key: cord-260392-hj9s5cnu authors: Lin, Peng; Ng, Tzi Bun title: A novel and exploitable antifungal peptide from kale (Brassica alboglabra) seeds date: 2008-05-30 journal: Peptides DOI: 10.1016/j.peptides.2008.05.020 sha: doc_id: 260392 cord_uid: hj9s5cnu The aim of this study was to purify and characterize antifungal peptides from kale seeds in view of the paucity of information on antifungal peptides from the family Brassicaceae, and to compare its characteristics with those of published Brassica antifungal peptides. A 5907-Da antifungal peptide was isolated from kale seeds. The isolation procedure comprised affinity chromatography on Affi-gel blue gel, ion exchange chromatography on SP-Sepharose and Mono S, and gel filtration on Superdex Peptide. The peptide was adsorbed on the first three chromatographic media. It inhibited mycelial growth in a number of fungal species including Fusarium oxysporum, Helminthosporium maydis, Mycosphaerella arachidicola and Valsa mali, with an IC(50) of 4.3 μM, 2.1 μM, 2.4 μM, and 0.15 μM, respectively and exhibited pronounced thermostability and pH stability. It inhibited proliferation of hepatoma (HepG2) and breast cancer (MCF7) cells with an IC(50) of 2.7 μM and 3.4 μM, and the activity of HIV-1 reverse transcriptase with an IC(50) of 4.9 μM. Its N-terminal sequence differed from those of antifungal proteins which have been reported to date. Antifungal proteins are a family of proteins employed to combat pathogenic fungi which can cause diseases in plants and animals. Those proteins have been purified from a diversity of flowering plants [8, [30] [31] [32] [33] 36, 37] , animals [3, 28] , bacteria [39] , and fungi [34, 35] . Plant tissues that produce antifungal proteins and peptides comprise seeds [1, 2, 4, 6, 11, 30, 31, 36] , bulbs [7, 32] , leaves [10, 13] , tubers [9] , fruits [33] , shoots [13] , and roots [12] . Monocots [4, 6, 11, 13, 14, 25, 32, 37] , dicots [9, 15, 16, 17, 24, 29, 33, 36, 38, 40] , and gymnosperms [10, 30] have been reported to produce antifungal proteins. Plant antifungal proteins are classified, based on structure or activity, into various types [26] . The different types include chitinases and chitinase-like proteins [29] , chitin-binding proteins [2, 10] , lipid transfer proteins [16, 17] , protease inhibitors [11, 40] , ribosome inactivating proteins [14, 24] , embryo abundant protein-like proteins [30] , thaumatin-like proteins [33] , and defensin-like peptides [38] . To date, only one antifungal peptide has been reported from Brassica campestris seeds [16, 17] in spite of the presence of multiple Brassica species. In new of the structural diversity manifested by the various aforementioned antifungal proteins and the presence of different antifungal proteins even in the same species [9, 29] , the intent of the present investigation was to isolate an antifungal peptide from the seeds of kale (Brassica alboglabra L.H. Bailey), another Brassica species, and to compare it with the antifungal peptide from B. campestris seeds [16] and other plant antifungal proteins. Protein concentration was determined by the dye-binding method (Bio-Red) using bovine serum albumin as a standard. Tricine-sodium dodecyl sulfate-polyacrylamide gel electrophoresis (tricine-SDS-PAGE) It was conducted according to the method of Schagger and von Jagow [27] . After electrophoresis using 18% acrylamide gel, the gel was stained with Coomassie Brilliant Blue. The molecular mass of the isolated antifungal peptide was determined by comparison of its electrophoretic mobility with those of , the extract of kale seeds was applied on an Affi-gel Blue gel column (5 cm T 20 cm). Unadsorbed proteins (fraction BG1) were eluted with the same buffer while adsorbed proteins (fraction BG2) were eluted with 10 mM Tris-HCl buffer (pH 7.8) containing 1 M NaCl as indicated by the arrows. In (B), fraction BG2 from the Affi-gel Blue gel column was dialyzed and applied on an SP-Sepharose column (2.5 cm T 20 cm) in 10 mM NH 4 OAc buffer (pH 4.5). After elution of unadsorbed proteins, the column was eluted stepwise with 0.2 M NaCl, 0.5 M NaCl and then with 1 M NaCl added to the buffer as indicated by the arrows. In (C), fraction SP2 from the SP-Sepharose column was loaded on a 1-ml Mono S column. Following elution of unadsorbed proteins with 10 mM NH 4 OAc buffer (pH 4.5), adsorbed proteins were eluted sequentially, first with a 0-0.4 M NaCl gradient and then with a 0.4-0.7 M and 0.7-1 M NaCl gradient. In (D), fraction S2 from the