- Email: [email protected]
In vitro antiviral activities of enzymatic hydrolysates extracted from byproducts of the Atlantic holothurian Cucumaria frondosa
Accepted Manuscript Title: IN VITRO ANTIVIRAL ACTIVITIES OF ENZYMATIC HYDROLYSATES EXTRACTED FROM BYPRODUCTS OF THE ATLANTIC HOLOTHURIAN CUCUMARIA FRONDOSA Author: Ludovic Tripoteau Gilles Bedoux Jacques Gagnon Nathalie Bourgougnon PII: DOI: Reference:
S1359-5113(15)00102-6 http://dx.doi.org/doi:10.1016/j.procbio.2015.02.012 PRBI 10360
To appear in:
Process Biochemistry
Received date: Revised date: Accepted date:
15-12-2014 10-2-2015 23-2-2015
Please cite this article as: Tripoteau L, Bedoux G, Gagnon J, Bourgougnon N, IN VITRO ANTIVIRAL ACTIVITIES OF ENZYMATIC HYDROLYSATES EXTRACTED FROM byproducts OF THE ATLANTIC HOLOTHURIAN CUCUMARIA FRONDOSA, Process Biochemistry (2015), http://dx.doi.org/10.1016/j.procbio.2015.02.012 This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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IN VITRO ANTIVIRAL ACTIVITIES OF ENZYMATIC HYDROLYSATES EXTRACTED FROM
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BYPRODUCTS OF THE ATLANTIC HOLOTHURIAN CUCUMARIA FRONDOSA
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Ludovic TRIPOTEAU
a,b
a
b
*, Gilles Bedoux , Jacques Gagnon , Nathalie Bourgougnon
a,
4 a. Laboratoire de Biotechnologie et Chimie Marines, EA3884, UBS, IUEM, F-56000 Vannes, France.
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b. Coastal Zones Research Institute Inc., Shippagan, New Brunswick, CANADA
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Highlights: -
Bioactive compounds were extracted from aquapharyngeal bulb of Cucumaria frondosa
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Enzymatic extraction permitted the recovery of antiherpetic compounds on our model
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Antiherpetic activities were highlighted on enzymatic hydrolysates of aquapharyngeal bulb
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High molecular weight molecules were demonstrated as active against HSV-1
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IN VITRO ANTIVIRAL ACTIVITIES OF ENZYMATIC HYDROLYSATES EXTRACTED FROM
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BYPRODUCTS OF THE ATLANTIC HOLOTHURIAN CUCUMARIA FRONDOSA
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Ludovic TRIPOTEAU
a,b
a
b
*, Gilles Bedoux , Jacques Gagnon , Nathalie Bourgougnon
a,
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20 a. Laboratoire de Biotechnologie et Chimie Marines, EA3884, UBS, IUEM, F-56000 Vannes, France.
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b. Coastal Zones Research Institute Inc., Shippagan, New Brunswick, CANADA
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23 *Corresponding author: Ludovic Tripoteau
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LBCM, Centre de recherche Yves Coppens. Campus de Tohannic – BP 573, 56017 Vannes Cedex. France.
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Tel.: +33 2 97 01 71 22
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E-mail address: [email protected]
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28 Pr. Nathalie Bourgougnon.
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LBCM, Centre de recherche Yves Coppens. Campus de Tohannic – BP 573, 56017 Vannes Cedex. France.
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Tel.: +33 2 97 01 71 55
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E-mail address: [email protected]
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Dr. Jacques Gagnon
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CZRI, PPM. 232B, avenue de l’église, Shippagan, NB, E8S 1J2 Canada
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Tel.: 1 506 336 6603
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E-mail address: [email protected]
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Dr. Gilles Bedoux
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LBCM, Centre de recherche Yves Coppens. Campus de Tohannic – BP 573, 56017 Vannes Cedex. France.
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Tel.: +33 2 97 01 71 57
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E-mail address: [email protected]
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ABSTRACT
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Herpes Simplex virus 1 (HSV-1), responsible for the common cold sore, can also lead to serious infections in immunocompromised people. Current antiviral chemotherapies face obstacles including
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the toxicity of therapeutic molecules, interference with normal cellular metabolism, genetic variability
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and the incurable nature of latent infections. Therefore, the search for new treatments is a public
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health issue. Marine invertebrates have held great potential for finding novel antiviral compounds.
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Little is known, about the antiviral activities of compounds isolated from holothurians. In New
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Brunswick, holothurian is fished for its edible bodywall and muscle, but its processing generates high
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amounts of byproducts. In vitro evaluation of the anti-HSV-1 activity by cell viability was performed on
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nine hydrolysates obtained by enzyme-assisted extraction and four solvent extractions from
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aquapharyngeal bulb and internal organs of Cucumaria frondosa at an MOI of 0.001 ID50/cells. After
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72 h, four enzymatic hydrolysates from the aquapharyngeal bulb presented effective antiherpetic
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activities (EC50=7.2–15.2 µg/mL) . After evaluation at a higher MOI (0.01 ID50/cells), the most efficient
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extract (Papain hydrolysate) was fractionated to identify the active fraction. The fraction superior to
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100 kDa showed the highest antiherpetic activity (EC50: 18.2 µg/mL). In conclusion, upgrading
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byproducts of sea cucumber fisheries offers new sources of bioactive molecules.
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Key words: Cucumaria frondosa; enzymatic hydrolysis; Herpes simplex virus type 1; byproducts.
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1. INTRODUCTION
64 Sea cucumbers are benthic marine invertebrates. Of the 1200 species living worldwide, over 60
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are known to be harvested for human consumption [1]. One of the species that is considered new on
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the market is the orange-footed sea cucumber Cucumaria frondosa (Gunnerus, 1767), which is
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approximately 25–30 cm long and can reach 50 cm when relaxed. The Atlantic sea cucumber
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Cucumaria frondosa is distributed abundantly in the north Atlantic from tide pools of the lower intertidal
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zone and to down to 300 m depth [2].
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Cucumaria frondosa is harvested in the Fundy Bay, New Brunswick (NB), Canada to be then
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transformed for the human consumption. The processing plant generates discards representing more
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than half of the total amount of raw matter (600 t). The waste is mainly used as fish meal or fish oil.
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Internal muscle bands and the dried body wall are the products from C. frondosa sold on Asian food
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markets. The rest of the sea cucumbers, comprising the aquapharyngeal bulb, gut, gonad, and
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respiratory tree, considered as byproducts, is rejected or underused. This biomass holds, however,
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considerable potential to generate new biological compounds and can be turned into a commercially
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viable business [3-4]. The process of enzymatic hydrolysis has been developed in order to transform
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marine byproducts into marketable forms. By the use of specific enzymes, this process has the ability
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to enhance the extraction of specific molecules with new properties (functional, biological, aromatic).
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Consequently, the action of proteases on marine byproducts rich in proteins may lead to the
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production of peptides, polypeptides and proteins with various biological activities [3].
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Sea cucumbers are a rich source of vitamins, minerals and bioactive components [5]. They are
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used as healthy foods, traditional medicines and dietary supplements. For example, they have been
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used for centuries, especially in Asia, as tonic foods and used in folk medicine to treat various ailments
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[6]. Dried forms of sea cucumber are used as dietary supplements. More recently, sea cucumbers
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have received increased attention because of their bioactive compounds such as triterpene glycosides
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[7-9], chondroitin sulfates [10], sulfated polysaccharides [11], sterols [12], phenolics [13], peptides [14],
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cerebrosides [15], and lectins [16].
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Several studies conducted on holothurians have shown antifungal [17-19] and antibacterial [14; 20-22] activities. Little is known about antiviral activities [23-27], especially regarding Herpes Simplex
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Virus 1 (HSV-1) [28-31]. Herpes simplex Virus, a DNA enveloped virus, is a common human pathogen
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with between 60 and up to 95% of certain populations infected with HSV-1, and between 6 and 50%
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infected with Herpes Simplex Virus type 2 (HSV-2). The frequency of HSV-seropositive males was
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significantly higher in populations infected with Human Immunodeficiency Virus (HIV). As the HIV
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disease progresses, cutaneous and mucosal complications become more severe and occur in up to
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92% of HIV-infected individuals. Medications available for systemic treatment of HSV are acyclovir,
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famciclovir and valacyclovir. Acyclovir and penciclovir are available for topical use. In clinical practice,
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treatment of primary HSV infections, while relieving symptoms and reducing the duration of viral
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shedding, does not prevent recurrences. Moreover, resistance to acyclovir has been reported in
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immuno-compromised patients. Therefore, there was a need to develop new therapeutic agents for
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the management of HSV infections. Moreover, the majority of commercially effective molecules are
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expected to join the public domain in 2015. The search for new treatments is therefore a major public
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health issue.
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The purpose of this study was to evaluate the in vitro antiherpetic activities of compounds
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obtained after enzyme-assisted extraction and solvent extractions of Cucumaria frondosa
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(Dendrochirotida, Cucumariidae) byproducts with a bioguided fractionation.
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2. MATERIALS AND METHODS
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2.1 Specimen collection
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2.2 Sample processing
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Specimens of Cucumaria frondosa were collected in Passamaquoddy Bay, Bay of Fundy, New
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Brunswick, Canada, between January and March 2012. Sea cucumbers (15-30 cm) were placed for
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acclimation at the Aquaculture Pavilion and Aquaculture Laboratories of the Coastal Zones Research
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Institute, Shippagan, New Brunswick, in 900L aerated tanks supplied with filtered seawater (4°C)
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pumped from Shippagan’s bay, prior to experiments.
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Specimens were sacrificed, then the aquapharyngeal bulb (A.B.) and internal organs (I.O.)
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were removed from the rest of the sea cucumbers to be separately crushed with a blender (LBC 15,
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Waring Laboratory Science, USA) and placed at -20°C prior to further treatments. Some of these
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samples were freeze-dried and placed in a labeled glass vial at -20ºC prior to the sequential solvent
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extraction.
123 Aqueous extraction assisted by enzymatic hydrolysis
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For each enzymatic hydrolysis, 1.5 kg of ground biomass was placed in a bioreactor (BioFlo
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110, New Brunswick Scientific, USA) with 1.5 L of distilled water. Nine different proteases were
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separately used: Alcalase (0.1%, w/w ; Alcalase® 2.4L FG, Novozymes AS, Denmark) with a
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declared activity of 2.4 AU/g (Anson Unit), Bromelain (0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a
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declared activity of 2000 GDU/g (Gelatin-Digesting Unit), Flavourzyme (0.1%, w/w ; Flavourzyme®
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Novozymes AS, Denmark) with a declared activity of 500 LAPU/g (Leucine Amino Peptidase Unit),
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Fungal Protease (0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a declared activity of 400 000 HU/g
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(Hemoglobin Unit), Neutral Protease (0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a declared activity of
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2 000 000 PC/g (Proteolytic unit), Papain (0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a declared activity
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of 6500 NFPU/g (Nuclear Floating Power Unit), Peptidase AM (Peptidase Aspergillus Melleus ; 0.1%,
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w/w ; Bio-Cat, Troy, VA, USA) with a declared activity of 500 LAPU/g, Peptidase AO (Peptidase
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Aspergillus Oryzae ; 0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a declared activity of 500 LAPU/g and
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Protamex (0.1%, w/w ; Protamex® Novozymes AS, Denmark) with a declared activity of 1.5 AU/g
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during 6 h at pH 8.0 and 50°C. After hydrolysis, enzymes were then inactivated at 90°C for 15 min and
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hydrolysates were centrifuged at 10,000xg for 20 min at 4°C to separate undigested residues and
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solubilized compounds. The supernatants were sampled, freeze-dried and stored at -20°C prior to
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cytotoxicity and antiviral evaluation [14]. The enzymatic hydrolysis process is summarized in Figure 1.
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Sequential solvent extraction
Hexane (OmniSolv® Hexanes), acetone (OmniSolv® Acetone) and methanol (OmniSolv®
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Methanol) are HPLC grade and were provided by Fisher Scientific (Canada). The sequential solvent
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extraction is summarized in Figure 2.
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Hexane extraction: 20 g of freeze-dried sample of raw matter were first submitted to hexane
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extraction into a 500 mL Erlenmeyer flask, and 300 mL (15 mL/g) of hexane was added. The sample
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was placed on a stir-plate, stirred for 30 min at room temperature and then placed in a sonicator for 15
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min. After filtration (Filter grade #4; Aldrich, Canada), the soluble part and the first residue (R1) were
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separately collected. The solvent was removed from the filtrate using reduced pressure on the rotary
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evaporator. The remaining solvent was removed by N2 stream in the heating block (40-50°C). The
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filtrate was then freeze-dried and placed in a labeled glass vial at -20ºC prior to cytotoxicity and
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antiviral evaluation.
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using the same procedure according to the sequential solvent extraction described in Figure 2.
For hexane, acetone, and methanol extraction, extractions were repeated twice and the
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Acetone extraction of R1 and methanol extraction of the second residue (R2) were carried out
fractions obtained were pooled.
