Antioxidant and tyrosinase inhibitory activities of traditional fermented Rosa from Dali Bai communities, Northwest Yunnan, China

Traditional fermented Rosa (TFR) is a typical food and medical product among the Dali Bai people, and its popularity is growing. A few studies have looked into TFR's medicinal advantages, linked germplasm resources, traditional processing procedures, and functional food qualities. Our goal was to look into Rosa's traditional processing, examine the dominant strains in TFR, and prove how these strains affected antioxidant and tyrosinase inhibitory activities. We used a snowball selection strategy to pick 371 informants for a semi-structured interview, supplemented with direct observations and sample collection. A microbial strain was isolated and identified from a TFR sample collected in the field. We synthesized TFR in the lab using the traditional way. Both of 2, 2-diphenyl-1 picrylhydrazyl (DPPH) free radical scavenging and tyrosinase inhibitory properties of the fermented solution of Rosa 'Dianhong' have been tested in this study. Altogether 15 species belonging to the genus Rosa, which are utilized in herbal medicine and fermented foods. Rosa 'Dianhong' was the Bai community's principal species with considerable cultural value and consumption. Raw Rosa petals included 15 major flavonoids and phenols, which were identified as TFR's active components. TFR-1 was discovered to be the dominating microbial strain in TFR, increasing total phenolic and flavonoid content in the fermented solution of Rosa 'Dianhong' by 0.45 mg GAE/ml and 0.60 mg RE/ml, respectively, after 30 days. TFR-1 also exhibited promising activity in terms of DPPH free radical scavenging and tyrosinase inhibition. TFR showed potent antioxidant and free-radical scavenger properties and is beneficial in skincare and nutrition, according to the findings. TFR's medicinal and edible properties suggest that it could be used as a cosmetic or nutraceutical product.

Fermentation has a long history in human food production and is a valuable process in food industries, making food products available throughout the year 1,2 . Fermentation of edible items improves product quality and creates diverse flavor components, which boosts consumer acceptability [3][4][5] . Furthermore, by adding salt and producing acid and ethanol, the fermentation process can improve the nutritional and functional qualities of foods while also extend their shelf life 2 . Microorganisms and their enzymes cause fermentation, which is a biochemical alteration of the fundamental food matrix. Traditional knowledge of the fermentation of edibles has shown pharmacological activity that can be used to cure a variety of diseases. Fermentation, for example, allows for the manufacture of broccoli products that are safe, stable, and high in sulforaphane. These fermented foods are fantastic dietary supplements 6 . It also contains anti-cancer 7,8 , anti-diabetes 9 , and anti-obesity 10 properties, as well as helping to alleviate behavioral issues linked with autism spectrum disorder 11 . Fermentation also enhances the antioxidant activity and tyrosinase inhibitory activity of phenols 12 and flavonoid antioxidants 13 .
The adaptive nature of the fermentation process within a given region arises from centuries of human relationships with the microbial community in the environment. Microorganisms, inorganic components, and their interactions all play a role in fermentation processes and product creation 14 . In traditional fermentation processes, such as those of Brassica oleracea L., Oryza sativa L., and Glycine max (Linn.) Merr., microbial sources are either internal to plants or derived from external surfaces and the surrounding environment. Fungi and bacteria, particularly yeast and lactic acid bacteria populations among the microorganisms that increase the quality of traditional fermentation products 3,4 . Traditional fermentation is a promising method for isolating certain microorganisms' impact on biosynthesis or breakdown of bioactive substances.
Traditional fermented Rosa (TFR) is a biocultural heritage among Dali Bai communities in northwest Yunnan, China, which has evolved over a long time as a result of interactions between local cultures and their environment 15 . TFR is widely acknowledged in Dlai Bai communities as a medical food that nourishes the body and keeps the skin smooth. However, until today, knowledge of traditional TFR processing has been preserved within the community. TFR's plant resources, fermentation method, and bioactivity have never been comprehensively described. When the globe is confronting a pandemic like Covid-19, research into traditional knowledge around such a vital food source and its bioactivity is critical. Functional foods with health advantages are in high demand. To that end, the goal of this study was to determine the main microbial strains and relative bioactivities of TFR, as well as clarify the plant resources and conventional processing methods employed in TFR. Our research not only contributes to biocultural preservation, but it also gives critical information for the future development of TFR-based pharmaceuticals and prospective nutraceuticals.

