• 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:
    Method for obtaining an extract of algae. The object of the invention is a method for obtaining an extract of algae that starts from the mass of algae, which is subjected to a solid-liquid extraction process, at a high temperature and at atmospheric pressure conditions. The product obtained from the claimed method and its use for the preparation of agricultural biostimulants is also an object of the invention. (Machine-translation by Google Translate, not legally binding)
    公开号:ES2796961A1
    申请号:ES201930478
    申请日:2019-05-30
    公开日:2020-11-30
    发明作者:Sendra Fernando Feliu;Sendra Carlos Feliu
    申请人:Plymag S L;
    IPC主号:
    专利说明:

    [0004] TECHNICAL SECTOR
    [0005] The present invention belongs to the technical field of the chemical industry and, in particular, it relates to an improved method for obtaining algae extract. In more particular it refers to a method for obtaining algae extract that comprises chopping the fresh algae, drying and / or dehydrating it, mixing with water, and macerating at a high temperature until obtaining a solid phase and a liquid phase, and then , stabilize the liquid phase and filter to finally obtain the algae extract. The present invention also relates to the use of the product obtained by the claimed method as a biostimulant in plant crops.
    [0007] BACKGROUND OF THE INVENTION
    [0008] At present, there are some substances that are gaining great importance within the agricultural industry called agricultural biostimulants and that act on the physiology of the plant in different ways and by different ways to improve the vigor of the crop, the yield and quality of Harvest. These products have various origins, and because, when applied to plants, they are capable of improving their efficiency in the absorption and assimilation of nutrients, tolerance to biotic or abiotic stress or improve any of their agronomic characteristics, their use each it is more and more widespread in a great variety of crops.
    [0010] One of the main origins of agricultural biostimulants is seaweed extracts. In fact, there are currently several companies worldwide that are producers of algae extracts in the agricultural sector, the company Kelp Products International, which produces an extract of the algae species Ecklonia maxima and is the holder of patent No. ZA201300362 (B ), the Afrikelp company, which also produces various seaweed extracts, for its own products and for other companies in the agricultural sector, and the PLYMAG company, holders of this patent application.
    [0011] In order to prepare biostimulants whose origin is algae, companies in the sector specialized in this type of product have developed different techniques to obtain their extract.
    [0013] In the previously referenced patent ZA201300362 (B), a process for obtaining the algae extract is described, which is called "Cold cell breaking technique", a process that consists of cutting and washing the algae, to later introduce it into a chamber of Pressure where the raw material is subjected to an extremely high pressure between 400 and 600 bar and which is only maintained for a short period of time. Subsequently, said pressure decreases rapidly to atmospheric pressure, through the use of an exhaust valve. This change Sudden pressure is what causes the cells to break. Finally, the liquid fraction is recovered, while the residue in the form of pulp remains inside the chamber. In this way, an algae extract is obtained without using products chemicals, heat, freezing or dehydration.
    [0015] On the other hand, the Afrikelp company has also developed its own process for obtaining algae extract, which it calls the Cold Micronization Process, which is based on micronizing and filtering fresh algae, without using any type of chemical product or making use of elevated temperatures.
    [0017] However, both the process described by patent ZA201300362 (B) and the one described by the Afrikelp company present a great limitation since their performance in both processes is conditioned by the amount of matter from which they start. In both procedures, it is necessary to start with a high amount of raw material in order to obtain a high amount of extract, which implies a high cost both in raw material and during the process of obtaining the algae extract.
    [0019] For this reason, it has been seen the need to develop a new procedure for extracting algae, which allows increasing its yield by obtaining more extract with the same amount of algae, without losing the activity of said extract.
    [0021] That is why the present invention aims to solve in an economically viable and efficient way the problem of high costs and technological difficulties of the methods currently used in the industry by means of a new procedure for obtaining completely algae extract. different from the previous ones, starting from the raw material, the high performance of the process, that is, obtaining a higher concentration of algae extract per unit volume of product, which also comprises surprisingly effective phytohormones.
