 6PPDQ can penetrate the blood–brain barrier and enhance blood–brain barrier permeability without compromising cell viability. The time spent in the top of the tank increased with rising 6PPDQ concentrations, as indicated by locomotion behavior tests. Furthermore, 6PPDQ influenced neurotransmitter levels and mRNA expression of neurotransmission-related genes in the brain and exhibited strong binding affinity to target neurotransmission-related proteins using computational simulations. The integrated biomarker response value associated with neurotoxicity showed a positive linear correlation with trout mortality. These findings significantly contribute to filling the knowledge gap between neurological impairments and apical outcomes, including behavioral effects and mortality, induced by 6PPDQ. [ABSTRACT FROM AUTHOR]

Published

2024

41. Analyzing the effects of helical flow in blood vessels using acoustofluidic-based dynamic flow generator.

Author

Kwak, Daesik, Im, Yongtaek, Nam, Hyeono, Nam, Ungsig, Kim, Seunggyu, Kim, Woohyuk, Kim, Hyun Jin, Park, Jinsoo, and Jeon, Jessie S.

Subjects

BLOOD vessels, BLOOD flow, ACOUSTIC streaming, ACOUSTIC surface waves, CARDIOVASCULAR system

Abstract

The effects of helical flow in a blood vessel are investigated in a dynamic flow generator using surface acoustic wave (SAW) in the microfluidic device. The SAW, generated by an interdigital transducer (IDT), induces acoustic streaming, resulting in a stable and consistent helical flow pattern in microscale channels. This approach allows rapid development of helical flow within the channel without directly contacting the medium. The precise design of the window enables the creation of distinct unidirectional vortices, which can be controlled by adjusting the amplitude of the SAW. Within this device, optimal operational parameters of the dynamic flow generator to preserve the integrity of endothelial cells are found, and in such settings, the actin filaments within the cells are aligned to the desired state. Our findings reveal that intracellular Ca2+ concentrations vary in response to flow conditions. Specifically, comparable maximum intensity and graphical patterns were observed between low-flow rate helical flow and high-flow rate Hagen-Poiseuille flow. These suggest that the cells respond to the helical flow through mechanosensitive ion channels. Finally, adherence of monocytes is effectively reduced under helical flow conditions in an inflammatory environment, highlighting the atheroprotective role of helical flow. Helical flow in blood vessels is well known to prevent atherosclerosis. However, despite efforts to replicate helical flow in microscale channels, there is still a lack of in vitro models which can generate helical flow for analyzing its effects on the vascular system. In this study, we developed a method for generating steady and constant helical flow in microfluidic channel using acoustofluidic techniques. By utilizing this dynamic flow generator, we were able to observe the atheroprotective aspects of helical flow in vitro, including the enhancement of calcium ion flux and reduction of monocyte adhesion. This study paves the way for an in vitro model of dynamic cell culture and offers advanced investigation into helical flow in our circulatory system. [Display omitted] [ABSTRACT FROM AUTHOR]

Published

2024

42. Enhancement of de novo lipogenesis by the IDH1 and IDH2-dependent reverse TCA cycle maintains the growth and angiogenic capacity of bone marrow-derived endothelial progenitor cells under hypoxia.

Author

He, Qiwei, Yu, Tiantian, Chen, Junxiong, Liang, Jianli, Lin, Dongni, Yan, Kaihao, Xie, Zijing, Song, Yuqi, and Chen, Zhenzhou

Subjects

*NEOVASCULARIZATION, *PROGENITOR cells, *ENDOTHELIAL cells, *RESPIRATION, *VASCULAR endothelial growth factors, *RNA interference, *HYPOXEMIA