Diversity of the genus of Rosa in Dali Bai communities. Our informants told the interviewers about
15 Rosa species used in Dali for traditional applications. Both wild and cultivated species are in use as food and medicine. Table 1 shows the usage information for these 15 species. The informants reported that Rosa species have anti-aging properties; cure rheumatism and dehydration; activate blood circulation; and possess detoxification, insecticidal, and diuretic properties. These plants are used as medicine, food, and fragrance, with different methods and frequency of use.
The Dali Bai communities primarily use 10 of the 15 species for medicine, 7 for food, and 2 for fragrance. Rosa damascena is one of the main species used for essential oil extraction. Of the seven edible species, Rosa 'Dianhong' scored the highest informant consensus factor (ICF) 16 and use frequency (f) 17 values, indicating its cultural value and extent of consumption (Table 1). Rosa 'Dianhong' is used in petal tea, wine, sugar, and TFR. TFR is the most popular among these uses.
The TFR in Dali Bai communities. TFR in Dali was prepared by natural fermentation. Petals picked from locally available edible Rosa plants were the main ingredient in TFR (Fig. 1). The traditional planting of edible Rosa resources including Rosa 'Dianhong' , Rosa 'Mohong' , Rosa laevigata, Rosa rugosa, Rosa roxburghii, Rosa gallica, and Rosa centifolia. Rosa 'Dianhong' was mainly used in TFR preparations, while Rosa 'Mohong' was used as an ingredient of TFR only in Heqing county. According to our informants, the thinner petals of Rosa 'Dianhong' have better flavor after fermentation compared with those of Rosa 'Mohong' .
All informants mentioned that TFR benefits the skin. The majority of informants (83.3%) told us that TFR can nourish the stomach, and a few informants mentioned that TFR is hepatoprotective and refreshing. Although none of the informants could explain the pharmacological reasons, these traditional uses hint at potential therapeutic value.
Microbial strain identification. Microbial strains were isolated from TFR prepared traditionally by the Bai people in Dali. The ITS fragment from the dominant strain, TFR-1 (Table 2), shared 99.84% similarity with that of Saccharomyces rouxii. Therefore, the strain TFR-1 was named Saccharomyces rouxii TFR-1. The strain is now preserved in the China General Microbial Culture Collection Center (CGMCC) with the sample number CGMCC19335.
Pharmacological properties of FSR. Antioxidant activity. The free radical scavenging activity of FSR after different periods of fermentation were examined. As shown in Fig. 2. At low concentration (i.e., 0.025 mg/ ml, 0.05 mg/ml, and 0.1 mg/ml), samples FSR-3, FSR-7, FSR-14, FSR-21, and FSR-30 showed better DPPH free scavenging activities than FSR-0. At a concentration of 0.05 mg/ml, this difference was significant (P < 0.05). www.nature.com/scientificreports/ FSR-21 had the highest DPPH scavenging activity, reaching 44.60%. At concentrations greater than 0.2 mg/ ml, there was no significant difference in the DPPH scavenging activity of FSR-3, FSR-7, FSR-14, FSR-21, and FSR-30 compared with that of FSR-0. However, with increasing concentration, the trend for greater scavenging activity with longer fermentation began to flatten. DPPH radical scavenging rates of these samples were higher than 85% after 30 days. Table 3 shows the IC 50 values for FSR and the positive control.