Water extraction: The dried filtered residue from methanol extraction (R3) was placed into a
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500 mL Erlenmeyer flask; 200 mL of deionized water (10 mL/g) was added, and the mixture was
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placed on a heating plate and heated to 80-90°C while being stirred. Once the temperature range was
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reached, it was kept for 2 h. The mixture was removed from heat, cooled to room temperature, and
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filtered by vacuum filtration. The filtrate was precipitate using ethanol (3V). After ethanol addition, the
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flask was placed in an ice bath for 2 h. Once fully precipitated, the solids were separated by
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centrifugation (2500 rpm /20 min). Solids were then freeze-dried and stored in a labeled glass vial at -
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20°C prior to cytotoxicity and antiviral evaluation. The final residue was not included in the library of
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extracts due to its low solubility.
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Library of extracts
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All the extractions carried out on C. frondosa byproducts represented twenty eight different
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extracts. For one type of byproduct, there were nine enzymatic hydrolysates, four extracts by
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sequential solvent extraction (hexane, acetone, methanol and water extract) and one byproduct
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without treatment (control).
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2.3 Virus and cell lines
African green monkey kidney cells (Vero cell line n°ATCC CCL81) were grown in Eagle's
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Minimum Essential Medium (MEM, Laboratory Eurobio, France) supplemented with 8% (v/v) fetal calf
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serum (FCS, Eurobio, France), to which 1% (v/v) of PCS (penicillin 10 000U, colimycin 25 000 U,
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streptomycin 10 mg, Sigma, France) was added. Cells were routinely passaged every 3 days.
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Virus stock of Herpes Simplex Virus type 1 was obtained from Pr. Agut, Laboratoire de
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Dynamique, épidémiologie et traitement des infections virales de la Pitié Salpêtrière (Paris, France).
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The virus stock was prepared by incubating Vero monolayers (75 cm culture flasks seeded with 350
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000 cells / mL) at low multiplicity and incubating at 37°C, in a 95% air, 5% CO2 (v/v) atmosphere. Two
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or three days after infection, the cultures were frozen and thawed twice before clearing the preparation
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by centrifugation at low speed to remove cell debris. The resulting supernatant aliquot was stored at -
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80°C until used. Virus titrations were performed by the Reed and Muench dilution method [32], using
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10 wells on 96-wells microtiter plates per dilution. The virus titer was estimated from cytopathogenicity
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and expressed as 50% infectious doses / mL (ID50/mL). The virus titer was evaluated at 2.10
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ID50/mL.
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2.4 Cytotoxicity and antiviral activity of drugs by neutral red dye method
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Screening for antiviral activities of the library of extracts
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Dilutions of samples (50 µL) were prepared in Eagle’s MEM supplemented with 8% FCS and
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distributed into the well plates of a 96-well microtest III tissue culture plate (Nunclon, Intermed,
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France). A series included 10 assays ranging from extreme concentrations of extracts of 0.25 up to
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250.00 µg/mL (4 wells/concentration). One hundred microliters of cellular suspension (3.5 x 10 Vero
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cells/mL) in Eagle’s MEM containing 8% FCS were distributed into the wells and infected with HSV-1.
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Fifty microliters of mock- and virus-infected cell suspensions at multiplicity of infection (MOI) of 0.001
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ID50/cells were then transferred into each well containing the dilution compound and were incubated
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for 3 days without change of the medium, at 37°C in 5% CO2. Cells and virus controls were run
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simultaneously. A MOI of 0.01 ID50/cells was used for the second step of screening on the most
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promising extracts with a kinetic of 48, 72 and 96 h of incubation.
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After microscopic examination to check the growth of the virus, 50 µL of neutral red dye (0.15% in
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saline, pH 5.5) was added to each well, and the cultures were incubated for 45 min at 37°C [33].
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Excess dye was removed by rinsing with phosphate buffered saline (PBS, pH 7.2; Biomérieux,
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France), and the neutral red incorporated by the viable cells was eluted into 100 µL/well of citrate
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ethanol buffer. After shaking the tray for a few minutes, whereby cell monolayers were completely
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destroyed, the optical density (OD) of the wells was read in a multichannel spectrophotometer
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(Packard Spectra Count , USA) at 540 nm. The OD was directly related to the percentages of viable
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cells that were inversely proportional to the cytophathogenecity effect (CPE) ratio. The straight line of
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the regression was determined for each assay and for each plate on the basis of cell controls (0%
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CPE) and virus controls (100% CPE) [34]. The 50% cytotoxic concentration (CC50) of the test
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compound was defined as the concentration that reduced the absorbance of mock-infected cells to
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50% of that of controls. The 50% antiviral effective concentration (EC50) was expressed as the
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concentration that achieved a 50% protection of virus-infected cells from the HSV-induced destruction.
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The following formula was used to calculate the percentage protection:
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[ (ODt) HSV - (ODc) HSV ] / [ (ODc) MOCK - (ODc) HSV ] x 100 (%)
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Where (ODt) HSV is the absorbance of the test sample, (ODc) HSV is the absorbance of the virus-
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infected control (no compound), and (ODc) MOCK is the absorbance of the mock-infected control. The
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ratio of (ODc) HSV to (ODc) MOCK is expressed as “% of control“. For all tests, the anti-herpetic
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compound acyclovir [9-(2-hydroxyethoxymethyl) guanine] (Wellcome Foundation Ltd, U.K.) was used
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as a reference.
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Antiviral activities and kinetics of the efficient extracts
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The freeze-dried extracts were tested at 10 different concentrations ranging from 0.25 to 250.00
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µg/mL (4 wells/concentration) at an MOI of 0.01 ID50/cells. Cytotoxicity and antiviral activity of extracts
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were evaluated by neutral red dye method after 48, 72, and 96 h of treatment.
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Antiviral bioguided fractionation by molecular mass fractionation
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After fractionation of the most efficient extract with six different membranes (2 kDa, 5 kDa, 10 kDa,
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30 kDa, 50 kDa and 100 kDa), the freeze-dried extracts were tested at 10 different concentrations
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ranging from 0.25 to 250.00 µg/mL (4 wells/concentration) at an MOI of 0.01 ID50/cells after 72 h of
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treatment.
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2.5 Analysis of the biochemical compositions of the efficient extracts Analysis of biochemical compositions of the efficient extracts and the control were performed. Compositions of freeze-dried samples were determined as described below. Proteins, humidity, and
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ash were determined in accordance with Association of Official Analysts Chemists (A.O.A.C.) official
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methods, 981.10, 952.08, and 938.08 respectively. Fats were determined according to the Folch
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method [35] and neutral sugars according to the Dubois method [36].
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The total free amino acid composition of freeze-dried hydrolysates and the control was determined after hydrolysis in 6 M HCl at 118°C for 18 h. Then, the samples were completely dried
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under nitrogen atmosphere and diluted by adding 2.5 mL of water. The amino acid analysis was
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performed according to the EZ faast™ (Phenomenex, France) procedure consisting of a solid phase
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extraction step followed by derivatization and liquid/liquid extraction. The solid phase extraction was
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performed via a sorbent packed tip that binds amino acids while allowing interfering compounds to
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flow through. Amino acids on sorbent were then extracted into the sample and quickly transformed
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with a reagent at room temperature in an aqueous solution. Derivatized amino acids concomitantly
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migrated to the organic layer for additional separation from interfering compounds. An aliquot from the
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organic phase was then analyzed on a GC-MS system. The mass spectrometer was an Agilent 5973
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series network mass selective detector (Agilent, CA, U.S.A.). The column was a Zebron ZB-AAA GC
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column (Phenomenex, France) for protein hydrolysates (max. temp. 320/340°C). The amino acids
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were quantified by their response factor relative to the internal standard Norvaline added at a
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concentration of 200 μmol/L [37].
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2.6 Molecular mass fractionation
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Molecular mass fractionation was prepared with ultrapure water at 1 mg/mL then fractionated
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using centrifugal concentrators (Vivaspin 2, Sartorius, France) at different Molecular Weight Cut-Off
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(MWCO). Centrifugations were carried out for 10 min at 12000 g for 2 kDa, 5 kDa, 10 kDa, 30 kDa and
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50 kDa PES (Polyethersulfone) membranes and 9000 g for 100 kDa PES membrane. Seven samples
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were obtained (<2 kDa, 2-5 kDa, 5-10 kDa, 10-30 kDa, 30-50 kDa, 50-100 kDa, >100 kDa) and freeze-
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dried.
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3. RESULTS AND DISCUSSION The dissection step showed that byproducts represented around 50% of the fresh weight of
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the whole sea cucumber. The major parts were internal organs (15 ±3% of the fresh weight) and the
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aquapharyngeal bulb (13 ±2% of the fresh weight)
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The hydrolysis parameters (ratio enzyme/substrate; pH and temperature) have been selected
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as the mean of the optimal conditions declared by the manufacturers for all enzymes. Concerning the
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time of hydrolysis, previous studies showed that the degree of hydrolysis (DH) of Alcalase, Bromelain,
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Flavourzyme, Protamex, reached a threshold value after 6 h. Therefore, this time value was selected
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for all enzyme assisted extraction experiments [14; 37-38].
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3.1 Evaluation of antiviral activities of the library of extracts by cell viability
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3.1.1
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Before evaluation of antiviral activity, cytotoxicity of extracts on Vero cells was studied using the
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Evaluation of cytotoxicity
neutral red incorporation in the aim to detect lysosomal functionality. This method is currently used for
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the screening of anti-HSV-1 molecules from marine organisms [28; 39-40]. An antiviral drug should be
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active against the virus without inducing significant toxicity on the host cell. Therefore, the
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concentration range of the extract that did not induce significant toxicity to the host cells was estimated
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and the 50% cytotoxic concentration (CC50) was determined for each one.
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Most of the extracts from aquapharyngeal bulb (A.B.) were well tolerated by Vero cells and their CC50 varied in the range of 74.5 and up to more than 500 µg/mL. Only two extracts obtained by
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solvent extraction were cytotoxic (hexane extract with a CC50 = 81.5 µg/mL and methanol extract with
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a CC50 = 74.5 µg/mL). None of the hydrolysates evaluated in our conditions induced visible changes in
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cell morphology and cell density.
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The CC50 of the extracts from internal organs (I.O.) varied in the range of 23.3 and up to more
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than 500 µg/mL. Half of them were cytotoxic in the concentrations tested. The evaluation of
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cytotoxicity of solvent extracts showed that extracts obtained by highly polar solvent extraction were
291
toxic (methanol extract with a CC50 = 56.7 µg/mL and water extract with a CC50 = 96.3 µg/mL). The
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majority of the enzymatic hydrolysates were also cytotoxic.
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The cytotoxic extracts found in the A.B. and especially in I.O. could be explained by the presence
294
of triterpene glycosides [41]. Indeed, these molecules, essentially extracted by alcoholic solvent, have
295
already been described in holothurians species and demonstrated as cytotoxic agents. As an
296
example, the major triterpene glycoside Frondoside A, isolated by solvent extraction from the bodywall
297
of C. frondosa, showed cytotoxicity on THP-1 and HeLa tumor cell lines with IC50 values of 4.5 and
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2.1 μg/mL, respectively [42-43]. Furthermore, a recent study demonstrated the richness of triterpene
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glycosides in holothurian internal organs [44].
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3.1.2
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Evaluation of antiviral activity against HSV-1 was examined using CPE inhibitory assay. The
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Evaluation of antiviral activity
reference standard ACV conferred protection (EC50 = 0.2 µg/ml) against HSV-1 with a low percentage
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of cell destruction. All 28 samples from the library of extracts were evaluated for their antiviral activity
305
at an MOI of 0.001 ID50/cells by cell viability. Results are summarized in Table 1. After 72 h of
306
treatment, seven of nine hydrolysates of the aquapharyngeal exhibited antiherpetic activities with EC50
307
between 7.2 and 170.9 µg/mL. Only the water extract of the aquapharyngeal bulb of C. frondosa
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demonstrated an antiherpetic activity with an EC50 of 140 µg/mL and the aquapharyngeal bulb without
309
treatment (control) showed an activity (EC50: 75.0 µg/mL). Among the extracts from internal organs,
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only the control extract showed an antiviral activity (EC50 = 72.5 µg/mL).
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Of 28 extracts evaluated, 10 extracts exhibited antiherpetic activities. The extracts from the
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aquapharyngeal bulb showed better antiviral activities in comparison to internal organs extracts. This
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screening also demonstrated that antiviral compounds seemed to be highly polar. Indeed only the
314
water extract and hydrolysates of the aquapharyngeal bulb possessed antiviral activities without
315
cytotoxicity. In a review, Zhong et al. [31] showed that of 188 plant, animal, or microorganism extracts,
316
162 (86.2%) with inhibitory activity against HSV have been obtained from highly polar solvents such as
317
aqueous solvents, methanol, ethanol, and acetic acid. It appears that most anti-HSV molecules are
318
soluble in polar solvents, including polyphenols and flavones with multiple hydroxyl groups, and this
319
solubility correlates with the reported compound types that have anti-HSV activity. Consequently, it
320
seems relevant to focus on aqueous fractions for the search of antiherpetic compounds. For example,
321
the use of enzymatic hydrolysis with proteases in highly controlled conditions permits the release of
322
bioactive peptides, even though they were inactive when included in the amino sequence of the parent
323
protein [45].
