Investigation of the HelioVital filter foil revealed protective effects against UVA1 irradiation-induced DNA damage and against UVA1-induced expression of matrixmetalloproteinases (MMP) MMP1, MMP2, MMP3 and MMP15

The damaging effects of solar ultraviolet (UV) radiation exposure to human skin are well known and can reach from accelerated skin aging (photoaging) to skin cancer. Much of the damaging effects of solar UVA (320–400 nm) radiation is associated with the induction of reactive oxygen species (ROS), which are capable to cause oxidative damage to DNA like the oxidized guanosine 8-hydroxy-2' -deoxyguanosine (8-OHdG). Therefore, new UV protective strategies, have to be tested for their efficiency to shield against UV induced damage. We investigated the protective effects of HelioVital sun protection filter foil against UVA1 irradiation in skin cells. It could be shown, that HelioVital sun protection filter foil has protective effects against UVA1 irradiation induced changes in matrix metalloproteinase (MMP) expression. Furthermore a UVA1-dependant regulation of MMP15 in human fibroblasts could be shown for the first time in this context. In addition, this study demonstrated the protective effect of the HelioVital filter film against UVA1-induced ROS production and DNA damage. These results could pave the way for clinical studies with HelioVital filter foil shielding against the damaging effects of phototherapy and other forms of irradiation therapy, thereby increasing the safety and treatment opportunities of these forms of therapy.


Introduction
Most of the solar UV radiation reaching the surface of the earth consists of UVA (320-400 nm, subdivided in UVA2 (320-340 nm) and UVA1 (340-400 nm) [1]) radiation (approximately 95%) and only approximately 5% of UVB (280-320 nm) radiation [2]. The UVA exposure of healthy people, considering the presence and quantity of UVA radiation in everyday life [2], can have negative effects on the skin at the cellular level. Compared to UVB, which can inflict direct damage by photon-mediated excitation of DNA and subsequent generation of pyrimidine dimers, UVA can damage cellular structures indirectly via the generation of reactive oxygen species (ROS) [3]. UVAinduced ROS can cause oxidative damage to DNA like 8-hydroxy-2' -deoxyguanosine   [4], DNA double-strand breaks [5], and mediate lipid and protein oxidation [6][7][8]. Furthermore, UVA can penetrate much deeper into the skin compared to UVB, increasing the amount of affected tissue [9]. The plethora of cellular damage caused by UVA can translate to macroscopic skin malformations such as accelerated skin aging (photoaging) [10] and skin cancer, like squamous cell carcinoma (SCC), basal cell carcinoma (BCC) and melanoma [11], with continuously increasing prevalence and high mortality [12,13].
Prominent markers of UVA-induced damage in the skin are matrix metalloproteinases (MMP). The UVAinduced expression of matrix metalloproteinases, especially MMP1, MMP2, and MMP3, is an important feature in the process of UV-induced skin aging, especially in photoaging [14]. These proteases degrade proteins of the extracellular matrix in the skin and promote the formation of wrinkles in photoaged skin. In addition to this, MMP1 and MMP2 are important players during carcinogenesis of melanoma and many other tumors [14]. These proteases can be secreted by the tumor stroma [15] or the cancer cells themselves and help initial melanoma cells to invade the extracellular matrix, which is an important prerequisite for metastasis and vascularization of tumors [16][17][18]. Furthermore, high expression of MMP15 has been associated with the progression of SCC [14].
Despite its role in skin cancer formation and photoaging, solar and artificial UV radiation has a continuously increasing spectrum of clinical applications [19] as part of artificial light therapy [20] and heliotherapy in form of outdoor sun exposure. As part of artificial light therapy, both broad-band UVA and long-wave UVA1 are implemented for the treatment of pruritus, prurigo, atopic dermatitis, polymorphous light eruption, and cancer (in the form of photochemotherapy (PUVA)) [20]. Exposure to natural sunlight can have effects on the treatment of mood disorders, atopic dermatitis and psoriasis [21][22][23].
However, as already mentioned, the damaging effects of UVA irradiation and their long-term consequences, which can develop years after exposure, are a major drawback to its clinical application [24][25][26][27].
A field that can greatly benefit from improved protection strategies against UVA-induced damage is the Photodynamic Therapy (PDT), a treatment usually prescribed in cases of actinic keratosis (AK), Bowen disease, and certain types of basal cell carcinoma [28,29]. The classical application of PDT requires specialized devices and trained medical personnel [30]. In recent years, Daylight-Mediated Photodynamic Therapy (daylight PDT) has been proposed as an alternative to classical PDT. Daylight PDT substitutes specialized therapeutic devices with a regulated outdoor sun exposure, resulting in greater benefits for the patients in form of lower cost, flexibility, and reduced stress and pain [31]. Daylight PDT-treatment proved effective against AK, independent of weather conditions. Even irradiation reduction by 83% due to cloud-cover resulted in successful treatment as long as a minimal irradiation dose of 3.5-8 J/cm 2 was achieved [31,32]. However, patients have reported increased pain load when treatment was performed on a sunny day, with the lowest pain-score recorded on rainy or cloudy days [31]. Furthermore, there are indications that cloudy weather conditions do not always correspond to reduction of solar irradiance. Depending on cloud formation and composition, it is possible to receive higher irradiation doses when the weather is cloudy compared to clear-sky conditions [33], which can be detrimental for the patients.
Despite recent advancement in UV-protection technology and materials [34][35][36], alternative means for UVA protection are still in high demand. New protective strategies have to be tested for their efficiency to shield against UV-induced damage without reducing its therapeutic potential.
In this work, we investigated in skin cells the protective effects of HelioVital filter foil against UVA1 irradiation. In detail, the protective effects of HelioVital filter foil against UVA1-induced changes in cell viability, expression of matrix metalloproteinases (MMP), reactive oxygen species (ROS), DNA damage (measured with comet assays) and UVA1-specific DNA damage (8-OHdG) were investigated. The results showed that UVA1 irradiation-induced DNA damage, MMP expression and ROS production can be ameliorated by Helio-Vital filter foil. An additional outcome of this study was the discovery of UVA1 regulation of MMP15-a metalloproteinase, which was not reported to have UV-dependent modulation in human fibroblasts [14].