Tyrosinase inhibition activity. At a concentration of 0.125 mg/ml, tyrosinase inhibition activity of FSR was insignificant at all time points compared with FSR-0, except in the FSR-30 sample (5.48%; P < 0.05) (Fig. 3). However, as the concentration of FSR increased, tyrosinase inhibition activity also increased. At a concentration of 0.5 mg/ml, tyrosinase inhibition by FSR-7, FSR-14, FSR-21, and FSR-30 was significantly different from that by FSR-0 (P < 0.05). The confidence level for the FSR-30 sample was higher (P < 0.001), and FSR-30 was also significantly different from the FSR-21 sample (P < 0.05). Although only the inhibitory activity of FSR-30 showed a statistical difference compared with FSR-0 at a concentration of 2 mg/ml, the mean value of tyrosinase inhibition increased with increasing fermentation time. At a concentration of 10 mg/ml, tyrosinase inhibition by FSR-3, FSR-7, FSR-14, FSR-21, and FSR-30 was significantly higher than that of FSR-0 (P < 0.001). The highest inhibition rate was 86.58% and was for FSR-30. Among all samples, longer FSR fermentation duration resulted in greater inhibition of tyrosinase activity. Table 4 shows the IC 50 values for FSR and the positive control.
Nutrients in FSR and phytochemical profile. The total phenolic contents of FSR-3, FSR-7, FSR-14, FSR-21, and FSR-30 were significantly higher than that of FSR-0 (P < 0.001) ( Table 5). Longer duration of fermentation increased the total phenolic contents of FSR. However, none of the differences between adjacent fermentation intervals, FSR-3, FSR-7, FSR-14, FSR-21, and FSR-30, were significant.      (Table 5). However, different from the total phenolic contents, across the whole fermentation process, the values for total flavonoid contents of FSR-7, FSR-21, and FSR-30 were significantly different from those at the previous time point (P < 0.05). This indicated that fermentation duration plays an important role in increasing total flavonoid content in FSR.
Correlation analysis. Our results revealed that an increase in total phenolic and flavonoid contents produced by increased fermentation time enhances the DPPH free radical scavenging rate and tyrosinase inhibition activity of FSR (Fig. 4). Pearson analysis demonstrated a moderate correlation between total phenolic content and DPPH free radical scavenging activity, but the difference was not statistically significant (P > 0.5) (Fig. 4A). Total phenolic contents were highly correlated with tyrosinase inhibition activity (P < 0.5) (Fig. 4B). These results indicate an increase in phenolic content after fermentation as an important factor triggering tyrosinase inhibition activity of FSR.
Pearson analysis showed that total flavonoid contents after fermentation were highly correlated with DPPH free radical scavenging rate and tyrosinase inhibitory activity (P < 0.5) (Fig. 4C,D). Moreover, the total flavonoid contents changed significantly with increases in fermentation time (Table 5).
Main effective compounds in the genus Rosa used by Bai people in Dali. Petals from 15 plant species of the genus Rosa used in traditional applications in Dali Bai communities were collected; most were included in the previous phytochemical and pharmacological studies. The contents of the petals varied, but most of them contained flavonoids and phenols, which are known to be bioactive in vitro. Antioxidation is an important bioactivity of TFR in vitro. For example, according to Vinokur et al. 18 , the radical scavenging activity in rose petals is mostly due to the high content of phenolic compounds, especially free gallic acid (1; Fig. 5). protocatechuic acid (2), syringic acid (3), anthocyanin (4), 4-hydroxybenzoic acid (5), chlorogenic acid (6), and catechin hydrate (7) are also predominant phenols in rose petals 19 . These phenols have more hydroxyls, including o-dihydroxy, which demonstrate strong free radical scavenging and antioxidant abilities 20 . Flavonoids possess a galloyl ester in the C ring, which are important structures for chelation of metal ions, formation of complexes with metal ions, and inhibition of metal-initiated lipid oxidation. Therefore, flavonoids are able to effectively scavenge hydroxyl and peroxyl radicals [21][22][23] . The high concentration of flavonoids in Rosa resulted from the presence of a large amount of naringenin (8), with quercitrin (9), hesperidin (10), quercextin (11), luteolin (12), apigenin (13), and kaempferol (14) also comprising the main effective flavonoid compounds in rose petals; these flavonoid compounds contribute towards the antioxidant capacities of rose 19 . According to Jin 24 , the main flavonoids in rose petals include rubin (15), quercetin (11), kaempferol (14), and their derivatives; these compounds contributed more than 60% to the flavonoids in TFR rose petals, and our correlation analysis showed that they were significantly related to antioxidant activity. Flavonoids also slow tyrosinase activities by interacting with copper ions essential to the active site of tyrosinase. Tyrosinase, a key enzyme in skin pigmentation, catalyzes hydroxylation of   26,27 . Therefore, flavonoids are considered to be a natural tyrosinase inhibitor.