Abstract

Bone marrow-derived endothelial progenitor cells (EPCs) play a dynamic role in maintaining the structure and function of blood vessels. But how these cells maintain their growth and angiogenic capacity under bone marrow hypoxic niche is still unclear. This study aims to explore the mechanisms from a perspective of cellular metabolism. XFe96 Extracellular Flux Analyzer was used to analyze the metabolic status of EPCs. Gas Chromatography-Mass Spectrometry (GC-MS) was used to trace the carbon movement of 13C-labeled glucose and glutamine under 1 % O 2 (hypoxia) and ∼20 % O 2 (normoxia). Moreover, RNA interference, targeting isocitrate dehydrogenase-1 (IDH1) and IDH2, was used to inhibit the reverse tricarboxylic acid (TCA) cycle and analyze metabolic changes via isotope tracing as well as changes in cell growth and angiogenic potential under hypoxia. The therapeutic potential of EPCs under hypoxia was investigated in the ischemic hindlimb model. Compared with normoxic cells, hypoxic cells showed increased glycolysis and decreased mitochondrial respiration. Isotope metabolic tracing revealed that under hypoxia, the forward TCA cycle was decreased and the reverse TCA cycle was enhanced, mediating the conversion of α-ketoglutarate (α-KG) into isocitrate/citrate, and de novo lipid synthesis was promoted. Downregulation of IDH1 or IDH2 under hypoxia suppressed the reverse TCA cycle, attenuated de novo lipid synthesis (DNL), elevated α-KG levels, and decreased the expression of hypoxia inducible factor-1α (HIF-1α) and vascular endothelial growth factor A (VEGFA), eventually inhibiting the growth and angiogenic capacity of EPCs. Importantly, the transplantation of hypoxia-cultured EPCs in a mouse model of limb ischemia promoted new blood vessel regeneration and blood supply recovery in the ischemic area better than the transplantation of normoxia-cultured EPCs. Under hypoxia, the IDH1- and IDH2-mediated reverse TCA cycle promotes glutamine-derived de novo lipogenesis and stabilizes the expression of α-KG and HIF-1α, thereby enhancing the growth and angiogenic capacity of EPCs. [Display omitted] • Hypoxia-induced reverse TCA cycle promotes de novo lipogenesis of bone marrow-derived EPCs. • IDH1 and IDH2 mediate the reverse TCA cycle. • The reverse TCA cycle stabilizes α-KG and sustains HIF-1α levels. • The EPCs cultured under hypoxia have better therapeutic effect on limb ischemia than that under normoxia. [ABSTRACT FROM AUTHOR]

Published

2024

43. Development of an In Vitro Model to Study Mechanisms of Ultrasound-Targeted Microbubble Cavitation–Mediated Blood–Brain Barrier Opening.

Author

Conway, Grace E., Paranjape, Anurag N., Chen, Xucai, and Villanueva, Flordeliza S.

Subjects

*BLOOD-brain barrier, *CELL imaging, *TIGHT junctions, *PERMEABILITY, *ENDOTHELIAL cells

Abstract

Ultrasound-targeted microbubble cavitation (UTMC)-mediated blood–brain barrier (BBB) opening is being explored as a method to increase drug delivery to the brain. This strategy has progressed to clinical trials for various neurological disorders, but the underlying cellular mechanisms are incompletely understood. In the study described here, a contact co-culture transwell model of the BBB was developed that can be used to determine the signaling cascade leading to increased BBB permeability. This BBB model consists of bEnd.3 cells and C8-D1A astrocytes seeded on opposite sides of a transwell membrane. Pulsed ultrasound (US) is applied to lipid microbubbles (MBs), and the change in barrier permeability is measured via transendothelial electrical resistance and dextran flux. Live cell calcium imaging (Fluo-4 AM) is performed during UTMC treatment. This model exhibits important features of the BBB, including endothelial tight junctions, and is more restrictive than the endothelial cell (EC) monolayer alone. When US is applied to MBs in contact with the ECs, BBB permeability increases in this model by two mechanisms: UTMC induces pore formation in the EC membrane (sonoporation), leading to increased transcellular permeability, and UTMC causes formation of reversible inter-endothelial gaps, which increases paracellular permeability. Additionally, this study determines that calcium influx into ECs mediates the increase in BBB permeability after UTMC in this model. Both transcellular and paracellular permeability can be used to increase drug delivery to the brain. Future studies can use this model to determine how UTMC-induced calcium-mediated signaling increases BBB permeability. [ABSTRACT FROM AUTHOR]

Published

2024

44. Ultrasound Modulates Calcium Activity in Cultured Neurons, Glial Cells, Endothelial Cells and Pericytes.

Author

Newman, Malachy, Rasiah, Pratheepa Kumari, Kusunose, Jiro, Rex, Tonia S., Mahadevan-Jansen, Anita, Hardenburger, Jacob, Jansen, E. Duco, Millis, Bryan, and Caskey, Charles F.