Protective effect of HelioVital filter foil against UVA1 induced changes in cell viability
In initial experiments, primary human skin fibroblasts were irradiated with sub-lethal doses of UVA1 for 4 consecutive days (spectral profile of the lamp and irradiation protocol are presented in Supplementary Fig. 1 and 2, respectively). The irradiation was conducted with and without protection by HelioVital filter (Fig. 1b), a filter foil which can absorb approximately 60% of solar UV radiation (Transmission of UVB-25.3%, UVA2-40.3%, UVA1-41.9%, see Fig. 1a and Supplementary Fig. 3). Repetitive UVA1 irradiation did not decrease cell viability (Fig. 2a). However, the significant decrease in the overall amount of viable cells points to UVA1-induced proliferation retardation (Fig. 2b). This observation was confirmed when the doubling times of the UVA1-treated and untreated cells were compared (Fig. 2c). The application of HelioVital filter foil ameliorated this UVA1-induced effect on proliferation (Fig. 2b, c), which might be due to less UVA1-induced DNA damage occurring in HelioVital filter foil protected skin cells.

Protective effect of HelioVital filter foil against UVA1-induced reactive oxygen species (ROS)
The UVA-induced ROS are an important mutagen, which can cause severe cellular damage [37]. To investigate the protective effect of HelioVital filter foil against UVA1 induced ROS, primary human skin fibroblasts were irradiated as described in the material and methods section with subsequent detection of ROS levels. To improve detection of ROS, a single dose of 18 J/cm 2 UVA1 was used. This single dose of 18 J/cm 2 is better suited than repetitive low-dose UVA1 treatment for ROS detection with our ROS detection system. When primary human skin fibroblasts are treated with UVA1 irradiation, the ROS level is increased in these cells. This effect can be decreased when skin cells are protected by a HelioVital filter foil during irradiation (Fig. 3a, b).

