Leaves of Bidens segetum (Asteraceae) were collected in March 2017 (Figure 1). The specimens were obtained from plants grown in beds at the Instituto de

Botânica-SP (Atlantic Forest domain) (Figure 2) from seeds from a wild population of B. segetum, brought from the Biological Reserve and Experimental Station of Mogi-Guaçu (Cerrado domain) São Paulo State, Brazil. The botanical identity of the plant material was confirmed by Dr. Inês Cordeiro (Center for Research in Vascular Plants, Instituto de Botânica, São Paulo, Brazil). A voucher specimen (Nascimento 452794-SP) was deposited at the Herbarium Maria Eneyda P. Kaufmann Fidalgo (SP), São Paulo, Brazil.

Extraction

Crude ethanolic extract (EEBs. 123.284 g, 23% yield) was obtained from fresh leaves (1.345 kg), frozen and lyophilized (485 g, 27%) by exhaustive extraction (6 days), ethanol 93˚ (485 g∙6 L⁻¹) at room temperature, filtration, concentration under reduced (Büchi^® rotary evaporator) pressure and drying in a water bath 40˚C.

Bio-guided fractionation and Analyses

EEBs (45.0 g) was performed by flash chromatography in vacuum system on column (silica gel 60 g, Merck 200 - 500 mµ) and gradient system with the solvents: hexane (100%); hexane + ethyl acetate 5:5 (v:v); ethyl acetate (100%); methanol + ethyl acetate 5:5 (v:v); methanol (100%) methanol + H₂O 2:8 (v:v). The ethyl acetate + methanol (FAcEOt + MeOH; 35% yield) active fraction on the DPPH assay was solubilized in MeOH (10 mL) and fractionated by exclusion liquid chromatography on a 25 cm open top chromatographic column in length and 5 cm in diameter prepared with Sephadex LH 20 (35 g, Pharmacia) and 150 mL MeOH (Merck PA) and eluted with 1400 mL MeOH (Merck PA) yielding 47 subfractions (AM1-AM47). The AM17-AM23 active subfractions were pooled and fractionated by reverse phase chromatography (SPE Discovery DSC-18 Tube, 10 g, 60 mL, SUPELCO®) with gradient solvent: 100 mL Milli-Q® H₂O, 100 mL Milli-Q® H₂O + MeOH (8:2, v:v), 100 mL Milli-Q® H₂O + MeOH (5:5, v:v) and 100 mL 100% MeOH and were obtained seven new subfractions. The FFR3 (23.6 mg) was fractionated by preparative thin layer chromatography (PTLC, 60 F₂₅₄, silica gel, 1 mm, Merck, Darmstadt, Germany) furnishing three active fractions (DPPH): PFFR3.1 (Rf = 0.36); PFFR3.2 (Rf = 0.63 and 0.48) and PFFR3.3 Rf =

0.36) with solvent system (BAW):n-Butanol:acetic acid: water (4:1:5, upper phase). All fraction was analyzed by HPLC-DAD.

Another part of the EEBs (75.0 g) was suspended in Milli-Q^® water and fractionated by liquid-liquid partition with solvents: hexane (Hex) and ethyl acetate, (FAcEOt) and was fractionated by preparative thin layer chromatography PTLC on 60 F₂₅₄ silica gel (1 mm; Merck, Darmstadt, Germany), eluted with 8:2 (v:v) CHCl₃: MeOH furnished the active PP4 subfraction that inhibits the growth of the spores of the Cladosporium sphaerospermum and Cladosporium cladosporioides fungi by bioautographic assay.

Analytical HPLC-DAD and semi-preparative HPLC-DAD

Analytical scale HPLC-DAD was performed on an Agilent model 1260 chromatograph consisting of a G1316A thermostatic furnace, a G1329B automatic injector, a G1330B thermostatic sample compartment, a G1311B pump equipped with a spectrum scan detector. Ultraviolet by arrangement of 60 mm flow cell photodiodes. The stationary phase for analytical scale analyzes was carried out using a reverse phase C₁₈ Zorbax Eclipse plus column (4.6 × 150 mm) with 3.5 µm particle diameter and a flow rate of 1.0 mL∙min⁻¹. The elution system employed was the gradient mode initiated and consisted of a mixture of 75% acidified H₂O with 0.1% acetic acid and 25% acetonitrile (ACN) for 2 min, from 2 to 7 min reaching 50% of ACN, from 7 to 25 min reaching 90% ACN, from 25 to 26 min 100% ACN, which was held for one more minute.

