• 专利附录
  • 专利说明
  • 权利要求
  • 类似技术
  • 同族专利
  • 引用文献
  • 法律状态
  • 优先权
    • 专利摘要:
    Process for the preparation of a liquid extract rich in phycocyanin from cyanobacteria or micro-algae containing phycocyanin, comprising a step of cell lysis of an aqueous suspension of said cyanobacteria or fresh micro-algae, a step of maceration of the lysate obtained for several hours in a solution of divalent cations, releasing the water-soluble molecules in the extracellular space and one or more steps of clarification and concentration of the suspension to isolate the water-soluble molecules, including phycocyanin. This process is carried out at a pH of between 5 and 8.5 at room temperature without drying. 99% of the phycocyanin of the starting biomass is recovered. The aqueous extract obtained is stable over time and comprises an undenatured phycocyanin content which may be greater than 0.5 g / L, exhibiting an antioxidant activity demonstrated in vivo.
    公开号:FR3064269A1
    申请号:FR1752452
    申请日:2017-03-24
    公开日:2018-09-28
    发明作者:Sebastien Jubeau;Jeremy Pruvost;Pascal JAOUEN;Jean Jenck;Olivier Lepine
    申请人:ALGOSOURCE;
    IPC主号:
    专利说明:

    FIELD OF THE INVENTION
    The present invention relates to the field of methods for extracting cyanobacteria or microalgae with a view to obtaining biologically active compounds, more particularly for obtaining extracts rich in phycocyanin.
    PRIOR ART Numerous methods have been developed in recent years to extract different types of cyanobacteria molecules, one of the most well-known and used of which is spirulina.
    Spirulina is rich in essential amino acids and proteins (almost 50% by mass), in iron, and also in carbohydrates and lipids (gammalinoleic acid) and in carotenoids (beta-carotene). It also contains many vitamins, in particular vitamins B1, B2, B6, B9, B12, and E, as well as mineral trace elements (calcium, magnesium, zinc, potassium ...). The interest in extracting these molecules is growing for uses in the food, cosmetic and / or therapeutic fields.
    Among proteins, phycobiliproteins are pigments that capture light energy. The main pigment in spirulina, phycocyanin, is an intense blue. Phycobiliproteins also include allophycocyanin and phycoerythrin
    In the following text, by phycocyanin is meant phycobiliproteins, in particular phycocyanin.
    There are many methods of extracting phycocyanin from spirulina. However, most of these methods use as starting material dried spirulina (CN 101560254) and / or possibly crushed (FR 2789389), or else, if the extraction is carried out from fresh spirulina, the methods include a step of drying or freeze drying. However it turns out that in the dry state spirulina, and therefore phycocyanin, are altered and their bioactive properties are degraded.
    PURPOSE OF THE INVENTION
    A first object of the invention is therefore to propose a process for extracting phycocyanin from fresh cyanobacteria, such as fresh spirulina or from microalgae, and which does not include any step in which the product is found in the dry state.
    Certain extraction methods use organic solvents for the extraction of phycocyanin, such as polyethylene glycol or glycerin (WO 2016/030643). These compounds are then found, at least in trace amounts, in the final product. Since phycocyanin is intended for food and / or medical use, it is desirable not to use such methods involving organic solvents. As a variant, the process must use very expensive purification steps (chromatography for example).
    Another object of the present invention is therefore to propose a process for the preparation of a phycocyanin extract which does not involve organic solvents, nor expensive purification steps.
    Document FR 2453199 discloses a phycocyanin extraction process using fresh cyanobacteria, but using large amounts of calcium salts CaCl 2, carbonates and alumina sulfate and leading, after lyophilization, to obtaining a blue powder, which can be kept and stored.
    Another object of the present invention is to provide a preparation process which limits the addition of salts, and makes it possible to obtain a phycocyanin extract in liquid form, an extract which is stable over time, without requiring lyophilization or drying. final.
