Your search keyword '"Anya Wernersson"' showing total 5 results

1. The Vbeta13 T Cell Receptor Monoclonal Antibody Reduces Hyaluronan and CD68+, CD3+, and CD8+ Cell Infiltrations to Delay Diabetes in Congenic BB DRLyp/Lyp Rats

Author

Marika Bogdani, Linda Faxius, Malin Fex, Anita Ramelius, Anya Wernersson, John P. Mordes, Elizabeth P. Blankenhorn, and Åke Lernmark

Subjects

autoimmune diabetes, BB rat, hyaluronan, insulitis, pancreatic islets, T-cell receptor, Diseases of the endocrine glands. Clinical endocrinology, RC648-665

Abstract

The depleting Vβ13a T cell receptor monoclonal antibody (mAb) 17D5 prevents both induced and spontaneous autoimmune diabetes in BB rats. Here it was tested in congenic DRLyp/Lyp rats, all of which spontaneously developed diabetes. Starting at 40 days of age, rats were injected once weekly with either saline, His42 Vβ16 mAb, or 17D5 mAb and monitored for hyperglycemia. Diabetes occurred in 100% (n = 5/5) of saline-treated rats (median age, 66 days; range 55–73), and in 100% (n = 6/6) of His42-treated rats (median age, 69 days; range 59–69). Diabetes occurred in fewer (n = 8/11, 73%) 17D5-treated rats at a later age (median 76 days, range 60–92). Three (27%) of the 17D5-treated rats were killed at 101–103 days of age without diabetes (17D5 no-diabetes rats). Survival analysis demonstrated that 17D5 mAb delayed diabetes onset. Saline- and His42-treated rats had severely distorted islets with substantial loss of insulin-positive cells. These rats exhibited prominent hyaluronan (HA) staining, with the intra-islet HA+ accumulations measuring 5,000 ± 2,400 µm2 and occupying 36 ± 12% of islet area, and severe (grade 4) insulitis with abundant infiltration by CD68+, CD3+, and CD8+ cells. The 17D5 mAb-treated rats with delayed diabetes onset exhibited less severe insulitis (predominantly grade 3). In contrast, the 17D5 no-diabetes rats had mostly normal islets, with insulin+ cells representing 76 ± 3% of islet cells. In these rats, the islet HA deposits were significantly smaller than in the diabetic rats; the intra-islet HA+ areas were 1,200 ± 300 µm2 and accounted for 8 ± 1% of islet area. Also, islet-associated CD68+ and CD3+ cells occurred less frequently (on average in 60 and 3% of the islets, respectively) than in the diabetes rats (present in >95% of the islets). No CD8+ cells were detected in islets in all 17D5 no-diabetes rats. We conclude that mAb 17D5 delayed diabetes in DRLyp/Lyp rats and markedly reduced expression of HA and concomitant infiltration of CD68+, CD3+, and CD8+ cells. Our findings underscore the importance of refining immune suppression in prevention or intervention clinical trials to use mAb reagents that are directed against specific T cell receptors.

Published

2021

2. Mitochondrial clearance of calcium facilitated by MICU2 controls insulin secretion

Author

David G. Nicholls, Anya Wernersson, Vamsi K. Mootha, Peter Spégel, Kimberli J. Kamer, H. Barnard, Elaine Cowan, Neelanjan Vishnu, Annika Bagge, Alexander Hamilton, Malin Fex, Anders Tengholm, Hindrik Mulder, and Y. Sancak

Subjects

0301 basic medicine, Male, Voltage-dependent calcium channels, chemistry.chemical_element, 030209 endocrinology & metabolism, Mitochondrial calcium uniporter, Calcium, Mitochondrion, Bioenergetics, 03 medical and health sciences, Mice, 0302 clinical medicine, Insulin-Secreting Cells, Insulin Secretion, Animals, Humans, Uniporter, Inner mitochondrial membrane, Molecular Biology, Internal medicine, Mice, Knockout, Calcium-Binding Proteins, Cell Biology, Hyperpolarization (biology), RC31-1245, Cell biology, Mitochondria, Rats, Cytosol, 030104 developmental biology, HEK293 Cells, chemistry, Cell culture, Gene Knockdown Techniques, Stimulus-secretion coupling, Mitochondrial Membranes, Original Article, Female, Calcium Channels, Intracellular, Knockout mice