Discussion
Traditional edible flowers have been utilized as a therapeutic food in China for thousands of years 28 because of their emollient, antibacterial, and anti-inflammatory properties. Many Dali Bai groups use specific plants because they are considered healthy, according to our ethnobotanical survey. Specific species, biochemical ingredients, or pharmacological qualities are the subject of most studies on the beneficial properties of food plants. Many researchers, for example, are looking for potential nutritional supplements against cancer in food plants. Antioxidants play a role in cancer prevention, and many types of research have been conducted on these substances. Apium nodiflorum, Humulus lupulus, Silene vulgaris 29 , Nasturtium officinale 30 , and Leopoldia comosa bulbs 31 all have strong antioxidant capabilities. Our survey showed that Rosa 'Dianhong' petals are most commonly employed in traditional meals as a classic sauce, and their phenolic and flavonoid components have been linked to health benefits. Fermentation changes the chemical composition of food, potentially increasing its biological activity 32 . Fermentation is traditionally employed for food preservation 3,33 , but it is also an important biotransformation process for producing new products or crude materials 6,34 . Fermentation appears to increase the total phenolic and flavonoid content of FSR, as suggested by our findings. According to Pearson analysis, there is a strong link between total phenolic and flavonoid content in FSR and tyrosinase inhibition, consistent with prior research 35 . TFR can play a crucial role in conferring antioxidant and tyrosinase inhibitory action by boosting phenols and flavonoids. PDA isolated TFR-1, which was later recognized as belonging to Saccharomyces rouxii. It is a yeast commonly employed in soy sauce fermentation and safe to consume as it has been consumed for a long time in human history. This strain can withstand high osmotic pressure because it produces sugars, alcohols, acids, and other chemicals involved in sugar and energy metabolism to protect cells under hypertonic culture conditions 36 . Traditional Rosa fermentation uses a 50 percent sugar concentration to retain sweetness and taste under sugar stress to generate a high osmotic pressure environment that inhibits putrefactive, pathogenic, and Only one strain, TFR-1, could tolerate the high osmotic pressure and play an important role in TFR processing in Dali Bai populations. Because of its excellent osmotic pressure resistance, non-toxicity to humans, and other possible functions in healthcare, the strain in this study is worth further investigation.

Conclusion
In the Dali Bai villages in Northwest Yunnan, China, TFR is a traditional medical food. As evidenced by our ethnobotanical survey, local people sustain the traditional TFR process, which has been passed down from generation to generation through these activities. Our findings show that TFR prepared traditionally contains strain TFR-1 (Saccharomyces rouxii) as the most important microbial content that facilitates fermentation and impacts TFR quality. It increased the antioxidant activity and tyrosinase inhibitory activity of FSR. These critical functional activity alterations provide applicable research for TFR products, mainly cosmetic or nutraceutical products. Traditional medical food culture promotes environmental protection, protects fast vanishing traditional knowledge, and has numerous applications in other domains of human activity. To that end, this work underlines the importance of continuing research on traditional fermented food products and related traditional knowledge as a method of discovering new strains and expanding the commercial potential. Our findings also highlight the importance of traditional items in creating modern healthcare, food, and cosmetic businesses.  40 . First, the purpose of the study was explained to key informants of Bai communities. Local community committees were then visited to obtain field study permission and request assistance. The assistance included introduction to community members and heirs of the intangible cultural heritage of TFR and organization of representative workshops. All field studies were carried out with informed consent. An eth-  (Table 6) using the snowball sampling method to select potential informants 41 . Herbalists, farmers, merchants, and indigenous people were among the informants. They were engaged in the collection, production, sales, and use of the genus Rosa.

