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    • 专利摘要:
    The present invention relates to a fermentative process for the enrichment in docosahexaenoic acid (or DHA) of the biomass of microalgae of the genus Thraustochytrium, more particularly Schizochytrium sp or Schizochytrium mangrovei, by controlled supply of oxygen.
    公开号:FR3015516A1
    申请号:FR1362962
    申请日:2013-12-19
    公开日:2015-06-26
    发明作者:Bernard Caulier
    申请人:Roquette Freres SA;
    IPC主号:
    专利说明:

    [0001] The present invention relates to a novel fermentative process for the enrichment of docosahexaenoic acid (or DHA) in the biomass of microalgae of the genus Thraustochytrium, more particularly Schizochytrium sp or Schizochytrium mangrovei. , as well as the oil extracted from this microalgae biomass. Lipids are one of three major families of macronutrients with proteins and carbohydrates. Among the lipids, there are especially triglycerides and phospholipids: - Triglycerides (also called triacylglycerols or triacylglycerides or TAG) are glycerides in which the three hydroxyl groups of glycerol are esterified with fatty acids. They are the main constituent of vegetable oil and animal fats. Triglycerides account for approximately 95% of dietary lipids ingested by humans. In the body, they are present mainly in adipose tissue and constitute the main form of energy storage. Phospholipids are amphiphilic lipids, that is to say consisting of a polar "head" (hydrophilic) and two "tails" aliphatic (hydrophobic). Phospholipids are lipids of structure because they are constituents of the cellular membranes of which they ensure among others the fluidity. Triglycerides and phospholipids are composed mainly of fatty acids which are both provided by the diet and, for some of them, synthesized by the body. The biochemical classification (based on the number of double bonds contained in the fatty acid molecule) distinguishes between saturated fatty acids (AGS), monounsaturated fatty acids (MUFA) and polyunsaturated fatty acids (PUFAs). From the physiological point of view, we distinguish: - the essential fatty acids necessary for the development and the good functioning of the human body, but which our body does not know how to manufacture; the so-called "conditionally" fatty acids that are essential, essential for the normal growth and the physiological functions of the cells, but which can be manufactured from their precursor if it is provided by the diet. They are therefore strictly required if their indispensable precursor is absent. - non-essential fatty acids.
    [0002] The essential and "conditionally" essential fatty acids are the essential fatty acids. Other fatty acids are called non-essential. Non-essential fatty acids include: - eicosapentaenoic acid (EPA) of the omega 3 family - oleic acid, the major monounsaturated fatty acid in our diet, and palmitoleic acid, saturated fatty acids, such as lauric acid, myristic acid or palmitic acid.
    [0003] Polyunsaturated fatty acids Polyunsaturated fatty acids are classified according to the position of the first double bond, from the final methyl function. Thus, in the nomenclature, for omega "x" or "nx", "x" corresponds to the position of the first unsaturation.
    [0004] There are two main families of essential fatty acids: omega-6 fatty acids (or n-6 PUFAs), whose precursor and major representative is linoleic acid (LA) and omega-3 fatty acids (or PUFAs). 3) whose precursor is alphalinolenic acid (ALA). The majority of the polyunsaturated fatty acids of biological interest belong to the family of omega 6 (arachidonic acid or ARA) or omega 3 (eicosapentaenoic acid or EPA, docosahexaenoic acid or DHA). In addition, in the nomenclature, the number of carbon constituting the chain is also defined; thus EPA is described as C20: 5 and DHA as C22: 6. The "5" and "6" thus correspond to the number of unsaturations of the carbon chain presented respectively by EPA and by DHA. DHA, from the family of omega 3 fatty acids, is a fatty acid that the body knows how to synthesize from alpha-linolenic acid, or that is brought by the consumption of fatty fish (tuna, salmon, herring, etc.). .). DHA plays an important role in the structure of membranes and in the development and functioning of the brain and retina. Fish oils are mainly used as a source of omega 3 fatty acids, such as DHA and EPA, but they are also found in microalgae oils from which they are extracted either as a mixture or separately, as this is the case for example with oils from certain selected strains, such as those of the genus Schizochytrium, which contain only traces of EPA but high levels of DHA.
    [0005] Saturated fatty acids Among saturated fatty acids, palmitic acid, also known as hexadecanoic acid or cetyl acid, is one of the most common C16: 0 saturated fatty acids found in animals and plants.
    [0006] Palmitic acid is the first fatty acid produced during lipogenesis; from it, longer fatty acids can be produced. In addition, it is the fatty acid preferentially used to synthesize ATP. The energy balance of its combustion indicates 129 ATP. It is thus an excellent energy food.
    [0007] Industrially, palmitic acid is also used for the manufacture of both margarine and hard soaps. In the field of paints, since it is saturated, palmitic acid can not polymerize and become rigid once in contact with oxygen in the air (unlike oleic, linoleic and linolenic acid). ). It therefore remains in the form of a soft solid and acts (with stearic acid) as a plasticizer for polymerized oily binders. Thus, with stearic acid, it provides the elasticity necessary for the proper preservation of oil paints over time. Monounsaturated fatty acids As a precursor of monounsaturated fatty acid, palmitic acid leads to palmitoleic acid (16: 1 n-7), naturally present in large quantities in the fruit or pulp of sea buckthorn. It has furthermore been described that an increased intake of palmitoleic acid in the diet could have hypocholesterolemic and hypotriglyceridemic effects, reduce the risk of stroke, and also improve the metabolism of vascular smooth muscle cells. Production of lipids, especially of fatty acids, by microalgae The culture of microalgae of the genus Schizochytrium is conventionally carried out in fermentors (heterotrophic conditions: in the dark in the presence of a carbon source).
    [0008] It should be noted that the profitable exploitation of these microalgae generally requires the control of the fermentation conditions. To achieve this result, first fermentation processes to obtain high cell densities (HCD for High-Cell-Density) were thus worked extensively, so as to obtain maximum yields and productivities in lipids. The objective of these HCD cultures was to obtain the highest possible concentration of the desired lipids in the shortest time.