Abstract

Objective Transport of Ca2+ into pancreatic β cell mitochondria facilitates nutrient-mediated insulin secretion. However, the underlying mechanism is unclear. Recent establishment of the molecular identity of the mitochondrial Ca2+ uniporter (MCU) and associated proteins allows modification of mitochondrial Ca2+ transport in intact cells. We examined the consequences of deficiency of the accessory protein MICU2 in rat and human insulin-secreting cells and mouse islets. Methods siRNA silencing of Micu2 in the INS-1 832/13 and EndoC-βH1 cell lines was performed; Micu2−/− mice were also studied. Insulin secretion and mechanistic analyses utilizing live confocal imaging to assess mitochondrial function and intracellular Ca2+ dynamics were performed. Results Silencing of Micu2 abrogated GSIS in the INS-1 832/13 and EndoC-βH1 cells. The Micu2−/− mice also displayed attenuated GSIS. Mitochondrial Ca2+ uptake declined in MICU2-deficient INS-1 832/13 and EndoC-βH1 cells in response to high glucose and high K+. MICU2 silencing in INS-1 832/13 cells, presumably through its effects on mitochondrial Ca2+ uptake, perturbed mitochondrial function illustrated by absent mitochondrial membrane hyperpolarization and lowering of the ATP/ADP ratio in response to elevated glucose. Despite the loss of mitochondrial Ca2+ uptake, cytosolic Ca2+ was lower in siMICU2-treated INS-1 832/13 cells in response to high K+. It was hypothesized that Ca2+ accumulated in the submembrane compartment in MICU2-deficient cells, resulting in desensitization of voltage-dependent Ca2+ channels, lowering total cytosolic Ca2+. Upon high K+ stimulation, MICU2-silenced cells showed higher and prolonged increases in submembrane Ca2+ levels. Conclusions MICU2 plays a critical role in β cell mitochondrial Ca2+ uptake. β cell mitochondria sequestered Ca2+ from the submembrane compartment, preventing desensitization of voltage-dependent Ca2+ channels and facilitating GSIS., Graphical abstract Image 1, Highlights • MICU2 deficiency impairs glucose-stimulated insulin secretion. • MICU2 deficiency abrogates mitochondrial calcium uptake. • Depolarization-evoked cytosolic calcium increases are lower in MICU2-deficient cells. • Mitochondria clear calcium from the subplasma membrane region, maintaining calcium influx.

Published

2021

3. The Vbeta13 T Cell Receptor Monoclonal Antibody Reduces Hyaluronan and CD68+, CD3+, and CD8+ Cell Infiltrations to Delay Diabetes in Congenic BB DRLyp/Lyp Rats

Author

Malin Fex, Marika Bogdani, Anya Wernersson, Anita Ramelius, Elizabeth P. Blankenhorn, Linda Faxius, Åke Lernmark, and John P. Mordes

Subjects

Blood Glucose, 0301 basic medicine, CD3 Complex, Endocrinology, Diabetes and Metabolism, medicine.medical_treatment, CD8-Positive T-Lymphocytes, insulitis, lcsh:Diseases of the endocrine glands. Clinical endocrinology, Endocrinology, 0302 clinical medicine, Insulin-Secreting Cells, Rats, Inbred BB, T-cell receptor, Hyaluronic Acid, Original Research, geography.geographical_feature_category, biology, Chemistry, BB rat, Antibodies, Monoclonal, Islet, medicine.anatomical_structure, medicine.medical_specialty, CD3, Receptors, Antigen, T-Cell, Antigens, Differentiation, Myelomonocytic, 030209 endocrinology & metabolism, Polymorphism, Single Nucleotide, autoimmune diabetes, Diabetes Mellitus, Experimental, hyaluronan, 03 medical and health sciences, Immune system, Antigens, CD, Internal medicine, Diabetes mellitus, medicine, Animals, geography, pancreatic islets, lcsh:RC648-665, Macrophages, Pancreatic islets, Insulin, medicine.disease, 030104 developmental biology, biology.protein, Insulitis, CD8