    SUMMARY OF THE INVENTION
    To this end, the present invention provides a process for the preparation of a liquid extract of phycobiliproteins, and in particular phycocyanin, from cyanobacteria or micro-algae containing phycocyanin, comprising the following successive steps:
    - i) a cell lysis step, by a physical or mechanical method, of an aqueous suspension of said cyanobacteria or fresh micro-algae,
    ii) a step of maceration of the lysate obtained in step i) in a solution of divalent cations, preferably cations of alkaline earth metals, with a view to releasing the water-soluble molecules in the extra cellular space of cyanobacteria or micro-algae,
    - iii) one or more stages of clarification and concentration of the suspension to isolate the water-soluble molecules, including phycocyanin, the whole of this process being carried out at a pH between 5 and 8.5, without drying and at a temperature less than or equal to 25 ° C allowing phycocyanin to retain its spatial structure, thus preserving its biological properties and giving it better bioavailability.
    The extract obtained is therefore an aqueous extract, without any trace of organic solvent, since no stage of said process of the invention involves the introduction of such molecules with a view to the extraction of phycocyanin.
    The method according to the invention does not include a drying step, which allows the phycocyanin not to be denatured and to retain its spatial structure, thus preserving its biological properties and giving it better bioavailability.
    Preferably, the destructuring or cell lysis step comprises a freeze-thaw phase.
    The freeze-thaw phase allows in particular the weakening of cell walls and membranes, in order to then facilitate the extraction of intracellular metabolites. Advantageously, the freezing-thawing phase comprises freezing and preserving the cyanobacteria or micro-algae frozen at a temperature below -18 ° C, preferably below -20 ° C, more preferably below -24 ° C for from one day to one year, preferably from two weeks to six months; this freezing is followed by a slow thawing step at a temperature above 0 ° C, and preferably below 5 ° C, for several hours.
    The maceration step of the lysate obtained in step i) is preferably carried out with stirring of said thermostatically controlled suspension at a temperature between 10 ° C and 25 ° C for several hours: advantageously for at least 3 hours, preferably for at least at least 4 hours, more preferably for at least 6 hours.
    The clarification step is advantageously carried out by centrifugation, then recovery of the supernatant solution. The purpose of this clarification is to reduce a large part of the particulate fraction present in the suspension obtained in step ii). These particles are essentially cellular debris (walls, membranes) and poorly or not water-soluble metabolites (lipids, hydrophobic proteins, etc.). It has been found that the presence of CaCb greatly favors the settling of the particles by increasing their sedimentation rate during centrifugation.
    Advantageously, the supernatant solution resulting from the centrifugation step is subjected to a microfiltration step, preferably a tangential microfiltration, by means of a membrane having a cutoff threshold of between 0.1 μm and 2 μm, of preferably between 0.1 pm and 1.4 pm, more preferably between 0.2 pm and 1 pm, then recovery of the filtrate.
    This microfiltration step makes it possible, on the one hand, to complete the clarification of the aqueous extract by eliminating all the non-decanted particles during centrifugation, and, on the other hand, to reduce the bacterial load of the product (filtration sterilizing).
    The water-soluble fraction comprising in particular proteins including phycocyanin, phycobiliproteins, and sugars will cross the membrane and end up in the filtrate (permeate).
    This filtrate from the microfiltration stage is then advantageously subjected to separation by ultrafiltration, preferably tangential ultrafiltration, by means of a membrane with cut-off threshold between 1 and 50 kDa, preferably between 5 and 25 kDa, making it possible to separate phycocyanin from small water-soluble molecules and to collect an aqueous solution enriched in phycocyanin.
    Thus this operation constitutes a stage of purification of phycocyanin, because phycocyanin is retained on the membrane which lets through the other smaller water-soluble molecules (in particular peptides, small sugars, salts).
    It also makes it possible to reduce the volume of the clarified phycocyanin solution, by concentrating it. In concentrated form, the phycocyanin solutions are then more stable during cold storage.