    [0009] However, it soon became apparent to those skilled in the art that, for example, microalgae must be subjected to a nutritional stress which limits their growth when they wish to produce large lipid reserves. It is therefore classically decoupling growth / production in fermentative processes. For example, to promote the accumulation of polyunsaturated fatty acids (here docosahexaenoic acid or DHA), the patent application WO 01/54510 recommends dissociating the cell growth and the production of polyunsaturated fatty acids. More particularly, there is claimed a process for the production of microbial lipids, comprising the steps of: (a) fermenting a medium comprising microorganisms, a carbon source and a limiting nutrient source and providing sufficient conditions for maintaining a dissolved oxygen level of at least about 4% of the saturation in said fermentation medium to increase the biomass; (b) then providing sufficient conditions to maintain a dissolved oxygen level of approximately 1% or less of saturation in said fermentation medium and to provide sufficient conditions to allow said microorganisms to produce said lipids; (c) and collecting said microbial lipids, wherein at least about 15% of said microbial lipids are polyunsaturated lipids; and wherein a biomass density of at least about 100 g / l is obtained during the fermentation. In the microalga Schizochytrium sp strain ATCC 20888, it is thus more particularly carried out a first phase of growth in the presence of a carbon source and a nitrogen source but without limitation in oxygen, so as to promote the obtaining of a cell density and then, in a second phase, stop the supply of nitrogen and gradually slow down the supply of oxygen (management of the dissolved oxygen pressure or pO 2 by 10%, at 4%, then 0.5%). ), in order to stress the microalgae, slow down its growth and trigger the production of the fatty acids of interest.
    [0010] In the microalgae Crypthecodinium cohnii, the highest content of DHA is obtained at low glucose concentration (of the order of 5 g / l), and thus at a low growth rate (Jiang and Chen, 2000, Process Biochem., 35 (10), 1205-1209). Therefore, in cases where the formation of the products is not correlated with high cell growth, it is taught that it is wise to control the rate of cell growth. In general, those skilled in the art choose to control the growth of microalgae by controlling the fermentation conditions (Tp, pH, etc.), or by the regulated supply of nutritional components of the fermentation medium (semi-continuous conditions called " fedbatch "). If he chooses to control the growth of microalgae in heterotrophy by the supply of carbon sources, the skilled person generally chooses to adapt the carbon source (pure glucose, acetate, ethanol ...) to the microalga (C. cohnii, Euglena gracilis ...) depending on the metabolite produced (for example a polyunsaturated fatty acid type DHA). Temperature can also be a key parameter. For example, it has been reported that the synthesis of polyunsaturated fatty acids in certain species of microalgae, such as EPA by Chlorella minutissima, is favored at a lower temperature than that required for optimal growth of said microalgae. To optimize the production of triglycerides, a person skilled in the art is also led to optimize the carbon flow towards the production of oil, by acting on the nutritional environment of the fermentation medium.
    [0011] It is thus known that the accumulation of oil occurs during a sufficient carbon supply, but under conditions of nitrogen deficiency. The C / N ratio is here decisive, and it is accepted that the best results are obtained by acting directly on the nitrogen content, the glucose content not being limiting.
    [0012] To optimize the production of oil, it is therefore essential for the skilled person to control the carbon flow by diverting it to the production of oil, to the detriment of the production of proteins; the carbon flux is redistributed and accumulates in lipid reserve substances when the microalgae are placed in nitrogen-deficient medium. Be that as it may, commercial preparations of microalgae biomass rich in DHA and palmitic acid are available thanks to the implementation of standard fermentation conditions. However, there remains an unmet need for an alternative method of producing biomass of high quality, high DHA and controlled content palmitic acid and / or palmitoleic acid microalgae.
    [0013] SUMMARY OF THE INVENTION The present invention relates to a method for producing a biomass of microalgae of the genus Thraustochytrium enriched in docosahexaenoic acid (DHA), characterized in that, during the culture phase in heterotrophic conditions, the oxygen supply is controlled to meet only oxygen requirements 1) for energy production required for cell maintenance, 2) for the production of base lipids, and 3) for growth of biomass excluding fatty acids.
    [0014] Preferably, the method is characterized in that the supply of oxygen necessary to satisfy only the requirements 1), 2) and 3) is calculated by the following equation 2 wherein q02 Target is the quantity of oxygen in grams per gram biomass off fatty acids and hour; qm is maintenance coefficient expressed in g of glucose per g of biomass excluding fatty acids and per hour; basal glipids is the rate of accumulation of basal lipids expressed in g of basal lipids per g of biomass excluding fatty acids and per hour; is the coefficient of oxygen consumption relative to the formation of lipids expressed in g of oxygen per g of lipids, it is the growth rate expressed in g of biomass excluding fatty acids formed per g of biomass excluding fatty acids and by hour, that is (h-1); yo2 / x is the coefficient of oxygen consumption compared to the formation of biomass excluding fatty acids expressed in g of oxygen per g of biomass excluding fatty acids. Optionally, no limitation of a nutrient, especially in a carbon or nitrogen source, is applied during the fermentative process.
    [0015] Optionally, the growth and production phases of DHA are concomitant. Preferably, the microalgae are of the genus Schizochytrium sp or Schizochytrium mangrovei. More specifically, the microalgae may be a strain selected from strains CNCM 1-4469 and CNCM 1-4702 deposited at the National Collection of Microorganism Cultures of the Institut Pasteur respectively on April 14, 2011 and November 22, 2012. Optionally the method may further comprise harvesting biomass, optionally preparing an extract or cell lysate from said biomass, and optionally extracting a crude oil rich in DHA.
    [0016] The process according to the present invention can be characterized in that the biomass obtained comprises - at least 40% of DHA by weight of total fatty acids; and / or - at most 40% of palmitic acid by weight of total fatty acids; and / or - at least 25% of fatty acids in dry weight of biomass. DETAILED DESCRIPTION OF THE INVENTION Within the scope of the invention, the applicant company has chosen to explore an original way of optimizing production. in DHA by proposing an alternative solution to those conventionally envisaged by those skilled in the art.
