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1. Primary cilia control cellular patterning of Meibomian glands during morphogenesis but not lipid composition

Author

Céline Portal, Yvonne Lin, Varuni Rastogi, Cornelia Peterson, Samuel Chi-Hung Yiu, James W. Foster, Amber Wilkerson, Igor A. Butovich, and Carlo Iomini

Subjects
Biology (General), QH301-705.5
Abstract

Meibomian gland (MG) cells are ciliated in early stages of development and primary cilium is required to regulate early MG cell patterning within developing glands, with cilia-mediated signaling pathways identified as therapeutic targets.

Published
2023
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2. In situ transduction of cells in human corneal limbus using adeno-associated viruses: an ex vivo study

Author

Hyeck-Soo Son, Albert S. Jun, James W. Foster, Wei Wang, Yassine Daoud, Gerd U. Auffarth, and Madhuparna Roy

Subjects
Medicine, Science
Abstract

Abstract This study aimed to evaluate the efficacy of in situ adeno-associated virus (AAV)-mediated gene delivery into the human corneal limbal region via targeted sub-limbal injection technique. Human cadaveric corneal tissues were fixed on an artificial anterior chamber. Feasibility of sub-limbal injection technique was tested using trypan blue and black India ink. An enhanced green fluorescent protein (eGFP) encoding AAV DJ was injected into sub-limbal region. After AAV injection, corneal tissues were incubated in air-lift culture and prepared for immunohistochemical analysis. Cell survivial and expression of eGFP, stem cell markers (p63α and cytokeratin 19 (KRT19)), and differentiation marker cytokeratin 3 (KRT3) were evaluated using confocal microscopy. Both trypan blue and black India ink stained and were retained sub-limbally establishing specificity of the injection technique. Immunohistochemical analysis of corneas injected with AAV DJ-eGFP indicated that AAV-transduced cells in the limbal region co-express eGFP, p63α, and KRT19 and that these transduced cells were capable of differentiating to KRT3 postitive corneal epithelial cells. Our sub-limbal injection technique can target cells in the human limbus in a reproducible and efficient manner. Thus, we demonstrate that in situ injection of corneal limbus may provide a feasible mode of genetic therapy for corneal disorders with an epithelial etiology.

Published
2022
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3. The Correlation between Corneal Findings and Disease Severity in Keratoconus per Scheimpflug Corneal Tomography

Author

Ahmed E. M. Shehata, James W. Foster, Albert S. Jun, and Uri S. Soiberman

Subjects
Ophthalmology, RE1-994
Abstract

Purpose. This study aims to correlate the clinical signs of keratoconus (KC) which include superficial apical scarring, Fleischer rings, and Vogt striae with best spectacle-corrected visual acuity (BSCVA) and corneal tomography findings. Patients and methods. A retrospective observational study. 72 consecutive KC patients seen by the senior author over the course of one year were included in this case series. Eyes with pellucid marginal degeneration, postrefractive ectasia, history of a corneal graft, prior corneal collagen cross-linking, intracorneal ring segments or hydrops were excluded from analysis. Subsequently, the final analysis included only treatment-naïve KC eyes with varying degrees of disease severity. Results. BSCVA with manifest refraction was 0.5 logMAR higher in eyes with apical scarring (p

Published
2020
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4. Single cell RNA-seq of human cornea organoids identifies cell fates of a developing immature cornea

Author

George Maiti, Maithê Rocha Monteiro de Barros, Nan Hu, Igor Dolgalev, Mona Roshan, James W Foster, Aristotelis Tsirigos, Karl J Wahlin, and Shukti Chakravarti

Abstract

The cornea is a protective and refractive barrier in the eye crucial for vision. Understanding the human cornea in health, disease, and cell-based treatments can be greatly advanced with cornea organoids developed in culture from induced pluripotent stem cells. While a limited number of studies have investigated the single-cell transcriptomic composition of the human cornea, its organoids have not been examined similarly. Here, we elucidated the transcriptomic cell fate map of 4-month-old human cornea organoids and human donor corneas. The organoids harbor cell clusters that resemble cells of the corneal epithelium, stroma, and endothelium, with subpopulations that capture signatures of early developmental states. Unlike the adult cornea where the largest cell population is stromal, the organoids contain large proportions of epithelial and endothelial-like cells. These corneal organoids offer a 3D model to study corneal diseases and integrated responses of different cell types.

Published
2022
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5. Targeting the integrated stress response in ophthalmology

Author

Hsiao Sang Chu, James W Foster, Albert S. Jun, and Cornelia Peterson

Subjects
medicine.medical_specialty, Context (language use), Activating Transcription Factor 4, Biology, Article, Cornea, 03 medical and health sciences, Cellular and Molecular Neuroscience, 0302 clinical medicine, Anterior Eye Segment, Stress, Physiological, Ophthalmology, Ultraviolet light, medicine, Humans, Integrated stress response, eIF2, ATF4, Environmental exposure, Sensory Systems, Oxidative Stress, 030221 ophthalmology & optometry, Signal transduction, 030217 neurology & neurosurgery, Signal Transduction
Abstract

The Integrated Stress Response (ISR) is a powerful and conserved signaling pathway that allows for cells to respond to a diverse array of both intracellular and extracellular stressors. The pathway is classically responsible for coordination of the cellular response to amino acid starvation, ultraviolet light, heme dysregulation, viral infection, and unfolded protein. Under normal circumstances it is considered pro-survival and a necessary mechanism through which protein translation is controlled. However, in cases of severe or prolonged stress the pathway can promote apoptosis, and loss of normal cellular phenotype. The activation of this pathway culminates in the global inhibition of cap-dependent protein translation and the canonical expression of the activating transcription factor 4 (ATF4). The eye is uniquely exposed to these stressors due to its environmental exposure and relative isolation from the circulatory system which are necessary for its function. In this review we will summarize the growing body of evidence of the role of the ISR in the context of ophthalmology, with special interest on the cornea and anterior segment. We will discuss how this pathway is critical for the proper function of the tissue, its role in development, as well as how targeting of the pathway could alleviate key aspects of diverse ophthalmic diseases.