    Thus, the phycocyanin-enriched solution obtained after the ultrafiltration step can contain a phycocyanin concentration greater than or equal to 0.5 g / L, preferably greater than or equal to 2 g / L, more preferably greater than or equal to 10 g / L. The phycocyanin content in said phycocyanin solution is advantageously determined by measuring the optical density at one or more wavelengths between 615 nm and 750 nm.
    As regards the aqueous solution of divalent cations of step ii), it advantageously contains between 10 mM and 100 mM, preferably between 10 mM and 60 mM, more preferably between 15 mM and 55 mM, of divalent cations. The addition of the aqueous solution of divalent cations allows better migration of the water-soluble molecules into the extracellular space, îo The divalent cations are preferably calcium ions, more particularly in the form of calcium chloride.
    If necessary, the pH is adjusted to a value between 5 and 7.5, preferably to a value between 5.5 and 7.0.
    The process for preparing a liquid extract rich in phycocyanin according to the present invention can be carried out from cyanobacteria chosen from spirulina Arthrospira platensis, Aphanizomenon flos-aquae, or
    Phormidium, molle, or any other cyanobacterium containing phycocyanin.
    The present invention also relates to a liquid extract of cyanobacteria or micro-algae prepared by the method described above, comprising a phycocyanin content greater than 0.5 g / L, preferably greater than or equal to 2 g / L, preferably still greater than or equal to 10 g / L. This aqueous extract is clear and stable over time, showing no sedimentation for several months of storage (at room temperature). It can be used in the form of a drink.
    BRIEF DESCRIPTION OF THE DRAWINGS
    The invention will be clearly understood on reading the following description of exemplary embodiments, with reference to the appended figures in which:
    - Figure 1 is a schematic diagram of the main steps of the process for preparing an aqueous extract rich in phycocyanin according to the present invention;
    - Figure 2 shows the extraction yield of phycocyanin as a function of the maceration time for a CaCl2 content of 10 mM;
    - Figure 3 shows the results of measurement of the total antioxidant status (TAS) on three groups of hamsters after 4 weeks and 11 weeks subjected to different diets, one of which included the extract according to the invention;
    FIG. 4 shows the results of measurement of superoxide dismutase (SOD) on three groups of hamsters after 4 weeks and 11 weeks of diet;
    - Figure 5 shows the measurement results of glutathione peroxidase (GPx) on three groups of hamsters after 11 weeks of diet; and
    - Figure 6 shows the results of measurement of plasma levels of malondialdehyde (MDA) on three groups of hamsters after 11 weeks of diet.
    EXAMPLES
    Example 1
    In this nonlimiting example illustrating the invention, the starting fresh cyanobacteria 1 are from the family of the spirulina Arthrospira platensis cultivated in bioreactors in brackish aqueous medium. These micro-algae are collected and drained on a 50 µm mesh screen. The dry matter content of this biomass is 20% by mass.
    The biomass is first of all subjected to a slow freezing step 2 (less than -1 ° C / min up to a temperature of -20 ° C) and stored at this temperature for 3 to 12 months, advantageously for reasons for seasonal production of spirulina.
    The conservation of the biomass in frozen form has the double advantage of ensuring the non-denaturation of compounds of interest contained in the cells but also of causing a destructuring of the biomass. This destructuring results from various phenomena involved in freezing, namely the formation of infra and extracellular ice, osmotic dehydration and rearrangement of the ice crystals resulting in high mechanical stresses on the cells. This latter phenomenon is quite slow and requires a significant period of freezing in order to ensure that the main barriers to extraction, which are the various membranes and the cell wall, are well destructured. This ensures, after thawing, good penetration of the extraction solvent and, thereby, good extraction yields.
    After this period of storage at very low temperature, the biomass is thawed to a temperature above 0 ° C while keeping it in an enclosure at around + 3 ° C. This low temperature, but positive, allows a slow thawing favoring cell permeabilization.