    [0017] The applicant company has thus found, contrary to technical prejudices on the subject, that it is possible to produce by fermentation biomasses of lipid-rich microalgae (more than 45% by dry weight of biomass) whose fatty acids are docosahexaenoic acid (DHA), while modulating or controlling the amount of palmitic acid and palmitoleic acid: without the need to decouple the growth phase of the microalga and the production phase lipids - on the contrary, the production of lipids is concomitant with cell growth and is therefore carried out in a single phase, without it being necessary, as described in the state of the art, to induce a limitation in nitrogen or any other nutrient, and without it being necessary to control the fermentation by p02. The Applicant Company has thus found that it is possible to control the lipid composition of the biomass, and in particular the proportions of DHA and of palmitic and palmitoleic acid by means of a control of the oxygenation of the fermentation medium.
    [0018] Indeed, the Applicant Company has understood that oxygen is used by microalgae according to the following priorities: production of energy for maintenance, production of a range of fatty acids, called basic lipids, of which DHA is the majority , growth of biomass excluding fatty acids, and production of palmitic acid with excess oxygen. In other words, the process according to the invention consists in satisfying the oxygen requirements corresponding to the first three points and thus providing the optimal amount of oxygen to obtain a biomass rich in DHA (whether produced by Schizochytrium sp or S. mangroves). Then, as will be demonstrated in the experimental part below, an additional oxygen supply can be realized and leads to a rapid overproduction of palmitic acid (well illustrated with S. mangroves), with or without palmitoleic acid (well illustrated with Schizochytrium sp).
    [0019] The applicant company has started work on the basis of the strain Schizochytrium sp ATCC 20888.
    [0020] By following the teachings of the state of the art, in particular those of the patent application WO 01/54510, the Applicant Company first found that, contrary to what is disclosed, a constant regulation of the pO 2 to 0% or more than 10% during the entire fermentation allowed to produce more than 35 (3/0 of PUFA in fatty acids (more than 25% of DHA on total fatty acids), just as with a pipe reasoned with a reduction of the pO 2 in cascade (10%, then 4%, then 0.5% of saturation) .In contrast, the latter conduct (according to the application WO 01/54510) applied to the strain CNCM 1-4702 results in the end, to the production of fatty acids, of which palmitic acid is a majority of more than 60%, while DHA does not reach 20%, which leads to the same results as those obtained for this strain with In addition, from a technical point of view, the measurement of pO 2 poses great difficulties. when it comes to transposing the laboratory protocol on an industrial scale (in other words, moving from the fermenter scale from 2 to 20 1 to the reactor scale from 1 to 200 m3). Indeed, the pO 2 is defined as the relative concentration of dissolved oxygen in the saturation fermentation must. For example, if water is vented in air, at room temperature and under atmospheric pressure, long enough, it is considered that the pO 2 is equal to 100% (which corresponds to the state of oxygenation of the fermenter at t = 0). However, when calibrating a p02 probe in a fermenter, the dissolved oxygen content is influenced by the concentration of residual salts and the fermentation temperature. Furthermore, it is conventionally admitted that, for a laboratory fermenter, the pO 2 is not influenced by the pressure generated by the height of the fermentation must and by the mixing effects. However, during the industrializations on fermenters of average (of the order of the m3) with large capacity (of the order of hundreds of m3), the height of the must of fermentation goes on the contrary: to have an influence on the pressure in oxygen dissolved; and cause complex phenomena in the fermenter "not perfectly agitated". In this sense, the value of pO 2 established at the laboratory scale can not be extrapolated on an industrial scale. In addition, the recommendations of patent WO 01/54510 described for Schizochytrium sp do not seem generalizable to all strains of the genus Thraustochytrium. In other words, in the present invention, there is no process here to reduce the oxygen supply so as to "stress" the microalgae so as to make it produce its reserve lipids (in this case the DHA), but to control the oxygen supply to the level of the needs expressed by said microalgae to modulate the orientation of its lipid production and, without referring to the pO 2. Moreover, the choice of the fermentation line by controlling the supply of oxygen has led the applicant company to obtain, without it being useful to limit the intake of certain nutrients or decouple growth phase and production, remarkable results: an increase in the overall lipid content of interest, and in particular DHA, and a reduction of odors (the reduction of the particularly intense scent of the biomasses harvested from the CNCM 1-4469 is remarkable. Microorganisms The strains to be used in the methods of the present invention are of the genus Thraustochytrium, more particularly Schizochytrium sp or Schizochytrium mangrovei, Such strains are known to those skilled in the art, for example the strain Schizochytrium sp ATCC No 20888, described and studied in the application WO 01/54510. The applicant company has identified in the course of its research several strains of microalgae pro DHA producers of great interest. In particular, the applicant company is particularly interested in two strains it has identified. The first strain is a strain of Schizochytrium sp., Deposited in France on April 14, 2011 with the National Collection of Microorganism Cultures of the Pasteur Institute (CNCM) under the number 1-4469 but also in China with the 25 CHINA CENTER FOR TYPE CULTURE COLLECTION (CCTCC) from Wuhan University, Wuhan 430072, PR China under the number M 209118. This strain mainly produces DHA and to a lesser extent palmitic acid and palmitoleic acid. It was characterized by partial sequencing of the gene encoding the 18S RNA (SEQ ID No. 1): 30 1 GAGGGTTTTA CATTGCTCTC aTTCCaATAG CAaGACGCGA AGCGCCCCGC ATTGATATTT 61 CTCGTCACTA CCTCGTGGAG TCCACATTGG GTAATTTACG CGCCTGCTGC CTTCCTTGGA 121 TGTGGTAGCC GTCTCTCAGG CTCCCTCTCC GGAGTCGAGC CCTAACTCCC CGTCACCCGT 181 TATAGTCACC GTAGGCCAAT ACCCTACCGT CGACAACTGA TGGGGCAGAA ACTCAAACGA 241 TTCATCGCTC CGAAAAGCGA TCTGCTCAAT TATCATGACT CACCAAGAGA GTTGGCTTAG 35,301 ACCTAATAAG TGCGGCCCTC CCCGAAAGTC GGGCCCGTAC AGCACGTATT AATTCCAGAA 361 TTACTGCAGG TATCCGTATA AAGGAACTAC CGAAGGGATT ATAACTGATA TAATGAGCCG 421 TTCGCAGTTT CACAGTATAA TTCGCTTATA CTTACACATG CATGGCTTAG TCTTTGAGA allowing to identify it as being a strain of Schizochytrium sp kind. This strain will be designated "CNCM 1-4469" later in this application. In addition, the second strain is a strain of Schizochytrium mangrovei.
