Explant cultures of hTM were obtained from the eye bank of the Ludwig-Maximilians-University, Munich, Germany. Methods of securing human tissue were humane, included proper consent and approval, complied with the Declaration of Helsinki and were approved by the ethic committee of the Department of Medicine of the Friedrich-Alexander-University Erlangen-Nuremberg. The consent statement was written (EK_No. 4346-CH). Monolayer cultures were established from eyes obtained 4 to 8 hours post mortem of five human donors (40–50 years) without any history of eye diseases. Cells were propagated in complete F10 (Ham's F10 medium supplemented with 10% fetal bovine serum [FBS], 10 U/ml penicillin, 10 µg/ml streptomycin, and 0.25 µg/ml Fungizone Mix; all from PAN™ Biotech GmbH, Aidenbach, Germany) under standard cell culture conditions in 6-well (RNA/ protein extraction) or 24 well (CCK-8/BrdU/IF-labeling) cell culture plates (Techno Plastic Products AG, Trasadingen, Switzerland).

To test the effects of ω-3 or ω-6 fatty acids, confluent hTM of passages 3 to 5 were pre-incubated in low F10 (Ham's F10/1% FBS) for 24 hours. Then the medium was substituted by low F-10 supplemented to nontoxic 50 µM ω-3 ^[30] or 16 µM ω-6 ^[31] fatty acids (both from Sigma-Aldrich, Taufkirchen, Germany). After 24 hours, medium was replaced by fresh ω-3 or ω-6 containing medium for an additional 24 hours incubation. After 48 hours in total, oxidative stress was induced by exposure to nontoxic 300 µM hydrogen peroxide ^[6] (H₂O₂, Sigma-Aldrich) for 1 hour. Afterwards the cells were washed with PBS and further cultured with the distinct media for 1 hour. In control cultures, the medium was changed at the same time points, but no H₂O₂ was added.

Mitochondrial metabolism was quantified at 0, 24 and 48 hours after indicated treatments with a Cell Counting Kit-8 (CCK-8, Dojindo Molecular Technologies, Rockville, MD) according to the manufactures' instructions. 100 µl aliquots of the medium were transferred to 96 well plates and absorbance at 450 nm was measured with a spectrophotometer (Multiscan® Spectrum; Thermo Electron Corporation, Karlsruhe, Germany). Measurements were done as triplicates of hTM from 5 different donors in 3 independent experiments. Values represent mean averages ± SD (n = 45).

hTM proliferation was quantified with a Bromodeoxyuridine (BrdU) detection kit (Cell Proliferation ELISA, BrdU [colorimetric]; Roche Diagnostics, Mannheim, Germany). Therefore, 1 µM BrdU labeling solution was added to the cells during treatment for 48 hours. Detection was done according to the manufactures' instructions. Absorbance was measured at 370 nm wavelength with a spectrophotometer (Multiscan® Spectrum; Thermo). The tests were done as triplicates of hTM from 5 different donors in 3 independent experiments. Values represent mean averages ± SD (n = 45).

Total RNA was isolated with a RNA isolation kit (RNeasy Fibrous Tissue Mini Kit; Qiagen N.V., Hilden, Germany) according to the manufactures' instructions. Structural integrity of the RNA samples was confirmed by electrophoresis in 1% Tris-acetate-EDTA (TAE)-agarose gels ^[32]. Yield and purity were determined photometrically. 200 ng of mRNA were transcribed to cDNA by reverse transcription using a reverse transcription-PCR kit (Access RT-PCR Introductory System; Promega Corporation, Madison, USA). Real-time PCR quantification was performed in 40 cycles in a thermocycler (LightCycler System; Roche Diagnostics, Penzberg, Germany). The selected primers for FN, PAI-1, CTGF, Hsp27, Hsp90, IL-1α, IL-6, IL-8, NFκB and glycerinaldehyd-3-phosphat-dehydrogenase (GAPDH) were purchased from Metabion (Metabion International AG, Martinsried, Germany); primer sequences are summarized in Table 1. Corresponding probes were selected with the ProbeFinder v2.04 software (Roche). The standard curve was obtained from probes of three different untreated hTM cultures. As internal control GAPDH was processed simultaneously in each assay and levels of FN-1, PAI-1, CTGF, Hsp27, Hsp90, IL-1α, IL-6, IL-8 and NFκB mRNAs were determined as relative ratios (RR) by division by GAPDH. Ratios in non-supplemented cells without H₂O₂ treatment were set to one and expression levels of treated cells are given as fold of that. All experiments were performed in triplicates with TM cultures from three different donors. Values represent mean averages ± SD (n = 9).