324
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Little is known about antiviral activities from holothurians. Tsushima et al. [23] showed that
325
cucumariaxanthin C from Cucumaria japonica exhibited an inhibitory effect on Epstein-Barr virus
326
(Herpesviridae) activation in a short-term in vitro assay. On the same species, Grishin et al. [24]
327
demonstrated that triterpene glycosides, and especially cucumarioside A2-2, can inhibit the cytopathic
12 Page 12 of 39
effect induced by Vesicular Stomatitis Virus (VSV), Poliovirus, and other viruses in cell culture.
329
According to Rodriguez et al. [25], holothurinosides from Holothuria forskalii can also inhibit the
330
cytopathic effect induced by VSV. Recently, it has been shown that glycosaminoglycan extracted from
331
Thelenota ananas may possess great potential to be further developed as a new Human
332
Immunodeficiency Virus (HIV) entry inhibitor [26-27].
333
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Liouvillosides A and B extracted from a whole specimen of Staurocucumis liouvilei [28],
thyonosides A and B from Thyone aurea [29], and a water extract of the body wall of Holothuria sp.
335
[30], have been shown to possess antiviral activities against Herpes simplex virus type 1. In particular,
336
triterpene glycosides from Staurocucumis liouvilei showed a virucidal effect at concentrations below 10
337
µg/mL, and the water extract of Holothuria sp. exhibited an intracellular antiviral activity with an IC50
338
value of 189.9 µg/mL.
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In comparison to solvent extraction, enzymatic hydrolysis recovers antiherpetic compounds from
340
the aquapharyngeal bulb. Moreover, this process is a softer technique without the solvent elimination
341
step and can allow a valorization of the entire raw matter, which is useful in a global context of marine
342
biological resources overexploitation [3-4; 46]. The most efficient extracts selected were obtained by
343
using four different proteases which have a common mechanism of action. Indeed, these enzymes
344
have endopeptidase activities resulting mainly in the production of polypeptides or proteins, compared
345
to exopeptidases which mainly promote the production of free amino acids.
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347
3.2 Biochemical composition of the effective extracts
348
The most effective extracts were selected according to EC50 values. In that way, four hydrolysates
349
from the aquapharyngeal bulb byproducts were chosen to continue the study: Papain hydrolysate
350
(EC50 = 7.2 µg/mL), Protamex hydrolysate (EC50 = 8.3 µg/mL), Neutral Protease hydrolysate (EC50 =
351
12.5 µg/mL) and Alcalase hydrolysate (EC50 = 15.2 µg/mL).
352
Analysis of the biochemical composition was carried out on the four aquapharyngeal bulb
353
hydrolysates and on the control (aquapharyngeal bulb without treatment). Results are presented in
354
Table 2. Results showed no significant differences between the extracts, except for the control.
355
Indeed, a small decrease of the lipid content and increase of the protein content were observed.
356
Compositions of the extracts showed a high protein content with an average of 54.9% (dry weight).
357
These results are in accordance with the previous study of Mamelona et al. [47] on hydrolysis of the
13 Page 13 of 39
358
viscera of the same animal with an average of 55%. Other studies also report that enzymatic
359
hydrolysis does not significantly change the protein percentage, but rather liberates small peptides
360
[48].
361
Total amino acids assays showed no significant differences between the four hydrolysates selected. The mean amino acid profile is presented in three groups of amino acids according to their
363
abundance. Values are expressed as a percentage of the total amino acids assayed: inferior to 4%:
364
Histidine (1.5%), Methionine (1.5%), Phenylalanine (3.5%), Lysine (2.3%), Hydroxyproline (3.5%), and
365
Tyrosine (2.0%); between 4 and 8%: Alanine (7.8%), Threonine (6.2%), Valine (5.1%), Isoleucine
366
(4.7%), Leucine (6.1%), and Serine (7.5%); superior to 8%: Aspartic acid (10.7%), Glutamic acid
367
(12.4%), Glycine (16.5%), and Proline (8.6%). These values are in accordance with the previous study
368
of Zhong et al. [49] on a biochemical comparison of the body wall of C. frondosa with or without
369
internal organs, on fresh or rehydrated matter, where major amino acids were the same as those
370
found in the extracts evaluated in our study. However, the total amino acid profile of the control was
371
slightly different. Indeed, the control was enriched in Leucine (8.2%), Phenylalanine (5.0%), Glycine
372
(25.8%) and Alanine (10.4%) but depleted in Aspartic acid (5.1%), Glutamic acid (5.7%) and Serine
373
(5.5%). In our conditions, the enzymatic hydrolysis process with proteases seems to recover amino
374
acids with acidic side chains and strongly loses the neutral amino acid Glycine.
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Lipid contents (average of 6.6%) are similar between hydrolysates, but twice as high as the
376
control. This difference can be explained by the ability of the enzymatic hydrolysis process to release
377
lipids in the soluble part. Dumay et al. [50] demonstrated on sardine byproducts that enzymatic
378
proteolysis can be used for high lipid recovery.
379
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Ash contents are similar with an average of 25.6%. Available data on the ash content of the
380
holothurian aquapharyngeal bulb are quite rare. Results found for C. frondosa are higher than the data
381
found for the viscera content of the same species (7-11%: [47]) and lower than the data found for the
382
body walls of other shallow-water holothuroids with an average of 52% [51]. These variations in ash
383
content can be explained by the structure of their internal anatomy, which is more or less rich in calcite
384
depending on the part of the animal considered [52].
385
Neutral sugar contents are around 1.8% for Alcalase, Papain and Protamex hydrolysates and are
386
similar for those found on the viscera of other shallow-water sea cucumbers [51] but slightly higher for
387
Neutral Protease hydrolysate with 3.1%.
14 Page 14 of 39
388
Studies on natural products with anti-HSV activities reported that most of these compounds targeted the viral attachment and the entry stage. The other major mechanism of action reported was
390
the DNA replication by inhibition of the HSV-encoded DNA polymerase. This latter is the mechanism
391
of action used by the anti-HSV-1 reference drug, acyclovir (ACV). The other mechanisms of action
392
described in natural compounds with antiviral activities target the inhibition of the virion assembly and
393
output, the cellular proteins and the promotion of the immune response [22].
ip t
389
The four selected hydrolysates showed a high protein content. Marine peptides and nucleosides
395
have already shown antiherpetic activities by inhibiting the viral protein synthesis of HSV-1 [53]. The
396
nucleoside spongouridine was used for the synthesis of the marine adenine arabinoside which is
397
rapidly converted into its triphosphate form, leading to the inhibition of the viral DNA polymerase and
398
DNA synthesis of HSV in infected cells [54]. Besides the antiviral activities of these compounds, other
399
chemical classes have also shown such activity. Fucosylated chondroitin sulfate (FuCS) found in sea
400
cucumbers from different species has revealed interesting bioactivities. Among these activities, FuCS
401
extracted from the holothurian T. ananas has shown highly effective antiviral activity against HIV
402
strains. FuCS showed a capacity to block the virus entry and replication on cell models and clinic
403
isolates [10].
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Sulfated polysaccharides are known to be active on HSV. These compounds are able to inhibit
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404
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394
viral infection by preventing adsorption of the virus into the host cells and/or by inhibiting the
406
production of new viral particles inside the host cells [55]. Natural carrageenans were identified as
407
potent and selective inhibitors of HSV-1 and HSV-2. Studies suggested that the main target for
408
antiviral action of the carrageenans was based on the virus adsorption, whereas no effect on virus
409
internalization or early or later protein synthesis was detected [56]. Alkaloids showed potent anti-HSV-
410
1 activity by impairing the virus penetration and inhibiting immediate early protein synthesis [57].
411
Glycolipids showed antiviral activity against HSV-1 and HSV-2 [58]. The antiviral action might be due
412
to the binding of the virus glycoprotein to the glycolipid leading to an irreversible denaturation that
413
blocks viral infection [59].
414
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405
Many marine compounds of different chemical classes with a broad range of mechanism of action
415
have been described as effective anti-HSV-1 agents. However, according to the biochemical
416
composition of the selected extracts and the differences in activity values modulated by the nature of
417
the enzymes used, the results suggested that the antiviral compounds might be from protein origin.
15 Page 15 of 39
418 419
3.3 Antiviral activities and kinetics of the effective extracts from aquapharyngeal bulb byproducts
420 421
After 48, 72, and 96 h of treatment, viability assay showed no cytotoxic effect of the compounds on Vero cells in the range of concentrations assayed for all four compounds.
422
ip t
The four hydrolysates showed anti-HSV-1 activities for an MOI of 0.01 ID50/cells. Results are summarized in Table 3 in comparison with the reference drug (ACV). After 48 h of incubation, the four
424
extracts exhibited an important antiviral activity: Papain hydrolysate (EC50 = 15.9 µg/mL) > Alcalase
425
hydrolysate (EC50 = 20.4 µg/mL) > Neutral protease hydrolysate (EC50 = 26.9 µg/mL) > Protamex
426
hydrolysate (EC50 = 52.2 µg/mL). After 72 h of incubation, the four extracts still showed an important
427
activity: Papain hydrolysate (EC50 = 25.2 µg/mL) > Neutral protease hydrolysate (EC50 = 36.9 µg/mL) >
428
Alcalase hydrolysate (EC50 = 43.9 µg/mL) > Protamex hydrolysate (EC50 = 102.9 µg/mL). After 96 h of
429
incubation, three of four hydrolysates remained active against HSV-1: Papain hydrolysate (EC50 =
430
44.3 µg/mL) > Protamex hydrolysate (EC50 = 144.9 µg/mL) > Alcalase hydrolysate (EC50 = 150.4
431
µg/mL).
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432
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423
Extracts seemed to act differently depending on the time of incubation, and the evolution of activities did not follow the same trend. This is well illustrated with a neutral protease hydrolysate
434
activity that, during 48 and 72 h of incubation, possessed interesting antiviral activities but completely
435
lost its activity after 96 h. Antiherpetic compounds from the extracts assayed seemed to act on early
436
cycles of replication but after 96 h faced obstacles with the release of newly formed virions [60].
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Results showed that Protamex hydrolysate was the second most efficient extract (EC50 = 8.3
438
µg/mL) at an MOI of 0.001 ID50/cells after 72 h of incubation. At an MOI of 0.01 ID50/cells, it became
439
less active (EC50 = 102.9 µg/mL) with the same concentrations assayed after the same period of
440
incubation. This observation can be explained by the fact that continuous replication of every virus
441
particle will produce an aggressive virus population. A culture infected with high virus multiplicity may
442
therefore need higher concentrations of antiviral compounds for viral inhibition than cells infected with
443
low multiplicity [61].
444
Among all these observations, the Papain hydrolysate remained the more active extract.
445
According to the specificities of each enzyme, a trend seemed to be emerging. Byproducts hydrolysed
446
with Alcalase and mostly with Papain possessed the highest antiviral activities. Papain, and Alcalase
16 Page 16 of 39
447
at a lower rate, have broad specificities to cleave peptide bonds but preferences for amino acids
448
bearing a large hydrophobic side chain compared to Neutral Protease and Protamex enzymes.
449
Ghanbari et al. [14] showed an antibacterial activity of enzymatic hydrolysates from the sea cucumber Actinopyga lecanora. The antibacterial activity was not only correlated to the size, the
451
molecular weight and the degree of hydrolysis, but also on the hydrophobicity of the resulting
452
peptides. Furthermore, Papain hydrolysates have already shown to possess activities such as
453
antioxidant activities [62] and ACE inhibition [63]
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454
On the same raw matter, the process of enzymatic hydrolysis with proteases induced different extracts with different activities against HSV-1; therefore, the nature of the enzyme used seems to be
456
a major parameter to modify the antiviral activity. The enzyme specificity is important to peptide
457
functionality because it strongly influences the molecular size and hydrophobicity of the hydrolysate
458
[3].