    [0021] It produces DHA and palmitic acid in a relatively equal proportion. It was filed by the company Applicant in France on November 22, 2012 with the National Collection of Microorganism Cultures of the Pasteur Institute (CNCM) under number CNCM 1-4702. It was characterized by sequencing of genes coding for rRNA 18S (SEQ ID No. 2): 1 61 121 181 241 301 361 CGT GGTTTTACAT CCTACCT GGTAGCCGTC AGTCACCGTA ATCGACCAAA CTAATAAGTG GGTATCCATA TGCTCTCATT CGTGGAGTCC TCTCAGGCTC GTCCAATACA AWAGTCAATC CAGCCCCATA TAAAAGAAAC CCGATAGCAA ACAGTGGGTA CCTCTCCGGA CTACCGTCGA TGCTCAATTA CAGGGCTCTT TACCGAAGAA AACGCATACA ATTTACGCGC GTCGAGCCCT CAACTGATGG TCATGATTCA ACAGCATGTA ATTATTACTG CGCTTCGCAT CTGCTGCTAT AACTCTCCGT GGCAGAAACT CCAATAAAAT TTATTTCCAG ATATAATGAG CGATATTTCT CCTTGGATAT CACCCGTTAT CAAACGATTC CGGCTTCAAT AATTACTGCA CCGTTCGCAG 421 TCTCACAGTA CAATCGCTTA TACTTACACA GCAG allowing to identify it as a type strain Schizochytrium mangrovei. This strain will be referred to as "CNCM 1-4702" later in this application. Determination and use of the quantity of oxygen necessary, in particular q02 The global oxygen flux introduced into the culture medium is variable and essentially depends on: the flow rate of the introduced air, the stirring speed which favors the dissolution of oxygen in the medium. This stream is named OTR (Acronym for Oxygen Transfer Rate). The oxygen consumption by the culture is named OUR (acronym for Oxygen Uptake Rate). As the biomass grows in the fermenter, its overall oxygen consumption increases to absorb all the oxygen transferred, the OUR is then considered equal to the OTR. OTR and OUR are data for the entire culture medium. Thus, the OUR for a volume of culture can be related to the quantity of cells occupying this volume.
    [0022] Thus, the cell consumption is called q02 and represents the amount of O 2 in grams absorbed per gram of cell per hour. This consumption is then calculated for the mass of cells as such, that is to say without the mass of fatty acids, since the lipid reserves have no active role in the absorption of oxygen.
    [0023] The method of the invention makes it possible, by a controlled supply of oxygen to the culture medium, to act on the production of the lipids and to optimize it according to the growth conditions of the microalgae (size of the inoculum, age of the culture...). The overall 02 consumption corresponds to the addition of the different uses of oxygen by the cell. The Applicant company distinguishes four oxygen consumption routes, which correspond to the basic needs of the cell, needs successively met with an order of priority up to the oxygen supply. These needs are as follows, in order of priority: 1. Cellular maintenance. 2. The production of basic lipids. 3. The formation of biomass off fatty acid. 4. An accumulation of lipids related to a metabolic overflow. The Applicant Company has found that the q02 is then determined by the following formula: Equation (1) (1) (2) (3) (4) The terms "qm", "basic qipides", <y ° / "< "° 2 /" "lipids of 2lipids, x overflow" of the equation must be understood as follows. Cellular maintenance. Term (1) of Equation Cell maintenance is the energy the cell needs for its maintenance, regardless of any lipid production or biomass growth. "Qm" is the amount of carbon substrate (usually glucose) used to produce this energy; it is expressed in g of glucose per g of biomass excluding fatty acids and per hour. This term is conventionally referred to in the field as maintenance energy or maintenance coefficient.
    [0024] The associated oxygen requirement is proportional. It takes 6 molecules of O2 (Molar mass: 32 g) to transform a molecule of glucose (Molar mass: 180 g). Hence the term "" in equation (1). The production of basic lipids. Term (2) of the Equation The applicant company has found that lipid accumulation is concomitant to growth and is not only a phenomenon appearing at the end of the latter. Lipid accumulation is a precursor to growth, if only for the formation of cell membranes. The composition of these basic lipids is different depending on the strain and includes among others palmitic acid or palmitoleic acid as precursors of the biosynthesis of DHA, but DHA is still the major constituent, whose quantification is illustrated by Example 2. The rate of accumulation of these lipids corresponds to a stream named "n, basic lipids" in equation (1).
    [0025] For strains CNCM 1-4469 Schizochytrium sp and CNCM 1-4702 Schizochytrium mangrovei, this speed is exemplified below. To obtain the associated oxygen requirement, this flow or rate is multiplied by the oxygen requirement to form lipids (also called oxygen consumption coefficient with respect to lipid formation), expressed by the term "y 02 / Lipids" In equation (1). Thus, the oxygen supply will serve secondly the production of basic lipids. The formation of biomass off fatty acid. Term (3) of Equation Total biomass includes lipid stores.
    [0026] The latter (consisting of fatty acids) are determined by assay and are subtracted from the total biomass. The formation of biomass excluding fatty acids (excluding "A.G.") corresponds to the growth of biomass rich in proteins, and therefore really active. The growth rate is symbolized by "μ" in equation (1) which represents the biomass (excluding A.G.) in g formed by g of biomass (excluding A.G.) and per hour ie (h-1). To obtain the associated oxygen requirement, this growth rate (p) is multiplied by the oxygen requirement to form the biomass excluding A.G., expressed as "y ° 2 / x" in equation (1).
    [0027] Thus, the oxygen supply will serve thirdly the production of biomass excluding fatty acids.
    [0028] Calculation of the biomass concentration excluding fatty acid The growth is continuous because, according to the method of the invention, there is no nutritional limitation. However, it is observed a slowing down of the growth rate independent of the exhaustion of the medium.
    [0029] The biomass concentration excluding A.G. varies according to the initial biomass concentration and increases according to its growth rate. To predict by calculation the biomass concentration at each instant and estimate the value of the growth rate, the Applicant Company recommends using the following equation (3).