Media of hTM were collected separately and concentrated six fold by centrifugation (Vivaspin20; Sartorius Stedim GmbH, Goettingen, Germany). Cells were directly lysed in RIPA buffer (150 mM NaCl, 1% NP-40, 0.5% DOC, 0.1% SDS, 50 mM Tris [pH 8.0], 4 mM DTT, 0.5 mM NaVanadate, 2 mM NaF, 2 mM phenylmethylsulfonyl fluoride) containing protease inhibitors (complete protease inhibitor cocktail; Roche). Protein contents of concentrated media and cell lysates were determined by the bicinchoninic acid (BCA) protein assay (Pierce, Rockford, USA). Samples were supplemented with one fourth SDS-loading buffer (Roti-load-1; Roth, Karlsruhe, Germany) and aliquots containing equal proteins were separated by SDS-polyacrylamide gel electrophoresis (PAGE). Proteins were transferred onto a nitrocellulose membrane (Protran Ba-183; Whatman, Dassel, Germany) by semi-dry or tank blotting. Further procedure was done as previously described ^[33] and primary antibodies (Table 2) were added over night at 4°C. Corresponding secondary alkaline phosphatase (AP) -conjugated antibodies (Table 2) were incubated for 30 minutes at room temperature. After substrate incubation (CDP-star; Roche) the signals were visualized by exposure to light sensitive films (Hyperfilm ECL; GE Healthcare, Munich, Germany), which were digitized and densitometrically quantified with the Multi Gauge V3.1 software (Fujifilm, Duesseldorf, Germany). All experiments were performed in triplicates with hTM cultures from three different donors. Values represent mean averages ± SD (n = 9).

Medium contents for FN were analyzed by ELISA according to the manufacturer's instructions (QuantiMatrix Human Fibronectin ELISA KIT; Millipore, Schwalbach, Germany). Aliquots of 50 µl of six-fold concentrated cell media were set in. Absorbance at 450 nm was measured with a spectrophotometer (Multiscan® Spectrum; Thermo). Measurements were done as triplicates of media from hTM cultures of 3 different donors in 3 independent experiments. Values represent mean averages ± SD (n = 9).

Amounts of secreted Interleukins (IL) -6 and -8 were analyzed by ELISA according to the manufacturer's instructions (QuantiGlo Chemiluminescent ELISA; R&D Systems, Minneapolis, USA). Aliquots of 100 µl and 50 µl of six-fold concentrated cell media were used for IL-6 and IL-8 determination, respectively. Light emission was measured with a luminometer (Fluoroskan Ascent FL; Thermo). Measurements were done as triplicates of hTM cell media from 3 different donors in 3 independent experiments. Values represent mean averages ± SD (n = 9).

Nuclear content of NFκB was tested in nuclear extracts with a NoShift™ NFκB Transcription Factor Assay (Novagen/Merck, Darmstadt, Germany) according to the manufacturer's instructions. For nuclear extracts, cells were collected from plates with Trypsine/EDTA (PAN™), washed three times in Hank's buffered salt solution (HBBS; PAN™) and lysed in three times packed cell volumes of low-salt hypotonic cell lysis buffer (20 mM HEPES pH 7.5, 10 mM KCl, 5 mM MgCl2, 0.5 mM EDTA, 0.1% TritonX-100, 10% glycerol, protease inhibitor cocktail [Roche]) for 10 min on ice. Nuclei were pelleted by centrifugation for 10 sec at 4°C and cytosolic fractions (supernatants) were discarded. Nuclei were washed once in low-salt hypotonic cell lysis buffer, and extracted using high-salt hypotonic cell lysis buffer (low-salt supplemented to 500 mM NaCl) for 10 min on ice. Debris was sedimented by centrifugation for 30 min at 4°C and nuclear extracts were transferred to fresh vials. After BCA protein determination extracts were stored at −80°C until use. For assays, equal masses of proteins were set in. Quantification was done by measurement of the absorbance at 450 nm with a spectrophotometer (Multiscan® Spectrum; Thermo). Measurements were done as triplicates of nuclear extracts of hTM cell cultures from 3 different donors in 3 independent experiments. Values represent mean averages ± SD (n = 9).