Published
2021
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6. The Correlation between Corneal Findings and Disease Severity in Keratoconus per Scheimpflug Corneal Tomography

Author

James W Foster, Uri Soiberman, Ahmed E. M. Shehata, and Albert S. Jun

Subjects
0301 basic medicine, Keratoconus, medicine.medical_specialty, Visual acuity, Article Subject, genetic structures, Scheimpflug principle, Pellucid marginal degeneration, 03 medical and health sciences, 0302 clinical medicine, Disease severity, Ectasia, Ophthalmology, medicine, Advanced disease, business.industry, Corneal tomography, RE1-994, medicine.disease, eye diseases, 030104 developmental biology, 030221 ophthalmology & optometry, sense organs, medicine.symptom, business, Research Article
Abstract

Purpose. This study aims to correlate the clinical signs of keratoconus (KC) which include superficial apical scarring, Fleischer rings, and Vogt striae with best spectacle-corrected visual acuity (BSCVA) and corneal tomography findings.Patients and methods. A retrospective observational study. 72 consecutive KC patients seen by the senior author over the course of one year were included in this case series. Eyes with pellucid marginal degeneration, postrefractive ectasia, history of a corneal graft, prior corneal collagen cross-linking, intracorneal ring segments or hydrops were excluded from analysis. Subsequently, the final analysis included only treatment-naïve KC eyes with varying degrees of disease severity.Results. BSCVA with manifest refraction was 0.5 logMAR higher in eyes with apical scarring (p<0.001). Eyes with apical scarring had worse vision than eyes with Fleischer rings alone (0.43 logMAR higher in the former,p<0.009). Eyes with apical scarring had higher keratometry readings (K2 = 64.56 ± 12.89 D versus 49.07 ± 6.61 D,p<0.001); this was also true for eyes with Fleischer rings compared with ring-free eyes (K2 = 56.23 ± 11.52 D versus 48.91 ± 7.79 D,p<0.001) and eyes with Vogt striae (K2 = 56.19 ± 10.27 D versus 50.68 ± 9.21 D,p=0.01). Atopic disease was a risk factor for scarring: odds ratio (OR) = 2.87 (p=0.03). The OR of observing Fleischer rings in KC eyes was 12% per year (p=0.001). Additionally, each mm of corneal apex displacement from the pupillary center led to a 0.76 logMAR increase in visual acuity (p=0.001).Conclusion. The presence of apical scarring and Fleischer rings on biomicroscopy can aid the clinician in making the distinction between severe or long-standing disease (respectively). Apical scarring is a sign of advanced disease and is associated with worse BSCVA and tomography findings. Fleischer rings are markers of intermediate disease and their presence correlates with disease duration.

Published
2020

7. A Guide to the Development of Human CorneaOrganoids from Induced Pluripotent Stem Cells in Culture

Author

Shukti Chakravarti, Karl J. Wahlin, and James W Foster

Subjects
0301 basic medicine, Induced Pluripotent Stem Cells, Cell Culture Techniques, Article, Cornea, Extracellular matrix, 03 medical and health sciences, Epithelial Differentiation, 0302 clinical medicine, medicine, Organoid, Humans, Induced pluripotent stem cell, Cell Proliferation, Corneal epithelium, Chemistry, Epithelium, Corneal, Cell Differentiation, eye diseases, Extracellular Matrix, Cell biology, Organoids, Endothelial stem cell, 030104 developmental biology, medicine.anatomical_structure, sense organs, 030217 neurology & neurosurgery
Abstract

The cornea is the outermost transparent and refractive barrier surface of the eye necessary for vision. Development of the cornea involves the coordinated production of extracellular matrix, epithelial differentiation, and endothelial cell expansion to produce a highly transparent tissue. Here we describe the production of multilayered three-dimensional organoids from human-induced pluripotent stem cells. These organoids have the potential for multiple downstream applications which are currently unattainable using traditional in vitro techniques.

Published
2020
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8. Induction of the integrated stress response in the rat cornea

Author

Albert S. Jun, Laura M. Ensign, James W Foster, Y.C. Kim, and C. Peterson

Subjects
Agonist, Keratoconus, Intraocular pressure, Pathology, medicine.medical_specialty, medicine.drug_class, medicine.medical_treatment, Corneal Keratocytes, Article, Collagen Type I, Cornea, Rats, Sprague-Dawley, Pathogenesis, Cellular and Molecular Neuroscience, In vivo, medicine, Animals, Integrated stress response, Corneal transplantation, Extracellular Matrix Proteins, business.industry, Thiourea, medicine.disease, Activating Transcription Factor 4, eye diseases, Sensory Systems, Rats, Collagen Type I, alpha 1 Chain, Disease Models, Animal, Ophthalmology, medicine.anatomical_structure, Cinnamates, Female, business
Abstract

Keratoconus (KC), a progressive, degenerative corneal disease, represents the second leading indication for corneal transplantation globally. We have previously demonstrated that components of the Integrated Stress Response (ISR) are upregulated in human keratoconic donor tissue, and treatment of normal tissue with ISR agonists attenuates collagen production. With no consistently accepted animal models available for translational KC research, we sought to establish an in vivo model based on ISR activation to elucidate its role in the development of the KC phenotype. Four-week-old female SD rats were treated with topical SAL003 formulated as a nanosuspension or vehicle every 48 h for four doses. Animals were subject to monitoring for ocular inflammation and discomfort before being euthanized at 1, 14, or 28 days after treatment was withdrawn. Schirmer's tear test, intraocular pressure, and body weight measurements were obtained at baseline and prior to euthanasia. Globes were subject to routine histopathology, immunohistochemistry for ATF4, and qPCR for Col1a1 expression. ANOVAs and Student's t tests were used to assess statistical significance (α = 0.05). SAL003 treatment did not produce any adverse ocular or systemic phenotype but did result in decreased keratocyte density. Col1a1 transcripts were reduced, corresponding to nuclear ATF4 expression within the axial cornea. In vivo topical treatment with a gel-formulated ISR agonist recapitulates key features of the activated ISR including nuclear ATF4 expression and decreased extracellular matrix (ECM) production. Exogenous ISR agonists may present one approach to establishing a rodent model for keratoconus, a charge essential for future evaluations of pathogenesis and therapeutic interventions.