    [0030] Equation (3) p _ elriaX [1 X x 'This equation illustrates the observed and unexplained reduction in growth rate. "It" represents the growth rate (expressed in h-1) and X the cell concentration excluding A.G. (expressed in g / L). The parameters are different for the two preferred strains and listed in Table I. Table I Strain 1.1 max X max (excluding AG) CNCM 1-4469 0.0811-1 45 g / L CNCM 1-4702 0.1711-1 40 g / L This phenomenon also reduces q02 because the growth rate (p) contributes to oxygen consumption (Equation 1).
    [0031] The biomass concentration is calculated from the amount of biomass introduced and known (Inoculum) and its rate of growth that evolves. The accumulation of lipids linked to a metabolic overflow. Term (4) of the Equation It has been determined by the Applicant Company that the latter stream exists only when the needs mentioned above have been met and the necessary oxygen is supplied. This oxygen supply, expressed in equation (1) by the term "n lipid overflow" X << Y ° 2 / lipids "causes an increase in the rate of consumption of glucose which will be transformed into a stream of fatty acid. This additional oxygen supply can be modulated so as to control the production of overflow lipids. This acceleration of fatty acid production, as illustrated in Example 1, causes a metabolic overflow and results in an accumulation of palmitic acid for Thraustochytrium and palmitic and palmitoleic acids for Schizochytrium sp. Without being bound by this theory, the applicant company considers that this overflow is related to the fact that the enzymes downstream of the metabolization pathway continue to act at the same rate while the enzymes at the beginning of the path accelerate their activity.
    [0032] Calculation of the Need in 02 to form the A.G. and the biomass out of A.G. The conversion yields on 02 make it possible to know the consumptions of 02 as a function of the productions of biomass except A.G or lipids. Conversion efficiencies are parameters well known to those skilled in the art which can therefore determine them by routine experiments. These values are shown in Table II and are specific to the two preferred strains. Table II 02 requirement for non-AG biomass production (g / g) 0.80 Y O2 / x O2 requirement for lipid production (g / g) 0.17 Y (1) 2 / lipids Obtained a biomass rich in DHA - Calculation of q02 target To increase the DHA content, the Applicant Company has established that it was appropriate to control the oxygen supply to satisfy only the first 3 uses of oxygen (maintenance, production base lipid, and non-AG biomass growth). This supply can be defined by the determination of the target q02, which corresponds to the amount of O 2 needed in grams per gram of cell per hour. The target q02 is then defined by equation (2), which includes only the first three components of equation (1) Equation 2:, qm - (2) (3) Then, this rate of consumption of 02 The cell is transposed to the fermenter by multiplying it by the non-AG biomass concentration, which can either be measured or predicted by calculation for each instant. This speed corresponds to the OUR. Since one places oneself in conditions where the OTR corresponds to the OUR, it will be this OTR that will be applied for each moment during the fermentative process. (1) The applicant company has found that it is by the respect of this control of the target oxygenation that a biomass rich in DHA is obtained. Oxygenation greater than the target results in producing more palmitic acid and / or palmitoleic acid and thus diluting DHA. Oxygenation below the target oxygenation level limits the amount of biomass produced. Since the target q02 varies with the evolution of the culture, reference is made in the following examples to the maximum observed OUR. Examples 1 and 2 illustrate the effect of the control of oxygenation on strains CNCM 1-4469 Schizochytrium sp and CNCM I-4702 Schizochytrium mangrovei and the method for obtaining the specific production rates. Example 3 illustrates, for the strain CNCM 1-4702 Schizochytrium mangrovei, the effect of a pipe in which the variation of the oxygenation makes it possible to modify the proportions of palmitic acid and DHA of the biomass.
    [0033] In an alternative embodiment, the oxygen supply necessary to satisfy the first three needs, namely the requirements (1), (2) and (3), can also be determined empirically. As illustrated in Example 3, one skilled in the art can carry out various fermentation processes in which a range of OTR is implemented and the amounts of lipids and biomass are measured. Based on these results, one skilled in the art can define the target OTR that satisfies the first three needs. The fermentative process according to the present invention makes it possible to obtain a biomass rich in fatty acids. In particular, the biomass comprises at least 25% of fatty acids in dry weight of biomass, preferably at least 30%. The level of fatty acids may depend on the strain used and may reach a minimum of 40% by dry weight of biomass for strain 1-4702. Moreover, and quite interestingly, this biomass rich in lipids has a high level of DHA. In particular, the fermentative process according to the present invention makes it possible to obtain a biomass comprising at least 40% by weight of DHA relative to the total fatty acids. Finally, the fermentative process according to the present invention makes it possible to obtain a biomass having a reduced content of palmitic acid. Thus, the biomass comprising at most 40% by weight of DHA relative to the total fatty acids. The level of palmitic acid may depend on the strain used and may reach a maximum of 10% by weight relative to the total fatty acids for the 1-4469 strain.
    [0034] Furthermore, the present invention also considers fermentation processes in which the oxygen supply is greater than that required to meet the first three needs, namely the needs (1), (2) and (3). In particular, this intake will be controlled so as to obtain the relative proportions of DHA and palmitic acids and / or palmitoleic desired, while optimizing the amount of biomass produced. In addition, the fermentative processes according to the present invention are carried out under heterotrophic culture conditions. These conditions adapted to the microalgae considered as well as the culture media are well known to those skilled in the art. The carbon source necessary for the growth of the microalga is preferably glucose. The nitrogen source can be yeast extracts, urea, sodium glutamate, ammonium sulfate, ammonia in pH regulation, alone or in combination. Generally, the culture step comprises a preculture step, to revive the strain, and then a culture or fermentation step itself. This last step corresponds to the production step of the lipids of interest, in particular DHA. In addition to biomass, the present invention also relates to an extract or cell lysate prepared from this biomass. In particular, this extract or lysate is prepared from the biomass recovered after fermentation. This extract or lysate rich in DHA, and optionally in palmitic and / or palmitoleic acids. The rupture of the cells for the extraction of the lipid content can be carried out by various ways, among which the mechanical, chemical and enzymatic pathways.