Subjects

*ASTROCYTES, *NEUROGLIA, *ENDOTHELIAL cells, *PERICYTES, *ULTRASONIC imaging, *ACOUSTICS

Abstract

Ultrasound is being researched as a method to modulate the brain. Studies of the interaction of sound with neurons support the hypothesis that mechanosensitive ion channels play an important role in ultrasound neuromodulation. The response of cells other than neurons (e.g., astrocytes, pericytes and endothelial cells) have not been fully characterized, despite playing an important role in brain function. To address this gap in knowledge, we examined cultured murine primary cortical neurons, astrocytes, endothelial cells and pericytes in an in vitro widefield microscopy setup during application of a 500 ms burst of 250 kHz focused ultrasound over a pressure range known to elicit neuromodulation. We examined cell membrane health in response to a range of pulses and used optical calcium indicators in conjunction with pharmacological antagonists to selectively block different groups of thermo- and mechanosensitive ion channels known to be responsive to ultrasound. All cell types experienced an increase in calcium fluorescence in response to ultrasound. Gadolinium (Gad), 2-aminoethoxydiphenyl borate (2-APB) and ruthenium red (RR) reduced the percentage of responding neurons and magnitude of response. The percentage of astrocytes responding was significantly lowered only by Gad, whereas both 2-APB and Gad decreased the amplitude of the fluorescence response. 2-APB decreased the percentage of responding endothelial cells, whereas only Gad reduced the magnitude of responses. Pericytes exposed to RR or Gad were less likely to respond to stimulation. RR had no detectable effect on the magnitude of the pericyte responses while 2-APB and Gad significantly decreased the fluorescence intensity, despite not affecting the percentage responding. Our study highlights the role of non-neuronal cells during FUS neuromodulation. All of the investigated cell types are sensitive to mechanical ultrasound stimulation and rely on mechanosensitive ion channels to undergo ultrasound neuromodulation. [ABSTRACT FROM AUTHOR]

Published

2024

45. Effect of serum from patients with ST-segment elevation myocardial infarction on endothelial cells.

Author

Ríos-Navarro, César, Gavara, José, de Dios, Elena, Pérez-Solé, Nerea, Molina-García, Tamara, Marcos-Garcés, Víctor, Ruiz-Saurí, Amparo, Bayés-Genís, Antoni, Carrión-Valero, Francisco, Chorro, Francisco J., and Bodí, Vicente

Abstract

Copyright of Revista Española de Cardiología (18855857) is the property of Elsevier B.V. and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published

2024

46. Osteogenic-angiogenic coupled response of cobalt-containing mesoporous bioactive glasses in vivo.

Author

Jiménez-Holguín, J., Lozano, D., Saiz-Pardo, M., de Pablo, D., Ortega, L., Enciso, S., Fernández-Tomé, B., Díaz-Güemes, I., Sánchez-Margallo, F.M., Portolés, M.T., and Arcos, D.

Subjects

BIOACTIVE glasses, VASCULAR endothelial cells, BONE regeneration, BONE grafting, BONE growth, ENDOTHELIAL cells