Protective effect of HelioVital filter foil against UVA1-induced DNA damage
It is well known that UVA -induced ROS can cause oxidative damage to DNA like 8-OHdG. However, UVA damage is not limited to oxidative lesions, there are many additional types of DNA damage induced by UVA irradiation, such as single or double strand breaks [38]. To detect these damages, comet assays were performed ( Fig. 4a-c).
In these assays, the damage is measured by the length of comet tails and the tail moment as described in the materials and methods section.
To investigate the protective effect of HelioVital filter foil against UVA1-induced DNA damage, primary human skin fibroblasts were irradiated with sub-lethal doses of UVA1, as described in the material and methods section and comet assay was performed to detect DNA damage. Repetitive UVA1 irradiation increased the tail moments ( Fig. 4a) and tail length (Fig. 4b), which can be reduced by protection with HelioVital filter foil during UVA1 irradiation.  foil against UVA1-induced DNA damage 8-OHdG, primary human skin fibroblasts were irradiated with sub-lethal doses of UVA1 as described in the material and methods section with subsequent detection of 8-OHdG levels. The 8-OHdG measurements were performed after 2 days UVA1-treatment since preliminary data (Supplementary Fig. 4) have shown that after 4 days irradiation the levels of 8-OHdG reach a plateau and no significant differences between irradiated and non-irradiated cells can be observed with the detection technology used. Repetitive UVA1 irradiation increased the 8-OHdG level in human fibroblasts compared to untreated controls. Application of HelioVital filter foil during UVA1 irradiation showed a tendency of 8-OHdG reduction (Fig. 5) compared to the level of UVA treatment. However, the difference in the 8-OHdG levels between UVA-treated cells with and without foil were not statistically significant.

HelioVital filter foil ameliorates UVA1 effects on the expression of matrix metalloproteinases (MMPs)
To investigate the protective effect of HelioVital filter foil against UVA1-induced expression of matrix metalloproteinases and tissue inhibitor of matrixmetalloproteinases (TIMP1), primary human skin fibroblasts were irradiated with sub-lethal doses of UVA1 for 4 consecutive days with and without protection by HelioVital filter foil.  Subsequently, the expression levels of matrixmetalloproteinases (MMP1; MMP2; MMP3; MMP9; MMP13; MMP15) and TIMP1 were measured. When primary human skin fibroblasts are irradiated, the expression of MMP2 (Fig. 6b), MMP3 (Fig. 6c), and MMP15 (Fig. 6d) is significantly increased in these cells compared to untreated controls. This effect can be reduced when skin cells are protected by a HelioVital filter foil during irradiation (Fig. 6a-d). The attenuation of UVA-induced MMP3 expression levels by the filter foil was not significant, but expression of MMP3 in UVA-irradiated filter foil protected cells was similar to the levels seen in untreated control cells with no statistically significant difference between these two levels (Fig. 6c).
Together with the filter-dependent attenuation of UVAinduced expression of MMP1, MMP2, MMP3 and MMP15, UVA induced TIMP1 expression also decreased after applying HelioVital filter foil (Fig. 6e). This could be explained as a coordinated effect of the treated cells. As there are less MMPs present in samples irradiated with HelioVital filter foil, less TIMP1 is needed.
Not all the investigated matrixmetalloproteinases are significantly influenced by UVA1 irradiation or filter foil protection ( Supplementary Fig. 5). This could be explained by a low expression level of MMP9 and MMP13 in these cells.
Taken together our results show that UVA1 induced an elevated expression of MMP2 and MMP15 and this effect can be ameliorated by HelioVital filter foil during UVA1 irradiation.