Published
2021
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9. Pathophysiology of Keratoconus: What Do We Know Today

Author

James W Foster, Albert S. Jun, Uri Soiberman, and Shukti Chakravarti

Subjects
0301 basic medicine, Morphology, Proteomics, TGF-β, medicine.medical_specialty, Keratoconus, genetic structures, Corneal epithelium, Disease, Pathogenesis, Abnormal protein, Article, 03 medical and health sciences, Corneal ectasia, 0302 clinical medicine, Ophthalmology, Cornea, Medicine, Cytokine, business.industry, medicine.disease, Pathophysiology, eye diseases, 030104 developmental biology, medicine.anatomical_structure, Oxidative stress, 030221 ophthalmology & optometry, Progressive visual impairment, sense organs, Keratocytes, business
Abstract

Keratoconus is a common corneal ectasia that leads to progressive visual impairment. Numerous studies have shown abnormal protein expression patterns in keratoconic corneas. However, the specific mechanisms causing this disease remain ambiguous. This review aims to provide an update on morphological studies of the keratoconic cornea, relate these early studies with current findings from proteomic, biochemical and cell culture studies and to postulate possible pathogenic pathways.

Published
2017

10. Transcriptomic and Immunohistochemical Analysis of Progressive Keratoconus Reveal Altered WNT10A in Epithelium and Bowman's Layer

Author

Mario Matthaei, Shukti Chakravarti, Albert S. Jun, Rupin N. Parikh, Kraig S. Bower, James W Foster, Charles G. Eberhart, Uri Soiberman, and Jiangxia Wang

Subjects
Adult, Male, 0301 basic medicine, Keratoconus, keratoconus, Blotting, Western, Biology, Real-Time Polymerase Chain Reaction, Collagen Type I, Cornea, Young Adult, 03 medical and health sciences, 0302 clinical medicine, Western blot, Gene expression, medicine, Humans, RNA, Messenger, Bowman Membrane, Corneal epithelium, corneal epithelium, Messenger RNA, medicine.diagnostic_test, Sequence Analysis, RNA, Epithelium, Corneal, medicine.disease, Wnt signaling, Immunohistochemistry, Molecular biology, eye diseases, Epithelium, WNT10A, Collagen Type I, alpha 1 Chain, Wnt Proteins, Phenotype, 030104 developmental biology, Real-time polymerase chain reaction, medicine.anatomical_structure, Gene Expression Regulation, 030221 ophthalmology & optometry, Female, sense organs, Transcriptome, Plasmids
Abstract

Purpose To identify global gene expression changes in the corneal epithelium of keratoconus (KC) patients compared to non-KC myopic controls. Methods RNA-sequencing was performed on corneal epithelium samples of five progressive KC and five myopic control patients. Selected results were validated using TaqMan quantitative PCR (qPCR) on 31 additional independent samples, and protein level validation was conducted using western blot analysis on a subset. Immunohistochemistry was performed on tissue microarrays containing cores from over 100 KC and control cases. WNT10A transcript levels in corneal epithelium were correlated with tomographic indicators of KC disease severity in 15 eyes. Additionally, WNT10A was overexpressed in vitro in immortalized corneal epithelial cells. Results WNT10A was found to be underexpressed in KC epithelium at the transcript (ratio KC/control = 0.59, P = 0.02 per RNA-sequencing study; ratio = 0.66, P = 0.03 per qPCR) and protein (ratio = 0.07, P = 0.06) levels. Immunohistochemical analysis also indicated WNT10A protein was decreased in Bowman's layer of KC patients. In contrast, WNT10A transcript level positively correlated with increased keratometry (Kmax ρ = 0.57, P = 0.02). Finally, WNT10A positively regulated COL1A1 expression in corneal epithelial cells. Conclusions A specific Wnt ligand, WNT10A, is reduced at the mRNA and protein level in KC epithelium and Bowman's layer. This ligand positively regulates collagen type I expression in corneal epithelial cells. The results suggest that WNT10A expression in the corneal epithelium may play a role in progressive KC.

Published
2021
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11. Cornea organoids from human induced pluripotent stem cells

Author

Karl J. Wahlin, David E. Birk, James W Foster, Shukti Chakravarti, Donald J. Zack, and Sheila M. Adams

Subjects
0301 basic medicine, Cell type, Stromal cell, Cellular differentiation, Induced Pluripotent Stem Cells, Cell Culture Techniques, Biology, Eye, Article, Extracellular matrix, Cornea, 03 medical and health sciences, 0302 clinical medicine, medicine, Organoid, Humans, Stem Cell Research - Embryonic - Human, Induced pluripotent stem cell, Eye Disease and Disorders of Vision, Multidisciplinary, Endothelial Cells, Epithelial Cells, Cell Differentiation, Stem Cell Research, eye diseases, Cell biology, Endothelial stem cell, Organoids, 030104 developmental biology, medicine.anatomical_structure, 030221 ophthalmology & optometry, sense organs, Stromal Cells
Abstract

The cornea is the transparent outermost surface of the eye, consisting of a stratified epithelium, a collagenous stroma and an innermost single-cell layered endothelium and providing 2/3 of the refractive power of the eye. Multiple diseases of the cornea arise from genetic defects where the ultimate phenotype can be influenced by cross talk between the cell types and the extracellular matrix. Cell culture modeling of diseases can benefit from cornea organoids that include multiple corneal cell types and extracellular matrices. Here we present human iPS cell-derived organoids through sequential rounds of differentiation programs. These organoids share features of the developing cornea, harboring three distinct cell types with expression of key epithelial, stromal and endothelial cell markers. Cornea organoid cultures provide a powerful 3D model system for investigating corneal developmental processes and their disruptions in diseased conditions.