    [0023] DESCRIPTION OF THE INVENTION
    [0024] The present invention refers to a new method for obtaining an extract of algae characterized in that it comprises:
    [0025] (a) Introduce algae mass with a humidity between 2 to 85% w / w in a reactor with water in a proportional amount Kg water / Kg algae between 0.5-15;
    [0026] (b) allow the mixture obtained in the previous step to marinate for a period of time from 0.5 to 48 hours at a temperature of between 40-98 ° C and, subsequently,
    [0027] (c) separating the solid phase from the liquid phase when the liquid phase has reached the desired dry residue of between 1.5 to 3.5% w / w,
    [0028] (d) filter the liquid phase obtained through a bag filter with a pore size equal to or greater than 80 µm.
    [0030] In step (c), a dry residue expressed in% w / w is obtained, which in the context of the present invention, reflects the amount of product that remains when all the water is removed from the sample. Serve as an illustrative example, in the event that in step (c) a dry residue of 3% w / w is obtained, it would indicate that if we take 100 g of the sample and eliminate the water it contains, 3 g of residue will be obtained dry, which in the case of not having added any external component, will be 3 g of pure solid extract of algae.
    [0032] It should be noted that the method object of the invention is carried out at atmospheric pressure. In this regard it is intended to indicate that the name of atmospheric pressure at a point is known as the "weight" of the column of air that is above said point until the atmosphere is exhausted. This value, as can be understood, is very difficult to determine because the density of the air decreases with height, affecting the mass and, as a consequence, the weight, in addition to varying with weather conditions. In general, the value of atmospheric pressure can vary around 1 atm, which corresponds to 101325 Pa, and can vary exclusively based on atmospheric conditions as indicated above.
    [0033] In a preferred embodiment of the present invention, the raw material used to carry out the method object of the invention is dehydrated Ecklonia maxima seaweed mass with a humidity comprised between 2 to 30% w / w and in a more preferred embodiment, said mass can have a humidity comprised between 3 to 15% w / w. Furthermore, in this preferred embodiment, taking into account the relative humidity of the starting material, the proportional amount of Kg water / Kg algae that is introduced into the reactor of stage (a) is between 7-15.
    [0035] In another preferred embodiment of the present invention, the raw material used to carry out the method object of the invention is Ecklonia maxima seaweed mass with a humidity comprised between 70 to 85% w / w and in a more preferred embodiment, said dough can have a moisture content of 77-83% w / w. Furthermore, in this preferred embodiment, taking into account the relative humidity of the starting material, the proportional amount of Kg water / Kg algae that is introduced into the reactor of stage (a) is between 0.5-7.
    [0037] Within the scope of protection of the claimed method, in the maceration stage the mixture obtained in step (a) is carried out for a period of time from 0.5 to 48 hours, being even more preferred, a period of time between 2 to 20 hours, and even more preferred in a time between 3 and 12 hours. On the other hand, said maturation is carried out at a temperature that can be comprised between 40-98 ° C, being in a preferred embodiment between 60 and 95 ° C, and even more preferred, between 70 and 95 ° C.
    [0039] In particular embodiments of the invention, the method may additionally comprise a stage where the liquid phase obtained in stage (c) can be stabilized by adding 0.1 to 1.5% w / w of an aqueous preservative within the scope of the present invention whose purpose is the microbiological control in systems highly susceptible to contamination. In a preferred embodiment of the present invention, the preservative used can be of the aqueous type and which also comprises in its base composition heterocycles and disinfectant aldehydes. Said use of the preservative aims to extend the useful life of the product, controlling the growth of any type of microorganism that may grow in said extract, deteriorating its composition.
    [0041] In particular embodiments of the invention, the method may additionally comprise a stage where the solid phase obtained in step (c) is macerated again with an amount of water comprised between 0.1-10 times the amount of solids present. in the extractor, for a period of time from 0.5 to 48 hours at a temperature between 40 to 98 ° C, obtaining a new liquid phase and a new solid phase. After this stage, the new liquid phase can be used in step (a) by substituting the proportional amount of water used in said step (a), repeating again the process of obtaining the extract. On the other hand, the solid phase obtained in said step can be reused as fertilizer or animal feed, and ultimately, discarded.
    [0043] On the other hand, in a preferred embodiment of the claimed method, the filtration of the liquid phase obtained in step (c) is carried out through a mesh filter of known diameter, said preferred diameter being up to a maximum of 80 µm , with a maximum size of 50 µm being even more preferred.
    [0045] One of the main characteristics that differentiate the method object of the invention with the methods that exist in the state of the art described previously in the present document is that the starting material is subjected to the solid-liquid extraction process, at a high temperature and atmospheric pressure.