    [0035] Subsequently, an oil can be extracted from the cell lysate, for example using hexane / ethanol in several successive extractions. The hexane fraction is then separated and the hexane is evaporated to isolate the crude oil. Thus, the method for producing lipids of interest, preferably DHA, and optionally palmitic and / or palmitoleic acids, comprises the fermentative process according to the present invention, the harvesting of the biomass, the preparation of an extract or lysate. and extraction of a crude oil comprising the lipids of interest, preferably DHA, and optionally palmitic and / or palmitoleic acids.
    [0036] EXAMPLES Example 1 Crop Conditions of Strains CNCM 1-4469 and CNCM 14702 and Determination of Specific Production Rates in Excess of Oxygenation Culture Conditions The protocol comprises a preculture in Erlens for a fermenter seeding with 0.1 g of biomass / L for the CNCM 1-4469 strain and at least 5g of biomass / L for the CNCM 1-4702 strain. Preculture The preculture (100 ml of medium) in 500 ml baffled Erlens lasts 24 hours at a temperature of 28 ° C. All the components of the medium is sterilized by filtration and introduced into an Erlen previously sterilized by autoclave after adding a drop of Clearol FBA antifoam 3107.
    [0037] Table III Preculture medium% (g / g) Glucose anhydrous 3 Yeast extract 0.4 Sodium monosodium glutamate 6.42 NaCl 1,25 MgSO 4 (H 2 O) 0.4 KCl 0.05 CaCl 2 (H 2 O) 0.01 NaHCO3 0.05 KH2PO4 0.4 Vitamins mother solution B1, B6, B12 0.1 Micronutrients mother solution 0.8 Culture The medium is sterilized in 3 parts.
    [0038] The glucose is sterilized with KH2PO4 in Erlen for an addition just before To. The rest of the salts are sterilized in fermenters with 0.05 ml / l of Clearol FBA 3107. The trace elements and vitamins are sterilized by filtration. The volume at To represents 75% of the final volume. The pH is adjusted to To by ammonia and then it is regulated at 6 with ammonia. Table IV A Fed batch of glucose (concentration: 500 g / L of Fed) is continuously fed from To to a constant rhythm (to be adapted according to calculations) not to be at a concentration lower than 20 g / L and 5g / L in the end. The culture is conducted at a temperature of 28 ° C and lasts from 65 to 85 hours. The use of corn steep liquor (acronym "CSL") or yeast extract (acronym "EL") as a source of nitrogen is possible, allowing slightly higher results in DHA.
    [0039] Matrix Solutions Table V Trace elements g / L MnCl 2 2H 2 O 8.60 00012 6H 2 O 2 NiSO 4 6H 2 O 7.50 Na 2 MoO 4 2H 2 O 0.15 ZnSO 4 7H 2 O 5.70 Cu Boa 5 h 20 6.50 FeSO 4 7 H 2 O 32 Acetate of Zinc 0.01 EDTA MisapH <3 Table VI Vitamins g / L B1 45 B6 45 B12 0.25 Determination of specific production rates To evaluate the specific production rates, a first culture was carried out at 10% P02, which means that it is ensured that there is always dissolved oxygen in the medium. This culture was conducted without limitation in nutritional sources. Culture Medium% (w / w) KH2PO4 0.80 (NH4) 2304 0.33 Na2SO4 0.67 NaCl 0.27 Ca 012 2 (H2O) 0.03 Mg SO4 7 (H2O) 1.00 Anhydrous Glucose 6, 00 Vitamins stock solution B1, B6, B12 0.20 Micronutrients stock solution 0.27 This method makes it possible to highlight the characteristics of the strains to be tested, in excess of oxygen (Figure 1). In Table VII, the results presented are those obtained at T65 from the culture of the biomasses of the two strains CNCM 1-4469 and CNCM 1-4702. Table VII: Biomass and fatty acid compositions CNCM 1-4469 CNCM 1-4702 Biomass (g / L) 51.2 79 Total AG / Biomass content (g / g) 0.38 0.57 DHA / AG (g / g) g) 0.34 0.19 palmitic acid / AG (g / g) 0.28 0.67 Other fatty acids / AG (g / g) 0.38 0.14 AG meaning Fatty Acid 10 The different fatty acids other than DHA and palmitic acids (in particular palmitoleic acid) are grouped under the name "other fatty acids" to highlight the effect on DHA and palmitic acid, but join the basal lipids with DHA in the calculation of the target q02. The calculation of the average speeds is done globally. The final biomass is analyzed by Gas Chromatography (GPC). The total biomass concentration, the content of each of the fatty acids and the overall content of the fatty acids are then known. The biomass excluding fatty acid, also called active biomass, is calculated by removing these fatty acids from the total biomass. The amount of each of the fatty acids produced is then divided by the average of the biomass excluding A.G. present and by time. The result obtained is a total specific production rate per unit of time and per g of biomass excluding A.G. These speeds are presented in the following Table VII.
    [0040] Table VIII: Calculation of Rates CNCM 1-4469 CNCM 1-4702 active biomass (h-1) 0.05 0.055 q Fat (g / g / h) 0.034 0.074 q (DHA) (g / g / h) 0.011 0.014 q (palm) (g / g / h) 0.009 0.050 q (other FA) (g / g / h) 0.013 0.010 Example 2: Cultures of strains CNCM 1-4469 and CNCM 1-4702 with a controlled oxygen supply The same culture conditions were used but the oxygen supply was controlled. The method consists in using half of the value of the observed transfer (OUR) during the culture at 10% (here, 50 mmol / L / h, see graph 1, ie 25 mmol / L / hr) (Figure 2). Moreover, for a fermenter of 201, to respect the proper operation of the fermenter, whatever the need for oxygenation, fixed at tc, minimum agitation, of the order of 150 rpm, during the first 10 to 15 hours of culture. In Table IX, the results presented are those obtained at T65 from the culture of the biomasses of the two strains CNCM 1-4469 and CNCM 1-4702 under controlled O 2 feed conditions. Table IX: Biomasses and fatty acid compositions CNCM 1-4469 CNCM 1-4702 Biomass (g / L) 34 59 Total AG / Biomass content (g / g) 0.29 0.45 DHA / AG (g / g) ) 0.52 0.44 palmitic acid / AG (g / g) 0.04 0.39 Other fatty acids / AG (g / g) 0.44 0.17 The calculation of the average velocities is carried out globally as indicated in Example 1. The results are given in Table X. Table X: Calculation of Velocities CNCM 1-4469 CNCM 1- 4702 active biomass (h-1) 0.05 0.055 q Fat (g / g / h) 0.021 0.045 q (DHA) (g / g / h) 0.011 0.02 q (palm) (g / g / h) 0.001 0.018 q (other FA) (g / g / h) 0.009 0.007 Comparing the overall specific production rates under conditions of excess oxygen (values in Table VIII) and controlled oxygen conditions, we find that: oxygen supply has reduced the rate of production of palmitic acid, the production rate of palmitic acid is decreased by a factor of 9 for the strain CNCM 1-4469 and by 3 for the strain CNCM 1-4702. This result is obtained while the production rates of biomass or DHA remain unchanged. Thus, the production of lipids is prevented in the context of a metabolic overflow.
