Extracellular Matrix and Integrin Expression Profiles in Fuchs Endothelial Corneal Dystrophy Cells and Tissue Model

Goyer, Benjamin; Thériault, Marius; Gendron, Sébastien P.; Brunette, Isabelle; Rochette, Patrick J.; Proulx, Stéphanie

doi:10.1089/ten.tea.2017.0128

Cited by 32 publications

(31 citation statements)

References 48 publications

(48 reference statements)

Supporting

Mentioning

Contrasting

Order By: Relevance

“…The goal of these experiments was to ascertain whether CECs from normal human corneas can be stimulated to proliferate in organ culture where the low basal proliferation may better reflect the in vivo situation 34 compared with dissociated culture systems that produce high levels of proliferation of normal and dystrophic/FECD CECs. 7,8,[44][45][46] In this human corneal organ culture model, unstimulated CECs in the mid zone had very few cells incorporating EdU, indicating that this model is more reflective of the in vivo situation where the number of cells changes only slowly.…”

Section: Discussionmentioning

confidence: 84%

Proliferation of Human Corneal Endothelia in Organ Culture Stimulated by Wounding and the Engineered Human Fibroblast Growth Factor 1 Derivative TTHX1114

Eveleth

Pizzuto

Weant

et al. 2020

Journal of Ocular Pharmacology and Therapeutics

View full text Add to dashboard Cite

Purpose: Corneal endothelial dystrophies are characterized by endothelial cell loss and dysfunction. Recent evidence suggests that corneal endothelial cells (CECs) can regenerate although they do not do so under normal conditions. This work sought to test whether CECs can be stimulated to proliferate in organ culture by wounding and/or by treatment with the engineered human fibroblast growth factor 1 (FGF1) derivative TTHX1114. Methods: Human donor corneas obtained from eye banks were maintained in organ culture in the presence or absence of TTHX1114. Wounds in the corneas were created by quartering the corneas. The CEC monolayer was identified as a regular layer by Hoechst staining of the nuclear DNA with cell outlines delineated by immunohistochemical identification of ZO-1. Nuclei and nuclei incorporating 5-ethynyl-2¢-deoxyuridine (EdU) were counted using ImageJ. Results: CECs in normal corneas in undisturbed monolayers had low, but measurable, rates of proliferation. CECs at the edge of a wound had higher rates of proliferation, probably due to the release of contact inhibition. TTHX1114 increased proliferation at wound edges. After 7 days of culture, proliferating CECs formed contiguous groups of labeled cells that did not migrate away from one another. TTHX1114-treated cells, including the EdU labeled proliferating cells, retained normal morphology, including cell/cell junction ZO-1 staining. Conclusions: Proliferation of CECs in organ-cultured corneas is low, but can be stimulated by wounding or by the administration of TTHX1114 with the effects of each being additive. The CEC monolayer appears to have a population of progenitor cells that are susceptible to stimulation.

show abstract

Section: Discussionmentioning

confidence: 84%

Proliferation of Human Corneal Endothelia in Organ Culture Stimulated by Wounding and the Engineered Human Fibroblast Growth Factor 1 Derivative TTHX1114

Eveleth

Pizzuto

Weant

et al. 2020

Journal of Ocular Pharmacology and Therapeutics

View full text Add to dashboard Cite

show abstract

“…Revealed underexpression (log2FC = −2.07) of IL7R could have contributed to the immunological imbalance in IUGR-affected samples. Also, fibronectin type III domain containing 4 ( FNDC4 ) dampen macrophage activation [57,58], and its robust upregulation results in the reduction of inflammation [59]. Considering mentioned functions, the identified underexpression of FNDC4 (log2FC = −2.38), in the growth-restricted placentas, may be associated with progression of pro-inflammatory state contributing to the severity of the disease [57,59].…”

Section: Discussionmentioning

confidence: 99%

Placenta Transcriptome Profiling in Intrauterine Growth Restriction (IUGR)

Majewska

Lipka

Paukszto

et al. 2019

IJMS

View full text Add to dashboard Cite

Intrauterine growth restriction (IUGR) is a serious pathological complication associated with compromised fetal development during pregnancy. The aim of the study was to broaden knowledge about the transcriptomic complexity of the human placenta by identifying genes potentially involved in IUGR pathophysiology. RNA-Seq data were used to profile protein-coding genes, detect alternative splicing events (AS), single nucleotide variant (SNV) calling, and RNA editing sites prediction in IUGR-affected placental transcriptome. The applied methodology enabled detection of 37,501 transcriptionally active regions and the selection of 28 differentially-expressed genes (DEGs), among them 10 were upregulated and 18 downregulated in IUGR-affected placentas. Functional enrichment annotation indicated that most of the DEGs were implicated in the processes of inflammation and immune disorders related to IUGR and preeclampsia. Additionally, we revealed that some genes (S100A13, GPR126, CTRP1, and TFPI) involved in the alternation of splicing events were mainly implicated in angiogenic-related processes. Significant SNVs were overlapped with 6533 transcripts and assigned to 2386 coding sequence (CDS), 1528 introns, 345 5’ untranslated region (UTR), 1260 3’UTR, 918 non-coding RNA (ncRNA), and 10 intergenic regions. Within CDS regions, 543 missense substitutions with functional effects were recognized. Two known mutations (rs4575, synonymous; rs3817, on the downstream region) were detected within the range of AS and DEG candidates: PA28β and PINLYP, respectively. Novel genes that are dysregulated in IUGR were detected in the current research. Investigating genes underlying the IUGR is crucial for identification of mechanisms regulating placental development during a complicated pregnancy.