Study area. This study was conducted in Dali Bai
Women are frequent users of the genus Rosa and accounted for 55% of informants. Men who are herbalists, farmers, and vendors are associated with the value chain of Rosa. All had long-term experience with the applications of the genus Rosa. Semi-structured interviews were conducted with the consent of local people. The interviews focused on the following questions: (1) Does the community use the Rosa species? If yes, how many species are in traditional use? (2) Where do you get these plants? (3) How do you use these plants?  Voucher specimens of 20 Rosa species naturally occurring in the study area were collected. A taxonomist and ethnobotanist at Kunming Institute of Botany identified the voucher specimens. All specimens collected during the field survey were deposited in the Herbarium of Kunming Institute of Botany.
Isolation, purification, and identification of strains. TFR prepared traditionally by the Bai people in Dali was used for strain isolation. TFR solution was prepared in sterile water at different concentrations (10 -1 -10 -5 ). The dilution coating method was applied 42 . The diluent was inoculated onto a PDA (potato dextrose agar) medium for culture of fungi 43 and onto NA (nutrient agar) medium for culture of bacteria 44,45 . After growth, fungal and bacterial colonies were purified using the plate streak method 45 . Purified materials, which were similar to yeast, were stored at 4 °C for preservation. PDA and NA medium were both from Qingdao Rishui Biotechnology Co., Ltd. The strain was named TFR-1 and deposited at the Kunming Institute of Botany, Chinese Academy of Sciences.
To ascertain the identity of strain TFR-1, its total genomic DNA was extracted using a DNA extraction kit from Beijing Tsingke Xinye Biotechnology Co., Ltd. (Tsingke) using the CTAB/SDS method 46 . The ITS1 region from the DNA sample was amplified by PCR using an Applied Biosystems 2720 thermal cycler, while fungal sequences were amplified using universal primers (Tsingke). Amplified PCR fragments were sequenced by Tsingke and used as a query sequence in a BLASTN search against the NCBI public database, following the method described by Blanc et al. 47 .
Preparation of Rosa fermentation and sampling. TFR was prepared in the laboratory following the traditional method. Petals of Rosa 'Dianhong' that is traditionally used in TFR preparation in Dali were purchased, and 0.5 kg of petals was cut into small pieces to maximize extraction. Brown sugar (0.5 kg) was added and the mixture was kneaded manually until fully wet. The mixture was then placed into a 1-l fermentation bottle and 500 ml sterile water was added. Three bottles of this solution were prepared as replicates. The bottles were exposed to ultraviolet light for 45 min for sterilization on a super purgative working table. After 24 h, 10 ml Rosa 'Dianhong' solution from each bottle was removed and stored as sample FSR-0. Then, TFR-1 solution (15 ml) with a concentration of 4.15 × 10 6 CFU/ml was added to the fermentation bottles, which were sealed with caps and stored at 28 °C in a thermostatic incubator. Fermentation solution of Rosa 'Dianhong' (FSR) from each bottle (10 ml) was sampled on days 3, 7, 14, 21, and 30 and labeled FSR-3, FSR-7, FSR-14, FSR-21, and FSR-30, respectively. Each of the samples was centrifuged at 4000 rpm for 15 min, and the supernatant liquid was stored at − 20 °C to cease further fermentation.
Determination of total phenolic contents. Total phenolic contents of FSR were determined spectrophotometrically using Folin-Ciocalteu's method as described by Kang et al. 48 with slight modification. Diluted FSR (0.4%, v/v) was used in the analysis. A 10-μl aliquot of FSR was mixed with 0.25 ml 1 N Folin-Ciocalteu's reagent in a 5-ml test tube. The mixture was covered and kept still for 2 min in the dark before 0.5 ml 12% (w/v) aqueous solution of Na 2 CO 3 and 1.24 ml distilled water were added. The mixture was incubated for 1 h at room temperature and then ultraviolet absorbance was measured at 765 nm using a UV-5500PC (METASH) against a control. The control sample contained the same amount of chemicals with the FSR replaced by distilled water. Gallic acid (GA) was used as a standard for preparing a calibration curve. Total phenolic contents were expressed as mg GA equivalents per FSR.