Mono S column was subjected to gel filtration on a Superdex Peptide HR 10/30 column in 10 mM NH 4 Mass spectrometric (MS) analysis of the antifungal peptide was performed on a Finnigan LCQ-MS, an instrument that essentially consists of an atmospheric pressure electrospray positive-ion source, attached to a triple-quadrupole mass analyzer. The purified peptide (100 pmol) was dissolved in water/methanol (50:50, v/v) containing 1% (v/v) acetic acid at a protein concentration of 5 mmol/l, and then applied on the MS instrument [16] . The N-terminal amino acid sequence of the purified peptide was performed by Edman degradation using a Hewlett-Packard amino acid sequencer [30] . The assay for antifungal activity was executed using 100 mm  15 mm petri plates containing 10 ml of potato dextrose agar. The fungal species tested included the following: Fusarium oxysporum, Helminthosporium maydis, Mycosphaerella arachidicola and Valsa mali. After the mycelial colony had developed, sterile blank paper disks (0.625 cm in diameter) were placed around and at a distance of 1 cm away from the rim of mycelial colony. An aliquot (8 ml containing 60 mg or 300 mg) of the purified peptide in 20 mM PBS buffer (pH 6.0) was introduced to a disk. The plates were incubated at 23 8C for 72 h until mycelial growth had enveloped peripheral disks containing the control (buffer) and had produced crescents of inhibition around disks containing samples with antifungal activity. To determine the IC 50 value for the antifungal activity of the isolated antifungal peptide, four doses of the peptide were added separately to four aliquots each containing 4 mil potato dextrose agar at 45 8C, mixed rapidly and poured into four separate small Petri dishes. After the agar had cooled down, a small amount of mycelia, the same amount to each plate was added. Buffer only without antifungal peptide served as a control. After incubation at 23 8C for 72 h, the area of the mycelial colony was measured and the inhibition of fungal growth determined. Inhibition of fungal growth = % reduction in area of mycelial colony = [(area of mycelial colony in absence of antifungal peptide À area in presence of antifungal peptide)/area in absence of antifungal peptide]  100%. A graph plotting % reduction in area of mycelial colony caused by antifungal peptide against the concentration of antifungal peptide was then plotted. The concentration of the isolated antifungal peptide that brought about 50% reduction in the area of mycelial colony is the IC 50 [30] . To investigate the thermal (0-100 8C) stability, pH (0-3 and 10-14) stability and effects of ions, the isolated antifungal peptide was pretreated accordingly and the antifungal assay was then conducted as mentioned above. A solution of the isolated antifungal peptide (1 mg/ml) was incubated with an equal volume of trypsin or pepsin (1 mg/ml) Only the kale and B. campestris antifungal peptides [17] exhibit antifungal activity. The remaining two proteins [5, 21] manifest trypsin inhibitory activity. The napin-like polypeptide also possesses antibacterial and antiproliferative activities [21] . p e p t i d e s 2 9 ( 2 0 0 8 ) 1 6 6 4 -1 6 7 1 at 37 8C for 1 h. At the end of the incubation, the reaction mixture was examined for antifungal activity. Breast cancer MCF-7 cell line and hepatoma HepG2 cell line were suspended in RPMI medium and adjusted to a cell density of 2  10 4 cells/ml. A 100 ml aliquot of this cell suspension was seeded to a well of a 96-well plate, followed by incubation for 24 h. Different concentrations of the antifungal peptide in 100 ml complete RPMI medium were then added to the wells and incubated for 72 h. After 72 h, 20 ml of 5 mg/ml [3-[4,5-dimethylthiazol-2-yl]-2,5-diphenyltetrazolium bromide] [MTT] in phosphate buffered saline was spiked into each well and the plates were incubated for 4 h. The plates were then centrifuged at 324  g for 5 min. The supernatant was carefully removed, and 150 ml of dimethyl sulfoxide was added in each well to dissolve the MTT-formazan at the bottom of the wells. After 10 min, the absorbance at 590 nm was measured by using a microplate reader [38] . The assay for HIV reverse transcriptase inhibitory activity was carried out according to instructions supplied with the assay kit from Boehringer Mannhein (Germany). The assay takes advantage of the ability of reverse transcriptase to synthesize DNA, starting from the template/primer hybrid poly (A) oligo (dT) 15. The digoxigenin-and biotin-labeled nucleotides