hTM were grown for 48 hours on microscope chamber slides (Lab-Tek®II; Nunc, Rochester, USA). After depicted treatments, slides were fixed in 4% paraformaldehyde (PFA), blocked in PBS (1% BSA, 0.1% Triton X-100) and primary antibodies (Table 2) were added in PBS (2% BSA, 0.2% Triton X-100) overnight at 4°C. Fluorophor conjugated secondary antibodies (Table 2) in PBS were added for 30 minutes at room temperature. The F-actin cytoskeleton was labeled by fluorescein conjugated phalloidin (Molecular Probes™, Eugene, USA) for 15 minutes at room temperature. Nuclei were counterstained by 4′,6′-diamidino-2-phenylindole (DAPI; Molecular Probes™). Cells were mounted in fluorescent mounting medium (Dako, Glostrup, Denmark) and analyzed by Laser confocal microscopy (Carl Zeiss, Goettingen, Germany). All experiments were performed in triplicates with hTM cultures from three different donors (n = 9).

Statistical analysis was done by a Student's t-test with the GraphPad Prism5 software (*p≤0.05; **p≤0.01; ***p≤0.001).

Mitochondrial activity of primary hTM cultured under standard conditions (controls) increased to 130±11% over 48 hours (Fig. 1A). Cells supplemented with ω-3 showed a similar activity at the same time point (122±16%; p = 0.2211), whereas the mitochondrial activity of cells preincubated with ω-6 was significantly lower at 87±8% (***p≤0.001; Fig. 1A) compared to the controls.

Exposure to H₂O₂ significantly reduced mitochondrial activity of controls to 60±7% (***p≤0.001; Fig. 1B), corresponding to a 71±13% reduction (Fig. 1C). The mitochondrial activity of ω-6 preincubated, H₂O₂ stimulated hTM was 39±16% (***p≤0.001; Fig. 1B), corresponding to a 48±17% (Fig. 1C) reduction compared to the ω-6-only incubated hTM. hTM preincubated with ω-3 in contrast, showed no significant reduction due to H₂O₂ (114±21%; Fig. 1B; reduction 5±18% Fig. 1C). Compared to the controls H₂O₂ mediated reductions were significantly reduced in both, ω-6 (**p≤0.01) and ω-3 (***p≤0.001) preincubated hTM (Fig. 1C).

Controls had a mean BrdU incorporation rate of 168±34% after 48 hours normalized to t = 0 hours. Cells preincubated with ω-3 showed a similar increase of incorporation rate as the controls up to 184±17% at 48 hours (p = 0.2447). In contrast, ω-6 preincubated cells' incorporation rate remained rather constant over 48 hours reaching a final value of 96±16%, which was significantly lower than in the controls and the ω-3 supplemented cells (***p≤0.001; Fig. 2A).

H₂O₂ exposure reduced BrdU incorporation in controls by 97±42% to 72±15% (***p≤0.001; Fig. 2B). In cells preincubated with fatty acids the incorporation rates were not reduced by H₂O₂ and were in the same range as in the corresponding controls at 88±11% (ω-6) and 161±26% (ω-3; Fig. 2B). The corresponding reductions were 8±17% (ω-6) and 23±23% (ω-3) respectively, both being significantly lower than in the controls (***p≤0.001; Fig. 2C).

Hsp27 mRNA levels were significantly increased after preincubation with ω-6 by 1.5±0.3 fold (**p≤0.01) normalized to the controls (Fig. 3A). Preincubation with ω-3, in contrast, significantly decreased the mRNA level by 0.5±0.2 fold (***p≤0.001; Fig. 3A). On protein level, however, amounts of Hsp27 were equal in controls and fatty acid preincubated cells (ω-6: 0.8±2.2 fold; p = 0.1923; ω-3: 0.9±0.1 fold; p = 0.3503; Fig. 3B, C).