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459
461
3.4 Antiviral activity by bioguided molecular mass fractionation
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460
After 72 h of treatment, a viability assay showing no cytotoxic effect of the compounds was observed on the Vero cells in the range of concentrations assayed for all seven compounds. Results
463
are presented in Table 4. Out of seven extracts tested, three extracts showed an effective antiviral
464
activity with EC50 of 55.1, 38.1, and 18.2 µg/mL at an MOI of 0.01 ID50/cells for the fractions 30-50
465
kDa, 50-100 kDa and superior to 100 kDa respectively. Other extracts were not active against HSV-1
466
in the range of concentrations tested. Active molecules were present on the last fractions, and activity
467
increased with the size of the cutoff from 30 kDa to over 100 kDa. It is assumed that the compounds
468
responsible for the antiherpetic activity are in an aqueous phase superior to 100 kDa due to the
469
highest activity found for the last fraction. High molecular weight compounds have already been
470
demonstrated as antiherpetic agents [64]. Indeed, sulfated polysaccharides isolated from two red
471
algae with an average molecular weight of 308 and 360 kDa were shown to exert in vitro anti-HSV-1
472
activity. They were capable of inhibiting the in vitro replication of HSV-1 on Vero cells with EC50 values
473
of 4.1 and 17.2 μg/mL [64]. These values have been obtained after an evaluation of 48 h at an MOI of
474
0.001 ID50/cells, ten times lower than the MOI used in the antiviral evaluation by bioguided molecular
475
mass fractionation (0.01 ID50/cells after an evaluation of 72 h). Recently, sulfated polysaccharides
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17 Page 17 of 39
476
isolated from the bodywall of C. frondosa showed biological effects. Indeed, they have demonstrated
477
in vitro the ability to act on the maturation of dendritic cells [11].
478
Generally, due to the poor permeability through membranes, molecular size, physical and chemical instability affect the bioavailability of peptides and more specifically proteins. In vivo, peptides
480
with two or six amino acids reach their target site more easily than a whole protein. However, some
481
marine proteins showed biological activities in animal models. Lectins are carbohydrate-binding
482
proteins found in a wide range of organisms even in holothurians. Bulgakov et al. [65] described a 44-
483
kDa, C-type mannan-binding lectin consisting of two identical subunits isolated from the coelomic fluid
484
of the holothurian Cucumaria japonica. A 400 kDa lectin named SPL-1 and a 68 kDa lectin named
485
SPL-2 were extracted from the holothurian species Stichopus (Apostichopus) japonicus. Inhibition of
486
HSV infections was demonstrated with lectins from plants which are able to recognize and bind to
487
polysaccharides or glycoproteins on cell surface in order to agglomerate the cells. The presence of
488
lectins in holothurians species, the wide range of molecular mass described and their bioactivities
489
might be a possible explanation for the antiviral compounds found in our study. Furthermore, the
490
presence of oligomers with different subunit sizes could also explain the antiviral activities of the two
491
fractions lower than 100 kDa. Glycosylation is essential to the virus for its cellular transport and
492
binding to cellular receptors, in this way, by binding to the glycosylated viral-envelope, lectins could act
493
as entry blockers.
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Protein hydrolysates have been investigated as an alternative for the upgrading of marine
Ac ce p
494
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479
495
byproducts to deal with the significant quantities of waste generated annually by the processing
496
industries [66]. These hydrolysates have broadly contributed to the discovery of new compounds with
497
activities that include the following: antioxidative, anticancer, calcium-binding peptides, appetite
498
suppression, anticoagulant, immunostimulant, hypocholesterolemic, hormone-regulating, and
499
antimicrobial and antiviral [38]. In our study, the aqueous fraction obtained by enzymatic proteolysis
500
from Cucumaria frondosa seems to be a promising extract for the search of active compounds against
501
Herpes Simplex virus.
502 503
In conclusion, this study confirms that, in comparison to solvent extraction, the enzymatic
504
extraction appears to be a promising softer technique for the recovery of industrially important
505
metabolites as antiviral compounds in a time-saving fashion, with less solvent and at lower cost. The
18 Page 18 of 39
specificity of enzymes used was also shown with different levels of response for the activity evaluated.
507
The aquapharyngeal bulb, for a long time considered as a byproduct with low value added, represents
508
a non-negligible part of the animal in terms of proportion but also mainly for its biochemical
509
composition. To our knowledge, no studies have demonstrated the presence of active molecules
510
against HSV-1 from C. frondosa byproducts. The results obtained in this study make the high
511
molecular weight extract from the Papain hydrolysate of the aquapharyngeal bulb from the sea
512
cucumber Cucumaria frondosa a great potential source of antiviral agent against Herpes Simplex virus
513
1. Literature suggested that lectins might be a possible explanation for the nature of the antiviral
514
compounds retrieved in the high molecular weight extract with a potential mechanism of action as
515
entry blockers. This extract could provide high added value to an underestimated biomass with the
516
added bonus of being environmentally friendly through the use of enzymes instead of solvents. These
517
compounds are currently undergoing purification in order to identify the active molecules as well as
518
their mechanism of action.
an
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ACKNOWLEDGMENTS This research was supported by the Atlantic Canada Opportunities Agency (Atlantic Innovation
te
521
Fund grant 193594). The authors thank Dr J.P. Bergé and C. Donnay-Moreno from the laboratory
524
BIORAFhe, IFREMER, Nantes, FRANCE for the amino acids analysis.
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19 Page 19 of 39
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[59] El Baroty GS, El Baz FKA-EI, Abd El-Baky HH, Ali MM, Ibrahim EA. Evaluation of Glycolipids of
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some Egyptian Marine Algae as A Source of Bioactive Substances. Int Res J Pharmacy. 2011.
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[60] Mat R, Zalilawati, Lahaye, Elodie, Defer, Diane, Douzenel, Philippe, Perrin, Bertrand,
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Bourgougnon, Nathalie, Sire, Olivier G. Isolation of a sulphated polysaccharide from a recently
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[61] Harmenberg J, Wahren B, Sundqvist V-A, Levén B. Multiplicity dependence and sensitivity of
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[62] You L, Zhao M, Cui C, Zhao H, Yang B. Effect of degree of hydrolysis on the antioxidant activity of
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Technologies. 2009;10:235-40.
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[63] Barbana C, Boye JI. Angiotensin I-converting enzyme inhibitory activity of chickpea and pea
766
protein hydrolysates. Food Research International. 2010;43:1642-9.
767 [64] Bouhlal R, Haslin C, Chermann J-C, Colliec-Jouault S, Sinquin C, Simon G, et al. Antiviral
769
Activities of Sulfated Polysaccharides Isolated from Sphaerococcus coronopifolius (Rhodophytha,
770
Gigartinales) and Boergeseniella thuyoides (Rhodophyta, Ceramiales). Marine Drugs. 2011;9:1187-
771
209.
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ip t
768
us
772
[65] Bulgakov AA, Eliseikina MG, Petrova IY, Nazarenko EL, Kovalchuk SN, Kozhemyako VB, et al.
774
Molecular and Biological Characterization of a Mannan-Binding Lectin from the Holothurian
775
Apostichopus Japonicus. Glycobiology. 2007;17:1284-98.
an
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M
776
[66] Harnedy PA, Fitzgerald RJ. Bioactive Proteins and Peptides from Macroalgae, Fish, Shellfish and
778
Marine Processing Waste. Marine Proteins and Peptides: John Wiley & Sons, Ltd; 2013. p. 5-39.
te Ac ce p
779
d
777
30 Page 30 of 39
779
Table 1 : Evaluation of anti-HSV activity at an MOI of 0.001 ID50/cells on Vero cell line of the
780
byproducts library of extracts from C. frondosa, by neutral red dye method after 72 h of incubation.
781
Acyclovir (ACV) was used as a reference drug. Treatment
Reagent
CC50 (µg/mL)
Aquapharyngeal bulb
None
None
>500
Enzymatic hydrolysis
Alcalase
>500
Bromelain
>500
cr
>250 160.5 ±8.7
>500
>250
>500
12.5 ±3.1
Papain
>500
7.2 ±1.9
Peptidase AM
>500
45.3 ±5.1
Peptidase AO
>500
170.9 ±7.5
Protamex
>500
8.3 ±2.7
Acetone
>500
>250
Hexane
81.5 ±3.8
7.9 ±3.4
Methanol
74.5 ±4.5
70.9 ±7.4
Water extract
>250
140.0 ±13.8
None
None
>250
72.5 ±9.8
Enzymatic hydrolysis
Alcalase
>500
>250
Bromelain
40.4 ±3.0
60.0 ±3.2
Flavourzyme
>500
>250
Fungal protease
29.0 ±3.0
10.4 ±1.5
Neutral protease
23.3 ±3.1
14.0 ±4.0
Papain
69.6 ±2.8
11.0 ±9.1
Peptidase AM
>500
>250
d
M
Neutral protease
Ac ce p
te
Solvent extraction
Internal organs
15.2 ±2.5
>500
an
Fungal protease
75.0 ±2.1
us
Flavourzyme
EC50 (µg/mL)
ip t
Organ
31 Page 31 of 39
ACV
None
7.8 ±9.5
Protamex
>500
>250
Acetone
>500
>250
Hexane
>500
>250
Methanol
56.7 ±5.8
Water extract
96.3 ±7.3
None
>500
7.9 ±1.8
33.2 ±4.8
0.2 ±0.1
us
Data are shown as mean ± S.D. (n=4).
ip t
74.9 ±4.8
cr
Solvent extraction
Peptidase AO
an
MOI: multiplicity of infection: ratio (virus titer)/(cells number/mL). CC50: the 50% cytotoxic concentration: concentration that reduced the absorbance of mock-infected cells to 50% of that of controls. EC50: the 50% antiviral effective concentration: concentration that achieved 50% protection of virus-infected cells from the HSV-induced destruction
Ac ce p
te
d
M
782 783
32 Page 32 of 39
Table 2: Proximate analysis on freeze-dried aquapharyngeal bulb of C. frondosa hydrolysates and without hydrolysis as a control group; n.d.: Not determined Control
Alcalase hydrolysate
Neutral Protease hydrolysate
Papain hydrolysate
Protamex hydrolysate
Crude protein (%)
58.8
54.5
54.7
55.4
54.9
Humidity (%)
6.5
5.8
5.9
4.7
Ash (%)
23.2
26.2
25.1
26.0
Fats (%)
2.8
6.3
6.5
Neutral sugars (%)
n.d.
1.8
3.1
ip t
Analysis
us
cr
4.3
27.6
7.0
6.4
1.9
1.7
an
783 784 785
786
Ac ce p
te
d
M
787
33 Page 33 of 39
787 Table 3 : Evaluation of anti-HSV activity at an MOI of 0.01 ID50/cells on Vero cell line of the most promising extracts from aquapharyngeal bulb of C. frondosa hydrolysed with: Alcalase (1), Neutral protease (2), Papain (3) and Protamex (4) by neutral red dye method at 48, 72 and 96 h of incubation. Acyclovir (ACV) was used as a reference drug. 96 h
EC50 (µg/mL)
CC50 (µg/mL)
EC50 (µg/mL)
CC50 (µg/mL)
EC50 (µg/mL)
1
>500.0
20.4 ±3.2
>500.0
43.9 ±5.2
>500.0
150.4 ±8.2
2
>500.0
26.9 ±4.4
>500.0
36.9 ±0.5
3
>500.0
15.9 ±2.2
>500.0
25.2 ±4.8
>500.0
44.3 ±3.2
4
>500.0
52.2 ±5.8
>500.0
102.9 ±8.7
>500.0
144.9 ±7.3
0.3 ±0.1
>500.0
0.3 ±0.1
>500.0
1.1 ±0.3
us
>500.0
>500
Ac ce p
te
d
794
an
Data are shown as mean ± S.D. (n=4).
cr
CC50 (µg/mL)
ACV >500.0 792 793
72 h
ip t
48 h
M
788 789 790 791
34 Page 34 of 39
794
801
< 2 kDa
>500.0
>500.0
2-5 kDa
>500.0
>500.0
5-10 kDa
>500.0
>500.0
10-30 kDa
>500.0
>500.0
30-50 KDa
>500.0
50-100 KDa
>500.0
us
> 100 kDa
>500.0
ACV
>500.0
cr
55.1 ±7.2 38.1 ±5.2
an
M
Data are shown as mean ± S.D. (n=4).
ip t
EC50 (µg/mL)
18.2 ±3.6 0.3 ±0.1
d
800
CC50 (µg/mL)
te
798 799
Table 4 : Evaluation of anti-HSV activity at an MOI of 0.01 ID50/cells on Vero cell line by molecular mass fractionation of aquapharyngeal bulb of C. frondosa hydrolysed with Papain after 72 h of incubation, by neutral red dye method. Acyclovir (ACV) was used as a reference drug.
Ac ce p
795 796 797
35 Page 35 of 39
801
Figure 1: Summary of the enzymatic hydrolysis process for the preparation of byproducts
802
hydrolysates from Cucumaria frondosa (A.B.: Aquapharyngeal Bulb and I.O.: Internal Organs); rpm:
803
rotation per minute.