Discussion
It is well known that UVA irradiation can damage cellular structures and can induce photoaging and carcinogenesis [10,39,40]. In this work, we have shown that the HelioVital filter foil has the capacity to reduce UVA-induced cellular damage. In regard to UVA1-induced oxidative damage, cells irradiated without the protection of the HelioVital filter had significantly increased ROS production compared to both untreated controls and cells irradiated with filter. The amount of reactive molecules that could potentially damage cellular components was significantly reduced when foil was applied compared to unprotected irradiation. Furthermore, the alkaline comet assay showed significant decrease in both tail moments as well as tail length in cells irradiated in the presence of HelioVital filter compared to un-filtered irradiation (Fig. 4a, b). In addition to that, a tendency of reduction in oxidative DNA-damage marker 8-OHdG was observed in cells protected by HelioVital filter foil (Fig. 5). Even though the reduction of ROS formation and DNA damage did not reach the level of untreated control cells, the data presented in this work show that the application of HelioVital filter ameliorates UVA1-induced damage.
Besides reducing the damaging effects of UVA1 on DNAlevel, the application of HelioVital filter resulted in significant reduction of MMP1, MMP2, MMP15, and TIMP1 expression compared to cells irradiated without foil protection. No significant changes in the expression of MMP3 could be observed between cells irradiated with and without foil, although the application of HelioVital filter resulted in reduction of expression to levels similar to the ones observed in un-irradiated controls. This data imply that the application of HelioVital filter could be beneficial for the reduction of photoaging and skin cancer-associated MMP expression.
In the context of MMP regulation, it is important to note that, as far as we know from literature, there have been no reports of MMP15 being UVA1-regulated in human fibroblasts. This work is the first describing such UVA-dependent modulation of expression in this type of non-malignant cells [14]. Such behavior of MMP15, however, is not surprising since Gendron et al. have reported of UVA-dependent MMP15 expression in aged human cornea [41]. In their work on UVA and melanoma, Kamenisch et al. have observed increased lactate secretion after UVA-irradiation and lactatedependent regulation of multiple MMPs, including MMP1, MMP2, and MMP15, and TIMP1. If this UVA-dependent metabolic change would be similar in dermal primary fibroblasts, it would be possible that the increased expression of MMP15 observed in the current work has a similar UVrelated metabolic regulation.
However, the TIMP1 upregulation after UVA radiation observed in the current work was unexpected. Up to now, studies have shown either no influence of UVA radiation on TIMP1 expression levels [42,43] or even a decrease expression [44]. However, our experimental setup was different from the ones described in these studies [42][43][44]. In the case of Herrmann et al., the used dose was a single 180 kJ/m 2 (18 J/cm 2 ) [42] while in our experiment, the cells were irradiated repeatedly with 60 kJ/m 2 (6 J/cm 2 ) three times per day for 4 days, yielding a cumulative dose of 720 kJ/m 2 (72 J/ cm 2 ). In the study by Catalgol et al., a decrease of TIMP1expression levels was observed 3 h after UVA radiation. [44], whereas in our experiments, the cells were incubated over night before mRNA collection was done to determine TIMP1 expression levels. Since it is known that MMPs and TIMPs have a temporal regulation [45], and since the cells used are healthy wild-type fibroblasts, it could expected that there is an upregulation of TIMP1 as an antagonist of MMPs to preserve "tissue homeostasis". In contrast, Naru et al. concluded that TIMP1 shows no UVA-dependent changes in expression, despite showing UVA-regulation of TIMP1 in "older" cultured cells at maximum irradiation dose of 20 J/ cm 2 [43]. However, the UVA radiation dose used by Naru et al. correlates closely to the cumulative 18 J/cm 2 daily dose used in our study and the cells used were obtained from an adult donor (compared to the fibroblasts used by Naru et al. [43]). Therefore, we believe that the findings described by Naru et al. do not contradict the data from our study.
In addition to its protective function, since there is only a partial block of the UVA1 irradiation by HelioVital foil (see Fig. 1a and Supplementary Fig. 3), it is possible to use the residual 40% transmittance of radiation in diverse therapeutic applications such as daylight PDT.
An effective daylight PDT requires at least 3.5-8 J/cm 2 of solar irradiation, a dose-range achieved even under weather conditions when up to 83% of irradiation is blocked by cloud cover [31,32]. Since the HelioVital filter foil absorbs approximately 60% of solar UV irradiation (Fig. 1), which is in a range mimicking cloudy or partially cloudy weather conditions [31][32][33], it could be applied as sun-shielding during daylight PDT, giving the patients the benefit of reduced pain load even on sunny days [31]. Furthermore, the application of a HelioVital filter on sunny days could provide the benefits of reduced radiation exposure of cloudy weather without the variable cloud formation.
In addition to the potential benefits of HelioVital filter foil for patients undergoing PDT, another aspect of interest could be its application in the field of hormetic therapies. For some years, the hypothesis of hormesis has attracted attention. It suggests that a small dose of stressors could be beneficial for the organism by improving long lasting defense strategies against these stressors [46,47]. This hypothesis was already tested for ROS and it was found that continuous small doses of ROS could activate antioxidant defense systems [46][47][48]. Since ROS are induced by UVA and are one major damaging effect of this type of irradiation, it can be assumed that small doses of UVA could also have beneficial hormetic effects. The newly developed HelioVital filter foil, can shield approximately 60% of the solar UV irradiation, but can pass a limited amount of UVA irradiation ( Fig. 1 and Supplementary Fig. 3). From the perspective of the hormesis theory, the resulting small amounts of oxidative damage to cells could be important stimulators to maintain antioxidative protection, like the expression of proteins of the antioxidative defense system [46,[49][50][51]. These possible applications of the HelioVital filter foil open the path for new UV protective strategies, which do not completely block, but attenuate the intensity of UV radiation.