Abstract

The incorporation of cobalt ions into the composition of bioactive glasses has emerged as a strategy of interest for bone regeneration purposes. In the present work, we have designed a set of bioactive mesoporous glasses SiO 2 -CaO-P 2 O 5 -CoO (Co-MBGs) with different amounts of cobalt. The physicochemical changes introduced by the Co2+ ion, the in vitro effects of Co-MBGs on preosteoblasts and endothelial cells and their in vivo behaviour using them as bone grafts in a sheep model were studied. The results show that Co2+ ions neither destroy mesoporous ordering nor inhibit in vitro bioactive behaviour, exerting a dual role as network former and modifier for CoO concentrations above 3 % mol. On the other hand, the activity of Co-MBGs on MC3T3-E1 preosteoblasts and HUVEC vascular endothelial cells is dependent on the concentration of CoO present in the glass. For low Co-MBGs concentrations (1mg/ml) cell viability is not affected, while the expression of osteogenic (ALP, RUNX2 and OC) and angiogenic (VEGF) genes is stimulated. For Co-MBGs concentration of 5 mg/ml, cell viability decreases as a function of the CoO content. In vivo studies show that the incorporation of Co2+ ions to the MBGs improves the bone regeneration activity of these materials, despite the deleterious effect that this ion has on bone-forming cells for any of the Co-MBG compositions studied. This contradictory effect is explained by the marked increase in angiogenesis that takes place inside the bone defect, leading to an angiogenesis-osteogenesis coupling that compensates for the partial decrease in osteoblast cells. The development of new bone grafts implies to address the need for osteogenesis-angiogenesis coupling that allows bone regeneration with viable tissue in the long term. In this sense the incorporation of cobalt ions into the composition of bioactive glasses has emerged as a strategy of great interest in this field. Due to the potential cytotoxic effect of cobalt ions, there is an important controversy regarding the suitability of their incorporation in bone grafts. In this work, we address this controversy after the implantation of cobalt-doped mesoporous bioactive glasses in a sheep model. The incorporation of cobalt ions in bioactive glasses improves the bone regeneration ability of these bone grafts, due to enhancement of the angiogenesis-osteogenesis coupling. [Display omitted] [ABSTRACT FROM AUTHOR]

Published

2024

47. Update of pericytes function and their roles in kidney diseases.

Author

Chou, Yu-Hsiang, Pan, Szu-Yu, Shih, Hong-Mou, and Lin, Shuei-Liong

Subjects

KIDNEY diseases, PERICYTES, RENAL fibrosis, ACUTE kidney failure, ENDOTHELIAL cells

Abstract

Studies have highlighted the significant involvement of kidney pericytes in renal fibrosis. Kidney pericytes, classified as interstitial mesenchymal cells, are extensively branched, collagen-producing cells that closely interact with endothelial cells. This article aims to provide an overview of the recent advancements in understanding the physiological functions of pericytes and their roles in kidney diseases. In a healthy kidney, pericytes have essential physiological function in angiogenesis, erythropoietin (EPO) production, and the regulation of renal blood flow. Nevertheless, pericyte–myofibroblast transition has been identified as the primary cause of disease progression in acute kidney injury (AKI)-to-chronic kidney disease (CKD) continuum. Our recent research has demonstrated that hypoxia-inducible factor-2α (HIF-2α) regulates erythropoietin production in pericytes. However, this production is repressed by EPO gene hypermethylation and HIF-2α downregulation which were induced by transforming growth factor-β1-activated DNA methyltransferase and activin receptor-like kinase-5 signaling pathway during renal fibrosis, respectively. Additionally, AKI induces epigenetic modifications in pericytes, rendering them more prone to extracellular matrix production, cell migration and proliferation, thereby contributing to subsequent capillary rarefaction and renal fibrosis. Further investigation into the specific functions and roles of different subpopulations of pericytes may contribute for the development of targeted therapies aimed at attenuating kidney disease and mitigating their adverse effects. [ABSTRACT FROM AUTHOR]

Published

2024

48. Every sheriff needs a deputy: Targeting non-parenchymal cells to treat hepatic fibrosis.

Author

McGettigan, Brett M. and Shah, Vijay H.

