High Throughput Assay Identifies Glafenine as a Corrector for the Folding Defect in Corneal Dystrophy–Causing Mutants of SLC4A11

Chiu, Anthony M.; Mandziuk, Jake; Loganathan, Sampath K.; Kumari, Aruna; Casey, Joseph R.

doi:10.1167/iovs.15-17802

Cited by 26 publications

(31 citation statements)

References 71 publications

(88 reference statements)

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“…pAMC1 encoding N-terminally HA-tagged human SLC4A11 in pcDNA3.1 20 or wild-type (WT) Luc-SLC4A11 with N-terminal luciferase tag 12 were used as template for mutagenesis experiments to create point mutants.…”

Section: Dna Constructsmentioning

confidence: 99%

“…SLC4A11 variants carried a double HA tag insertion in extracellular loop 3, following amino acid 564, and have been previously reported as normal in functional activity and cell surface localization. 20 One hour post transfection, cells were treated with 500 lL of drug to a final concentration as indicated in the Table in 0.2% DMSO (vol/ vol), or DMSO alone as control. Forty-eight hours later, cells were washed in PBS, fixed with 4% paraformaldehyde in PBS for 10 minutes, followed by a quenching step with 100 mM glycine in PBS for 5 minutes at 208C.…”

Section: Confocal Immunofluorescencementioning

confidence: 99%

“…cDNA for SLC4A11 variants encoded a shortened version of splicing variant 2 of human SLC4A11 (891 amino acid, NCBI reference: NG_017072.1) with an N-terminal HA tag, as previously described previously. 20 One hour post transfection, cells were treated with the final concentration of drug in 0.2% DMSO (Table), and control cells received DMSO to a final concentration of 0.2% DMSO (vol/vol). Forty-eight hours later, coverslips were mounted in a 35-mm diameter Attofluor Cell Chamber (Molecular Probes, Ottawa, ON, Canada) and washed with PBS.…”

Section: Assay Of Osmotically Driven Water Fluxmentioning

confidence: 99%

“…The tag was inserted into extracellular loop 3 of SLC4A11, following P564, and does not affect cell surface trafficking or water flux function of SLC4A11. 20 Representative CHED (E143K) and FECD (G709E) mutants were tested in this assay. Cells were treated with indicated ophthalmic NSAIDs in 0.2% DMSO (Table).…”

Section: Confocal Immunofluorescence Microscopy Of Slc4a11 Cell Surfamentioning

confidence: 99%

“…7,10,[14][15][16][17][18][19] Most SLC4A11 mutations lead to biosynthetic defects marked by accumulation in the ER, and protein degradation before reaching the plasma membrane. 12 A small-scale drug screen showed that Glafenine, a disused NSAID, was able to move some SLC4A11 mutants to the cell surface, 20 suggesting that other NSAIDs might also have therapeutic potential. We thus set out to screen NSAIDs available as eye drops for their ability to correct the cell-surfacing trafficking of SLC4A11 proteins, using a bioluminescence resonance energy transfer (BRET) assay that enabled rapid analysis of SLC4A11 cell surface abundance.…”

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confidence: 99%

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Ophthalmic Nonsteroidal Anti-Inflammatory Drugs as a Therapy for Corneal Dystrophies Caused by SLC4A11 Mutation

Kumari

Casey

2018

Invest. Ophthalmol. Vis. Sci.

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Citation: Alka K, Casey JR. Ophthalmic nonsteroidal anti-inflammatory drugs as a therapy for corneal dystrophies caused by SLC4A11 mutation. Invest Ophthalmol Vis Sci. 2018;59:4258-4267. https://doi.org/ 10.1167/iovs.18-24301 PURPOSE. SLC4A11 is a plasma membrane protein of corneal endothelial cells. Some mutations of the SLC4A11 gene result in SLC4A11 protein misfolding and failure to mature to the plasma membrane. This gives rise to some cases of Fuchs' endothelial corneal dystrophy (FECD) and congenital hereditary endothelial dystrophy (CHED). We screened ophthalmic nonsteroidal anti-inflammatory drugs (NSAIDs) for their ability to correct SLC4A11 folding defects.METHODS. Five ophthalmic NSAIDs were tested for their therapeutic potential in some genetic corneal dystrophy patients. HEK293 cells expressing CHED and FECD-causing SLC4A11 mutants were grown on 96-well dishes in the absence or presence of NSAIDs. Ability of NSAIDs to correct mutant SLC4A11 cell-surface trafficking was assessed with a bioluminescence resonance energy transfer (BRET) assay and by confocal microscopy. The ability of mutant SLC4A11-expressing cells to mediate water flux (SLC4A11 mediates water flux across the corneal endothelial cell basolateral membrane as part of the endothelial water pump) was measured upon treatment with ophthalmic NSAIDs.RESULTS. BRET-assays revealed significant rescue of SLC4A11 mutants to the cell surface by 4 of 5 NSAIDs tested. The NSAIDs, diclofenac and nepafenac, were effective in moving endoplasmic reticulum-retained missense mutant SLC4A11 to the cell surface, as measured by confocal immunofluorescence. Among intracellular-retained SLC4A11 mutants, 20 of 30 had significant restoration of cell surface abundance upon treatment with diclofenac. Diclofenac restored mutant SLC4A11 water flux activity to the level of wild-type SLC4A11 in some cases.CONCLUSIONS. These results encourage testing diclofenac eye drops as a treatment for corneal dystrophy in patients whose disease is caused by some SLC4A11 missense mutations.