show abstract

“…Moreover, the majority of cells in culture were shown to downregulate various proteins involved in β-catenin activation. Of those proteins, Endoglin 43 , ITGB5 78 , and SPARC 79 were previously found to be expressed in CEnC (Supplementary Table S2 ). β-catenin is indeed generally fast degraded once in the cytoplasm 75 , and the condition captured by the proteomic analysis showed how β-catenin may have been already digested by the proteasome or moving back to the cell membrane (Fig.…”

Section: Introductionmentioning

confidence: 99%

A fine-tuned β-catenin regulation during proliferation of corneal endothelial cells revealed using proteomics analysis

Maurizi

Schiroli

Zini

et al. 2020

Sci Rep

View full text Add to dashboard Cite

Corneal endothelial (CE) dysfunction is the main indication for corneal transplantation, an invasive procedure with several limitations. Developing novel strategies to reactivate CE regenerative capacity is, therefore, of fundamental importance. This goal has proved to be challenging as corneal endothelial cells (CEnC) are blocked in the G0/G1 phase of the cell cycle in vivo and, albeit retaining proliferative capacity in vitro, this is further hindered by endothelial-to-mesenchymal transition. Herein we investigated the mechanisms regulating CEnC proliferation in vitro. Comparing the proteome of non-proliferating (in vivo-G0/G1) and proliferating (in vitro-G2/M) rabbit CEnC (rCEnC), 77 proteins, out of 3,328 identified, were differentially expressed in the two groups (p < 0.005). Literature and Gene Ontology analysis revealed β-catenin and transforming growth factor (TGF-β) pathways to be correlated with the identified proteins. Treatment of rCEnC with a β-catenin activator and inhibitor showed that β-catenin activation was necessary during rCEnC proliferation, but not sufficient for its induction. Furthermore, both pro-proliferative activity of basic fibroblast growth factor and anti-proliferative effects of TGF-β were regulated through β-catenin. Overall, these results provide novel insights into the molecular basis underlying the proliferation process that CEnC reactivate in vitro, consolidating the role of β-catenin and TGF-β. The corneal endothelium (CE) is a monolayer of cells localised in the innermost segment of the cornea, regulating solutes transport from and to the aqueous humor (pump-leak hypothesis) 1. Corneal endothelial cells (CEnC) are generally considered non-dividing in vivo 2 and arrested in the G0/G1 phase of the cell cycle 3,4. The presence of anti-proliferative factors in the aqueous humor, the stress-induced premature senescence, and the contact inhibition between cells are the main events triggering the expression of cell cycle regulators that induce CEnC mitotic block 2. For this reason, as CEnC density decreases by 0.6% each year 5,6 , cell loss is compensated through migration and cell enlargement 2,7. When, as a consequence of pathologies or surgical treatments, endothelial cell density falls below 500 cells/mm 2 , cell enlargement is no longer able to compensate for the passive leaking 7. In this case, the impaired CE results in corneal swelling and, if untreated, in the subsequent severe loss of corneal transparency, ultimately leading to blindness. CEnC dysfunction is the underlying cause of about 40% of all corneal transplants performed worldwide 7. Corneal grafts, despite decisive advancements in the last decades, are still complex and invasive procedures, with some severe limitations, including immune graft rejection, graft failure, and a general scarcity of donor corneas 7. Alternative clinical procedures have been recently proposed in order to increase the number of patients that can be treated and to improve their quality of life. Currently, descemetorhexis is the only therap...

show abstract

Extracellular Matrix and Integrin Expression Profiles in Fuchs Endothelial Corneal Dystrophy Cells and Tissue Model

Cited by 32 publications

References 48 publications

Proliferation of Human Corneal Endothelia in Organ Culture Stimulated by Wounding and the Engineered Human Fibroblast Growth Factor 1 Derivative TTHX1114

Proliferation of Human Corneal Endothelia in Organ Culture Stimulated by Wounding and the Engineered Human Fibroblast Growth Factor 1 Derivative TTHX1114

Placenta Transcriptome Profiling in Intrauterine Growth Restriction (IUGR)

A fine-tuned β-catenin regulation during proliferation of corneal endothelial cells revealed using proteomics analysis

Contact Info

Product

Resources

About