Abstract

The depleting Vβ13a T cell receptor monoclonal antibody (mAb) 17D5 prevents both induced and spontaneous autoimmune diabetes in BB rats. Here it was tested in congenic DRLyp/Lyp rats, all of which spontaneously developed diabetes. Starting at 40 days of age, rats were injected once weekly with either saline, His42 Vβ16 mAb, or 17D5 mAb and monitored for hyperglycemia. Diabetes occurred in 100% (n = 5/5) of saline-treated rats (median age, 66 days; range 55–73), and in 100% (n = 6/6) of His42-treated rats (median age, 69 days; range 59–69). Diabetes occurred in fewer (n = 8/11, 73%) 17D5-treated rats at a later age (median 76 days, range 60–92). Three (27%) of the 17D5-treated rats were killed at 101–103 days of age without diabetes (17D5 no-diabetes rats). Survival analysis demonstrated that 17D5 mAb delayed diabetes onset. Saline- and His42-treated rats had severely distorted islets with substantial loss of insulin-positive cells. These rats exhibited prominent hyaluronan (HA) staining, with the intra-islet HA+ accumulations measuring 5,000 ± 2,400 µm2 and occupying 36 ± 12% of islet area, and severe (grade 4) insulitis with abundant infiltration by CD68+, CD3+, and CD8+ cells. The 17D5 mAb-treated rats with delayed diabetes onset exhibited less severe insulitis (predominantly grade 3). In contrast, the 17D5 no-diabetes rats had mostly normal islets, with insulin+ cells representing 76 ± 3% of islet cells. In these rats, the islet HA deposits were significantly smaller than in the diabetic rats; the intra-islet HA+ areas were 1,200 ± 300 µm2 and accounted for 8 ± 1% of islet area. Also, islet-associated CD68+ and CD3+ cells occurred less frequently (on average in 60 and 3% of the islets, respectively) than in the diabetes rats (present in >95% of the islets). No CD8+ cells were detected in islets in all 17D5 no-diabetes rats. We conclude that mAb 17D5 delayed diabetes in DRLyp/Lyp rats and markedly reduced expression of HA and concomitant infiltration of CD68+, CD3+, and CD8+ cells. Our findings underscore the importance of refining immune suppression in prevention or intervention clinical trials to use mAb reagents that are directed against specific T cell receptors.

Published

2021

4. Human enteroviral infection impairs autophagy in clonal INS(832/13) cells and human pancreatic islet cells

Author

Elaine Cowan, Anya Wernersson, Corrado M. Cilio, Luis Sarmiento, and Malin Fex

Subjects

0301 basic medicine, Autophagosome, Male, Endocrinology, Diabetes and Metabolism, Cell, Blotting, Western, 030209 endocrinology & metabolism, Balanced salt solution, Virus spread, Virus Replication, Article, 03 medical and health sciences, Islets of Langerhans, 0302 clinical medicine, Internal Medicine, medicine, Autophagy, Viral replication, Humans, Pancreas, Enterovirus, Type 1 diabetes, Chemistry, Insulin secretion, Beta cells, medicine.disease, Molecular biology, 030104 developmental biology, medicine.anatomical_structure, Cell culture, Female, Beta cell, Lysosomes, Homeostasis