    [0047] Furthermore, another advantageous characteristic of the claimed process is that thanks to its configuration, the starting material can be both dehydrated seaweed material and fresh seaweed material, obtaining in both cases a high extraction performance of the extract.
    [0049]
    [0051] Table 1. Comparison of the method of patent application No. ZA201300362 (B), with respect to the method described in the present document.
    [0053] As indicated above, the method object of the invention is presented as an alternative to the methods for obtaining algae extract that currently exist in the state of the art, being totally novel and with a series of advantages that are indicated then.
    [0054] The main advantage of the claimed method is that a higher concentration of active matter can be extracted than that obtained with known methods and particularly, with the method defined by patent No. ZA201300362 (B). The main cause of the limitation of the process developed by the company Kelp Products International is that the final concentration of its product is limited by the active material / moisture ratio of the raw material from which the extraction method initially starts, since the extract is obtained directly from fresh algae, without concentrating or adding water.
    [0056] On the contrary, the method object of the invention allows the extraction parameters to be varied to obtain a desired concentration, regardless of the quality of the raw material or the humidity that the algae present.
    [0058] Likewise, the claimed method allows different concentration ranges to be obtained, since said method allows the temperature and the water / algae ratio to be varied, allowing in turn to control the richness of the extract obtained regardless of the quality of the algae used as raw material. .
    [0060] It should be noted that the claimed method, as indicated previously in the present document, is carried out under atmospheric pressure conditions, while the methods that currently exist in the state of the art use pressures between 400 and 600 bars.
    [0062] The algae extract obtained by the claimed method is also an object of the present invention. In a particular embodiment of the claimed method, when the raw material used is the algae is Ecklonia maxima, an extract of algae is obtained that presents surprisingly high auxinic and cytokinetic activity, as shown in examples 3 and 4 of this document. .
    [0064] Auxins are plant hormones that promote growth by facilitating cell elongation through their effects on the components of the cell wall. In addition, they can promote cell division and are involved in the development of lateral and adventitious roots. However, high concentrations of this hormone can also have a negative effect on growth. Fruit growth is another phenomenon controlled by auxins, together with the apical dominance of the terminal bud.
    [0065] Cytokinins are phytohormones that promote tissue cell division. In mature plants, one of the main synthesis sites is the root, from where they travel to the aerial part through the xylem. Also, cytokinins have an antisenescent or youth-maintaining effect. This effect is produced by preserving the levels of chlorophyll, proteins and nucleic acids, probably because they decrease their degradation rate and also because they maintain the integrity of the membranes. In turn, the mobilization of nutrients induced by cytokinins has been described, as well as the promotion of chloroplast development. These hormones are also involved in the promotion of lateral bud growth, and therefore, in the inhibition of apical dominance. The best known cytokinins are kinetin and zeatin.
    [0066] Finally, the use of a product obtained by the claimed method for the preparation of agricultural biostimulants is also an object of the present invention.
    [0068] BRIEF DESCRIPTION OF THE FIGURES
    [0069] For a better understanding of the present specification, the following figures are attached, by way of illustration and not limitation of the invention:
    [0070] • Figure 1 shows the primary leaves of bean plants submerged in the different treatments of indoleacetic acid solutions (IAA) and of the extract obtained by the method claimed from the product to be tested, keeping 1 cm of the leaf petiole.
    [0071] • Figure 2 shows the bean leaves in Petri dishes with filter paper moistened with distilled water.
    [0072] • Figure 3 shows the development of adventitious roots in petioles of bean leaves treated with the extract obtained by the claimed method.
    [0073] • Figure 4 is a graph showing the number of adventitious roots that have developed in exposed bean leaves with respect to treatments T, E, E 1: 2 and E 1: 5.
    [0074] • Figure 5 shows the development of callus (a) and adventitious roots (b) in the petioles of bean leaves treated with the extract obtained by the claimed method.
    [0075] • Figure 6 is a graph showing the relationship between the variables number of adventitious roots and IAA concentration after 2 weeks of treatment.
    [0076] • Figure 7 shows the cytokinetic activity bioassay based on the maintenance of chlorophyll concentration. The treatments analyzed were from left to right and from top to bottom: E, E 1: 2, E 1: 5, T, K -2, K -3, K -4, K -5, K -6.