Conclusion
We could show that UVA1-induced damage to skin cells can be ameliorated by HelioVital sun protection filter foil. Furthermore, we could show for the first time UVA1-dependant regulation of MMP15 in human fibroblasts. HelioVital sun protection filter foil had protective effects against UVA1 irradiation-induced changes in cell proliferation and MMP expression and against UVA1 irradiation-induced ROS production and DNA damage. These results pave the way for clinical studies with HelioVital filter foil shielding against the damaging effects of phototherapy and other forms of irradiation therapy, thereby increasing the safety of these treatments. Furthermore, protection with HelioVital filter foil could increase the number of applications of these therapies and could contribute to achieve a balance between potential beneficial effects and damaging effects of UVA1 exposure.
As basis for later applications of these HelioVital filter foil as sun protection or as filter in artificial light therapy and heliotherapy, more in vitro safety studies with low doses of repetitive UVA1 treatment have to be performed.

Isolation and culturing of human fibroblasts
Skin biopsy samples of healthy volunteers were obtained from the University Hospital Regensburg (Ethic vote number 14101 0001). The whole skin biopsy was put on a Primaria cell culture dish (Corning, USA), containing a single drop of DMEM-Cipro (DMEM 1 g/L glucose (Gibco, Thermo Fisher) supplemented with 10% FCS (Fetal + High Performance Serum, anprotec), 1% Penicillin/Streptomycin (Sigma-Aldrich), 1% Ciprofloxacin (Fresenius Kabi)), and incubated for 30 min at 37 °C to ensure that the skin sample sticks on the dish surface. Afterward, 3 ml DMEM-Cipro were added to the skin sample. It was cultivated at 37 °C, 5% CO 2 until cell-outgrowth of fibroblasts was enough for a transfer to a T25 cell culture flask. Subsequently, the cells were transferred to a T75 flask, cultured in DMEM without Ciprofloxacin, and used for further experiments under the designation Re5.

Irradiation protocols for skin cells
The irradiation of Re5 fibroblasts was performed as follows. Cells were seeded at 5 × 10 4 cells per well on a 6-well plate and left to grow over night before the start of UVA1-treatment. The standard irradiation protocol is shown schematically ( Supplementary Fig. 2), and described in detail below. It had the duration of 4 days, with 3 × 6 J/cm 2 per day. All irradiations contained three test groups − 0 J/cm 2 , 6 J/cm 2 and 6 J/cm 2 + Filter foil. After the fourth day of irradiation and overnight incubation, the cells were counted, viability was determined, and the cells were collected for further analysis. mRNA and DNA was isolated for qPCR analysis and 8-OHdG measurement, respectively (Data for 8-OHdG after 4 days of UVA1 irradiation are shown in Supplementary Fig. 4). Additional data for 8-OHdG were collected after 2 days of UVA1 irradiation. A complete protocol of the 8-OHdG measurement can be found in Sect. 5.6.
At the beginning of irradiation, the medium was aspired form each well. Cells were irradiated in 1 ml PBS. The amount of UVA1 per single irradiation was set at 6 J/cm 2 and provided by a Sellamed 1200 Lamp [Sellas Medizinische Geräte GmbH, Germany) with an emission spectrum 340-420 nm (see Supplementary Fig. 1)]. The PBS was then aspired and 5 ml fresh medium were added to each well after the first irradiation. Before all subsequent irradiations the medium was aspired and collected in separate falcons and returned to the corresponding wells after wards. Three irradiations per day were performed. There was 4 h resting period between single irradiations with ON rest after the last daily irradiation. The duration of total irradiation was 4 days. Before the first irradiation of day 3, 1 ml fresh medium was added to each well to compensate for medium loss. The HelioVital Filter LTL-3-130om (PP-PET-met.-multilayerfilm) was added between UVA1 lamp and cells in one of the experimental groups. After overnight incubation, cells were collected for RNA extraction.
A separate irradiation protocol of a single irradiation (1 × 18 J/cm 2 ) was performed for the purpose of ROS detection. A graphic representation of the treatment can be found in Supplementary Fig. 2 and the complete procedure of ROS detection can be found in Sect. 5.5.

