Galectin‐1 promotes choroidal neovascularization and subretinal fibrosis mediated<i>via</i>epithelialmesenchymal transition

Wu, Di; Kanda, Atsuhiro; Liu, Ye; Kase, Satoru; Noda, Kousuke; Ishida, Susumu

doi:10.1096/fj.201801227r

Cited by 53 publications

(56 citation statements)

References 50 publications

(82 reference statements)

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“…Total RNA isolation was performed from cells using SuperPrep II Cell Lysis & RT Kit for qPCR (TOYOBO) and from tissue samples using TRI reagent (Molecular research centre), as previously described . The following primers were used: human LGALS1 (forward 5′‐CGC TAA GAG CTT CGT GCT GAA C‐3′, reverse 5′‐CAC ACC TCT GCA ACA CTT CCA G‐3′), human HIF1A (HIF‐1α; forward 5′‐TGC TCA TCA GTT GCC ACT TC‐3′, reverse 5′‐TCC TCA CAC GCA AAT AGC TG‐3′), human VEGFA (forward 5′‐CAG ATT ATG CGG ATC AAA CCT CA‐3′; reverse 5′‐CAA GGC CCA CAG GGA TTT TC‐3′), human TSC22D3 (forward 5′‐ATC TGC AAC CGC AAC ATC GAC C‐3′, reverse 5′‐GCA TAC ATC AGA TGA TTC TTC ACC‐3′), human DUSP1 (forward 5′‐CTG CCT TGA TCA ACG TCT CA‐3′, reverse 5′‐CTG TGC CTT GTG GTT GTC CT‐3′), human ACTB (β‐actin; forward 5′‐CTG GAA CGG TGA AGG TGA CA‐3′, reverse 5′‐ AAG GGA CTT CCT GTA ACA ATG CA‐3′), mouse Lgals1 (forward 5′‐GTC TCA GGA ATC TCT TCG CTT C‐3′, reverse 5′‐TCC CCG AAC TTT GAG ACA TTC‐3′, probe 5′‐TTC AAT CAT GGC CTG TGG TCT GGT‐3′), mouse Tsc22d3 (forward 5′‐TCA ATG AGG GCA TCT GCA ACC G‐3′, reverse 5′‐CAT CAG GTG GTT CTT CAC GAG G‐3′), and mouse Actb (forward 5′‐CAT CCG TAA AGA CCT CTA TGC CAA C‐3′, reverse 5′‐ATG GAG CCA CCG ATC CAC A‐3′).…”

Section: Methodsmentioning

confidence: 99%

“…Immunofluorescence analyses were performed as described previously . Serial sections were incubated with the following primary antibodies: goat anti‐galectin‐1 (1:100, R&D systems), rabbit anti‐glial fibrillary acidic protein (1:200, GFAP; Leica), mouse anti‐HIF‐1α (1:100, Novus Biologicals), rabbit anti‐HIF‐1α (1:100, Cell signaling technology) and mouse anti‐TSC22D3 (1:50, Santa Cruz Biotechnology) antibodies.…”

Section: Methodsmentioning

confidence: 99%

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Glucocorticoid‐transactivated TSC22D3 attenuates hypoxia‐ and diabetes‐induced Müller glial galectin‐1 expression via HIF‐1α destabilization