    [0077] • Figure 8 is a graph showing the concentration of total chlorophylls in spinach leaves exposed for one week with respect to treatments T, E, E 1: 2 and E 1: 5.
    [0078] • Figure 9 shows the chlorosis status of spinach leaf discs after one week in dark conditions. The treatments being compared in the image are from left to right: T, K -3, E, and E 1: 2.
    [0079] • Figure 10 shows spinach leaf discs after one week of treatment in the dark. The treatments shown from left to right and top to bottom are: T, KIN -3, KIN -4, KIN -5, KIN -6, E and E 1: 2.
    [0080] • Figure 11 is a graph that shows the relationship between the variables concentration of total chlorophylls and Kinetin.
    [0082] PREFERRED EMBODIMENT OF THE INVENTION
    [0083] In order to contribute to a better understanding of the invention, and in accordance with a practical embodiment thereof, a series of examples is attached as an integral part of this description: a preferred embodiment of the claimed method, a comparative study of the extract obtained by the method in relation to other products found on the market, as well as studies of auxinic and cytokinetic activity of the extract obtained by the claimed method.
    [0085] Example 1: Method for obtaining an extract of algae where the raw material is the alga Ecklonia maxima.
    [0087] Next, a preferred embodiment of the method described herein is shown where the raw material is the alga Ecklonia maxima. This method comprises the following phases:
    [0088] (a) Introduce dehydrated seaweed mass with a humidity between 5 to 15% w / w in a reactor with water in a proportional amount Kg water / Kg seaweed of 9.29, (b) allow the mixture obtained in step to macerate above for a period of time of 3 to 6 hours at a temperature of between 80-90 ° C and then separate the solid phase from the liquid phase when the liquid phase has reached the dry residue of between 1.9 to 2.1 % w / w,
    [0089] (c) stabilize the liquid phase obtained in the previous step by adding 0.5% w / w of a preservative, and then, it is filtered through a membrane with a pore size equal to or greater than 80 µm.
    [0090] Example 2: Comparison of the extract obtained by the claimed method when the raw material is the alga Ecklonia maxima.
    [0092] Starting from the extract obtained by the method described in Example 1, a comparison is made of its composition with respect to the other extracts obtained from Ecklonia maxima that currently exist in the labeling and that are used as biostimulants.
    [0094]
    [0097] Table 2. Comparison of the composition of the different products that exist on the market that consist of extracts obtained from Ecklonia maxima with respect to Ecklonia maxima extract obtained in example 1.
    [0099] Example 3: Study on the auxin activity of the Ecklonia maxima extract obtained by the method claimed and described in example 1.
    [0101] In order to determine the auxin activity of the Ecklonia maxima extract obtained by the claimed method, leaves were used that were dipped in different treatments and dilutions of the extract obtained by the claimed method. It should be clarified at this point that some plants spontaneously produce roots at the terminations of split leaves or cuttings. However, in many other species roots do not develop, and treatment with auxins will allow such formation.
    [0103] The natural auxin in plants is a very simple substance, Indolacetic Acid (IAA). This compound is synthesized in the plant from the amino acid tryptophan. To level nursery, for vegetative propagation synthetic auxins such as indole butyric acid (IBA) and naphthaleacetic acid (ANA) are used.
    [0105] Based on this, for the auxin activity tests of the extract obtained by the claimed method, primary leaves of bean plants were used that were treated with IAA solutions of known concentration together with the product to be tested, keeping 1 cm of the petiole of the leaves immersed for 2 hours in said solution (Figure 1). After these 2 hours, the excised leaves were transferred to Petri dishes with filter paper moistened with distilled water (Figure 2). The plates were kept for 2 weeks in diffuse light and at room temperature in the laboratory. After 2 weeks, the development of roots in isolated leaves was analyzed by determining the number of roots formed.
    [0107] The treatments to which the leaves were subjected are the following:
    [0108] • Control (T) (distilled water)
    [0109] • Undiluted extract (E)
    [0110] • Extract dilution 1: 2 (E 1: 2)
    [0111] • Extract dilution 1: 5 (E 1: 5)
    [0112] • AIA 100 | jg ml-1 (AIA 100)
    [0113] • AIA 10 jg ml-1 (AIA 10)
    [0114] • IAA 1 jg ml-1 (IAA 1)
    [0115] • IAA 0.1 jg ml-1 (IAA 0.1)
    [0117] The results were statistically analyzed using the IBM SPSS program (v. 24) through a one-way ANOVA analysis of variance and the Tukeyb posterior test (p <0.05).