Two-in-one cell count and viability test
To determine the number of cells, as well as their viability, a LUNA-FL Dual Fluorescence Cell Counter (Logos Biosystems, Inc., South Korea) in combination with Acridine orange/Propidium iodide (AO/PI) staining (BioCat) was used. Acridine orange (AO) and propidium iodide (PI) are nucleic acid binding dyes. AO can permeate both live and dead cells and intercalates with DNA, generating green fluorescence. PI can only enter dead cells who have poor membrane integrity. It then generates red fluorescence in all dead nucleated cells. In addition, in cells containing both AO and PI, the green fluorescence is quenched and the cells still fluorescent red. With this, all live nucleated cells fluoresce green and all dead nucleated cells fluoresce red, allowing for clear distinction between viable and non-viable populations.
To perform the actual cell-count, 18 µl of cell suspension were mixed with 2 µl AO/PI dye. From this mixture, 10 µl were pipetted on LUNA cell counting slides and measured in fluorescence modus with LUNA-FL.
To calculate the doubling times of the counted cells, the following formulas were used: a is the initial cells (seeded at the beginning of the experiment); b is the end cells (counted at the end of the experiment, see Supplementary Fig. 2); n is the number of doublings; h is the hours in culture; t is the doubling time.

RNA extraction, reversed transcription and qPCR analysis
RNA extraction from the treated cells was performed via NucleoSpin RNA-isolation kit (Macherey-Nagel, Germany) using the standard isolation protocol for adherent cells. The samples were stored at − 20 °C until further use. The concentration of RNA in the samples was determined via NanoDrop. For the reverse transcription, 500 ng RNA per sample were used. A master mix was prepared for the reverse transcription, containing 1 µl random primer, 4 µl 5 × buffer, 1 µl dNTPs (New England BioLabs), 1 µl DTT and 2 µl water per sample (Invitrogen Reverse Transcription Kit, Thermo Fisher Scientific, USA). Up to 10 µl RNA were added to the mix and the rest of the volume up to 19 µl was filled with water. The RNA was stretched for 10 min at 70 °C. Afterwards 1 µl Superscript enzyme (Invitrogen Reverse Transcription Kit, Thermo Fisher Scientific, USA) was added to each sample at room temperature followed by 45 min incubation at 42 °C and subsequently 10 min at 70 °C. At the end of the reverse transcription, the sample were cooled and stored at 4 °C. For the qPCR analysis following each sample contained 10 µl SybrGreen (Roche, Switzerland), 0.5 µl forward primer, 0.5 µl reverse primer, 8 µl water and 1 µl cDNA. For negative control 1 µl water was used instead of cDNA. 20 µl from each sample were pipetted in duplicates on a Roche 96-well LightCycler plate. Optimal annealing temperatures were determined for each gene of interest as shown in Table 1.
The LightCycler was programmed for 45 cycles of amplification. The end results were calculated with LightCycler 96 software and presented as ratio to housekeeper (b-Actin).