Published
2017
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12. Small Molecule Modulation of the Integrated Stress Response Governs the Keratoconic Phenotype In Vitro

Author

Yassine J. Daoud, Ahmed Mahmoud Shehata, James W Foster, Albert S. Jun, Tempest Young, Shukti Chakravarti, Michelle Lu, and Uri Soiberman

Subjects
collagen, 0301 basic medicine, keratoconus, Blotting, Western, Cell Count, Corneal Keratocytes, Real-Time Polymerase Chain Reaction, Collagen Type I, Cornea, 03 medical and health sciences, chemistry.chemical_compound, cell stress, 0302 clinical medicine, Stress, Physiological, Protein Phosphatase 1, Acetamides, medicine, Humans, Integrated stress response, Prospective Studies, ATF4, Enzyme Inhibitors, ISR, Fibroblast, Sirius Red, Cells, Cultured, Cyclohexylamines, Chemistry, Corneal Transplant, In vitro, Collagen Type I, alpha 1 Chain, Hydroxyproline, Phenotype, 030104 developmental biology, medicine.anatomical_structure, Matrix Metalloproteinase 9, 030221 ophthalmology & optometry, Cancer research, Matrix Metalloproteinase 2, Tumor necrosis factor alpha, Signal transduction, Ex vivo
Abstract

Purpose The degenerative corneal disease keratoconus is a leading indicator for corneal transplant with an unknown etiology. We recently identified the activation of the integrated stress response (ISR) in ex vivo human corneas and in vitro cell culture. Utilizing small molecules to modulate the ISR we sought to investigate the effects of stimulating the ISR in healthy cells to recapitulate aspects of the in vitro keratoconic phenotype and whether relieving the ISR signaling would recover the disease phenotype. Methods Corneal fibroblasts were extracted from patients undergoing corneal transplant or unaffected cadaverous donor limbal rings. Cells were exposed to the DNA damage-inducible protein (GADD34) inhibitor SAL003 to stimulate the ISR, or Trans-ISRIB to relieve ISR signaling pathway. Collagen production was assessed through hydroxyproline production, Sirius Red incorporation, or quantitative (q)PCR. Western blotting, hydroxyproline, and qPCR were used to assess components of the ISR pathway and collagen production. Results ISR stimulation through SAL003 resulted in significant decrease of hydroxyproline and COL1A1 transcription and eventual apoptosis in normal fibroblasts. Patient (KC) fibroblast production of hydroxyproline was increased in response to ISRIB, while matrix metalloproteinase (MMP)9 production was lowered. The prospective biomarker of keratoconus prolactin-inducible factor was also upregulated in KC fibroblast cultures in response to ISRIB. Inflammatory markers TNFα and IL-1β were unaffected. Conclusions Activation of the ISR is sufficient to recapitulate many key aspects of the KC phenotype in unaffected cells in vitro. Inhibition of the ISR also relieves many of the hallmarks of KC in affected cells. Therefore, targeting of the ISR through small molecules is a potential therapeutic path for small molecule treatment of keratoconus.

Published
2019
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13. Integrated Stress Response and Decreased ECM in Cultured Stromal Cells From Keratoconus Corneas

Author

Gajanan Sathe, Yassine Dauoud, Jiang Qian, James W Foster, Akhilesh Pandey, Shukti Chakravarti, Sheng Liu, Uri Soiberman, Albert S. Jun, Vishal Shinde, and Julius Wan

Subjects
Adult, Male, Proteomics, collagen, 0301 basic medicine, Stromal cell, Cell Survival, Corneal Stroma, keratoconus, extracellular matrix, Blotting, Western, Corneal Keratocytes, Matrix metalloproteinase, Real-Time Polymerase Chain Reaction, Mass Spectrometry, Cornea, Extracellular matrix, Young Adult, 03 medical and health sciences, 0302 clinical medicine, Stress, Physiological, cellular stress, Humans, Integrated stress response, Cells, Cultured, Aged, Aged, 80 and over, Extracellular Matrix Proteins, biology, Chemistry, Middle Aged, Tissue Donors, Fibronectins, Cell biology, ADAMTS2, Fibronectin, Blot, Hydroxyproline, 030104 developmental biology, Cell culture, 030221 ophthalmology & optometry, biology.protein, Female
Abstract

Purpose Keratoconus (KC) is a multifactorial disease where progressive thinning and weakening of the cornea leads to loss of visual acuity. Although the underlying etiology is poorly understood, a major endpoint is a dysfunctional stromal connective tissue matrix. Using multiple individual KC corneas, we determined that matrix production by keratocytes is severely impeded due to an altered stress response program. Methods KC and donor (DN) stromal keratocytes were cultured in low glucose serum-free medium containing insulin, selenium and transferrin. Fibronectin, collagens and proteins related to their chaperone, processing and export, matrix metalloproteinase, and stress response related proteins were investigated by immunoblotting, immunocytochemistry, hydroxyproline quantification, and gelatin zymography. Multiplexed mass spectrometry was used for global proteomic profiling of 5 individual DN and KC cell culture. Transcription of selected proteins was assayed by qPCR. Results DN and KC cells showed comparable survival and growth. However, immunoblotting of selected ECM proteins and global proteomics showed decreased fibronectin, collagens, PCOLCE, ADAMTS2, BMP1, HSP47, other structural and cytoskeletal proteins in KC. Phosphorylated (p) eIF2α, a translation regulator and its target, ATF4 were increased in KC cultured cells and corneal sections. Conclusions The profound decrease in structural proteins in cultured KC cells and increase in the p-eIF2α, and ATF4, suggest a stress related blockade in structural proteins not immediately needed for cell survival. Therefore, this cell culture system reveals an intrinsic aggravated stress response with consequent decrease in ECM proteins as potential pathogenic underpinnings in KC.