Kanda

Hirose

Noda

et al. 2020

J Cellular Molecular Medi

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Galectin-1/LGALS1, a newly recognized angiogenic factor, contributes to the pathogenesis of diabetic retinopathy (DR). Recently, we demonstrated that glucocorticoids suppressed an interleukin-1β-driven inflammatory pathway for galectin-1 expression in vitro and in vivo. Here, we show glucocorticoid-mediated inhibitory mechanism against hypoxia-inducible factor (HIF)-1α-involved galectin-1 expression in human Müller glial cells and the retina of diabetic mice. Hypoxia-induced increases in galectin-1/LGALS1 expression and promoter activity were attenuated by dexamethasone and triamcinolone acetonide in vitro. Glucocorticoid application to hypoxia-stimulated cells decreased HIF-1α protein, but not mRNA, together with its DNA-binding activity, while transactivating TSC22 domain family member (TSC22D)3 mRNA and protein expression. Co-immunoprecipitation revealed that glucocorticoid-transactivated TSC22D3 interacted with HIF-1α, leading to degradation of hypoxia-stabilized HIF-1α via the ubiquitin-proteasome pathway. Silencing TSC22D3 reversed glucocorticoid-mediated ubiquitination of HIF-1α and subsequent down-regulation of HIF-1α and galectin-1/LGALS1 levels. Glucocorticoid treatment to mice significantly alleviated diabetes-induced retinal HIF-1α and galectin-1/Lgals1 levels, while increasing TSC22D3 expression. Fibrovascular tissues from patients with proliferative DR demonstrated co-localization of galectin-1 and HIF-1α in glial cells partially positive for TSC22D3. These results indicate that glucocorticoid-transactivated TSC22D3 attenuates hypoxia-and diabetes-induced retinal glial galectin-1/LGALS1 expression via HIF-1α destabilization, highlighting therapeutic implications for DR in the era of anti-vascular endothelial growth factor treatment. K E Y W O R D S diabetic retinopathy, galectin-1, glucocorticoid, HIF-1α, hypoxia, Müller glia, transactivation, TSC22D3

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Glucocorticoid‐transactivated TSC22D3 attenuates hypoxia‐ and diabetes‐induced Müller glial galectin‐1 expression via HIF‐1α destabilization

Kanda

Hirose

Noda

et al. 2020

J Cellular Molecular Medi

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“…Immunofluorescence analyses were performed as described previously . Serial sections were incubated with the following primary antibodies: mouse anti‐galectin‐1 (1:50, Santa Cruz Biotechnology), mouse and rabbit anti‐glial fibrillary acidic protein (GFAP) (1:200, Leica), rabbit anti‐phosphorylated ATF2 (1:100), rabbit anti‐phosphorylated c‐Fos (1:100), and rabbit anti‐phosphorylated c‐Jun (1:100, Cell Signaling Technology), rabbit anti‐DUSP1 (1:100, Millipore) and rabbit anti‐GR (1:100, Thermo Fisher Scientific) antibodies.…”

Section: Methodsmentioning

confidence: 99%

“…Immunofluorescence analyses were performed as described previously. 4,5,15 Serial sections were incubated with the following primary antibodies: mouse anti-galectin-1 (1:50, Santa Cruz Biotechnology), mouse and rabbit anti-glial fibrillary acidic protein (GFAP) (1:200, Leica), rabbit anti-phosphorylated ATF2 (1:100), rabbit anti-phospho-…”

Section: Immunofluorescence Microscopymentioning

confidence: 99%

“…Total RNA isolation and reverse transcription were performed from cells using SuperPrep Cell Lysis & RT Kit for qPCR (TOYOBO) and from tissues using PureLink RNA Mini Kit (Thermo Fisher Scientifc) and GoScrip Reverse Transcriptase (Promega), as previously described. 4,5,15 All primers are listed in Table S1. Real-time qPCR was performed using the GoTaq qPCR Master Mix (Promega) and…”

Section: Real-time Quantitative Pcr (Qpcr)mentioning

confidence: 99%

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Glucocorticoid receptor inhibits Müller glial galectin‐1 expression via DUSP1‐dependent and ‐independent deactivation of AP‐1 signalling