    [0041] The velocities evaluated by this method serve as a basis for calculating the q02 Target. Calculation of qL2) s with Equations 1 and 2 The lipid production rates of Table X represent here the constant flux of base lipids (da1-, liptclesdebase in equations 1 and 2), of which DHA is the major constituent but which also includes some palmitic acid. The metabolic overflow flow corresponds to the additional flow, between the speeds of Table VIII and that of Table X.
    [0042] Qm is negligible in non-stressing culture conditions; a value of 0.006 g / g / h is retained. The growth rate is reduced with increasing biomass concentration; the maximum growth rate can be maintained up to 4 g / L of biomass without lipids for CNCM 1-4702 and 7 g / L for CNCM 1-4469 inoculated at 5 g / L.
    [0043] It is possible to transpose the q02 (consumption at the cellular level) to the OTR (contribution corresponding to the level of the fermenter) by taking into account the biomass concentration.
    [0044] For the CNCM 1-4469 strain at pm "EQ 2: q02ciblex-0.006 * 1.07 + (0.011 + 0.001 + 0.009) * 0.17 + 0.08 * 0.8 = 0.106 g / g / hr which corresponds to: OTRcible = 0.106 * 7 = 0.74 g of O 2 per L of culture per hour or OTRcible = 0.106 * 7 * 1000/32 = 23 mmol of O 2 / L of culture and per hour For the strain CNCM 1-4702 by placing at "EQ 2: q02cible - 0.006 * 1.07 + (0.02 + 0.018 + 0.07) * 0.17 + 0.17 * 0.8 = 0.218 g / g / h which corresponds to: OTRcible = 0.218 * 4 = 0.87 (g of 02 per L of culture per hour) OTRcible = 0.218 * 4 * 1000/32 = 27.4 mmol of 02 / L of culture and by / h The use of these equations given by the data of Table X makes it possible to simulate the culture, and to determine OTRcible to be applied. The latter is reduced with the decrease in the growth rate, but this is partially offset by the increase in biomass concentration. TARGET remains close to that expressed above until reaching a growth rate of biomass excluding zero lipids. Example 3: Fermentation line with different OTR conditions The tests carried out in Examples 1 and 2, without limitation in nutrient sources, make it possible to establish a model by which it is possible to control the production of lipids while respecting a target q02. defined by equation 2 (which is 27.4 mmol of O 2 / L of culture and per hr - see Example 2). From this initial target q02, variations were tested. The levels of variation, on both sides of this target q02, are illustrated here by the max OTR at the beginning of culture.
    [0045] The maximum OTR value of between 25 and 30 corresponds to the optimum OUR at the beginning of culture defined in the context of the invention for controlling the supply of oxygen and in order to respect the target q02.
    [0046] Table XI presents the fermentation parameters measured at T65 with CNCM 1-4702. Table XI Concentrations% of q02 OTR Max Biomass Fatty Acids Palmitic acid DHA target (mmol / L / h) (g / L) (g / 100g) of (g / 100 g lipid) (g / 100 g at the beginning of biomass lipid culture) 60 15 41 41 36 48 75 20 52 41 36 46 100 25 57 47 39 45 30 60 48 43 43 150 40 74 55 49 37 200 50 81 61 57 30 Thus, on the basis of these results, it is possible to note that when the oxygen is brought in excess of the value defined by the equation 2, there is a dilution of DHA in the overflow lipids, especially palmitic acid. On the other hand, when the oxygen supply is suboptimal compared to the value defined by equation 2, the quantity of DHA produced is smaller.
    [0047] Example 4 Comparative Example with and Without Limited Nitrogen Deficiency The tests were carried out with: in Control: the strain CNCM 1-4702, cultivated under the conditions defined in the state of the art constituted by the patent application WO 01/54510, that is to say decoupling growth and production phase, itself induced during the step of limiting the supply of nitrogen source. This limitation has here been induced by the interruption of pH regulation with ammonia at the end of the first third of the culture. In order to account only for the behavior of the CNCM 1-4702 strain in its lipid production under nitrogen deficiency conditions, the aeration was not cascade regulated, but maintained at a pO 2 greater than 10% . a fermentation in which, during the entire duration of the culture, no nutritional limitation was imposed on the strain, and the pO 2 was also regulated at 10%. The results are as follows: Table XII No nutrient limitation Nitrogen limitation Biomass (g / L) 76 86 Fatty acids on biomass (g / g) 0.57 0.65 Palmitic / AG (g / g) 0.67 0.62 DHA / AG (g / g) 0.21 0.24 The fatty acid content of biomass is only slightly reduced without any nutritional restrictions. Contrary to the technical prejudices in the field, a nitrogen source limitation is therefore not necessary to induce the production of lipids. Example 5 Comparative Example with the ATCC 20888 Strain The culture protocol used is that described in Example 4 of Patent Application WO 01/54510. The strain used is Schizochytrium sp ATCC 20888.
    [0048] It is followed by the teaching of the said request, in comparison with the following two modes of conduct: 1. A permanent regulation higher than 10 (3/0 2. A p02 of 0% constant The results obtained are presented in the following table XIII .