804
806
Figure 2: Summary of the sequential solvent extraction of the freeze-dried byproducts of
ip t
805
Cucumaria frondosa (A.B.: Aquapharyngeal Bulb and I.O.: Internal Organs; RT: Room Temperature.
cr
807
Ac ce p
te
d
M
an
us
808
36 Page 36 of 39
Ac ce p
te
d
M
an
us
cr
ip t
Figure1
Page 37 of 39
Ac ce p
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d
M
an
us
cr
ip t
Figure2
Page 38 of 39
cr M
an
us
*Graphical Abstract
L.TRIPOTEAU L.TRIPOTEAU
Extraction of the byproducts
L.TRIPOTEAU
ed
Enzymatic hydrolysis Enzymatic and Solvent extraction hydrolysis (variation of proteases nature, pH, temperature, time)
ce
pt
Collection of specimens
Ac
Identification of a potent antiherpetic extract : - > 100 kDa
- Papain hydrolysate - Aquapharyngeal bulb
Selection
Molecular mass fractionation
Antiviral and cytotoxic evaluation of the fractions
Antiviral and cytotoxic evaluation of the selected extracts
Page 39 of 39
Antiviral and cytotoxic evaluation of the library of extracts
S1359-5113(15)00102-6 http://dx.doi.org/doi:10.1016/j.procbio.2015.02.012 PRBI 10360
To appear in:
Process Biochemistry
Received date: Revised date: Accepted date:
15-12-2014 10-2-2015 23-2-2015
Please cite this article as: Tripoteau L, Bedoux G, Gagnon J, Bourgougnon N, IN VITRO ANTIVIRAL ACTIVITIES OF ENZYMATIC HYDROLYSATES EXTRACTED FROM byproducts OF THE ATLANTIC HOLOTHURIAN CUCUMARIA FRONDOSA, Process Biochemistry (2015), http://dx.doi.org/10.1016/j.procbio.2015.02.012 This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
1
IN VITRO ANTIVIRAL ACTIVITIES OF ENZYMATIC HYDROLYSATES EXTRACTED FROM
2
BYPRODUCTS OF THE ATLANTIC HOLOTHURIAN CUCUMARIA FRONDOSA
3
Ludovic TRIPOTEAU
a,b
a
b
*, Gilles Bedoux , Jacques Gagnon , Nathalie Bourgougnon
a,
4 a. Laboratoire de Biotechnologie et Chimie Marines, EA3884, UBS, IUEM, F-56000 Vannes, France.
6
b. Coastal Zones Research Institute Inc., Shippagan, New Brunswick, CANADA
9
Highlights: -
Bioactive compounds were extracted from aquapharyngeal bulb of Cucumaria frondosa
-
Enzymatic extraction permitted the recovery of antiherpetic compounds on our model
-
Antiherpetic activities were highlighted on enzymatic hydrolysates of aquapharyngeal bulb
-
High molecular weight molecules were demonstrated as active against HSV-1
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8
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7
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10 11 12 13
d te Ac ce p
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14 15
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5
1 Page 1 of 39
16
IN VITRO ANTIVIRAL ACTIVITIES OF ENZYMATIC HYDROLYSATES EXTRACTED FROM
17
BYPRODUCTS OF THE ATLANTIC HOLOTHURIAN CUCUMARIA FRONDOSA
18 19
Ludovic TRIPOTEAU
a,b
a
b
*, Gilles Bedoux , Jacques Gagnon , Nathalie Bourgougnon
a,
ip t
20 a. Laboratoire de Biotechnologie et Chimie Marines, EA3884, UBS, IUEM, F-56000 Vannes, France.
22
b. Coastal Zones Research Institute Inc., Shippagan, New Brunswick, CANADA
cr
21
23 *Corresponding author: Ludovic Tripoteau
25
LBCM, Centre de recherche Yves Coppens. Campus de Tohannic – BP 573, 56017 Vannes Cedex. France.
26
Tel.: +33 2 97 01 71 22
27
E-mail address: [email protected]
an
us
24
28 Pr. Nathalie Bourgougnon.
30
LBCM, Centre de recherche Yves Coppens. Campus de Tohannic – BP 573, 56017 Vannes Cedex. France.
31
Tel.: +33 2 97 01 71 55
32
E-mail address: [email protected]
33
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29
Dr. Jacques Gagnon
35
CZRI, PPM. 232B, avenue de l’église, Shippagan, NB, E8S 1J2 Canada
36
Tel.: 1 506 336 6603
37
E-mail address: [email protected]
38
Ac ce p
34
39
Dr. Gilles Bedoux
40
LBCM, Centre de recherche Yves Coppens. Campus de Tohannic – BP 573, 56017 Vannes Cedex. France.
41
Tel.: +33 2 97 01 71 57
42
E-mail address: [email protected]
43
2 Page 2 of 39
43
ABSTRACT
44 45
Herpes Simplex virus 1 (HSV-1), responsible for the common cold sore, can also lead to serious infections in immunocompromised people. Current antiviral chemotherapies face obstacles including
47
the toxicity of therapeutic molecules, interference with normal cellular metabolism, genetic variability
48
and the incurable nature of latent infections. Therefore, the search for new treatments is a public
49
health issue. Marine invertebrates have held great potential for finding novel antiviral compounds.
50
Little is known, about the antiviral activities of compounds isolated from holothurians. In New
51
Brunswick, holothurian is fished for its edible bodywall and muscle, but its processing generates high
52
amounts of byproducts. In vitro evaluation of the anti-HSV-1 activity by cell viability was performed on
53
nine hydrolysates obtained by enzyme-assisted extraction and four solvent extractions from
54
aquapharyngeal bulb and internal organs of Cucumaria frondosa at an MOI of 0.001 ID50/cells. After
55
72 h, four enzymatic hydrolysates from the aquapharyngeal bulb presented effective antiherpetic
56
activities (EC50=7.2–15.2 µg/mL) . After evaluation at a higher MOI (0.01 ID50/cells), the most efficient
57
extract (Papain hydrolysate) was fractionated to identify the active fraction. The fraction superior to
58
100 kDa showed the highest antiherpetic activity (EC50: 18.2 µg/mL). In conclusion, upgrading
59
byproducts of sea cucumber fisheries offers new sources of bioactive molecules.
62
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Key words: Cucumaria frondosa; enzymatic hydrolysis; Herpes simplex virus type 1; byproducts.
Ac ce p
60
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46
3 Page 3 of 39
62 63
1. INTRODUCTION
64 Sea cucumbers are benthic marine invertebrates. Of the 1200 species living worldwide, over 60
66
are known to be harvested for human consumption [1]. One of the species that is considered new on
67
the market is the orange-footed sea cucumber Cucumaria frondosa (Gunnerus, 1767), which is
68
approximately 25–30 cm long and can reach 50 cm when relaxed. The Atlantic sea cucumber
69
Cucumaria frondosa is distributed abundantly in the north Atlantic from tide pools of the lower intertidal
70
zone and to down to 300 m depth [2].
us
cr
ip t
65
Cucumaria frondosa is harvested in the Fundy Bay, New Brunswick (NB), Canada to be then
72
transformed for the human consumption. The processing plant generates discards representing more
73
than half of the total amount of raw matter (600 t). The waste is mainly used as fish meal or fish oil.
74
Internal muscle bands and the dried body wall are the products from C. frondosa sold on Asian food
75
markets. The rest of the sea cucumbers, comprising the aquapharyngeal bulb, gut, gonad, and
76
respiratory tree, considered as byproducts, is rejected or underused. This biomass holds, however,
77
considerable potential to generate new biological compounds and can be turned into a commercially
78
viable business [3-4]. The process of enzymatic hydrolysis has been developed in order to transform
79
marine byproducts into marketable forms. By the use of specific enzymes, this process has the ability
80
to enhance the extraction of specific molecules with new properties (functional, biological, aromatic).
81
Consequently, the action of proteases on marine byproducts rich in proteins may lead to the
82
production of peptides, polypeptides and proteins with various biological activities [3].
M
d
te
Ac ce p
83
an
71
Sea cucumbers are a rich source of vitamins, minerals and bioactive components [5]. They are
84
used as healthy foods, traditional medicines and dietary supplements. For example, they have been
85
used for centuries, especially in Asia, as tonic foods and used in folk medicine to treat various ailments
86
[6]. Dried forms of sea cucumber are used as dietary supplements. More recently, sea cucumbers
87
have received increased attention because of their bioactive compounds such as triterpene glycosides
88
[7-9], chondroitin sulfates [10], sulfated polysaccharides [11], sterols [12], phenolics [13], peptides [14],
89
cerebrosides [15], and lectins [16].
90 91
Several studies conducted on holothurians have shown antifungal [17-19] and antibacterial [14; 20-22] activities. Little is known about antiviral activities [23-27], especially regarding Herpes Simplex
4 Page 4 of 39
Virus 1 (HSV-1) [28-31]. Herpes simplex Virus, a DNA enveloped virus, is a common human pathogen
93
with between 60 and up to 95% of certain populations infected with HSV-1, and between 6 and 50%
94
infected with Herpes Simplex Virus type 2 (HSV-2). The frequency of HSV-seropositive males was
95
significantly higher in populations infected with Human Immunodeficiency Virus (HIV). As the HIV
96
disease progresses, cutaneous and mucosal complications become more severe and occur in up to
97
92% of HIV-infected individuals. Medications available for systemic treatment of HSV are acyclovir,
98
famciclovir and valacyclovir. Acyclovir and penciclovir are available for topical use. In clinical practice,
99
treatment of primary HSV infections, while relieving symptoms and reducing the duration of viral
100
shedding, does not prevent recurrences. Moreover, resistance to acyclovir has been reported in
101
immuno-compromised patients. Therefore, there was a need to develop new therapeutic agents for
102
the management of HSV infections. Moreover, the majority of commercially effective molecules are
103
expected to join the public domain in 2015. The search for new treatments is therefore a major public
104
health issue.
cr
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The purpose of this study was to evaluate the in vitro antiherpetic activities of compounds
M
105
ip t
92
obtained after enzyme-assisted extraction and solvent extractions of Cucumaria frondosa
107
(Dendrochirotida, Cucumariidae) byproducts with a bioguided fractionation.
108
te
d
106
2. MATERIALS AND METHODS
110
2.1 Specimen collection
116
Ac ce p
109
117
2.2 Sample processing
111
Specimens of Cucumaria frondosa were collected in Passamaquoddy Bay, Bay of Fundy, New
112
Brunswick, Canada, between January and March 2012. Sea cucumbers (15-30 cm) were placed for
113
acclimation at the Aquaculture Pavilion and Aquaculture Laboratories of the Coastal Zones Research
114
Institute, Shippagan, New Brunswick, in 900L aerated tanks supplied with filtered seawater (4°C)
115
pumped from Shippagan’s bay, prior to experiments.
118
Specimens were sacrificed, then the aquapharyngeal bulb (A.B.) and internal organs (I.O.)
119
were removed from the rest of the sea cucumbers to be separately crushed with a blender (LBC 15,
120
Waring Laboratory Science, USA) and placed at -20°C prior to further treatments. Some of these
5 Page 5 of 39
121
samples were freeze-dried and placed in a labeled glass vial at -20ºC prior to the sequential solvent
122
extraction.
123 Aqueous extraction assisted by enzymatic hydrolysis
125
For each enzymatic hydrolysis, 1.5 kg of ground biomass was placed in a bioreactor (BioFlo
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124
110, New Brunswick Scientific, USA) with 1.5 L of distilled water. Nine different proteases were
127
separately used: Alcalase (0.1%, w/w ; Alcalase® 2.4L FG, Novozymes AS, Denmark) with a
128
declared activity of 2.4 AU/g (Anson Unit), Bromelain (0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a
129
declared activity of 2000 GDU/g (Gelatin-Digesting Unit), Flavourzyme (0.1%, w/w ; Flavourzyme®
130
Novozymes AS, Denmark) with a declared activity of 500 LAPU/g (Leucine Amino Peptidase Unit),
131
Fungal Protease (0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a declared activity of 400 000 HU/g
132
(Hemoglobin Unit), Neutral Protease (0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a declared activity of
133
2 000 000 PC/g (Proteolytic unit), Papain (0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a declared activity
134
of 6500 NFPU/g (Nuclear Floating Power Unit), Peptidase AM (Peptidase Aspergillus Melleus ; 0.1%,
135
w/w ; Bio-Cat, Troy, VA, USA) with a declared activity of 500 LAPU/g, Peptidase AO (Peptidase
136
Aspergillus Oryzae ; 0.1%, w/w ; Bio-Cat, Troy, VA, USA) with a declared activity of 500 LAPU/g and
137
Protamex (0.1%, w/w ; Protamex® Novozymes AS, Denmark) with a declared activity of 1.5 AU/g
138
during 6 h at pH 8.0 and 50°C. After hydrolysis, enzymes were then inactivated at 90°C for 15 min and
139
hydrolysates were centrifuged at 10,000xg for 20 min at 4°C to separate undigested residues and
140
solubilized compounds. The supernatants were sampled, freeze-dried and stored at -20°C prior to
141
cytotoxicity and antiviral evaluation [14]. The enzymatic hydrolysis process is summarized in Figure 1.
143 144
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Sequential solvent extraction
Hexane (OmniSolv® Hexanes), acetone (OmniSolv® Acetone) and methanol (OmniSolv®
145
Methanol) are HPLC grade and were provided by Fisher Scientific (Canada). The sequential solvent
146
extraction is summarized in Figure 2.