    Then, the aqueous extraction aims to release the phycocyanin from the cell envelope in order to find it in solution in the extracellular aqueous phase. To this end, the thawed biomass is first suspended in an aqueous solution (solid / liquid mass ratio: 15/85). This aqueous solution 3 comprises 0.2 μm microfiltered water and 10 mM calcium chloride CaCl2. The pH is adjusted if necessary to 7. The solution thermostatically controlled at 20 ° C. is subjected to a maceration 4 with stirring for 7 hours in the dark.
    The presence of both a large amount of water relative to the biomass and calcium chloride allows the migration of the major part of the water-soluble molecules in the extracellular space. We then find in this fraction extracted more than 95%, even 99% of the phycocyanin present in the initial biomass (cf. example 2 below).
    This suspension is then subjected to a centrifugation step 5 (15000 g, for 10 minutes at 20 ° C.) which makes it possible to remove a large part of the particulate fraction present (cellular debris, and poorly or not water-soluble metabolites. It was noted that the presence of calcium chloride promotes the settling of these particles.The algae residue 6 is discarded and is only kept the supernatant solution 7 colored blue.
    This solution 7 is then subjected to a new clarification step. For this, a tangential microfiltration operation 8 is carried out. The cut-off threshold is 0.2 µm (it is therefore a sterilizing filtration). The water-soluble fraction (phycocyanin and sugars in particular) crosses this membrane and is found in the permeate 10. The retentate 9 is evacuated.
    The purpose of the ultrafiltration step 11 which follows is to concentrate the volume of this phycocyanin solution and to eliminate the small contaminating molecules. It is a tangential ultrafiltration with a cutoff threshold of 10 kDa. This cut-off threshold retains phycocyanin while letting other smaller water-soluble molecules (peptides, small sugars, salts) pass through permeate 12. This step therefore also constitutes a step of purifying the phycocyanin. A clear, concentrated and purified phycocyanin solution 13 is thus obtained.
    The phycocyanin content (several grams per liter up to 50 g / L) is determined by measuring the optical density at 615 nm, 652 nm and 750 nanometers (see formula I of Example 2). This solution is stable for several months without adding a stabilizing agent or preservative, and can be packaged in sterile ampoules.
    EXAMPLE 2 Yield of Phycocyanin ίο
    Spirulina paste frozen at about 20% dry matter is placed in water at room temperature and at a CaCl2 concentration of 10 mM (1.1 g / L) according to the ratio 15/85 (m / m) . The mixture is then placed in the dark with stirring.
    A first fraction of this suspension obtained is centrifuged (10 min, Tambiant, 13000 x g) in order to follow the extraction of phycocyanin (PC). The aqueous supernatant extract thus obtained is then analyzed by a spectrophotometer by measuring the absorbance at different wavelengths: 615 is respectively calculated in Cell. Biol., 419to nm, 652 nm and 750 nm. The phycocyanin concentration using the following equation (I) (according to Bennett and Bogorad, J. 435, 1973):
    Γη /, Τ _ ”0., 474 (j46s 652 “ j4is 75 £ taHa ) '“CM (I)
    In order to calculate the extraction yields, the total amount of phycocyanin must be determined. To do this, a second fraction of the same suspension of spirulina was treated in a cell destructor by high dynamic pressures which makes it possible to obtain a total lysis of the cells and a release of all the water-soluble molecules contained in the cells. The ground product thus obtained is then clarified and then analyzed by spectrophotometry like the previous aqueous extracts.
    The results showing the extraction yield of phycocyanin as a function of the extraction time are presented in Figure 2 attached.
    After 400 minutes of extraction according to the protocol detailed above, it is found in particular that more than 95% of the total phycocyanin was extracted according to the process of the present invention.
    Example 3 Properties in vivo
    An aqueous extract of spirulina was prepared according to the method as described in Example 1. This extract contains 1 g / L of phycocyanin.