    [0049] Table XIII pO 2 0% constant pO 2 according to pO 2 10% constant protocol WO 01/54510 (8 - 4 - 0.5 to 0%) Time (h) 74 74 74 PUFA / total fatty acids (%) 44.0 43, 8 36.1 DHA / total fatty acids (%) 33.6 32.8 27.1 total fatty acids (%) Biomass 45.9 44.6 44.8 Total biomass (g / L) 166 147 187 DHA g / L / h 0.35 0.29 0.31 DHA% Biomass 15 15 12 Inoculum (indicative) g / L 23 10.5 11 Following the teachings of the state of the art, including those of the patent application WO 01/54510, it is thus found that, contrary to what is disclosed, a constant regulation of the pO 2 at 0% or at more than 10% during the entire duration of the fermentation made it possible to produce more than 35% PUFA in fatty acids, just as with a reasoned conduct with a reduction of the pO 2 in cascade (10%, then 4%, then 0.5% of saturation).
    权利要求:
    Claims (4)
    [0001]
    CLAIMS1- A process for producing a microalgae biomass of Thraustochytrium genus enriched in docosahexaenoic acid (DHA), characterized in that, during the culture phase under heterotrophic conditions, the oxygen supply is controlled so as to satisfy only the requirements of oxygen 1) for the production of energy necessary for cell maintenance,
    [0002]
    2) for the production of basic lipids, and
    [0003]
    3) for the growth of biomass excluding fatty acids. 2- Method according to claim 1, characterized in that the supply of oxygen necessary to satisfy only the needs 1), 2) and 3) is calculated by the following equation 2 q02Cible = (qm X 6x32 (glipiddebase xy nhipides) + (1.1 y 02/0 in which q02Cible is the quantity of oxygen in gram per gram of biomass excluding fatty acids and hour; qm is maintenance coefficient expressed in g of glucose per g of biomass excluding fatty acids and per hour; base is the rate of accumulation of basal lipids expressed in g of basal lipids per g of biomass excluding fatty acids per hour, y02iiedes is the coefficient of oxygen consumption compared to the formation of lipids expressed in g d oxygen per g of lipids, p is the growth rate expressed in g of biomass excluding fatty acids formed per g of biomass excluding fatty acids and per hour, that is (h-1), y ° 2 /, is the coefficient of consumption of oxygen in relation to your biomass formation excluding fatty acids expressed in g of oxygen per g of biomass excluding fatty acids. 3- Process according to any one of the preceding claims, characterized in that no limitation of a nutrient, especially carbon source or nitrogen, is applied during the fermentation process.
    [0004]
    4. Process according to any one of the preceding claims, characterized in that the microalgae are of the genus Schizochytrium sp or Schizochytrium mangrovei. A process according to any one of the preceding claims, characterized in that the microalgae are a strain selected from strains CNCM 1-4469 and CNCM 1-4702 deposited in the National Collection of Cultures of Microorganisms of the Institut Pasteur on April 14, 2011 and November 22, 2012. 6- Process according to any one of the preceding claims, characterized in that it further comprises the harvesting of biomass, optionally the preparation of an extract or cell lysate from this biomass, then optionally the extraction of a crude oil rich in DHA. 7- Process according to any one of the preceding claims, characterized in that the biomass obtained comprises at least 40% of DHA by weight of total fatty acids. 8- Process according to any one of the preceding claims, characterized in that the biomass obtained comprises at most 40% of palmitic acid by weight of total fatty acids. 9- Process according to any one of the preceding claims, characterized in that the biomass obtained comprises at least 25% fatty acids by dry weight of biomass.
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    同族专利:
    公开号 | 公开日
    ES2738672T3|2020-01-24|
    CN105829540B|2019-11-22|
    EP3083973A1|2016-10-26|
    CA2931233A1|2015-06-25|
    US10392636B2|2019-08-27|
    AU2014369524A1|2016-06-09|
    LT3083973T|2019-09-25|
    CN105829540A|2016-08-03|
    AU2014369524B2|2018-04-12|
    JP2017500044A|2017-01-05|
    FR3015516B1|2016-01-22|
    US20160298149A1|2016-10-13|
    WO2015092301A1|2015-06-25|
    KR20160098233A|2016-08-18|
    EP3083973B1|2019-05-08|
    JP6584409B2|2019-10-02|
    KR102247276B1|2021-05-03|
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    优先权:
    申请号 | 申请日 | 专利标题
    FR1362962A|FR3015516B1|2013-12-19|2013-12-19|PROCESS FOR ENHANCING DHA BIOMASS OF MICROALGUES OF THE GENUS THRAUSTOCHYTRIUM|FR1362962A| FR3015516B1|2013-12-19|2013-12-19|PROCESS FOR ENHANCING DHA BIOMASS OF MICROALGUES OF THE GENUS THRAUSTOCHYTRIUM|
    AU2014369524A| AU2014369524B2|2013-12-19|2014-12-18|Method for enriching the biomass of Thraustochytrium genus microalgae with DHA|
    US15/100,377| US10392636B2|2013-12-19|2014-12-18|Method for enriching the biomass of Thraustochytrium genus microalgae with DHA|
    CA2931233A| CA2931233A1|2013-12-19|2014-12-18|Method for enriching the biomass of thraustochytrium genus microalgae with dha|
    LTEP14830829.9T| LT3083973T|2013-12-19|2014-12-18|Dha enrichment process of the traustochytrium species microalgae|
    CN201480068877.2A| CN105829540B|2013-12-19|2014-12-18|Method for being enriched with the biomass of the genus thraustochytrium microalgae with DHA|
    EP14830829.9A| EP3083973B1|2013-12-19|2014-12-18|Dha enrichment process of the traustochytrium species microalgae|
    ES14830829T| ES2738672T3|2013-12-19|2014-12-18|DHA enrichment procedure of the microalgae biomass of the Traustochytrium genus|
    JP2016541224A| JP6584409B2|2013-12-19|2014-12-18|Method for concentrating biomass of microalgae of the genus Schizochytrium with DHA|
    KR1020167015420A| KR102247276B1|2013-12-19|2014-12-18|Method for enriching the biomass of thraustochytrium genus microalgae with dha|
    PCT/FR2014/053430| WO2015092301A1|2013-12-19|2014-12-18|Method for enriching the biomass of thraustochytrium genus microalgae with dha|
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