Abstract

Aim/hypothesis Human enteroviral infections are suggested to be associated with type 1 diabetes. However, the mechanism by which enteroviruses can trigger disease remains unknown. The present study aims to investigate the impact of enterovirus on autophagy, a cellular process that regulates beta cell homeostasis, using the clonal beta cell line INS(832/13) and human islet cells as in vitro models. Methods INS(832/13) cells and human islet cells were infected with a strain of echovirus 16 (E16), originally isolated from the stool of a child who developed type 1 diabetes-associated autoantibodies. Virus production and release was determined by 50% cell culture infectious dose (CCID50) assay and FACS analysis. The occurrence of autophagy, autophagosomes, lysosomes and autolysosomes was detected by western blot, baculoviral-mediated expression of microtubule-associated protein light chain 3 (LC3)II-GFP and LysoTracker Red, and quantified by Cellomics ArrayScan. Autophagy was also monitored with a Cyto-ID detection kit. Nutrient deprivation (low glucose [2.8 mmol/l]), amino acid starvation (Earle’s Balanced Salt Solution [EBSS]) and autophagy-modifying agents (rapamycin and chloroquine) were used in control experiments. Insulin secretion and the expression of autophagy-related (Atg) genes and genes involved in autophagosome–lysosome fusion were determined. Results E16-infected INS(832/13) cells displayed an accumulation of autophagosomes, compared with non-treated (NT) cells (grown in complete RPMI1640 containing 11.1 mmol/l glucose) (32.1 ± 1.7 vs 21.0 ± 1.2 μm2/cell; p = 0.05). This was accompanied by increased LC3II ratio both in E16-infected cells grown in low glucose (LG) (2.8 mmol/l) (0.42 ± 0.03 vs 0.11 ± 0.04 (arbitrary units [a.u.]); p p p = 0.012) and grown in media containing 11.1 mmol/l glucose (1.79 ± 0.39 vs 0.66 ± 0.15 (a.u.); p = 0.0078). mRNA levels of genes involved in autophagosome formation and autophagosome–lysosome fusion remained unchanged in E16-infected cells, except Atg7, which was significantly increased when autophagy was induced by E16 infection, in combination with LG (1.48 ± 0.08-fold; p = 0.02) and at 11.1 mmol/l glucose (1.26 ± 0.2-fold; p = 0.001), compared with NT controls. Moreover, autophagosomes accumulated in E16-infected cells to the same extent as when cells were treated with the lysosomal inhibitor, chloroquine, clearly indicating that autophagosome turnover was blocked. Upon infection, there was an increased viral titre in the cell culture supernatant and a marked reduction in glucose-stimulated insulin secretion (112.9 ± 24.4 vs 209.8 ± 24.4 ng [mg protein]–1 h–1; p = 0.006), compared with uninfected controls, but cellular viability remained unaffected. Importantly, and in agreement with the observations for INS(832/13) cells, E16 infection impaired autophagic flux in primary human islet cells (46.5 ± 1.6 vs 34.4 ± 2.1 μm2/cell; p = 0.01). Conclusions/interpretation Enteroviruses disrupt beta cell autophagy by impairing the later stages of the autophagic pathway, without influencing expression of key genes involved in core autophagy machinery. This results in increased viral replication, non-lytic viral spread and accumulation of autophagic structures, all of which may contribute to beta cell demise and type 1 diabetes.

Published

2020

5. Mitochondrial clearance of Ca2+ controls insulin secretion

Author

Kimberli J. Kamer, Alexander Hamilton, Anders Tengholm, Annika Bagge, Anya Wernersson, Hindrik Mulder, Neelanjan Vishnu, David G. Nicholls, Malin Fex, H. Barnard, Peter Spégel, Elaine Cowan, Y. Sancak, and Vamsi K. Mootha

Subjects

0303 health sciences, Chemistry, Depolarization, Hyperpolarization (biology), Mitochondrion, Cell biology, 03 medical and health sciences, Cytosol, 0302 clinical medicine, Mitochondrial matrix, Knockout mouse, Inner membrane, Uniporter, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

SUMMARYTransport of Ca2+from the cytosol to the mitochondrial matrix of insulin-secreting pancreatic β-cells facilitates nutrient-mediated insulin secretion. However, the underlying mechanism is unclear. The establishment of the molecular identity of the mitochondrial Ca2+uniporter (MCU) and associated proteins has allowed mitochondrial Ca2+transport to be modified in intact cells. We examined the consequences of deficiency of the accessory protein, MICU2, in rat and human insulin-secreting cell lines as well as in mouse islets. Glucose-induced mitochondrial Ca2+elevation and inner membrane hyperpolarization were reduced, together with cytosolic ATP/ADP-ratios and insulin secretion. Insulin secretion inMicu2knock out mice was attenuatedin vitroas well asin vivo. While KCl-evoked sub-plasmalemmal Ca2+increases were more pronounced, the global cytosolic Ca2+response was, surprisingly, diminished inMICU2-deficient cells. These findings were supported by selective inhibition of mitochondrial Ca2+uptake by mitochondrial depolarization. It is concluded that mitochondrial Ca2+transport plays an additional and hitherto unrecognized role in stimulated β-cells by regulating net Ca2+entry across the plasma membrane. This is likely accounted for by clearing of sub-plasmalemmal Ca2+levels by mitochondria located near the plasma membrane.

Published

2019