Published
2018
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15. Functions of Peptidoglycan Recognition Proteins (Pglyrps) at the Ocular Surface: Bacterial Keratitis in Gene-Targeted Mice Deficient in Pglyrp-2, -3 and -4

Author

Shukti Chakravarti, Rachel L. Redfern, Jihane Frikeche, Ranjita N. Gowda, Sudarshan Pinglay, James W Foster, Leslie Cope, and Carolina Lema

Subjects
Antimicrobial peptides, lcsh:Medicine, Gene Expression, Biology, medicine.disease_cause, Keratitis, Microbiology, chemistry.chemical_compound, Mice, Gene expression, medicine, Animals, lcsh:Science, Mice, Knockout, Mice, Inbred BALB C, Multidisciplinary, Pseudomonas aeruginosa, lcsh:R, Wild type, Epithelium, Corneal, Bacterial Infections, N-Acetylmuramoyl-L-alanine Amidase, medicine.disease, Antimicrobial, Beta defensin, chemistry, Gene Targeting, Cytokines, lcsh:Q, Peptidoglycan, Inflammation Mediators, Carrier Proteins, Research Article
Abstract

Purpose Functions of antimicrobial peptidoglycan recognition proteins (Pglyrp1-4) at the ocular surface are poorly understood. Earlier, we reported an antibacterial role for Pglyrp-1 in Pseudomonas aeruginosa keratitis. Here we investigated functions of three other related genes Pglyrp-2, -3 and -4 in a mouse model of P. aeruginosa keratitis. Methods Wild type (WT) and each of the Pglyrp-null genotypes were challenged with P. aeruginosa keratitis. The eyes were scored in a blinded manner 24 and 48h post infection. Viable bacterial counts and inflammatory factors (IL-12, TNF-α, IFN-γ, CCL2, IL-6 and IL-10) were measured in whole eye homogenates using cytometric bead arrays. Expressions of Pglyrp-1-4, mouse beta defensins (mBD)-2,-3, cathelicidin-related antimicrobial peptide (CRAMP) were determined by qRTPCR in total RNA extracts of uninfected and infected eyes of WT and each of the Pglyrp-null mouse types. Results The Pglyrp-2-/- mice showed reduced disease and lower induction of pro-inflammatory TNF-α (p = 0.02) than WT or the other Pglyrp null mice. Viable bacterial yield was significantly lower in the Pglyrp-2-/- (p = 0.0007) and the Pglyrp-4-/- (p = 0.098) mice. With regards to expression of these antimicrobial genes, Pglyrp-2 expression was induced after infection in WT mice. Pglyrp-3 expression was low before and after infection in WT mice, while Pglyrp-4 expression was slightly elevated after infection in WT, Pglyrp-2 and -3 null mice. Pglyrp-1 expression was slightly elevated after infection in all genotypes without statistical significance. Transcripts for antimicrobial peptides mBD2, mBD3 and CRAMP were elevated in infected Pglyrp-2-/- males without statistical significance. Conclusions Efficient resolution of keratitis in the Pglyrp-2-/- mice may be due to a reduced pro-inflammatory microenvironment and synergistic antibacterial activities of defensins, CRAMP and Pglyrp-1. Therefore, in ocular infections the pro-inflammatory functions of Pglyrp-2 must be regulated to benefit the host.

Published
2015

16. Low-glucose enhances keratocyte-characteristic phenotype from corneal stromal cells in serum-free conditions

Author

James W Foster, Che J. Connon, and Ricardo M. Gouveia

Subjects
Pathology, medicine.medical_specialty, Stromal cell, Cell Survival, Lumican, CD34, Corneal Keratocytes, Culture Media, Serum-Free, Article, Cornea, Cell Movement, Cyclic AMP, medicine, Humans, Cell Proliferation, Microscopy, Multidisciplinary, biology, Phenotype, In vitro, Cell biology, ALDH1A1, Glucose, medicine.anatomical_structure, biology.protein, Stromal Cells, Keratocan, Biomarkers
Abstract

The avascular cornea is a uniquely-isolated organ, with its stroma constituting a nutrient-poor environment. Consequently, the availability of metabolites such as glucose to corneal stromal cells is considerably reduced compared with other tissues, or indeed with media commonly used to culture these cells in vitro. However, the role of glucose in the behaviour of human corneal keratocytes has been overlooked. As such, we sought to investigate the effects of low-glucose formulations on the phenotype of human corneal stromal cells. Cells cultured in low-glucose were able to survive for extended periods when compared to high-glucose, serum-free conditions. Furthermore, low-glucose enhanced their reversal to a keratocyte-characteristic phenotype. Specifically, cells within low-glucose medium assumed dendritic morphologies, with bean-shaped condensed nuclei, absence of alpha-smooth muscle actin or stress fibres and a corresponding reduction in migratory and contractile activities when compared with high-glucose, serum-free conditions. Moreover, cells within low-glucose uniquely recovered the ability to express a robust keratocyte-characteristic marker, CD34, while still expressing elevated levels of other representative phenotypic markers such as keratocan, lumican, ALDH1A1 and ALDH3A1. These results indicate that low-glucose enhances keratocyte-characteristic phenotype above and beyond established media formulations and thus has important implications for corneal biology in health and disease.

Published
2015
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17. Differential nuclear expression of Yap in basal epithelial cells across the cornea and substrates of differing stiffness

Author

Christian A. Bippes, Che J. Connon, James W Foster, Ricardo M. Gouveia, and Roanne R. Jones

Subjects
Pathology, medicine.medical_specialty, Cell, Cell Count, Biology, Limbus Corneae, Cellular and Molecular Neuroscience, Cornea, medicine, Animals, Mechanotransduction, Corneal epithelium, Adaptor Proteins, Signal Transducing, Cell Proliferation, Cell Nucleus, Stem Cells, Epithelium, Corneal, Cell Differentiation, Epithelial Cells, eye diseases, Sensory Systems, In vitro, Cell biology, Ophthalmology, medicine.anatomical_structure, Cytoplasm, Trans-Activators, Cattle, sense organs, Stem cell, Homeostasis, Biomarkers, Compliance
Abstract

Corneal epithelium is maintained throughout life by well-orchestrated proliferation of limbal epithelial stem cells, followed by migration and maturation centripetally across the ocular surface. The present study sets out to explore the role tissue stiffness (compliance) may have in directing both differentiation and centripetal migration of limbal epithelial stem cells during homeostasis. For that, we analysed the localization of the Yes-associated protein (Yap), a transcriptional co-activator previously shown to mediate cellular response and mechanical stimuli. Using both models of ocular surface compliance and normal bovine corneas we evaluated the nuclear/cytoplasmic expression ratio of Yap. Expression levels within corneal epithelial cells were compared in situ between the limbus and central cornea, and in vitro between limbal epithelial stem cells expanded upon biomimetic collagen gels of increasing stiffness. Nuclear expression of Yap was shown to increase within the expanded cells upon substrates of increasing stiffness. Subsequently, Yap was used as a novel molecular probe to investigate the mechanical microenvironment within a normal ocular surface. The in situ localization of Yap was predominantly cytoplasmic within basal limbal epithelial cells and nuclear within basal central corneal epithelial cells. Furthermore, nuclear p63 expression was not co-localized with Yap in basal limbal epithelial cells. In conclusion, the current investigation provides new insights into the relationship between Yap and distinct cell populations across the ocular surface indicating that cells experience a different mechanical environment between the limbus and central cornea. A new hypothesis is put forward, in which centripetal differences in substrate stiffness drives the migration and differentiation of limbal epithelial stem cells, thus controlling corneal epithelium homeostasis.