Hsp90 mRNA was increased by both fatty acids by 33±8 fold (ω-6; ***p≤0.001) and 17±6 fold (ω-3; ***p≤0.001; Fig. 3A), respectively. Hsp90 protein levels were also increased by both fatty acids by 1.4±0.2 fold (ω-6; *p≤0.05) and 1.6±0.1 fold (ω-3; ***p≤0.001; Fig. 3B, C).

ω-6 fatty acid significantly increased the fibronectin (FN) mRNA by 2.5±0.5 fold (***p≤0.001) compared to controls, while ω-3 supplementation did not have a significant effect (1.5±0.8 fold; p = 0.1158; Fig. 4A). Intracellular FN protein levels were not changed upon fatty acid supplementation (ω-6: 1.1±0.1 fold; p = 0.3073; ω-3: 0.8±0.1 fold; p = 0.0584; Fig. 4C, D), amounts of secreted FN in the medium were also not affected (ω-3: p = 0.8279; ω-6: p = 0.9382; Fig. 4G).

In the controls, H₂O₂ addition increased the FN mRNA by 3.7±0.7 fold (***p≤0.001; Fig. 4B), and the intracellular FN protein by 1.3±0.1 fold (***p≤0.001; Fig. 4C, D). In ω-6 pre-treated cells, H₂O₂ led to a further increase of FN mRNA to 5.2±2.5 fold (*p≤0.05), whereas the amount of intracellular FN protein did not increase (1.5±0.1 fold) compared to the corresponding controls (p = 0.2168; Fig. 4C, D). Pre-treatment with ω-3 prevented the H₂O₂ stimulation of FN mRNA (1.6±1.1 fold; p = 0.8420; Fig. 4B) and intracellular FN (0.6±0.1 fold; ***p≤0.001; Fig. 4C, D). In ELISA analysis H₂O₂ increased FN in the medium to 1.6±0.3 fold (*p≤0.05). Both fatty acids appeared to impede this stimulation, in case of ω-3 even to a statistically significant extent (*p≤0.05; ω-6: p = 0.0573; Fig. 4G).

Plasminogen activator inhibitor (PAI-)1 mRNA expression was significantly increased by 2.5±0.5 fold in ω-6 supplemented cells (*p≤0.05), whereas ω-3 reduced the expression level compared to the controls (0.8±0.1 fold; ***p≤0.001; Fig. 4A). On the protein level, in contrast, PAI-1 was significantly increased to 1.5±0.1 fold in ω-3 supplemented cells (***p≤0.001), while ω-6 did not affect PAI-1 protein levels (1.1±0.2 fold; p = 0.3462; Fig. 4C, E).

Exposure to H₂O₂ stimulated PAI-1 mRNA expression in the controls by 5.6±0.2 fold (***p≤0.001) and cellular PAI-1 protein levels were increased to 1.4±0.2 fold (**p≤0.01; Fig. 4C, E). In cells pre-treated with ω-6 fatty acid the PAI-1 mRNA was not further increased by H₂O₂ (3.1±1.1; p = 0.3824). The same applied for the PAI-1 protein levels, which remained constant after H₂O₂ stimulation (1.3±0.1 fold; p = 0.3276; Fig. 4C, E). In cells preincubated with ω-3 the PAI-1 mRNA expression even dropped to 0.05±0.02 fold after H₂O₂ addition (***p≤0.001; Fig. 4B), protein levels, however, were in the same range than in their corresponding controls (1.2±0.1 fold; p = 0.0598; Fig. 4C, E).

Connective tissue growth factor (CTGF) mRNA expression was significantly upregulated in cells supplemented with fatty acids compared to the controls (ω-6:14.4±5.7 fold; ***p≤0.001; ω-3: 26.6±1.7 fold; ***p≤0.001; Fig. 4A). The ω-6 mediated activation of CTGF was also observed on the protein level by a 1.4±0.05 fold increase (***p≤0.001). Protein levels in ω-3 treated cells were not increased (1.1±0.1 fold; p = 0.2721; Fig. 4C, F).