in an optimized ratio are incorporated into one of the same DNA molecule, which is freshly synthesized by the reverse transcriptase (RT). The detection and quantification of synthesized DNA as a parameter for RT activity follows a sandwich ELISA protocol. Biotin-labeled DNA binds to the surface of microtiter plate modules that have been precoated with streptavidin. In the next step, an antibody to digoxigenin, conjugated to peroxidase, binds to the digoxigeninlabeled DNA. In the final step, the peroxidase substrate is added. The peroxidase enzyme catalyzes the cleavage of the substrate, producing a colored reaction product. The absorbance of the sample at 405 nm can be determined using a microtiter plate (ELISA) reader and is directly correlated to the level of RT activity. A fixed amount (4-6 ng) of recombinant HIV-1 reverse transcriptase was used. The inhibitory activity of the antifungal peptide was calculated as percent inhibition as compared to a control without the antifungal peptide [32, 33] . Assay of ability to inhibit HIV-1 integrase The assay was conducted as described in Ref. [19] . The ribosome inactivating protein trichosanthin was used as a positive control [19] . Screening for inhibitory effect on severe acute respiratory syndrome (SARS) coronavious (CoV) protease The assay was conducted as described by Leung et al. [15] . Trypsin activity was determined by using N-a-benzoyl-Larginine ethyl ester hydrochloride (BAEE) as the substrate. A similar assay was conducted using casein as substrate instead of BAEE [22, 23, 40 ]. The assay was carried out as described earlier. Con A was used as positive control and bovine serum albumin as a negative control [38] . The crude extract was fractionated on Affi-gel blue gel into a larger unadsorbed fraction (BG1) eluted by the starting buffer and a smaller adsorbed fraction (BG2) eluted by starting buffer containing 1 M NaCl (Fig. 1A) . Antifungal activity resided only in fraction BG2, which was then resolved on SP-Sepharose into an unadsorbed fraction and three adsorbed fractions (SP1, SP2 and SP3) of approximately equal size which were desorbed with 0.2 M NaCl, 0.5 M NaCl and 1 M NaCl, respectively (Fig. 1B) . Antifungal activity was concentrated in fraction SP2. Fraction SP2 was separated on Mono S into a tiny unadsorbed fraction (S1) and two adsorbed fractions (S2 and S3) (Fig. 1C) . Antifungal activity was detected in the sharp adsorbed fraction S2 eluted soon after application of the 0.3-0.6 M NaCl gradient. Final purification of S2 on Superdex Peptide resulted in a major and a tiny absorbance peak, the former representing purified antifungal peptide (Fig. 1D ) with a molecular weight of 5.9 kDa in SDS-PAGE ( Fig. 2A ). Its molecular weight as determined by mass spectrometry was 5907 Da (Fig. 2B) . The yields of the chromatographic fractions with antifungal activity from 500 g seeds are as follows: crude extract (13765 mg), fraction BG2 (6648 mg), fraction SP2 (1023 mg), fraction S2 (342 mg) and purified antifungal peptide (32 mg). It differed from known Brassica antifungal proteins, napins and trypsin inhibitors in N-terminal sequence (Table 1) (Fig. 3) . The antifungal activity of the peptide was retained after exposure to temperatures in the range 20-80 8C for 10 min (Fig. 4A) and to the pH ranges 2-3 and 10-11 for 30 min (Fig. 4B) . It inhibited proliferation of HepG2 cells (Fig. 5A ) and MCF7 cells (Fig. 5B) with an IC 50 of 2.7 mM and 3.4 mM, respectively, and reduced the activity of HIV-1 reverse transcriptase with an IC 50 of 4.9 mM (Fig. 5C) . It was devoid of mitogenic activity, HIV-1 integrase inhibitory, and SARS proteinase inhibitory activities (data not shown). A 9-kDa nonspecific lipid transfer with antifungal activity has been isolated from B. campestris seeds [16] . The present study constitutes the second report on the isolation of an antifungal seeds did not exhibit trypsin inhibitory activity and also did not resemble B. napus trypsin inhibitor in N-terminal sequence. This is noteworthy in view of the fact that some of the trypsin inhibitors demonstrate antifungal activity [40] and that trypsin inhibitors and napins are produced by Brassica seeds. The two Brassica antifungal peptides were also isolated by using similar protocols. Ion exchange chromatography on Q-Sepharose, affinity chromatography on Affi-gel blue gel, ion exchange chromatography on Mono S, and gel filtration on Superdex Peptide were used for isolation of B. campestris antifungal peptide, the only