Abstract

BackgroundKeratoconus (KC) is associated with oxidative stress and hypoxia and as several times discussed, potentially with inflammatory components. Inflammation, hypoxia, and oxidative stress may result in metabolic dysfunction and are directly linked to each other. In the current study, we investigate the effect of hypoxia through NF-κB signaling pathways on iNOS, hypoxia-induced factors (HIF), ROS, and proliferation of normal and KC human corneal fibroblasts (HCFs), in vitro.MethodsPrimary human KC-HCFs and normal HCFs were isolated and cultured in DMEM/Ham’s F12 medium supplemented with 5% fetal calf serum. Hypoxic conditions were generated and quantitative PCR and Western blot analysis were performed to examine NF-κB, iNOS, HIF, and PHD2 expression in KC and normal HCFs. ROS level was analyzed using flow cytometry and proliferation by BrdU-ELISA.ResultsHypoxia increased NF-κB mRNA and protein expression in normal HCFs, but in KC-HCFs NF-κB mRNA and protein expression remained unchanged. Hypoxic conditions upregulated iNOS mRNA expression of normal HCFs, but iNOS mRNA expression of KC-HCFs and iNOS protein expression of both HCF types remained unchanged. Hypoxia downregulated HIF-1α and HIF-2α mRNA expression in normal and KC-HCFs. PHD2 mRNA expression is upregulated under hypoxia in KC-HCFs, but not in normal HCFs. PHD2 protein expression was upregulated by hypoxia in both HCF types. Total ROS concentration is downregulated in normal and KC-HCFs under hypoxic conditions. Proliferation rate of KC-HCFs was upregulated through hypoxia, but did not change in normal HCFs.ConclusionsHypoxia increases NF-κB and iNOS mRNA expression in normal HCFs, but there does not seem to be enough capacity in KC-HCFs to increase NF-κB and iNOS mRNA expression under hypoxia, maybe due to the preexisting oxidative stress. HIF and PHD2 do not show altered iNOS regulation under hypoxic conditions in KC-HCFs, and therefore do not seem to play a role in keratoconus pathogenesis. An increased proliferation of cells may refer to compensatory mechanisms under hypoxia in KC. Understanding the mechanism of the altered regulation of NF-κB and iNOS in KC-HCFs will provide better insight into the potential inflammatory component of the KC pathogenesis.

Highlights

  • Keratoconus (KC) is associated with oxidative stress and hypoxia and as several times discussed, potentially with inflammatory components

  • We investigated the regulation of nuclear factor kappa B (NF-κB), inducible nitric oxide synthase (iNOS), hypoxia-induced factors (HIF)-1α, HIF-2α, and PHD expression; reactive oxidative species (ROS), and proliferation under hypoxic conditions in keratoconus corneal fibroblasts compared with normal control cells, in vitro

  • NF-κB mRNA is displayed after 4 h and iNOS, HIF-1α, HIF-2α, and hypoxia-inducible factor prolylhydroxylase 2 (PHD2) mRNA after 48 h of hypoxic conditions

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Summary

Introduction

Keratoconus (KC) is associated with oxidative stress and hypoxia and as several times discussed, potentially with inflammatory components. Proliferation rate of KC-HCFs was upregulated through hypoxia, but did not change in normal HCFs. Conclusions Hypoxia increases NF-κB and iNOS mRNA expression in normal HCFs, but there does not seem to be enough capacity in KC-HCFs to increase NF-κB and iNOS mRNA expression under hypoxia, maybe due to the preexisting oxidative stress. HIF and PHD2 do not show altered iNOS regulation under hypoxic conditions in KC-HCFs, and do not seem to play a role in keratoconus pathogenesis. Keratoconus has been characterized as a non-inflammatory corneal disease, but several studies suggest an inflammatory component in its development. Hypoxia increases NF-κB and iNOS mRNA expression in normal human corneal fibroblasts (HCFs), but there does not seem to be enough capacity in keratoconus human corneal fibroblasts (KC-HCFs) to increase NF-κB and iNOS mRNA expression under hypoxia, maybe due to the preexisting oxidative stress

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