    The antioxidant activity of this spirulina extract has been demonstrated by a study carried out for 11 weeks on three groups of 6 hamsters having followed different diets:
    - Group T: subject to a standard diet
    - Group H: subjected to a hyperlipidic diet
    - Group HL: subjected to a hyperlipidic diet with supplementation with liquid spirulina (phycocyanin at 1 g / L: spirulina extract is provided in hamsters' drinking water at a dose of 1 ml / day).
    Since the hyperlipid diet is known to induce oxidative stress, the balance of this stress is determined by various measurements carried out in week no. 4 and / or in week no. 11:
    - Measurement of total antioxidant status (TAS):
    The total antioxidant status measured with the TAS-NX 2332 Kit (Randox Laboratories Ltd) reflects the activity potential of the antioxidant system to protect tissues against the effects of free radicals. The results presented in FIG. 3 show that supplementation with extract rich in phycocyanin leads to a better antioxidant status, which makes it possible to increase the cell's ability to defend itself against damage from oxidative stress.
    - Measurement of superoxide dismutase (SOD):
    It is the first enzyme in the free radical reduction chain. SOD is the enzyme necessary for the maintenance of life in the presence of oxygen, it eliminates active oxygen species toxic to cells. SOD is measured on blood using the Ransod SD 125 kit ((Randox Laboratories Ltd).
    The amount of SOD present in the blood is increased by 30 to 50% in hamsters subjected to the diet with spirulina extract (see Figure 4). Spirulina extract increases the amount of SOD available in the blood by stimulating its production.
    - Measurement of glutathione peroxidase (GPx):
    Glutathione peroxidase has the property of reducing oxidized free radicals by oxidizing reduced glutathione (GSH) to glutathione. It is measured with the Ransel kit - RS 505 (Randox Laboratories Ltd).
    At week 11, there is a significant increase in GPx îo activity (see FIG. 5) thanks to the spirulina extract according to the invention which thus allows an effective fight against free radicals.
    - Measurement of lipid peroxidation:
    Malondialdehyde (MDA) is naturally present in the tissues, it is one of the products of fatty acid oxidation, a high level is a marker of oxidative stress. It is measured on plasma with the MDA kit, ref. 1203.001 (Sobioda).
    The results presented in FIG. 6 show that supplementation with spirulina extract allows a drop in the level of MDA and therefore an inhibition of lipid peroxidation allowing a reduction in oxidative stress.
    All of the above results therefore show that the spirulina extract prepared according to the process of the present invention has good bioavailability and an antioxidant activity demonstrated in vivo.
    权利要求:
    Claims (13)
    [1" id="c-fr-0001]
    1. Process for the preparation of a liquid extract of phycobiliproteins, and in particular phycocyanin, from cyanobacteria or micro-algae containing phycocyanin, comprising the following successive steps:
    - i) a cell lysis step, by a physical or mechanical method, of an aqueous suspension of said cyanobacteria or fresh micro-algae,
    ii) a step of maceration of the lysate obtained in step i) in a solution of divalent cations, preferably cations of alkaline earth metals, with a view to releasing the water-soluble molecules in the extra cellular space of cyanobacteria or micro-algae,
    - iii) one or more stages of clarification and concentration of the suspension to isolate the water-soluble molecules, including phycocyanin, the whole of this process being carried out at a pH between 5 and 8.5, without drying and at a temperature less than or equal to 25 ° C allowing phycocyanin to retain its spatial structure, thus preserving its biological properties and giving it better bioavailability.
    [2" id="c-fr-0002]
    2. Method according to claim 1, characterized in that the destructuring or cell lysis step comprises a freeze-thaw phase.