difference from the present protocol for kale antifungal peptide being replacement of SP-Sepharose by Q-Sepharose. The antifungal peptide from kale seeds had a smaller molecular mass (5.9 kDa) than that (9 kDa) of B. campestris antifungal peptide. Its yield (64 mg/kg) was lower than that of B. campestris antifungal peptide (175 mg/kg) [16] . Its HIV-1 reverse transcriptase inhibitory activity (IC 50 = 4.9 mM) was similar to that of B. campestris antifungal peptide (IC 50 = 4 mM), but more potent than many anti-HIV-1 natural products [18] . Its antiproliferative activity toward HepG2 cells and MCF-7 cells (IC 50 = 2.7 mM and 3.4 mM, respectively) was also analo-gous to that of B. campestris antifungal peptide (IC 50 = 5.8 mM and 1.6 mM, respectively). Both kale and B. campestris antifungal peptide were devoid of mitogenic activity toward mouse splenocytes. It has previously been demonstrated that some [7, 38, 40] but not other [17] antifungal proteins/peptides exhibit mitogenic activity. Neither kale nor B. campestris antifungal peptide demonstrated HIV-1 integrase inhibitory and SARS proteinase inhibitory activities, in line with the observation on French bean defensin-like antifungal peptide [15] . Napin-like polypeptides with trypsin-inhibitory activity but devoid of antifungal activity have been purified from seeds of various Brassica species [20] [21] [22] [23] . A trypsin-inhibitor has also been isolated from Brassica napus seeds [5] . These proteins demonstrate N-terminal amino acid sequences distinctly different from those of the antifungal peptide from kale. The isolation of this antifungal peptide adds to the literature on proteins from Brassica seeds. The chromatographic behavior of kale antifungal peptide on ion exchanger and Affi-gel blue gel is similar to non-Brassica antifungal proteins [30] [31] [32] [33] [34] [35] [36] 38, 40] . Its molecular mass is similar to those of some antifungal peptides from non-Brassica plants [24, 30] . Its remarkable thermostability and pH stability resemble those of leguminous defensins [38] . Its broad spectrum of antifungal activity is interesting in view of the observation that shallot and asparagus antifungal proteins are activity toward only one out of several fungal species tested [31, 32] . The antifungal activity of kale antifungal peptide is more potent than that of the antifungal proteins [31, 32, 40] . Its potent antiproliferative and HIV-1 reverse transcriptase inhibitory activities are noteworthy since not all antifungal proteins have been reported to possess these potentially exploitable activities. In summary, the antifungal peptide isolated from kale (B. alboglabra L.H. Bailey) seeds has potentially exploitable activities such as stable and broad-spectrum antifungal activity, HIV-1 reverse transcriptase inhibitory activity and antiproliferative activity toward tumor cells. In contrast, some antifungal proteins like mungbean chitinase [17] lack the last two activities. There are very few reports on the presence of defense proteins such as antifungal proteins, antiviral proteins, antibacterial proteins and lectins from B. alboglabra except for the demonstration of a napin-like peptide with antiproliferative, antibacterial and translation-inhibitory activities [23] . The antifungal peptide isolated in this study would add to the existing literature. 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Ginkbilobin, a novel antifungal protein from Ginkgo biloba seeds with sequence similarity to embryo-abundant protein Isolation of a novel deoxyribonuclease with antifungal activity from Asparagus officinalis seeds Ascalin, a new antifungal peptide with human immunodeficiency virus type 1 reverse transcriptase inhibitory activity from shallot bulbs Isolation of an antifungal thaumatinlike protein from kiwi fruits Eryngin. a novel antifungal peptide from fruiting bodies of the edible mushroom Pleurotus eryngii Alveolarin. a novel antifungal polypeptide from the wild mushroom, Polyorus alveolaris Isolation of cucurmoschin, a novel antifungal peptide abundant in arginine, glutamate and glycine residues from black pumpkin seeds Pilot-scale purification of zeamatin, an antifungal protein from maize Gymnin, a potent defensin-like antifungal peptide from the Yunnan bean Gymnocladus chinensis Baill An antifungal protein from Escherichia coli A Bowman-Birk-type trypsinchymotrypsin inhibitor from broad beans We thank Miss Kathy Lau and Miss Grace Chan for excellent secretarial assistance.r e f e r e n c e s