H₂O₂ addition induced expression of CTGF mRNA by 21.2±3.1 fold (***p≤0.001) in the controls. In ω-6 pre-treated cells, H₂O₂ further increased mRNA expression to 23.7±8.6 fold (*p≤0.05), which was not observed in ω-3 pre-treated cells (26.7±11.6; p = 0.4423; Fig. 4B). On the protein level, H₂O₂ resulted in a weak, but significant upregulation of CTGF in the controls (1.2±0.05 fold; **p≤0.01). In ω-6 pre-treated cells, H₂O₂ exposure led to a reduced protein level than in the corresponding controls (1.1±0.05 fold; **p≤0.01). In ω-3 pre-treated cells, H₂O₂ exposure had no effect on CTGF protein level (1.0±0.05 fold; p = 0.1670 Fig. 4C, F).

Expression of IL-1α mRNA was significantly stimulated by ω-6 (7.5±1.0 fold; ***p≤0.001), whereas ω-3 had no effect (1.6±0.9 fold; p = 0.3408; Fig. 5A). Exposition to H₂O₂ doubled IL-1α mRNA expression (2.6±0.5 fold; **p≤0.01; Fig. 5A). Neither ω-3, nor ω-6 could significantly inhibited this stimulation (ω-3: p = 0.0669; ω-6: p = 0.0596; Fig. 5A). Expression in H₂O₂/ω-6 double treated cells appeared lower than in ω-6 supplemented hTM, differences, however, did not reach the level of statistical significance (p = 0.0513; Fig. 5A).

IL-6 mRNA expression was not altered by both fatty acids (ω-3: p = 0.7306; ω-6: p = 0.2828; Fig. 5B). H₂O₂ stimulation increased IL-6 mRNA to 3.4±1.4 fold (*p≤0.05), which could not be impeded by both fatty acids (ω-3: p = 0.1720; ω-6: p = 0.8920; Fig. 5B). ELISA analysis of the medium revealed that ω-6 stimulated IL-6 secretion (*p≤0.05) which was not observed upon ω-3 supplementation (p = 0.0791; Fig. 5D). H₂O₂ lead to a 1.6±0.3 fold induction of IL-6 protein (*p≤0.05; Fig. 5D). Both fatty acids appeared to reduce this stimulation, however, only the effect of ω-3 was significant (*p≤0.05; ω-6: p = 0.1675; Fig. 5D).

IL-8 mRNA expression appeared to be slightly activated by both fatty acids. However, this was statistically significant for ω-3 only (**p≤0.01; ω-6: p = 0.1017; Fig. 5C). Incubation with H₂O₂ increased IL-8 synthesis to 4.8±1.7 fold (*p≤0.05), which could be counteracted by ω-3 supplementation (*p≤0.05; Fig. 5C). Addition of ω-6 was inefficient here (p = 0.2174). Analysis of IL-8 in the cells medium indicated that fatty acids alone had no effect on IL-8 contents (ω-3: p = 0.0506; ω-6: p = 0.9324; Fig. 5E). Exposition to H₂O₂ led to a 2.0±0.2 fold increase of IL-8, which was statistically significant (**p≤0.01; Fig. 5E). With respect to H₂O₂ counteraction, both fatty acids were ineffective (ω-3: p = 0.5258; ω-6: p = 0.9256; Fig. 5E).

Realtime PCR analysis of NFκB expression did not reveal any significant influences of both fatty acids on this transcription factor (Fig. 6A). Data suggested that H₂O₂ slightly stimulated NFκB, but statistical significance was not reached (p = 0.1087; Fig. 6A). Notably, such an indication of increase was not detected in fatty acid supplemented hTM (Fig. 6A). On the protein level, a similar regulation was observed. Fatty acids alone did not affect the nuclear NFκB level, whereas H₂O₂, though insignificantly, stimulated nuclear contents (Fig. 6B). Again, such a slight increase was not observed in ω-3 or ω-6 supplemented hTM (Fig. 6B).

Phalloidin labeling of F-actin revealed no explicit differences between controls and fatty acid supplemented cells with respect to formation of cross-linked actin networks (CLANs; Fig. 7A). It appeared that ω-6 treated cells tended to form increased numbers of stress fibers than the controls as well as ω-3 treated cells (Fig. 7A). H₂O₂ exposure promoted accumulation of stress fibers and CLAN formation (Fig. 7B) in the controls. In ω-6 preincubated cells, CLAN formation and stress fibre accumulation appeared even more pronounced (Fig. 7B) than in the stimulated controls and in ω-3 pre-treated cells. ω-3 pre-treated cells showed a similar frequency of CLANs and stress fibres as the unstimulated controls (Fig. 7B).