147
Hexane extraction: 20 g of freeze-dried sample of raw matter were first submitted to hexane
148
extraction into a 500 mL Erlenmeyer flask, and 300 mL (15 mL/g) of hexane was added. The sample
149
was placed on a stir-plate, stirred for 30 min at room temperature and then placed in a sonicator for 15
150
min. After filtration (Filter grade #4; Aldrich, Canada), the soluble part and the first residue (R1) were
6 Page 6 of 39
151
separately collected. The solvent was removed from the filtrate using reduced pressure on the rotary
152
evaporator. The remaining solvent was removed by N2 stream in the heating block (40-50°C). The
153
filtrate was then freeze-dried and placed in a labeled glass vial at -20ºC prior to cytotoxicity and
154
antiviral evaluation.
158 159
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using the same procedure according to the sequential solvent extraction described in Figure 2.
For hexane, acetone, and methanol extraction, extractions were repeated twice and the
cr
156
Acetone extraction of R1 and methanol extraction of the second residue (R2) were carried out
fractions obtained were pooled.
Water extraction: The dried filtered residue from methanol extraction (R3) was placed into a
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155
500 mL Erlenmeyer flask; 200 mL of deionized water (10 mL/g) was added, and the mixture was
161
placed on a heating plate and heated to 80-90°C while being stirred. Once the temperature range was
162
reached, it was kept for 2 h. The mixture was removed from heat, cooled to room temperature, and
163
filtered by vacuum filtration. The filtrate was precipitate using ethanol (3V). After ethanol addition, the
164
flask was placed in an ice bath for 2 h. Once fully precipitated, the solids were separated by
165
centrifugation (2500 rpm /20 min). Solids were then freeze-dried and stored in a labeled glass vial at -
166
20°C prior to cytotoxicity and antiviral evaluation. The final residue was not included in the library of
167
extracts due to its low solubility.
170
Library of extracts
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All the extractions carried out on C. frondosa byproducts represented twenty eight different
171
extracts. For one type of byproduct, there were nine enzymatic hydrolysates, four extracts by
172
sequential solvent extraction (hexane, acetone, methanol and water extract) and one byproduct
173
without treatment (control).
174 175 176
2.3 Virus and cell lines
African green monkey kidney cells (Vero cell line n°ATCC CCL81) were grown in Eagle's
177
Minimum Essential Medium (MEM, Laboratory Eurobio, France) supplemented with 8% (v/v) fetal calf
178
serum (FCS, Eurobio, France), to which 1% (v/v) of PCS (penicillin 10 000U, colimycin 25 000 U,
179
streptomycin 10 mg, Sigma, France) was added. Cells were routinely passaged every 3 days.
7 Page 7 of 39
180
Virus stock of Herpes Simplex Virus type 1 was obtained from Pr. Agut, Laboratoire de
181
Dynamique, épidémiologie et traitement des infections virales de la Pitié Salpêtrière (Paris, France).
182
The virus stock was prepared by incubating Vero monolayers (75 cm culture flasks seeded with 350
183
000 cells / mL) at low multiplicity and incubating at 37°C, in a 95% air, 5% CO2 (v/v) atmosphere. Two
184
or three days after infection, the cultures were frozen and thawed twice before clearing the preparation
185
by centrifugation at low speed to remove cell debris. The resulting supernatant aliquot was stored at -
186
80°C until used. Virus titrations were performed by the Reed and Muench dilution method [32], using
187
10 wells on 96-wells microtiter plates per dilution. The virus titer was estimated from cytopathogenicity
188
and expressed as 50% infectious doses / mL (ID50/mL). The virus titer was evaluated at 2.10
189
ID50/mL.
7.57
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2.4 Cytotoxicity and antiviral activity of drugs by neutral red dye method
192
Screening for antiviral activities of the library of extracts
193
Dilutions of samples (50 µL) were prepared in Eagle’s MEM supplemented with 8% FCS and
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191
distributed into the well plates of a 96-well microtest III tissue culture plate (Nunclon, Intermed,
195
France). A series included 10 assays ranging from extreme concentrations of extracts of 0.25 up to
196
250.00 µg/mL (4 wells/concentration). One hundred microliters of cellular suspension (3.5 x 10 Vero
197
cells/mL) in Eagle’s MEM containing 8% FCS were distributed into the wells and infected with HSV-1.
198
Fifty microliters of mock- and virus-infected cell suspensions at multiplicity of infection (MOI) of 0.001
199
ID50/cells were then transferred into each well containing the dilution compound and were incubated
200
for 3 days without change of the medium, at 37°C in 5% CO2. Cells and virus controls were run
201
simultaneously. A MOI of 0.01 ID50/cells was used for the second step of screening on the most
202
promising extracts with a kinetic of 48, 72 and 96 h of incubation.
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After microscopic examination to check the growth of the virus, 50 µL of neutral red dye (0.15% in
204
saline, pH 5.5) was added to each well, and the cultures were incubated for 45 min at 37°C [33].
205
Excess dye was removed by rinsing with phosphate buffered saline (PBS, pH 7.2; Biomérieux,
206
France), and the neutral red incorporated by the viable cells was eluted into 100 µL/well of citrate
207
ethanol buffer. After shaking the tray for a few minutes, whereby cell monolayers were completely
208
destroyed, the optical density (OD) of the wells was read in a multichannel spectrophotometer
209
(Packard Spectra Count , USA) at 540 nm. The OD was directly related to the percentages of viable
TM
8 Page 8 of 39
cells that were inversely proportional to the cytophathogenecity effect (CPE) ratio. The straight line of
211
the regression was determined for each assay and for each plate on the basis of cell controls (0%
212
CPE) and virus controls (100% CPE) [34]. The 50% cytotoxic concentration (CC50) of the test
213
compound was defined as the concentration that reduced the absorbance of mock-infected cells to
214
50% of that of controls. The 50% antiviral effective concentration (EC50) was expressed as the
215
concentration that achieved a 50% protection of virus-infected cells from the HSV-induced destruction.
216
The following formula was used to calculate the percentage protection:
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210
217 218
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[ (ODt) HSV - (ODc) HSV ] / [ (ODc) MOCK - (ODc) HSV ] x 100 (%)
219
Where (ODt) HSV is the absorbance of the test sample, (ODc) HSV is the absorbance of the virus-
221
infected control (no compound), and (ODc) MOCK is the absorbance of the mock-infected control. The
222
ratio of (ODc) HSV to (ODc) MOCK is expressed as “% of control“. For all tests, the anti-herpetic
223
compound acyclovir [9-(2-hydroxyethoxymethyl) guanine] (Wellcome Foundation Ltd, U.K.) was used
224
as a reference.
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Antiviral activities and kinetics of the efficient extracts
227
The freeze-dried extracts were tested at 10 different concentrations ranging from 0.25 to 250.00
te
226
µg/mL (4 wells/concentration) at an MOI of 0.01 ID50/cells. Cytotoxicity and antiviral activity of extracts
229
were evaluated by neutral red dye method after 48, 72, and 96 h of treatment.
230
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231
Antiviral bioguided fractionation by molecular mass fractionation
232
After fractionation of the most efficient extract with six different membranes (2 kDa, 5 kDa, 10 kDa,
233
30 kDa, 50 kDa and 100 kDa), the freeze-dried extracts were tested at 10 different concentrations
234
ranging from 0.25 to 250.00 µg/mL (4 wells/concentration) at an MOI of 0.01 ID50/cells after 72 h of
235
treatment.
236 237 238 239
2.5 Analysis of the biochemical compositions of the efficient extracts Analysis of biochemical compositions of the efficient extracts and the control were performed. Compositions of freeze-dried samples were determined as described below. Proteins, humidity, and
9 Page 9 of 39
240
ash were determined in accordance with Association of Official Analysts Chemists (A.O.A.C.) official
241
methods, 981.10, 952.08, and 938.08 respectively. Fats were determined according to the Folch
242
method [35] and neutral sugars according to the Dubois method [36].
243
The total free amino acid composition of freeze-dried hydrolysates and the control was determined after hydrolysis in 6 M HCl at 118°C for 18 h. Then, the samples were completely dried
245
under nitrogen atmosphere and diluted by adding 2.5 mL of water. The amino acid analysis was
246
performed according to the EZ faast™ (Phenomenex, France) procedure consisting of a solid phase
247
extraction step followed by derivatization and liquid/liquid extraction. The solid phase extraction was
248
performed via a sorbent packed tip that binds amino acids while allowing interfering compounds to
249
flow through. Amino acids on sorbent were then extracted into the sample and quickly transformed
250
with a reagent at room temperature in an aqueous solution. Derivatized amino acids concomitantly
251
migrated to the organic layer for additional separation from interfering compounds. An aliquot from the
252
organic phase was then analyzed on a GC-MS system. The mass spectrometer was an Agilent 5973
253
series network mass selective detector (Agilent, CA, U.S.A.). The column was a Zebron ZB-AAA GC
254
column (Phenomenex, France) for protein hydrolysates (max. temp. 320/340°C). The amino acids
255
were quantified by their response factor relative to the internal standard Norvaline added at a
256
concentration of 200 μmol/L [37].
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2.6 Molecular mass fractionation
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Molecular mass fractionation was prepared with ultrapure water at 1 mg/mL then fractionated
260
using centrifugal concentrators (Vivaspin 2, Sartorius, France) at different Molecular Weight Cut-Off
261
(MWCO). Centrifugations were carried out for 10 min at 12000 g for 2 kDa, 5 kDa, 10 kDa, 30 kDa and
262
50 kDa PES (Polyethersulfone) membranes and 9000 g for 100 kDa PES membrane. Seven samples
263
were obtained (<2 kDa, 2-5 kDa, 5-10 kDa, 10-30 kDa, 30-50 kDa, 50-100 kDa, >100 kDa) and freeze-
264
dried.
265 266
3. RESULTS AND DISCUSSION The dissection step showed that byproducts represented around 50% of the fresh weight of
267
the whole sea cucumber. The major parts were internal organs (15 ±3% of the fresh weight) and the
268
aquapharyngeal bulb (13 ±2% of the fresh weight)
10 Page 10 of 39
The hydrolysis parameters (ratio enzyme/substrate; pH and temperature) have been selected
270
as the mean of the optimal conditions declared by the manufacturers for all enzymes. Concerning the
271
time of hydrolysis, previous studies showed that the degree of hydrolysis (DH) of Alcalase, Bromelain,
272
Flavourzyme, Protamex, reached a threshold value after 6 h. Therefore, this time value was selected
273
for all enzyme assisted extraction experiments [14; 37-38].
274
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3.1 Evaluation of antiviral activities of the library of extracts by cell viability
276
3.1.1
277
Before evaluation of antiviral activity, cytotoxicity of extracts on Vero cells was studied using the
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Evaluation of cytotoxicity
neutral red incorporation in the aim to detect lysosomal functionality. This method is currently used for
279
the screening of anti-HSV-1 molecules from marine organisms [28; 39-40]. An antiviral drug should be
280
active against the virus without inducing significant toxicity on the host cell. Therefore, the
281
concentration range of the extract that did not induce significant toxicity to the host cells was estimated
282
and the 50% cytotoxic concentration (CC50) was determined for each one.
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Most of the extracts from aquapharyngeal bulb (A.B.) were well tolerated by Vero cells and their CC50 varied in the range of 74.5 and up to more than 500 µg/mL. Only two extracts obtained by
285
solvent extraction were cytotoxic (hexane extract with a CC50 = 81.5 µg/mL and methanol extract with
286
a CC50 = 74.5 µg/mL). None of the hydrolysates evaluated in our conditions induced visible changes in
287
cell morphology and cell density.
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The CC50 of the extracts from internal organs (I.O.) varied in the range of 23.3 and up to more
289
than 500 µg/mL. Half of them were cytotoxic in the concentrations tested. The evaluation of
290
cytotoxicity of solvent extracts showed that extracts obtained by highly polar solvent extraction were
291
toxic (methanol extract with a CC50 = 56.7 µg/mL and water extract with a CC50 = 96.3 µg/mL). The
292
majority of the enzymatic hydrolysates were also cytotoxic.
293
The cytotoxic extracts found in the A.B. and especially in I.O. could be explained by the presence
294
of triterpene glycosides [41]. Indeed, these molecules, essentially extracted by alcoholic solvent, have
295
already been described in holothurians species and demonstrated as cytotoxic agents. As an
296
example, the major triterpene glycoside Frondoside A, isolated by solvent extraction from the bodywall
297
of C. frondosa, showed cytotoxicity on THP-1 and HeLa tumor cell lines with IC50 values of 4.5 and
11 Page 11 of 39
298
2.1 μg/mL, respectively [42-43]. Furthermore, a recent study demonstrated the richness of triterpene
299
glycosides in holothurian internal organs [44].