    [3" id="c-fr-0003]
    3. Method according to claim 2, characterized in that the freeze-thaw phase comprises freezing and preserving the cyanobacteria or micro-algae frozen at a temperature below -18 ° C, preferably below -20 ° C, more preferably below -24 ° C for a period ranging from one day to one year, preferably from two weeks to six months, followed by a slow thawing step at a temperature above 0 ° C, and preferably below at 5 ° C, for several hours.
    [4" id="c-fr-0004]
    4. Method according to any one of the preceding claims, characterized in that the step of maceration of the lysate obtained in step i) is carried out with stirring of said suspension thermostatically controlled at a temperature
    [5" id="c-fr-0005]
    5 between 10 ° C and 25 ° C for several hours.
    5. Method according to any one of the preceding claims, characterized in that the clarification step is carried out by centrifugation, then recovery of the supernatant solution.
    [6" id="c-fr-0006]
    6. Method according to claim 5, characterized in that the supernatant solution resulting from the centrifugation step is subjected to a microfiltration step, preferably a tangential microfiltration, by means of a membrane having a cutoff threshold of between 0 , 1 pm and 2 pm, from
    Preferably between 0.1 µm and 1.4 µm, more preferably between 0.2 µm and 1 µm, followed by recovery of the filtrate.
    [7" id="c-fr-0007]
    7. Method according to claim 6, characterized in that the filtrate of the microfiltration step is subjected to separation by ultrafiltration, preferably
    20 a tangential ultrafiltration, by means of a membrane with a cutoff threshold of between 1 and 50 kDa, preferably between 5 and 25 kDa, making it possible to separate the phycocyanin from the small water-soluble molecules and to collect an aqueous solution enriched in phycocyanin.
    25
    [8" id="c-fr-0008]
    8. Method according to claim 7, characterized in that the solution enriched in phycocyanin obtained after the ultrafiltration step contains a phycocyanin concentration greater than or equal to 0.5 g / L, preferably greater than or equal to 2 g / L, preferably still greater than or equal to 10 g / L, the content of phycocyanin in said phycocyanin solution being
    30 determined by measuring the optical density at one or more wavelengths between 615 nm and 750 nm.
    [9" id="c-fr-0009]
    9. Method according to any one of the preceding claims, characterized in that the aqueous solution of divalent cations of step ii) contains between 10 mM and 100 mM, preferably between 10 and 60 mM, more preferably between 15 mM and 55 mM, in divalent cations.
    [10" id="c-fr-0010]
    10. Method according to any one of the preceding claims, characterized in that the pH is adjusted to a value between 5 and 7.5, preferably to a value between 5.5 and 7.
    [11" id="c-fr-0011]
    11. Method according to any one of the preceding claims, characterized in that the divalent cations are calcium ions.
    [12" id="c-fr-0012]
    12. Method according to any one of the preceding claims, characterized in that the cyanobacteria are chosen from spirulina Arthrospira platensis, Aphanizomenon flos-aquae, or Phormidium molle.
    [13" id="c-fr-0013]
    13. Liquid extract of cyanobacteria or microalgae prepared by the process according to any one of the preceding claims, comprising a phycocyanin content greater than 0.5 g / L, preferably greater than or equal to 2 g / L , preferably still greater than or equal to 10 g / L.
    Extraction yield in PC (%)
    类似技术:
    公开号 | 公开日 | 专利标题
    EP3601319B1|2020-12-23|Method for preparing a liquid extract of phycobiliproteins, in particular phycocyanin, from cyanobacteria or microalgae and extract thus obtained
    CA2885277A1|2014-03-27|Method for extracting and stabilising phycocyanin and the uses thereof
    FR2904773A1|2008-02-15|SLIMMING COSMETIC COMPOSITION CONTAINING NEOCHLORIS OLEOABUNDANS ALGAE BIOMASS EXTRACT
    EP3193821B1|2019-01-02|Method for producing a stable precipitate enriched in phycobiliproteins
    EP3169696B1|2019-06-12|Method for extracting soluble proteins from microalgal biomass
    FR2976490A1|2012-12-21|USE OF SUBSTANCES ACTING ON IGF-1 AND / OR IGF-1R FOR ANTI-AGING ACTIVITY
    EP3601318A2|2020-02-05|Purification of phycobiliproteins
    FR2958163A1|2011-10-07|PREPARATION FROM IN VITRO CULTURE OF NON-ELICITED ARGANIER DIFFERENTIAL CELLS, USE THEREOF FOR THE TREATMENT OF SKIN AGING, INFLAMMATION AND HEALING, AND OBTAINING THEM.