Published
2014

18. Transforming growth factor β and insulin signal changes in stromal fibroblasts of individual keratoconus patients

Author

Wai Hong Wu, Albert S. Jun, Yassine J. Daoud, James W Foster, Mehak Bassi, Sherri Gae Scott, Walter J. Stark, Divya Mohan, and Shukti Chakravarti

Subjects
medicine.medical_specialty, Cell biology, Cell signaling, Stromal cell, Glucose uptake, Science, Signal transduction, Biochemistry, Internal medicine, Molecular Cell Biology, medicine, Medicine and Health Sciences, AKT signaling cascade, Fibroblast, Protein kinase B, Extracellular Matrix Proteins, Multidisciplinary, biology, Biology and life sciences, Proteins, Signaling cascades, Transforming growth factor beta, 3. Good health, Extracellular Matrix, Transplantation, Ophthalmology, medicine.anatomical_structure, Endocrinology, TGF-beta signaling cascade, Cell culture, biology.protein, Corneal Disorders, Medicine, sense organs, Cellular Structures and Organelles, Transforming growth factor, Research Article
Abstract

Keratoconus (KC) is a complex thinning disease of the cornea that often requires transplantation. The underlying pathogenic molecular changes in this disease are poorly understood. Earlier studies reported oxidative stress, metabolic dysfunctions and accelerated death of stromal keratocytes in keratoconus (KC) patients. Utilizing mass spectrometry we found reduced stromal extracellular matrix (ECM) proteins in KC, suggesting ECM-regulatory changes that may be due to altered TGFβ signals. Here we investigated properties of stromal cells from donor (DN) and KC corneas grown as fibroblasts in serum containing DMEM: F12 or in serum-free medium containing insulin, transferrin, selenium (ITS). Phosphorylation of SMAD2/3 of the canonical TGFβ pathway, was high in serum-starved DN and KC fibroblast protein extracts, but pSMAD1/5/8 low at base line, was induced within 30 minutes of TGFβ1 stimulation, more so in KC than DN, suggesting a novel TGFβ1-SMAD1/5/8 axis in the cornea, that may be altered in KC. The serine/threonine kinases AKT, known to regulate proliferation, survival and biosynthetic activities of cells, were poorly activated in KC fibroblasts in high glucose media. Concordantly, alcohol dehydrogenase 1 (ADH1), an indicator of increased glucose uptake and metabolism, was reduced in KC compared to DN fibroblasts. By contrast, in low glucose (5.5 mM, normoglycemic) serum-free DMEM and ITS, cell survival and pAKT levels were comparable in KC and DN cells. Therefore, high glucose combined with serum-deprivation presents some cellular stress difficult to overcome by the KC stromal cells. Our study provides molecular insights into AKT and TGFβ signal changes in KC, and a mechanism for functional studies of stromal cells from KC corneas.

Published
2014

19. GASTROINTESTINAL PARASITES OF MOUNTAIN GORILLAS (GORILLA GORILLA BERINGEI) IN THE PARC NATIONAL DES VOLCANS, RWANDA

Author

Lisa L. Meader, James W. Foster, Jonathan M. Sleeman, Sharon Patton, and Antoine B. Mudakikwa

Subjects
Male, Veterinary medicine, food.ingredient, Mountain gorilla, Entamoeba, Feces, Entamoeba histolytica, food, Strongyloides, parasitic diseases, Animals, Trichostrongylus, Mites, Gorilla gorilla, General Veterinary, biology, Anoplocephala, Giardia, Endolimax nana, Rwanda, Entamoeba coli, General Medicine, fictional_universe, fictional_universe.character_species, biology.organism_classification, Trichuris, Female, Animal Science and Zoology, Chilomastix, Trematoda, Entamoeba hartmanni, Digestive System
Abstract

Ninety-eight fecal samples were collected from 74 free-living mountain gorillas (Gorilla gorilla beringei) from the Parc National des Volcans, Rwanda, between July 1995 and January 1997 and examined for parasites by Sheather's sugar and zinc sulfate flotation methods, trichrome staining, and larval cultures. All samples contained at least one parasite. Seventeen endoparasites were identified, including eight protozoa, seven nematodes, one cestode, and one trematode. Two species of arthropod mite were also recovered from the fecal samples. Parasites observed on fecal examinations included strongyle/trichostrongyle-type eggs (72/74) (representing Oesphagostomum sp., Trichostrongylus sp., Hyostrongylus spp., and possibly Murshidia sp.), Strongyloides sp. (1/74), Trichuris trichiura (2/74), Probstmayria sp. (7/74), Anoplocephala sp. (63/74), Entamoeba hartmanni cysts and trophozoites (19/70), Endolimax nana cysts (31/70), Iodamoeba buetschlii cysts (11/70), Endolimax nana or Iodamoeba buetschlii trophozoites (63/70). Entamoeba coli cysts and trophozoites (14/70), Entamoeba histolytica trophozoite (1/70), Chilomastix sp. cysts and trophozoites (31/70), and Giardia sp. cysts (2/70). In addition, one ascarid and one trematode egg were seen. There were no significant differences in the prevalence of parasites between males and females and between age groups: however, infants and juveniles appeared to have a lower prevalence of Anoplocephala gorillae, and the silverbacked males appeared to have a higher prevalence of Probstmayria sp. Parasite prevalence was consistent among the five social groups studied except Susa group had a significantly lower prevalence of Anoplocephala gorillae. Trichuris trichiura, Strongyloides sp., Chilomastix sp., and Endolimax nana were identified for the first time in this population, and it is possible that these parasites were of human origin. Although there were no obvious clinical effects due to the presence of these parasites, six parasites identified (Trichuris trichiura, Strongyloides sp., Oesphagostomum sp., Trichostrongylus sp., Entamoeba histolytica, and Giardia sp.) could potentially be pathogenic. Some of the parasite products and cultured larvae could not be speciated.