Subjects

*HEPATIC fibrosis, *LIVER cells, *SHERIFFS, *ENDOTHELIAL cells, *LIVER diseases

Published

2024

49. Reprogramming endothelial cells to empower cancer immunotherapy.

Author

Cleveland, Abigail H. and Fan, Yi

Subjects

*ENDOTHELIAL cells, *MYELOID-derived suppressor cells, *CANCER cells, *METABOLIC reprogramming, *MYELOID cells

Abstract

The tumor vascular niche drives intratumoral immunosuppression, leading to immune evasion and immunotherapy resistance. Tumor endothelial cells educate myeloid suppressor cells and lymphocytes by angiocrines. Aberrant endothelial metabolism induces T cell exclusion and inactivation. Abnormal vasculature in tumors forms a pathophysiological barrier that hampers T cell infiltration. Genetic and metabolic reprogramming of endothelial cells may reverse tumor immunosuppression and overcome tumor resistance to immunotherapy. Cancer immunity is subject to spatiotemporal regulation by leukocyte interaction with the tumor microenvironment. Growing evidence suggests an emerging role for the vasculature in tumor immune evasion and immunotherapy resistance. Beyond the conventional functions of the tumor vasculature, such as providing oxygen and nutrients to support tumor progression, we propose multiplex mechanisms for vascular regulation of tumor immunity: The immunosuppressive vascular niche locoregionally educates circulation-derived immune cells by angiocrines, aberrant endothelial metabolism induces T cell exclusion and inactivation, and topologically and biochemically abnormal vascularity forms a pathophysiological barrier that hampers lymphocyte infiltration. We postulate that genetic and metabolic reprogramming of endothelial cells may rewire the immunosuppressive vascular microenvironment to overcome immunotherapy resistance, serving as a next-generation vascular targeting strategy for cancer treatment. [ABSTRACT FROM AUTHOR]

Published

2024

50. PEGylated nanoparticles interact with macrophages independently of immune response factors and trigger a non-phagocytic, low-inflammatory response.

Author

Asoudeh, Monireh, Nguyen, Nicole, Raith, Mitch, Denman, Desiree S., Anozie, Uche C., Mokhtarnejad, Mahshid, Khomami, Bamin, Skotty, Kaitlyn M., Isaac, Sami, Gebhart, Taylor, Vaigneur, Lauren, Gelgie, Aga, Dego, Oudessa Kerro, Freeman, Trevor, Beever, Jon, and Dalhaimer, Paul

Subjects

*PHAGOCYTOSIS, *IMMUNE response, *LIPOPROTEIN receptors, *BLOOD proteins, *MACROPHAGES, *HIGH density lipoproteins, *ENDOTHELIAL cells, *MACROPHAGE colony-stimulating factor

Abstract

Poly-ethylene-glycol (PEG)-based nanoparticles (NPs) - including cylindrical micelles (CNPs), spherical micelles (SNPs), and PEGylated liposomes (PLs) - are hypothesized to be cleared in vivo by opsonization followed by liver macrophage phagocytosis. This hypothesis has been used to explain the rapid and significant localization of NPs to the liver after administration into the mammalian vasculature. Here, we show that the opsonization-phagocytosis nexus is not the major factor driving PEG-NP – macrophage interactions. First, mouse and human blood proteins had insignificant affinity for PEG-NPs. Second, PEG-NPs bound macrophages in the absence of serum proteins. Third, lipoproteins blocked PEG-NP binding to macrophages. Because of these findings, we tested the postulate that PEG-NPs bind (apo)lipoprotein receptors. Indeed, PEG-NPs triggered an in vitro macrophage transcription program that was similar to that triggered by lipoproteins and different from that triggered by lipopolysaccharide (LPS) and group A Streptococcus. Unlike LPS and pathogens, PLs did not increase transcripts involved in phagocytosis or inflammation. High-density lipoprotein (HDL) and SNPs triggered remarkably similar mouse bone-marrow-derived macrophage transcription programs. Unlike opsonized pathogens, CNPs, SNPs, and PLs lowered macrophage autophagosome levels and either reduced or did not increase the secretion of key macrophage pro-inflammatory cytokines and chemokines. Thus, the sequential opsonization and phagocytosis process is likely a minor aspect of PEG-NP – macrophage interactions. Instead, PEG-NP interactions with (apo)lipoprotein and scavenger receptors appear to be a strong driving force for PEG-NP – macrophage binding, entry, and downstream effects. We hypothesize that the high presence of these receptors on liver macrophages and on liver sinusoidal endothelial cells is the reason PEG-NPs localize rapidly and strongly to the liver. [Display omitted] [ABSTRACT FROM AUTHOR]

Published

2024