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Section: Dna Constructsmentioning

confidence: 99%

Section: Confocal Immunofluorescencementioning

confidence: 99%

Section: Assay Of Osmotically Driven Water Fluxmentioning

confidence: 99%

Section: Confocal Immunofluorescence Microscopy Of Slc4a11 Cell Surfamentioning

confidence: 99%

mentioning

confidence: 99%

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Ophthalmic Nonsteroidal Anti-Inflammatory Drugs as a Therapy for Corneal Dystrophies Caused by SLC4A11 Mutation

Kumari

Casey

2018

Invest. Ophthalmol. Vis. Sci.

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SLC4A11 Three-Dimensional Homology Model Rationalizes Corneal Dystrophy-Causing Mutations

2016

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We studied the structural effects of point mutations of a membrane protein that cause genetic disease. SLC4A11 is a membrane transport protein (OH /H /NH /H O) of basolateral corneal endothelium, whose mutations cause some cases of congenital hereditary endothelial dystrophy and Fuchs endothelial corneal dystrophy. We created a three-dimensional homology model of SLC4A11 membrane domain, using Band 3 (SLC4A1) crystal structure as template. The homology model was assessed in silico and by analysis of mutants designed on the basis of the model. Catalytic pathway mutants p.Glu675Gln, p.His724Arg, and p.His724Ala impaired SLC4A11 transport. p.Ala720Leu, in a region of extended structure of the proposed translocation pore, failed to mature to the cell surface. p.Gly509Lys, located in an open region at the core domain/gate domain interface, had wild-type level of transport function. The molecular phenotype of 37 corneal dystrophy-causing point mutants was rationalized, based on their location in the homology model. Four map to the substrate translocation pathway, 25 to regions of close transmembrane helix packing, three to the dimeric interface, and five lie in extramembraneous loops. The model provides a view of the spectrum of effects of disease mutations on membrane protein structure and provides a tool to analyze pathogenicity of additional newly discovered SLC4A11 mutants.

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Molecular phenotype of SLC4A11 missense mutants: Setting the stage for personalized medicine in corneal dystrophies

Kumari

Casey

2018

Human Mutation

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SLC4A11 mutations cause cases of congenital hereditary endothelial dystrophy (CHED), Harboyan syndrome (HS), and Fuchs endothelial corneal dystrophy (FECD). Defective water reabsorption from corneal stroma by corneal endothelial cells (CECs) leads to these corneal dystrophies. SLC4A11, in the CEC basolateral membrane, facilitates transmembrane movement of H 2 O, NH 3 , and H + -equivalents. Some SLC4A11 disease mutants have impaired folding, leading to a failure to move to the cell surface, which in some cases can be corrected by the drug, glafenine. To identify SLC4A11 mutants that are targets for folding-correction therapy, we examined 54 SLC4A11 missense mutants. Cell-surface trafficking was assessed on immunoblots, by the level of mature, high molecular weight, cell surface-associated form, and using a bioluminescence resonance energy transfer assay. Low level of cell surface trafficking was found in four out of 18 (20%) of FECD mutants, 19/ out of 31 (61%) of CHED mutants, and three out of five (60%) of HS mutants.Amongst ER-retained mutants, 16 showed increased plasma membrane trafficking when grown at 30 • C, suggesting that their defect has potential for rescue. CHED-causing point mutations mostly resulted in folding defects, whereas the majority of FECD missense mutations did not affect trafficking, implying functional impairment. We identified mutations that make patients candidates for folding correction of their corneal dystrophy.

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High Throughput Assay Identifies Glafenine as a Corrector for the Folding Defect in Corneal Dystrophy–Causing Mutants of SLC4A11

Cited by 26 publications

References 71 publications

Ophthalmic Nonsteroidal Anti-Inflammatory Drugs as a Therapy for Corneal Dystrophies Caused by SLC4A11 Mutation

Ophthalmic Nonsteroidal Anti-Inflammatory Drugs as a Therapy for Corneal Dystrophies Caused by SLC4A11 Mutation

SLC4A11 Three-Dimensional Homology Model Rationalizes Corneal Dystrophy-Causing Mutations

Molecular phenotype of SLC4A11 missense mutants: Setting the stage for personalized medicine in corneal dystrophies

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