    [0119] As observed in Figure 3, the extract obtained by the claimed method was significantly effective in inducing the development of roots in petioles of bean leaves. Furthermore, this effect was independent of the dilution of the product used (Figure 4). It should be noted that the control treatment did not present any root development.
    [0121] After two weeks of the treatment with auxins or the extract, the petioles of the bean leaves showed in some cases the development of adventitious roots to a greater or lesser degree, from callus formation to well-differentiated roots (Figure 5).
    [0122] If the correlation is established between the number of roots developed in the excised leaves and the concentration of known IAA applied to the petioles of the leaves, we can extrapolate the auxin activity of the tested product. Figure 6 shows the mathematical relationship between both variables, after which the equivalent concentration of auxins of the product and their dilutions were calculated.
    [0124] The results of the auxin activity of the product are shown in Table 4:
    [0128] Table 4. Equivalent auxin concentration of the extract obtained by the claimed method.
    [0130] The extract obtained by the claimed method presented an auxin activity equivalent to 25 ppm, this activity being understood not as the concentration of auxins present in the product, but as its ability to stimulate root development. This response was independent of the dilution of the product used.
    [0132] Example 4: Study on the cytokinetic activity of the Ecklonia maxima extract obtained by the claimed method and described in example 1.
    [0134] In order to determine the cytokinetic activity of the Ecklonia maxima extract obtained by the claimed method, spinach spinach leaves were used.
    [0136] The excised leaves suffer an irreversible loss of chlorophylls that results in chlorosis, in addition to reducing their protein and nucleic acid content. This progressive senescent process can be delayed through the application of cytokinins, the concentration of chlorophylls being maintained proportional to the concentration of hormone applied.
    [0138] In this particular study, leaf discs were obtained from spinach leaves of known area with punches for maintenance in a Petri dish. 20 ml of the corresponding solution were added to each Petri dish, in which the leaf discs were placed with the underside in contact with the solution (Figure 7). Petri dishes are They were kept in darkness for a week, after which the concentration of total chlorophylls (chlorophylls a + b) was quantified spectrophotometrically after extraction in 96% ethanol and in a thermostatized bath at 80 ° C.
    [0140] The compared treatments were:
    [0141] • Control (T) (distilled water)
    [0142] • Undiluted extract (E)
    [0143] • Extract dilution 1: 2 (E 1: 2)
    [0144] • Extract dilution 1: 5 (E 1: 5)
    [0145] • Kinetin 10-2 M (K -2)
    [0146] • Kinetin 10-3 M (K -3)
    [0147] • Kinetin 10-4 M (K -4)
    [0148] • Kinetin 10-5 M (K -5)
    [0149] • Kinetin 10-6 M (K -6)
    [0151] The results were statistically analyzed using the IBM SPSS program (v. 24) through a one-way ANOVA analysis of variance and the Tukeyb posterior test (p <0.05).
    [0153] As seen in Figure 8, the extract obtained by the method of Example 1 was significantly effective in delaying foliar senescence determined as the degradation of chlorophylls after one week of tissue excision and under dark conditions. The dilution of the product with the factor 1: 5, even reducing the concentration of chlorophylls in comparison with the undiluted product, showed a significant antisenescent effect. In Figure 9, the comparison of the chlorosis status of the leaf discs can be observed after the week that the bioassay lasts. While the control treatment showed clear signs of chlorosis, both the high concentrations of Kinetin and the extract obtained in example 1 allowed to reduce said senescence. The visual comparison of all the treatments is shown in Figure 10. The decrease in the degradation of chlorophylls caused by the tested product could lead to a better maintenance of the photosynthetic rate and therefore, of the production.
    [0155] On the other hand, if the correlation between the concentration of chlorophylls present in the leaves is established as a function of a known applied Kinetin concentration, the cytokinetic activity of the tested product can be extrapolated. Figure 11 shows one of the correlations established between both variables as an example. One time Once the mathematical relationship between them was established, the equivalent concentration of Kinetin of the product and its dilutions were calculated. The results are shown in Table 4.
    [0160] Table 5. Kinetin equivalent concentration of extract obtained in example 1.