DCFDA-ROS detection
Cells were seeded on 10 cm dish at density 5 × 10 5 cells per dish in DMEM. The cells were cultured for 2 days at 37 °C. Afterwards the dishes were washed 1 × with DMEM without FCS. From that point on, all remaining steps were performed in the dark. The cells were stained with 100 µM DCFDA (Sigma-Aldrich, Germany), dissolved in DMEM without FCS. The staining was performed for 35 min at 37 °C in the dark. Some cells were left unstained to be later used as background control. After the end of incubation, the cells were washed 2 × with medium without FCS. They were thereafter trypsinized, counted and seeded on two black clear bottom 96-well plates at density 1 × 10 4 cells per well in a total volume of 100 µl per well. One plate was left as 0 J/cm 2 un-irradiated control and the other was immediately irradiated with a single dose of 18 J/cm 2 UVA1 to induce ROS (For irradiation protocol see Supplementary Fig. 2). After the irradiation, both plates were incubated for 30 min The viability of the irradiated cells was performed 30 min after irradiation at the same time as the ROS measurement was performed (see Irradiation Protocol 2 in Supplementary  Fig. 2).

DNA extraction and detection of 8-OHdG as a sign of UVA1-induced DNA damage
To retrieve DNA for subsequent 8-OHdG experiments, UVA1 treated cells (2 days and 4 days) and controls cultured on 20 cm petri dishes at seeding density of 8 × 10 5 , were trypsinized, centrifuged and re-suspended in 200 µl/ sample PBS. From then on, a QUIamp Mini Kit (QIAGEN, Germany) was used for the isolation using standard kit protocol for adherent cells.
The method used to detect oxidative DNA damage in UVA1-irradiated cells was based on the OxiSelect™ ELISA Kit (Cell Biolabs Inc., USA). This kit is a competitive enzyme immunoassay for detection and quantitation of 8-OHdG in DNA samples. After performing staining according to the kit protocol, the absorbance the microwell plate was measured with a Varioscan Flash plate reader at 450 nm.
For data analysis, the values from the standard were plotted in GraphPad Prism and the unknown values for the samples were extrapolated from the resulting curve.

Comet assay
In preparation for the comet assay, the cells were irradiated in accordance with the 4 days irradiation protocol described in point 5.2. Afterwards the cells were counted and resuspended at 1 × 10 5 cells/ml. Afterward, the comet assay was performed in accordance with Comet Assay protocol (Trevigen, USA) for Alkaline Comet Assay. SYBR-Gold was used for the subsequent DNA-staining and visualization. For the evaluation of the comets, the CometScore software Version 2.0.0.0 was used.

Heliovital Filter Foil specifications and measurements of the transmittance
As shown in Fig. 1b, the HelioVital Filter Foil (HelioVital Filter LTL-3-130om (PP-PET-met.-multilayer-film) used in these experiments consists of multiple layers: • Protective and weary layer-UV transparent polypropylene layer approved by food law (used to protect filter layer from external chemical or physical induced damages) (Fig. 1b layer 1 and 8); • Adhesive layer-connecting layer (Fig. 1b layer 2 and  7); • Print layer-connecting layer (Fig. 1b layer 3), • Metallization--functional part contributing to the filter properties of foil ( Fig. 1b layer 4); • Filter layer-PET (Polyethyleneterephthalate) layer for pigmentation (functional part of filter properties of foil) ( Fig. 1b layer 5); • Pigmentation layer-functional part contributing to the filter properties of the foil (Fig. 1b layer 6).
The primary selective filtration of wavelengths in the UV range is achieved by the absorption behavior of the special polymers of the PET membrane and its thickness. This very thin PET membrane is also the substrate for the following secondary relative filtration layers by means of metallisation through vacuum sputtering and by means of printed pigment ducks, which are also partly components of the adhesives. The cover layers made of PP protect the entire modular film composite and thus enable practical handling and processing. The Filter foils had, following transmission in the UVR-range: UVB-25.3%, UVA2-40.3%, UVA1-41.9%, (see Fig. 1a).
Measurements of the transmittance of the HelioVital filer foil (HelioVital Filter LTL-3-130om (PP-PET-Met.-Multilayer-Film)) and glasses ( Fig. 1 and Supplementary  Fig. 3) were made in 1-nm increments using a high-precision dual-beam UV-VIS-NIR spectrophotometer of the type Cary 500 from Varian (now Agilent). Funding Open Access funding enabled and organized by Projekt DEAL. This work was partially funded by HelioVital (HelioVital GmbH, Zollernring 32, 72186 Empfingen, Deutschland).

Availability of data and materials
Detailed information about used materials, methods and data are available upon request.
Code availability Not applicable.

Conflicts of interest/competing interests The authors have no conflict of interest.
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