Hirose

Kanda

Noda

et al. 2019

J Cellular Molecular Medi

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Galectin‐1/LGALS1 is a hypoxia‐induced angiogenic factor associated with diabetic retinopathy (DR). Recently, we elucidated a hypoxia‐independent pathway to produce galectin‐1 in Müller glial cells stimulated by interleukin (IL)‐1β. Here we revealed glucocorticoid receptor (GR)‐mediated inhibitory mechanisms for Müller glial galectin‐1/LGALS1 expression. Activator protein (AP)‐1 site in the LGALS1 enhancer region, to which activating transcription factor2, c‐Fos and c‐Jun bind, was shown to be essential for IL‐1β‐induced galectin‐1/LGALS1 expression in Müller cells. Ligand (dexamethasone or triamcinolone acetonide)‐activated GR induced dual specificity phosphatase (DUSP)1 expression via the glucocorticoid response element and attenuated IL‐1β‐induced galectin‐1/LGALS1 expression by reducing phosphorylation of these AP‐1 subunits following AKT and extracellular signal‐regulated kinase (ERK)1/2 deactivation. Moreover, activated GR also caused DUSP1‐independent down‐regulation of IL‐1β‐induced LGALS1 expression via its binding to AP‐1. Administration of glucocorticoids to mice attenuated diabetes‐induced retinal galectin‐1/Lgals1 expression together with AKT/AP‐1 and ERK/AP‐1 pathways. Supporting these in vitro and in vivo findings, immunofluorescence analyses showed co‐localization of galectin‐1 with GR and phosphorylated AP‐1 in DUSP1‐positive glial cells in fibrovascular tissues from patients with DR. Our present data demonstrated the inhibitory effects of glucocorticoids on glial galectin‐1 expression via DUSP1‐dependent and ‐independent deactivation of AP‐1 signalling (transactivation and transrepression), highlighting therapeutic implications for DR.

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Bioactive decellularized adipose matrix prepared using a rapid, nonchemical/enzymatic method for adipogenesis

Yang,

Tang,

Dang

et al. 2023

Biotech & Bioengineering

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Recent developments in the field of regenerative surgeries and medical applications have led to a renewed interest in adipose tissue‐enriched mesenchymal stem cell scaffolds. Various advantages declared for the decellularized adipose matrix (DAM) have caused its extensive use in the transfer of stem cells or growth factors for soft tissue regeneration induction. Meanwhile, the long‐term application of detergents toward DAM regeneration has been assumed as a risky obstacle in this era. Herein, a rapid, mechanical protocol was developed to prepare DAM (M‐DAM) without chemicals/enzymes and was comprehensively compared with the ordinary DAM (traditional chemical method). Accordingly, this method could effectively hinder oils and cells, sustain the structural and biological elements, and contain a superior level of collagen content. In addition, more protein numbers, as well as higher basement membrane elements, glycoproteins, and extracellular matrix‐related proteins were detected in the regenerated M‐DAM. Also, superior adipogenesis and angiogenesis proteins were distinguished. The noncytotoxicity of the M‐DAM was also approved, and a natural ecological niche was observed for the proliferation and differentiation of stem cells, confirming its great potential for vascularization and adipogenesis in vivo. The suggested technique could effectively prepare the modified DAM in variant constructions of tablets, powders, emulsions, hydrogels, and different three‐dimensional‐printed structures. Hence, this rapid, mechanical process can produce bioactive DAM, which has the potential to be widely used in various research fields of regenerative medicine.

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Galectin‐1 promotes choroidal neovascularization and subretinal fibrosis mediatedviaepithelialmesenchymal transition

Cited by 53 publications

References 50 publications

Glucocorticoid‐transactivated TSC22D3 attenuates hypoxia‐ and diabetes‐induced Müller glial galectin‐1 expression via HIF‐1α destabilization

Glucocorticoid‐transactivated TSC22D3 attenuates hypoxia‐ and diabetes‐induced Müller glial galectin‐1 expression via HIF‐1α destabilization

Glucocorticoid receptor inhibits Müller glial galectin‐1 expression via DUSP1‐dependent and ‐independent deactivation of AP‐1 signalling

Bioactive decellularized adipose matrix prepared using a rapid, nonchemical/enzymatic method for adipogenesis

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