Published
2000
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20. FIELD ANESTHESIA OF FREE-LIVING MOUNTAIN GORILLAS (GORILLA GORILLA BERINGEI) FROM THE VIRUNGA VOLCANO REGION, CENTRAL AFRICA

Author

John-Bosco Nizeyi, Kenneth Cameron, Susanne Anderson, Barkley Hastings, Elizabeth J. Macfie, Antoine B. Mudakikwa, James W. Foster, Jonathan M. Sleeman, H. Melvyn Richardson, and John E. Cooper

Subjects
Male, Tiletamine / Zolazepam, Body Temperature, Benzodiazepines, Heart Rate, medicine, Animals, Anesthesia, Ketamine, Low hemoglobin, Retrospective Studies, Anesthetics, Dissociative, Tiletamine, Gorilla gorilla, General Veterinary, business.industry, Respiration, Rwanda, Central africa, Zolazepam, General Medicine, Anesthetics, Combined, Gorilla gorilla beringei, Oxygen, Anti-Anxiety Agents, Anesthetic, Democratic Republic of the Congo, Female, Animal Science and Zoology, business, medicine.drug
Abstract

Twenty-six anesthetic procedures involving 24 free-living mountain gorillas (Gorilla gorilla beringei) from Rwanda or the Democratic Republic of Congo were performed between February 1987 and October 1997. Sixteen procedures were performed to remove snares or to treat snare-related wounds, and four of the animals died without recovering consciousness because of their severe medical conditions. Ketamine was used for induction 19 times, tiletamine/zolazepam was used five times, and the agent was not recorded for two procedures. The mean (+/- SD) ketamine dosage for four animals of known weight was 7.1 +/- 0.9 mg/kg. All induction agents were delivered i.m. by remote injection, and mean induction times for ketamine and tiletamine/zolazepam were 5.5 +/- 2.6 min (n = 12) and 5.4 +/- 3.7 min (n = 5), respectively. Mean recovery times were significantly shorter with ketamine compared with tiletamine/zolazepam (42.0 +/- 24.9 min, n = 9 vs. 75.25 +/- 22.1 min, n = 4). Low hemoglobin oxygen saturation (mean = 86.7%) was recorded in three cases under ketamine anesthesia, and oxygen insufflation is therefore recommended to prevent hypoxemia. Gorillas induced with tiletamine/zolazepam had significantly higher respiratory rates compared with animals given ketamine. Successful anesthesia and recovery, in particular, depended on the assistance of local personnel.

Published
2000
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21. Influence of substrate on corneal epithelial cell viability within ocular surface models

Author

Che J. Connon, James W Foster, Yun Feng, Bo Chen, and Shengli Mi

Subjects
Stromal cell, Cell Survival, Cell, Cell Count, Models, Biological, Cell Line, Cellular and Molecular Neuroscience, Tissue engineering, Cornea, medicine, Humans, MTT assay, Viability assay, Fluorescent Antibody Technique, Indirect, Polycarboxylate Cement, Tight junction, Tissue Engineering, Tissue Scaffolds, Chemistry, Reverse Transcriptase Polymerase Chain Reaction, Integrin beta4, Epithelium, Corneal, Membrane Proteins, Sodium Dodecyl Sulfate, Anatomy, Phosphoproteins, Sensory Systems, Epithelium, Ophthalmology, medicine.anatomical_structure, Biophysics, Microscopy, Electron, Scanning, Zonula Occludens-1 Protein, Collagen
Abstract

Corneal tissue engineering has improved dramatically over recent years. It is now possible to apply these technological advancements to the development of superior in vitro ocular surface models to reduce animal testing. We aim to show the effect different substrates can have on the viability of expanded corneal epithelial cells and that those which more accurately mimic the stromal surface provide the most protection against toxic assault. Compressed collagen gel as a substrate for the expansion of a human epithelial cell line was compared against two well-known substrates for modelling the ocular surface (polycarbonate membrane and conventional collagen gel). Cells were expanded over 10 days at which point cell stratification, cell number and expression of junctional proteins were assessed by electron microscopy, immunohistochemistry and RT-PCR. The effect of increasing concentrations of sodium lauryl sulphate on epithelial cell viability was quantified by MTT assay. Results showed improvement in terms of stratification, cell number and tight junction expression in human epithelial cells expanded upon either the polycarbonate membrane or compressed collagen gel when compared to a the use of a conventional collagen gel. However, cell viability was significantly higher in cells expanded upon the compressed collagen gel. We conclude that the more naturalistic composition and mechanical properties of compressed collagen gels produces a more robust corneal model.

Published
2012

22. Differential coupling of self-renewal signaling pathways in murine induced pluripotent stem cells

Author

Heather K. Bone, Melanie J. Welham, Luca Orlando, Claudia Giachino, Yolanda Sanchez-Ripoll, and James W Foster

Subjects
Time Factors, Somatic cell, MAP Kinase Signaling System, Cellular differentiation, Induced Pluripotent Stem Cells, Cell Culture Techniques, lcsh:Medicine, Biology, Leukemia Inhibitory Factor, 03 medical and health sciences, Glycogen Synthase Kinase 3, Mice, Phosphatidylinositol 3-Kinases, 0302 clinical medicine, Model Organisms, Molecular Cell Biology, Animals, Signaling in Cellular Processes, Induced pluripotent stem cell, lcsh:Science, Cell Shape, PI3K/AKT/mTOR pathway, Cells, Cultured, 030304 developmental biology, Cell Proliferation, Genetics, 0303 health sciences, Multidisciplinary, Stem Cells, lcsh:R, Animal Models, Cellular Reprogramming, Embryonic stem cell, Cell biology, Culture Media, Enzyme Activation, 030220 oncology & carcinogenesis, lcsh:Q, Signal transduction, Cellular Types, Leukemia inhibitory factor, Reprogramming, Signal Transduction, Research Article, Developmental Biology
Abstract