300 301
3.1.2
302
Evaluation of antiviral activity against HSV-1 was examined using CPE inhibitory assay. The
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Evaluation of antiviral activity
reference standard ACV conferred protection (EC50 = 0.2 µg/ml) against HSV-1 with a low percentage
304
of cell destruction. All 28 samples from the library of extracts were evaluated for their antiviral activity
305
at an MOI of 0.001 ID50/cells by cell viability. Results are summarized in Table 1. After 72 h of
306
treatment, seven of nine hydrolysates of the aquapharyngeal exhibited antiherpetic activities with EC50
307
between 7.2 and 170.9 µg/mL. Only the water extract of the aquapharyngeal bulb of C. frondosa
308
demonstrated an antiherpetic activity with an EC50 of 140 µg/mL and the aquapharyngeal bulb without
309
treatment (control) showed an activity (EC50: 75.0 µg/mL). Among the extracts from internal organs,
310
only the control extract showed an antiviral activity (EC50 = 72.5 µg/mL).
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Of 28 extracts evaluated, 10 extracts exhibited antiherpetic activities. The extracts from the
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311
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303
aquapharyngeal bulb showed better antiviral activities in comparison to internal organs extracts. This
313
screening also demonstrated that antiviral compounds seemed to be highly polar. Indeed only the
314
water extract and hydrolysates of the aquapharyngeal bulb possessed antiviral activities without
315
cytotoxicity. In a review, Zhong et al. [31] showed that of 188 plant, animal, or microorganism extracts,
316
162 (86.2%) with inhibitory activity against HSV have been obtained from highly polar solvents such as
317
aqueous solvents, methanol, ethanol, and acetic acid. It appears that most anti-HSV molecules are
318
soluble in polar solvents, including polyphenols and flavones with multiple hydroxyl groups, and this
319
solubility correlates with the reported compound types that have anti-HSV activity. Consequently, it
320
seems relevant to focus on aqueous fractions for the search of antiherpetic compounds. For example,
321
the use of enzymatic hydrolysis with proteases in highly controlled conditions permits the release of
322
bioactive peptides, even though they were inactive when included in the amino sequence of the parent
323
protein [45].
324
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Little is known about antiviral activities from holothurians. Tsushima et al. [23] showed that
325
cucumariaxanthin C from Cucumaria japonica exhibited an inhibitory effect on Epstein-Barr virus
326
(Herpesviridae) activation in a short-term in vitro assay. On the same species, Grishin et al. [24]
327
demonstrated that triterpene glycosides, and especially cucumarioside A2-2, can inhibit the cytopathic
12 Page 12 of 39
effect induced by Vesicular Stomatitis Virus (VSV), Poliovirus, and other viruses in cell culture.
329
According to Rodriguez et al. [25], holothurinosides from Holothuria forskalii can also inhibit the
330
cytopathic effect induced by VSV. Recently, it has been shown that glycosaminoglycan extracted from
331
Thelenota ananas may possess great potential to be further developed as a new Human
332
Immunodeficiency Virus (HIV) entry inhibitor [26-27].
333
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Liouvillosides A and B extracted from a whole specimen of Staurocucumis liouvilei [28],
thyonosides A and B from Thyone aurea [29], and a water extract of the body wall of Holothuria sp.
335
[30], have been shown to possess antiviral activities against Herpes simplex virus type 1. In particular,
336
triterpene glycosides from Staurocucumis liouvilei showed a virucidal effect at concentrations below 10
337
µg/mL, and the water extract of Holothuria sp. exhibited an intracellular antiviral activity with an IC50
338
value of 189.9 µg/mL.
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In comparison to solvent extraction, enzymatic hydrolysis recovers antiherpetic compounds from
340
the aquapharyngeal bulb. Moreover, this process is a softer technique without the solvent elimination
341
step and can allow a valorization of the entire raw matter, which is useful in a global context of marine
342
biological resources overexploitation [3-4; 46]. The most efficient extracts selected were obtained by
343
using four different proteases which have a common mechanism of action. Indeed, these enzymes
344
have endopeptidase activities resulting mainly in the production of polypeptides or proteins, compared
345
to exopeptidases which mainly promote the production of free amino acids.
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339
347
3.2 Biochemical composition of the effective extracts
348
The most effective extracts were selected according to EC50 values. In that way, four hydrolysates
349
from the aquapharyngeal bulb byproducts were chosen to continue the study: Papain hydrolysate
350
(EC50 = 7.2 µg/mL), Protamex hydrolysate (EC50 = 8.3 µg/mL), Neutral Protease hydrolysate (EC50 =
351
12.5 µg/mL) and Alcalase hydrolysate (EC50 = 15.2 µg/mL).
352
Analysis of the biochemical composition was carried out on the four aquapharyngeal bulb
353
hydrolysates and on the control (aquapharyngeal bulb without treatment). Results are presented in
354
Table 2. Results showed no significant differences between the extracts, except for the control.
355
Indeed, a small decrease of the lipid content and increase of the protein content were observed.
356
Compositions of the extracts showed a high protein content with an average of 54.9% (dry weight).
357
These results are in accordance with the previous study of Mamelona et al. [47] on hydrolysis of the
13 Page 13 of 39
358
viscera of the same animal with an average of 55%. Other studies also report that enzymatic
359
hydrolysis does not significantly change the protein percentage, but rather liberates small peptides
360
[48].
361
Total amino acids assays showed no significant differences between the four hydrolysates selected. The mean amino acid profile is presented in three groups of amino acids according to their
363
abundance. Values are expressed as a percentage of the total amino acids assayed: inferior to 4%:
364
Histidine (1.5%), Methionine (1.5%), Phenylalanine (3.5%), Lysine (2.3%), Hydroxyproline (3.5%), and
365
Tyrosine (2.0%); between 4 and 8%: Alanine (7.8%), Threonine (6.2%), Valine (5.1%), Isoleucine
366
(4.7%), Leucine (6.1%), and Serine (7.5%); superior to 8%: Aspartic acid (10.7%), Glutamic acid
367
(12.4%), Glycine (16.5%), and Proline (8.6%). These values are in accordance with the previous study
368
of Zhong et al. [49] on a biochemical comparison of the body wall of C. frondosa with or without
369
internal organs, on fresh or rehydrated matter, where major amino acids were the same as those
370
found in the extracts evaluated in our study. However, the total amino acid profile of the control was
371
slightly different. Indeed, the control was enriched in Leucine (8.2%), Phenylalanine (5.0%), Glycine
372
(25.8%) and Alanine (10.4%) but depleted in Aspartic acid (5.1%), Glutamic acid (5.7%) and Serine
373
(5.5%). In our conditions, the enzymatic hydrolysis process with proteases seems to recover amino
374
acids with acidic side chains and strongly loses the neutral amino acid Glycine.
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362
Lipid contents (average of 6.6%) are similar between hydrolysates, but twice as high as the
376
control. This difference can be explained by the ability of the enzymatic hydrolysis process to release
377
lipids in the soluble part. Dumay et al. [50] demonstrated on sardine byproducts that enzymatic
378
proteolysis can be used for high lipid recovery.
379
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375
Ash contents are similar with an average of 25.6%. Available data on the ash content of the
380
holothurian aquapharyngeal bulb are quite rare. Results found for C. frondosa are higher than the data
381
found for the viscera content of the same species (7-11%: [47]) and lower than the data found for the
382
body walls of other shallow-water holothuroids with an average of 52% [51]. These variations in ash
383
content can be explained by the structure of their internal anatomy, which is more or less rich in calcite
384
depending on the part of the animal considered [52].
385
Neutral sugar contents are around 1.8% for Alcalase, Papain and Protamex hydrolysates and are
386
similar for those found on the viscera of other shallow-water sea cucumbers [51] but slightly higher for
387
Neutral Protease hydrolysate with 3.1%.
14 Page 14 of 39
388
Studies on natural products with anti-HSV activities reported that most of these compounds targeted the viral attachment and the entry stage. The other major mechanism of action reported was
390
the DNA replication by inhibition of the HSV-encoded DNA polymerase. This latter is the mechanism
391
of action used by the anti-HSV-1 reference drug, acyclovir (ACV). The other mechanisms of action
392
described in natural compounds with antiviral activities target the inhibition of the virion assembly and
393
output, the cellular proteins and the promotion of the immune response [22].
ip t
389
The four selected hydrolysates showed a high protein content. Marine peptides and nucleosides
395
have already shown antiherpetic activities by inhibiting the viral protein synthesis of HSV-1 [53]. The
396
nucleoside spongouridine was used for the synthesis of the marine adenine arabinoside which is
397
rapidly converted into its triphosphate form, leading to the inhibition of the viral DNA polymerase and
398
DNA synthesis of HSV in infected cells [54]. Besides the antiviral activities of these compounds, other
399
chemical classes have also shown such activity. Fucosylated chondroitin sulfate (FuCS) found in sea
400
cucumbers from different species has revealed interesting bioactivities. Among these activities, FuCS
401
extracted from the holothurian T. ananas has shown highly effective antiviral activity against HIV
402
strains. FuCS showed a capacity to block the virus entry and replication on cell models and clinic
403
isolates [10].
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Sulfated polysaccharides are known to be active on HSV. These compounds are able to inhibit
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404
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394
viral infection by preventing adsorption of the virus into the host cells and/or by inhibiting the
406
production of new viral particles inside the host cells [55]. Natural carrageenans were identified as
407
potent and selective inhibitors of HSV-1 and HSV-2. Studies suggested that the main target for
408
antiviral action of the carrageenans was based on the virus adsorption, whereas no effect on virus
409
internalization or early or later protein synthesis was detected [56]. Alkaloids showed potent anti-HSV-
410
1 activity by impairing the virus penetration and inhibiting immediate early protein synthesis [57].
411
Glycolipids showed antiviral activity against HSV-1 and HSV-2 [58]. The antiviral action might be due
412
to the binding of the virus glycoprotein to the glycolipid leading to an irreversible denaturation that
413
blocks viral infection [59].
414
Ac ce p
405
Many marine compounds of different chemical classes with a broad range of mechanism of action
415
have been described as effective anti-HSV-1 agents. However, according to the biochemical
416
composition of the selected extracts and the differences in activity values modulated by the nature of
417
the enzymes used, the results suggested that the antiviral compounds might be from protein origin.
15 Page 15 of 39
418 419
3.3 Antiviral activities and kinetics of the effective extracts from aquapharyngeal bulb byproducts
420 421
After 48, 72, and 96 h of treatment, viability assay showed no cytotoxic effect of the compounds on Vero cells in the range of concentrations assayed for all four compounds.
422
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The four hydrolysates showed anti-HSV-1 activities for an MOI of 0.01 ID50/cells. Results are summarized in Table 3 in comparison with the reference drug (ACV). After 48 h of incubation, the four
424
extracts exhibited an important antiviral activity: Papain hydrolysate (EC50 = 15.9 µg/mL) > Alcalase
425
hydrolysate (EC50 = 20.4 µg/mL) > Neutral protease hydrolysate (EC50 = 26.9 µg/mL) > Protamex
426
hydrolysate (EC50 = 52.2 µg/mL). After 72 h of incubation, the four extracts still showed an important
427
activity: Papain hydrolysate (EC50 = 25.2 µg/mL) > Neutral protease hydrolysate (EC50 = 36.9 µg/mL) >
428
Alcalase hydrolysate (EC50 = 43.9 µg/mL) > Protamex hydrolysate (EC50 = 102.9 µg/mL). After 96 h of
429
incubation, three of four hydrolysates remained active against HSV-1: Papain hydrolysate (EC50 =
430
44.3 µg/mL) > Protamex hydrolysate (EC50 = 144.9 µg/mL) > Alcalase hydrolysate (EC50 = 150.4
431
µg/mL).
us
an
M
432
cr
423
Extracts seemed to act differently depending on the time of incubation, and the evolution of activities did not follow the same trend. This is well illustrated with a neutral protease hydrolysate
434
activity that, during 48 and 72 h of incubation, possessed interesting antiviral activities but completely
435
lost its activity after 96 h. Antiherpetic compounds from the extracts assayed seemed to act on early
436
cycles of replication but after 96 h faced obstacles with the release of newly formed virions [60].
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d
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Results showed that Protamex hydrolysate was the second most efficient extract (EC50 = 8.3
438
µg/mL) at an MOI of 0.001 ID50/cells after 72 h of incubation. At an MOI of 0.01 ID50/cells, it became
439
less active (EC50 = 102.9 µg/mL) with the same concentrations assayed after the same period of
440
incubation. This observation can be explained by the fact that continuous replication of every virus
441
particle will produce an aggressive virus population. A culture infected with high virus multiplicity may
442
therefore need higher concentrations of antiviral compounds for viral inhibition than cells infected with
443
low multiplicity [61].
444
Among all these observations, the Papain hydrolysate remained the more active extract.
445
According to the specificities of each enzyme, a trend seemed to be emerging. Byproducts hydrolysed
446
with Alcalase and mostly with Papain possessed the highest antiviral activities. Papain, and Alcalase
16 Page 16 of 39
447
at a lower rate, have broad specificities to cleave peptide bonds but preferences for amino acids
448
bearing a large hydrophobic side chain compared to Neutral Protease and Protamex enzymes.