    EP3024923B1|2017-07-05|Method for optimising the production efficiency, organoleptic quality and stability over time of a protein-rich microalgae biomass
    FR2863615A1|2005-06-17|Stabilizing phycobiliproteins against light, useful in cosmetic, dermatological, neutraceutical and pharmaceutical compositions, by adding ascorbic acid to algal extracts
    EP3119872A1|2017-01-25|Method for thermal permeabilization of a microalgae biomass
    WO2018033814A1|2018-02-22|A process for the extraction of phycocyanin
    EP3169695B1|2019-11-13|Method for extracting soluble proteins from microalgal biomass
    EP1652435B1|2017-06-14|Use of red algae subjected to extreme temperature and light conditions.
    WO2015071477A1|2015-05-21|Method for obtaining extracts of marine algae
    FR2789399A1|2000-08-11|Preparing extracts from photosynthetic microorganisms, useful in nutritional, cosmetic and therapeutic compositions, comprises lysing cells grown on induction medium
    EP3164140B1|2019-09-25|Microalga enriched with silicon in a water-soluble form
    CA2757156A1|2010-10-14|Method for producing and using active principles of limestone
    JP2006028412A|2006-02-02|Antioxidant derived from green algae
    WO2018229364A1|2018-12-20|Method for extracting water-soluble compounds from microalgae and/or cyanobacteria
    FR2582312A1|1986-11-28|PROCESS FOR PRODUCING NATURAL ANTHOCYANIC COLOR, COLORED COMPOSITIONS CONTAINING THE SAME, AND METHODS FOR PRODUCING STABLE COLOR USING THE SAME
    FR2879596A1|2006-06-23|PROCESS FOR OBTAINING STABILIZED NATURAL POLYPHENOLS, POLYPHENOLS OBTAINED THEREBY, AND USE OF THESE POLYPHENOLS IN CARBOHYDRATE METABOLISM
    FR2978915A1|2013-02-15|Macerate, useful as an antioxidant for preventing/delaying/treating cellular damage caused by free radicals and for reducing/preventing skin aging, comprises a mixture of Gelidium sesquipedale algae and solvent containing seawater
    同族专利:
    公开号 | 公开日
    DK3601319T3|2021-03-15|
    FR3064269B1|2021-07-09|
    US20200140496A1|2020-05-07|
    EP3601319B1|2020-12-23|
    WO2018172708A1|2018-09-27|
    ES2859781T3|2021-10-04|
    PT3601319T|2021-03-08|
    EP3601319A1|2020-02-05|
    引用文献:
    公开号 | 申请日 | 公开日 | 申请人 | 专利标题
    FR2453199A1|1979-04-06|1980-10-31|Inst Francais Du Petrole|PROCESS FOR SELECTIVE EXTRACTION OF DYES CONTAINED IN CYANOPHYCEA ALGAE|
    FR2863615A1|2003-12-12|2005-06-17|Minard Florence|Stabilizing phycobiliproteins against light, useful in cosmetic, dermatological, neutraceutical and pharmaceutical compositions, by adding ascorbic acid to algal extracts|
    FR2929957A1|2008-04-10|2009-10-16|Zesiger Michel Claude Hours|Metal-phycocyanin comprising combination of protein constituent of cyanobacteria, and phycocyanin, with a divalent metal e.g. chromium and copper, useful for the preparation of compositions e.g. for micro-nutrition and cosmetics|FR3103106A1|2019-11-19|2021-05-21|Algosource|Aqueous liquid extract of Spirulina for the prevention and / or treatment of chemo-induced peripheral neuropathies and their corresponding symptoms, composition and use.|