Semi-preparative scale HPLC-DAD was performed on Agilent model 1200 chromatograph and a C₁₈ reverse phase Zorbax eclipse plus LC-18 column (25 cm × 10 mm) with 5 µm diameter particles and a flow rate of 4.0 mL∙min⁻¹. The elution system employed was the same as that used in the analytical scale HPLC. All solvents used were HPLC grade (T. J. Baker).

LC-DAD-MS/MS/ESI⁺ and NMR

Analytical LC-DAD-MS/MS/ESI⁺ spectra the PP4 was performed on Shimadzu model CBM-20A chromatograph, pumps: LC-20AD, with detector: SPD-20A-Oven: CTO-20A and autoinjector: SIL 20AC (Shimadzu) and Esquire 3000 plus—Bruker Daltonics mass spectrometer, with 4000 V capillary, 27 Psi nebulizer, 300˚C and 7 L∙min⁻¹ gas flow. Operating in MS and MS/MS data acquisition mode with electron spray source in positive mode (ESI⁺). Subfraction PP4 (5mg) obtained from EEBs was solubilized in MeOH (Merck, PA). Chromatography conditions. Phenomenex Luna C18 column (250 × 4.6 mm − 5 um). The mobile phase was solvent A: H₂O acidifies with 0.1% formic acid and solvent B acetonitrile (ACN, HPLC grade). The solvent system was isocratic as follows: 0 min 95% A and 5% B, 50 min 0% A, 100% B. The flow rate was 1 ml∙min⁻¹. Temperature 40˚C and injection volume: 10 μL∙min⁻¹ (1 mg∙mL⁻¹). The chromatograms were monitored at 315 nm and 250 nm and retention times (Rt) detected. The TIC (Total ions chromatographic) were analyzed based on ion of mass/charge (m/z) of the [M + H]⁺ Dalton unit (Da) detected in the MS¹ spectrum. The fragment ion 100% it’s chromatography peak from (MS²) spectrum of major relative abundance.

NMR spectra of PP4 were performed on Bruker III 500 MHz spectrometer. PP4 in deuterated chloroform (CDCl₃) was analyzed by ¹H NMR and bidimensional HSQC and HMBC (http://ca.iq.usp.br/novo/).

Bioautographic Assay

Strains used in the antifungal assays belonged to C. sphaerospermum Penzig and C. cladosporioides (Fresen) de Vries, from the mycology collection of Instituto de Botânica, São Paulo, Brazil (CCIBt 491; CCIBt140). To obtain spore solutions for the bioautographic assay, C. sphaerospermum and C. cladosporioides were maintained on plates with potato-dextrose-agar (PDA) medium, incubated at 27˚C in the dark for 14 days. Conidial suspensions of fungi were obtained in salt and glucose solution prepared as follows: a stock solution contains 8.4 g KH₂PO₄; 2.4 g Na₂HPO₄ + 2H₂O; 4.8 g KNO₃; 1.2 g MgSO₄, 7H₂O; 1.2 g NaCl per 1200 mL of distilled water. The solution is homogenized at 120˚C for 20 min. Just before making the conidial suspension 10 mL of a 30% aqueous solution of glucose is added per 60 ml of this solution. The conidial suspension is stored in a freezer.

The antifungal activity of the extracts and subfractions was evaluated by qualitative bioautographic method on TLC [29]. Cladosporium sphaerospermum and C. cladosporioides were used in bioassays. For this assessment, samples were solubilized separately in methanol, and aliquots of 200 µg of samples were applied to silica gel 60 F₂₅₄ (0.2 mm; Merck, Darmstadt Germany) TLC and eluted in the solvent system CHCl₃: MeOH (9:1 v:v), for about 1 h, using nystatin standard and cinnamic acid (Sigma-Aldrich) as positive control (1 µg). The TLC plates were sprayed separately with the conidia fungi suspension of each species (>5 × 10⁷ conidia mL⁻¹) and incubated in a moist chamber at 27˚C for 48 h in darkness. A clear inhibition zone appeared against a dark background, indicating the presence of fungitoxic compounds since the dark background is due to fungal growth, and the lack of growth indicates fungicidal activities. Retention factor values (Rf) of the spot are determined for each inhibition zone observed. Each bioautography was repeated three times for each of the fungi tested and photographed in the Camag System—Repostar 3.