The ability to reprogram somatic cells to induced pluripotent stem cells (iPSCs), exhibiting properties similar to those of embryonic stem cells (ESCs), has attracted much attention, with many studies focused on improving efficiency of derivation and unraveling the mechanisms of reprogramming. Despite this widespread interest, our knowledge of the molecular signaling pathways that are active in iPSCs and that play a role in controlling their fate have not been studied in detail. To address this shortfall, we have characterized the influence of different signals on the behavior of a model mouse iPSC line. We demonstrate significant responses of this iPSC line to the presence of serum, which leads to profoundly enhanced proliferation and, depending on the medium used, a reduction in the capacity of the iPSCs to self-renew. Surprisingly, this iPSC line was less sensitive to withdrawal of LIF compared to ESCs, exemplified by maintenance of expression of a Nanog-GFP reporter and enhanced self-renewal in the absence of LIF. While inhibition of phosphoinositide-3 kinase (PI3K) signaling decreased iPSC self-renewal, inhibition of Gsk-3 promoted it, even in the absence of LIF. High passages of this iPSC line displayed altered characteristics, including genetic instability and a reduced ability to self-renew. However, this second feature could be restored upon inhibition of Gsk-3. Collectively, our data suggest modulation of Gsk-3 activity plays a key role in the control of iPSC fate. We propose that more careful consideration should be given to characterization of the molecular pathways that control the fate of different iPSC lines, since perturbations from those observed in naive pluripotent ESCs could render iPSCs and their derivatives susceptible to aberrant and potentially undesirable behaviors.

Published
2012

23. RG 9200-L11-001 Vietnam Mailbag Records

Author

James W. Foster and James W. Foster

Abstract

Bio, service info., weighing post-war plans for education and jobs, soliciting donations for an orphanage; Envelope/Letter

Published
2013

24. Kin selection and gorilla reproduction

Author

James W. Foster

Subjects
Reproductive success, Ecology, media_common.quotation_subject, Receptivity, Gorilla, Kin selection, Biology, Breed, biology.animal, Captive breeding, Animal Science and Zoology, Reproduction, Paternal care, Ecology, Evolution, Behavior and Systematics, Demography, media_common
Abstract

Surveys on captive gorillas indicate that males at the blackback (subadult) age are capable of reproducing, and often do. Such information further suggests that male reproductive success decreases dramatically after reaching adulthood at approximately 13 years of age. Field data support the present hypothesis that this early breeding behavior is not idiosyncratic, but a reproductive strategy based on kin selection. The dominant male permits subadult and subordinate males to remain in the troop, breed with receptive females and assist in infant defens. Infanticide is practiced by adult males during aggressive intertroop encounters to hasten the female's return to receptivity, and thereby facilitate her transfer to their troop. The proposed hypothesis and a review of current field data are used to develop criteria for a captive breeding plan.

Published
1982
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25. Testicular biopsy in the study of gorilla infertility

Author

James W. Foster and Mavis J. Rowley

Subjects
Infertility, Testicular biopsy, media_common.quotation_subject, Physiology, Gorilla, Fertility, Human Males, Disease, Biology, Hyperplasia, medicine.disease, biology.animal, Interstitial tissue, medicine, Animal Science and Zoology, Ecology, Evolution, Behavior and Systematics, media_common
Abstract

Testicular biopsy has long been accepted as a tool for evaluating fertility of human males. This study examined the use of testicular biopsy for evaluating fertility of gorillas. Biopsies were collected from six captive adult gorillas. Hyperplasia of interstitial tissue was noted in three subjects, but other evidence suggests that this may be fairly characteristic of gorillas, even in natural settings. The most notable finding was that spermatogenesis was interrupted in the spermatid stage in each examined. This condition is present in about 1/3 of human infertility cases. Potential causes include the following: chemical agents (lead, insecticides, other airborne toxins) and physical agents (especially those resulting in localized temperature elevation). Failure to provide the basis for even minimum environmental contexts for behavioral development, disease and nutritional deficiency are other potential causes of gorilla infertility.

Published
1982
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26. Potomac River Maps of 1737 by Robert Brooke and Others

Author

James W. Foster

Subjects
Cultural Studies, History, Geodetic survey, business.industry, Lettering, Rappahannock, Plan (archaeology), Surveyor, people.ethnicity, people, business, Archaeology
Abstract

Robert Brooke's manuscript map, A Plan of Potomack River, from the Mouth of Sherrendo, down to Chpapcwamsick, Surveyed in the year 1737, mentioned in the Magazine for April last, where the circumstances surrounding the survey of the Potomac in connection with the effort to determine the bounds of Lord Fairfax's Northern Neck grant were described, is but one of a number of maps that were prepared in the course of the extended investigation at this date. In addition to the joint survey of the River from what is now Harper's Ferry to the head waters (the resulting map of which has been reproduced in these pages) the Crown commissioners ordered the surveyor of each county bounded either by the Potomac or Rappahannock rivers to prepare a map of the waters adjacent to his county.1 The result was a series of minor maps which in turn formed the foundation for the two general maps, one by John Warner and the other by William Mayo, that were sent to England and laid before the Lords Commissioners of Trade. It appears that but two of these county maps survive, though a third, that of Stafford county by John Savage, is perpetuated by a tracing in the library of the Coast and Geodetic Survey at Washington. Of the original surviving maps, both in the Enoch Pratt Free Library, Baltimore, one is an untitled and unsigned plan of the Potomac borders of Westmoreland County, an account of which is here appended. The other is, of course, the excellent map of Brooke which, by reason of its careful execution, the names of settlers shown and the later import of the sites it includes (Washington and Mt. Vernon) merits fuller discussion. It should be noted at the outset that the map of identical title in the Coast and Geodetic Library, recorded by Philips and also by Swem in their lists of Virginia maps and reproduced in Fairfax Harrison's Landmarks of Old Prince William,2 is a comparatively late tracing of a portion of the map herewith reproduced. The northern limit of the tracing is at the Great Falls and all key numbers from 1 to 24 are omitted. Consequently that part of the present plan and key above this point-in the original a strip 17%2 by 11 inches-is here shown in print for the first time. Incidentally, the tracing fails exactly to follow the original lettering (e. g. "Ro. Brooke" was

Published
1938
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