449
Ghanbari et al. [14] showed an antibacterial activity of enzymatic hydrolysates from the sea cucumber Actinopyga lecanora. The antibacterial activity was not only correlated to the size, the
451
molecular weight and the degree of hydrolysis, but also on the hydrophobicity of the resulting
452
peptides. Furthermore, Papain hydrolysates have already shown to possess activities such as
453
antioxidant activities [62] and ACE inhibition [63]
cr
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450
454
On the same raw matter, the process of enzymatic hydrolysis with proteases induced different extracts with different activities against HSV-1; therefore, the nature of the enzyme used seems to be
456
a major parameter to modify the antiviral activity. The enzyme specificity is important to peptide
457
functionality because it strongly influences the molecular size and hydrophobicity of the hydrolysate
458
[3].
an
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459
461
3.4 Antiviral activity by bioguided molecular mass fractionation
M
460
After 72 h of treatment, a viability assay showing no cytotoxic effect of the compounds was observed on the Vero cells in the range of concentrations assayed for all seven compounds. Results
463
are presented in Table 4. Out of seven extracts tested, three extracts showed an effective antiviral
464
activity with EC50 of 55.1, 38.1, and 18.2 µg/mL at an MOI of 0.01 ID50/cells for the fractions 30-50
465
kDa, 50-100 kDa and superior to 100 kDa respectively. Other extracts were not active against HSV-1
466
in the range of concentrations tested. Active molecules were present on the last fractions, and activity
467
increased with the size of the cutoff from 30 kDa to over 100 kDa. It is assumed that the compounds
468
responsible for the antiherpetic activity are in an aqueous phase superior to 100 kDa due to the
469
highest activity found for the last fraction. High molecular weight compounds have already been
470
demonstrated as antiherpetic agents [64]. Indeed, sulfated polysaccharides isolated from two red
471
algae with an average molecular weight of 308 and 360 kDa were shown to exert in vitro anti-HSV-1
472
activity. They were capable of inhibiting the in vitro replication of HSV-1 on Vero cells with EC50 values
473
of 4.1 and 17.2 μg/mL [64]. These values have been obtained after an evaluation of 48 h at an MOI of
474
0.001 ID50/cells, ten times lower than the MOI used in the antiviral evaluation by bioguided molecular
475
mass fractionation (0.01 ID50/cells after an evaluation of 72 h). Recently, sulfated polysaccharides
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17 Page 17 of 39
476
isolated from the bodywall of C. frondosa showed biological effects. Indeed, they have demonstrated
477
in vitro the ability to act on the maturation of dendritic cells [11].
478
Generally, due to the poor permeability through membranes, molecular size, physical and chemical instability affect the bioavailability of peptides and more specifically proteins. In vivo, peptides
480
with two or six amino acids reach their target site more easily than a whole protein. However, some
481
marine proteins showed biological activities in animal models. Lectins are carbohydrate-binding
482
proteins found in a wide range of organisms even in holothurians. Bulgakov et al. [65] described a 44-
483
kDa, C-type mannan-binding lectin consisting of two identical subunits isolated from the coelomic fluid
484
of the holothurian Cucumaria japonica. A 400 kDa lectin named SPL-1 and a 68 kDa lectin named
485
SPL-2 were extracted from the holothurian species Stichopus (Apostichopus) japonicus. Inhibition of
486
HSV infections was demonstrated with lectins from plants which are able to recognize and bind to
487
polysaccharides or glycoproteins on cell surface in order to agglomerate the cells. The presence of
488
lectins in holothurians species, the wide range of molecular mass described and their bioactivities
489
might be a possible explanation for the antiviral compounds found in our study. Furthermore, the
490
presence of oligomers with different subunit sizes could also explain the antiviral activities of the two
491
fractions lower than 100 kDa. Glycosylation is essential to the virus for its cellular transport and
492
binding to cellular receptors, in this way, by binding to the glycosylated viral-envelope, lectins could act
493
as entry blockers.
cr
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d
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Protein hydrolysates have been investigated as an alternative for the upgrading of marine
Ac ce p
494
ip t
479
495
byproducts to deal with the significant quantities of waste generated annually by the processing
496
industries [66]. These hydrolysates have broadly contributed to the discovery of new compounds with
497
activities that include the following: antioxidative, anticancer, calcium-binding peptides, appetite
498
suppression, anticoagulant, immunostimulant, hypocholesterolemic, hormone-regulating, and
499
antimicrobial and antiviral [38]. In our study, the aqueous fraction obtained by enzymatic proteolysis
500
from Cucumaria frondosa seems to be a promising extract for the search of active compounds against
501
Herpes Simplex virus.
502 503
In conclusion, this study confirms that, in comparison to solvent extraction, the enzymatic
504
extraction appears to be a promising softer technique for the recovery of industrially important
505
metabolites as antiviral compounds in a time-saving fashion, with less solvent and at lower cost. The
18 Page 18 of 39
specificity of enzymes used was also shown with different levels of response for the activity evaluated.
507
The aquapharyngeal bulb, for a long time considered as a byproduct with low value added, represents
508
a non-negligible part of the animal in terms of proportion but also mainly for its biochemical
509
composition. To our knowledge, no studies have demonstrated the presence of active molecules
510
against HSV-1 from C. frondosa byproducts. The results obtained in this study make the high
511
molecular weight extract from the Papain hydrolysate of the aquapharyngeal bulb from the sea
512
cucumber Cucumaria frondosa a great potential source of antiviral agent against Herpes Simplex virus
513
1. Literature suggested that lectins might be a possible explanation for the nature of the antiviral
514
compounds retrieved in the high molecular weight extract with a potential mechanism of action as
515
entry blockers. This extract could provide high added value to an underestimated biomass with the
516
added bonus of being environmentally friendly through the use of enzymes instead of solvents. These
517
compounds are currently undergoing purification in order to identify the active molecules as well as
518
their mechanism of action.
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ACKNOWLEDGMENTS This research was supported by the Atlantic Canada Opportunities Agency (Atlantic Innovation
te
521
Fund grant 193594). The authors thank Dr J.P. Bergé and C. Donnay-Moreno from the laboratory
524
BIORAFhe, IFREMER, Nantes, FRANCE for the amino acids analysis.
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19 Page 19 of 39
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30 Page 30 of 39
779
Table 1 : Evaluation of anti-HSV activity at an MOI of 0.001 ID50/cells on Vero cell line of the
780
byproducts library of extracts from C. frondosa, by neutral red dye method after 72 h of incubation.
781
Acyclovir (ACV) was used as a reference drug. Treatment
Reagent
CC50 (µg/mL)
Aquapharyngeal bulb
None
None
>500
Enzymatic hydrolysis
Alcalase
>500
Bromelain
>500
cr
>250 160.5 ±8.7
>500
>250
>500
12.5 ±3.1
Papain
>500
7.2 ±1.9
Peptidase AM
>500
45.3 ±5.1
Peptidase AO
>500
170.9 ±7.5
Protamex
>500
8.3 ±2.7
Acetone
>500
>250
Hexane
81.5 ±3.8
7.9 ±3.4
Methanol
74.5 ±4.5
70.9 ±7.4
Water extract
>250
140.0 ±13.8
None
None
>250
72.5 ±9.8
Enzymatic hydrolysis
Alcalase
>500
>250
Bromelain
40.4 ±3.0
60.0 ±3.2
Flavourzyme
>500
>250
Fungal protease
29.0 ±3.0
10.4 ±1.5
Neutral protease
23.3 ±3.1
14.0 ±4.0
Papain
69.6 ±2.8
11.0 ±9.1
Peptidase AM
>500
>250
d
M
Neutral protease
Ac ce p
te
Solvent extraction
Internal organs
15.2 ±2.5
>500
an
Fungal protease
75.0 ±2.1
us
Flavourzyme
EC50 (µg/mL)
ip t
Organ
31 Page 31 of 39
ACV
None
7.8 ±9.5
Protamex
>500
>250
Acetone
>500
>250
Hexane
>500
>250
Methanol
56.7 ±5.8
Water extract
96.3 ±7.3
None
>500
7.9 ±1.8
33.2 ±4.8
0.2 ±0.1
us
Data are shown as mean ± S.D. (n=4).
ip t
74.9 ±4.8
cr
Solvent extraction
Peptidase AO
an
MOI: multiplicity of infection: ratio (virus titer)/(cells number/mL). CC50: the 50% cytotoxic concentration: concentration that reduced the absorbance of mock-infected cells to 50% of that of controls. EC50: the 50% antiviral effective concentration: concentration that achieved 50% protection of virus-infected cells from the HSV-induced destruction
Ac ce p
te
d
M
782 783
32 Page 32 of 39
Table 2: Proximate analysis on freeze-dried aquapharyngeal bulb of C. frondosa hydrolysates and without hydrolysis as a control group; n.d.: Not determined Control
Alcalase hydrolysate
Neutral Protease hydrolysate
Papain hydrolysate
Protamex hydrolysate
Crude protein (%)
58.8
54.5
54.7
55.4
54.9
Humidity (%)
6.5
5.8
5.9
4.7
Ash (%)
23.2
26.2
25.1
26.0
Fats (%)
2.8
6.3
6.5
Neutral sugars (%)
n.d.
1.8
3.1
ip t
Analysis
us
cr
4.3
27.6
7.0
6.4
1.9
1.7
an
783 784 785
786
Ac ce p
te
d
M
787
33 Page 33 of 39
787 Table 3 : Evaluation of anti-HSV activity at an MOI of 0.01 ID50/cells on Vero cell line of the most promising extracts from aquapharyngeal bulb of C. frondosa hydrolysed with: Alcalase (1), Neutral protease (2), Papain (3) and Protamex (4) by neutral red dye method at 48, 72 and 96 h of incubation. Acyclovir (ACV) was used as a reference drug. 96 h
EC50 (µg/mL)
CC50 (µg/mL)
EC50 (µg/mL)
CC50 (µg/mL)
EC50 (µg/mL)
1
>500.0
20.4 ±3.2
>500.0
43.9 ±5.2
>500.0
150.4 ±8.2
2
>500.0
26.9 ±4.4
>500.0
36.9 ±0.5
3
>500.0
15.9 ±2.2
>500.0
25.2 ±4.8
>500.0
44.3 ±3.2
4
>500.0
52.2 ±5.8
>500.0
102.9 ±8.7
>500.0
144.9 ±7.3
0.3 ±0.1
>500.0
0.3 ±0.1
>500.0
1.1 ±0.3
us
>500.0
>500
Ac ce p
te
d
794
an
Data are shown as mean ± S.D. (n=4).
cr
CC50 (µg/mL)
ACV >500.0 792 793
72 h
ip t
48 h
M
788 789 790 791
34 Page 34 of 39
794
801
< 2 kDa
>500.0
>500.0
2-5 kDa
>500.0
>500.0
5-10 kDa
>500.0
>500.0
10-30 kDa
>500.0
>500.0
30-50 KDa
>500.0
50-100 KDa
>500.0
us
> 100 kDa
>500.0
ACV
>500.0
cr
55.1 ±7.2 38.1 ±5.2
an
M
Data are shown as mean ± S.D. (n=4).
ip t
EC50 (µg/mL)
18.2 ±3.6 0.3 ±0.1
d
800
CC50 (µg/mL)
te
798 799
Table 4 : Evaluation of anti-HSV activity at an MOI of 0.01 ID50/cells on Vero cell line by molecular mass fractionation of aquapharyngeal bulb of C. frondosa hydrolysed with Papain after 72 h of incubation, by neutral red dye method. Acyclovir (ACV) was used as a reference drug.
Ac ce p
795 796 797
35 Page 35 of 39
801
Figure 1: Summary of the enzymatic hydrolysis process for the preparation of byproducts
802
hydrolysates from Cucumaria frondosa (A.B.: Aquapharyngeal Bulb and I.O.: Internal Organs); rpm:
803
rotation per minute.
804
806
Figure 2: Summary of the sequential solvent extraction of the freeze-dried byproducts of
ip t
805
Cucumaria frondosa (A.B.: Aquapharyngeal Bulb and I.O.: Internal Organs; RT: Room Temperature.
cr
807
Ac ce p
te
d
M
an
us
808
36 Page 36 of 39
Ac ce p
te
d
M
an
us
cr
ip t
Figure1
Page 37 of 39
Ac ce p
te
d
M
an
us
cr
ip t
Figure2
Page 38 of 39
cr M
an
us
*Graphical Abstract
L.TRIPOTEAU L.TRIPOTEAU
Extraction of the byproducts
L.TRIPOTEAU
ed
Enzymatic hydrolysis Enzymatic and Solvent extraction hydrolysis (variation of proteases nature, pH, temperature, time)
ce
pt
Collection of specimens
Ac
Identification of a potent antiherpetic extract : - > 100 kDa
- Papain hydrolysate - Aquapharyngeal bulb
Selection
Molecular mass fractionation
Antiviral and cytotoxic evaluation of the fractions
Antiviral and cytotoxic evaluation of the selected extracts
Page 39 of 39
Antiviral and cytotoxic evaluation of the library of extracts