Determination of total flavonoid contents. Total flavonoid contents of FSR were measured using the aluminum chloride colorimetric assay 49 with slight modification. Diluted FSR (concentration at 1.6%, v/v) was used in the analysis. A 40-μl aliquot of FSR was added into a 5-ml test tube containing 1.31 ml of distilled water and 75 μl of 5% (w/v) NaNO 2 was then added. After 5 min, 75 μl 10% (w/v) AlCl 3 was added and allowed to react for 6 min before 1 ml of 4% (w/v) NaOH dissolved in distilled water was added. The solution was mixed and kept for 12 min at room temperature before ultraviolet absorbance was measured against the control at 510 nm using a UV-5500PC (METASH). Control samples contained the same amount of chemicals except the FSR was replaced with distilled water. Rutin was used as a standard for constructing a calibration curve. Total flavonoid contents were expressed as mg rutin equivalents per of FSR.
Free radical scavenging activity. The free radical scavenging activity of FSR was examined in vitro using DPPH (2, 2-diphenyl-1 picrylhydrazyl) radical as described by El Atki et al. 49 . Different concentrations of FSR or GA were added to ethanolic solution and mixed with DPPH dissolved in ethanolic solution so that the final concentration of DPPH was 0.1 mmol. The absorbance of the mixture was measured using a UV-5500PC (METASH) at 517 nm after 30 min of incubation at room temperature in darkness. A control mixture in which FSR was replaced by the equivalent amount of ethanolic solution was prepared following the same procedures. The percentage of inhibition was calculated using the following equation: %DPPH scavenging activity = 1 − OD sample /OD control × 100 www.nature.com/scientificreports/ Here, OD control is the absorbance of the negative control and OD sample is the absorbance of the sample. GA served as positive control. IC 50 values were calculated as the concentration of causing a 50% inhibition of DPPH radical.
Tyrosinase inhibition activity. Tyrosinase inhibitory activity was examined in vitro as described by Elena et al. 50 . Different concentrations of FSR or kojic acid (KA) were mixed with tyrosinase dissolved in 0.2 M phosphate buffer (pH 6.8) and kept still for 15 min at 37 °C. Next, 12.5 mM L-Dopa dissolved in 0.2 M phosphate buffer (pH 6.8) was added, so that the final concentration of tyrosinase was 25 U/ml and that of L-Dopa was 1.25 mM in the solution. Absorbance at 475 nm was measured using a UV-5500PC (METASH) after incubation for 5 min at room temperature. FSR was replaced by the equivalent amount of phosphate buffer in the control mixture prepared following the same procedures. The percentage of inhibition was calculated using the following equation: OD control is the absorbance of the negative control and OD sample is the absorbance of the sample. KA served as a positive control. IC 50 values were calculated as the concentration of causing a 50% inhibition of tyrosinase.
Statistical analysis. SPSS 22 (Statistical Product and Service Solutions, https:// www. ibm. com/ produ cts/ spss-stati stics) was used for statistical analysis. Probit regression analysis was used to analyze the IC 50 of DPPH free radical and tyrosinase inhibition. Pearson correlation analysis was used to determine the correlation of total phenolic and flavonoid contents with DPPH free radical scavenging activity and tyrosinase inhibition activity. Differences between means were determined using the least significant difference test at P < 0.05, and figures were drawn using OriginPro 2017 (https:// www. origi nlab. com).
Ethics approval and consent to participate. The Authors confirm that no animal/human studies have been carried out in the present. This study was part of a wider project entitled "Study on traditional fermented rose in Dali Bai Nationality". We conducted this research in accordance with International Society of Ethnobiology (2006), ISE Code of Ethics (with 2008 additions), and the protocol was approved by Kunming Institute of Botany, Chinese Academy of Sciences (KIB) ethics committee (Supporting documents S1) and Center of Biodiversity and Indigenous Knowledge(CBIK) ethics committee (Supporting documents S2). Before data collection, we described the goals of this research to local informants and asked them to sign a Free andInformed Consent Term. We were authorized to collect plant specimens by Forestry and grassland Bureau of Dali Bai Autonomous Prefecture.