    EP3892329A1|2020-04-06|2021-10-13|Algosource|Composition for use in preventing atherosclerosis developpment|FR2789389B3|1999-02-10|2001-03-09|Sanofi Sa|NOVEL PIPERIDINE DERIVATIVES, PROCESS FOR THEIR PRODUCTION AND PHARMACEUTICAL COMPOSITIONS CONTAINING THEM|
    CN101560254B|2009-05-19|2011-08-17|江南大学|Enrichment and separation method of blue green algae phycocyanin|
    FR3025202A1|2014-08-28|2016-03-04|Algobiotech|PROCESS FOR OBTAINING STABLE PRECIPITATION ENRICHED WITH PHYCOBILI PROTEINS|US10822373B2|2019-01-09|2020-11-03|Chenghui Zheng|Methods for synthesizing phycocyanin using a biological substance|
    FR3106726B1|2020-02-04|2022-02-18|Degro0Te Jacques|Preparation of an extract rich in phycobiliproteins|
    法律状态:
    2018-03-23| PLFP| Fee payment|Year of fee payment: 2 |
    2018-09-28| PLSC| Search report ready|Effective date: 20180928 |
    2018-09-28| EXTE| Extension to a french territory|Extension state: PF |
    2020-03-19| PLFP| Fee payment|Year of fee payment: 4 |
    2021-03-23| PLFP| Fee payment|Year of fee payment: 5 |
    优先权:
    申请号 | 申请日 | 专利标题
    FR1752452|2017-03-24|
    FR1752452A|FR3064269B1|2017-03-24|2017-03-24|PROCESS FOR PREPARING A LIQUID EXTRACT OF PHYCOBILIPROTEINS, IN PARTICULAR PHYCOCYANIN, FROM CYANOBACTERIA OR MICROALGAE AND EXTRACT THUS OBTAINED|FR1752452A| FR3064269B1|2017-03-24|2017-03-24|PROCESS FOR PREPARING A LIQUID EXTRACT OF PHYCOBILIPROTEINS, IN PARTICULAR PHYCOCYANIN, FROM CYANOBACTERIA OR MICROALGAE AND EXTRACT THUS OBTAINED|
    PCT/FR2018/050700| WO2018172708A1|2017-03-24|2018-03-22|Method for preparing a liquid extract of phycobiliproteins, in particular phycocyanin, from cyanobacteria or microalgae and extract thus obtained|
    US16/496,725| US20200140496A1|2017-03-24|2018-03-22|Method for preparing a liquid extract of phycobiliproteins, in particular phycocyanin, from cyanobacteria or microalgae and extract thus obtained|
    PT187152236T| PT3601319T|2017-03-24|2018-03-22|Method for preparing a liquid extract of phycobiliproteins, in particular phycocyanin, from cyanobacteria or microalgae and extract thus obtained|
    ES18715223T| ES2859781T3|2017-03-24|2018-03-22|Process for preparing a liquid extract of phycobiliproteins, in particular phycocyanin, from cyanobacteria or microalgae, and the extract thus obtained|
    EP18715223.6A| EP3601319B1|2017-03-24|2018-03-22|Method for preparing a liquid extract of phycobiliproteins, in particular phycocyanin, from cyanobacteria or microalgae and extract thus obtained|
    DK18715223.6T| DK3601319T3|2017-03-24|2018-03-22|PROCEDURE FOR THE PREPARATION OF A LIQUID EXTRACT OF PHYCOBILI PROTEINS, NAMELY OF PHYCOCYANINE, FROM CYANOBACTERIZES OR MICRO-ALGAE AND OBTAINED EXTRACT|
    [返回顶部]