DPPH free radical scavenging activity

This assay was performed by 2,2-diphenyl-1-picrylhydrazyl (DPPH) stable free radical photocolorimetry method [30] [31]. Aliquots of 100 µg the PFRR3.3 subfraction and the 5-CQA standard (1 mg∙mL⁻¹, Sigma-Aldrich) were analyzed by TLC eluting with the upper phase of BAW (n-butanol: glacial acetic acid: H₂O 4:1:5, v:v). The plates were sprayed with a methanolic solution of the 2,2-diphenyl-1-picrylhydrazyl radical (0.2%—DPPH). After approximately 30 min white spots appeared under a purple background indicating that the DPPH radical was active in free radical DPPH scavenging. Chromatography profile was visualized under white light (Camag System—Repostar 3) and the retention factor (Rf) calculated. The active PFFR3.3 subfraction and 5-CQA standard (Sigma-Aldrich) by DPPH assay were quantified in 96-well microplate in triplicate (KC4-Bio-Tek Instrument INC., USA). For this purpose, 70 µL of methanol solution of DPPH (0.3 mM) and 178.5 µL of the sample (concentrations of 25, 50, 100, 150, 200, 250, 300 µg∙mL⁻¹) and authentic standard 5-CQA to determine the percentage of purple-colored DPPH free radical scavenger absorbing at 518 nm. IC₅₀ determination was calculated using the GraphPad Prims 5 program.

Cell Culture

The human melanocyte cell line (NGM) was acquired from the Rio de Janeiro Cell Bank (code BCRJ 0190) and was grown in DMEMf12 medium (Thermofisher, Carlsbad, CA) supplemented with20@ fetal bovine serum (Invitrogen, Scotland, UK), 2 mM glutamine, 1.4 µM hydrocortisone, 1 nM T3 hormone, 10 µg∙mL⁻¹ insulin (Sigma), 10 µg∙mL⁻¹ transferrin and 10 ng∙mL⁻¹ epidermal growth factor. Human melanoma lineages corresponding to different stages of tumor progression: radial growth melanoma (Wm1552), vertical growth melanoma (Wm1366) and metastatic (Lu1205) cell lines were kindly provided by Dr. Meenhard Merley from Institute Wistar (https://wistar.org/our-scientists/meenhard-herlyn) were cultured in 20% Leibovitz medium (GIBCO, Carlsbad, CA) at pH 7.2 plus 80% MCD153 medium (Sigma) supplemented with 2% fetal bovine serum and 1.68 mM CaCl₂. The cultures were kept in incubator at 37˚C in a humidified atmosphere containing 5% CO₂.

Dihydroethidium (DHE) antioxidant activity in melanoma and melanocyte cells

Intracellular superoxide anion (O⁻) amount was measured using dihydroethidium (DHE; Molecular Probes, Eugene, OR, USA), a non-fluorescent cell permeable indicator for superoxide anion and analyzed by fluorometric assay. Melanocytes and human melanoma cell lines Wm1552, Wm1366 and Lu1205 were treated or not (control) with 0.5, 1.0, 10 and 100 µg∙mL⁻¹ of PFFR3.3 and PP4 subfractions for 5, 15 and 30 min. Then, medium containing the treatments was removed, cells were washed with phosphate-buffered saline (PBS) and incubated with 25 µm DHE for 40 min at 37˚C in the dark. After washing, fluorescence was evaluated in Spectromaxi3 (Molecular Devices) (excitation wavelength 480 nm; emission wavelength 567 nm).

To evaluate the results, we relied on Student’s t-test for two-group experiments and analysis of variance (factorial ANOVA) with Dunnett’s post-test for experiments with three or more groups using the GraphPad Prism 7.0^® statistical software (GraphPad, San Diego, CA). The significance level was established at p < 0.05.