    [0162] The equivalent concentration of Kinetin of the extract obtained in Example 1 is of the order of 2500ppm (Table 4), understanding this cytokinetic activity not as the concentration of cytokinins in the product, but as its antisenescent capacity delaying the degradation of chlorophylls. As might be expected, this activity decreases significantly when the product is diluted 5 times.
    [0164] Example 5: Method for obtaining an extract of algae where the raw material is fresh Ecklonia maxima algae .
    [0166] Next, a preferred embodiment of the method described herein is shown where the raw material is the alga Ecklonia maxima. This method comprises the following phases:
    [0167] (a) Introduce hydrated seaweed mass with a humidity between 70 to 85% w / w in a reactor with water in a proportional amount Kg water / Kg seaweed of 0.5 -1.5, (b) let the mixture marinate obtained in the previous step over a period of time of 3 to 6 hours at a temperature between 80 ° C-90 ° C, and then
    [0168] (c) separating the solid phase from the liquid phase when the liquid phase has reached the dry residue of between 1.9 to 2.1% w / w,
    [0169] (d) stabilize the liquid phase obtained in the previous step by adding 0.5% w / w of a preservative, and then, it is filtered through a membrane with a pore size equal to or greater than 80 µm.
    权利要求:
    Claims (12)
    [1]
    1. A method for obtaining an extract of algae characterized in that it comprises:
    (a) Introduce mass of algae with a humidity comprised between 2 to 85% w / w in a reactor with water in a proportional quantity Kg water / Kg algae of 0.5-15;
    (b) let the mixture obtained in the previous step marinate for a period of time from 0.5 to 48 hours and at a temperature of between 40-98 ° C,
    (c) separating the solid phase from the liquid phase when the liquid phase has reached the dry residue of between 1.5 to 3.5% w / w,
    (d) filtering through a filter membrane with a pore size equal to or greater than 80 µm.
    [2]
    2. The method according to claim 1, characterized in that the mass of algae that is introduced into the reactor of step (a) is mass of dehydrated algae with a humidity comprised between 2 to 30% w / w.
    [3]
    3. The method according to claim 2, where the proportional amount of Kg water / Kg algae that is introduced into the reactor of stage (a) is between 7-15.
    [4]
    4. The method according to claim 1, characterized in that the mass of algae that is introduced into the reactor of step (a) is mass of fresh algae with a humidity comprised between 70 to 85% w / w.
    [5]
    5. The method according to claim 4, wherein the proportional amount of Kg water / Kg algae that is introduced into the reactor of step (a) is between 0.5-7.
    [6]
    6. The method according to any one of claims 1 to 5, characterized in that the method additional step where the liquid phase obtained in step (c) is stabilized by adding 0.1 to 1.5% w / w of a preservative.
    [7]
    7. The method according to claim 6, wherein the preservative can be a disinfecting heterocycle and / or aldehyde compound.
    [8]
    8. The method according to any one of claims 1 to 7, characterized in that it comprises an additional step where the solid phase obtained in step (c) is It macerates with a quantity of water between 0.1-10 times the quantity of solids present in the extractor, for a period of time from 0.5 to 48 hours at a temperature between 40 to 98 ° C, obtaining a new liquid phase and a new solid phase.
    [9]
    The method according to any one of claims 1 to 8, wherein the new liquid phase obtained in step (c) is used in step (a) by substituting the proportional amount of water used in said step (a).
    [10]
    10. The method according to any one of claims 1 to 9, wherein the species of algae from which the mass that is introduced into the reactor of step (a) is obtained is Ecklonia maxima.
    [11]
    11. Product obtained from the method described in claims 1 to 10.
    [12]
    12. Use of a product according to claim 11 for the preparation of agricultural biostimulants.
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    同族专利:
    公开号 | 公开日
    ES2796961B2|2021-05-21|
    CO2021017298A2|2022-01-17|
    WO2020260734A1|2020-12-30|
    引用文献:
    公开号 | 申请日 | 公开日 | 申请人 | 专利标题
    GB2150552A|1983-11-30|1985-07-03|Clearfield Nv|Fertilizer from seaweed|
    WO2013108188A1|2012-01-17|2013-07-25|Slack, Roy|Product for enhancing plant growth|
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    优先权:
    申请号 | 申请日 | 专利标题
    ES201930478A|ES2796961B2|2019-05-30|2019-05-30|METHOD FOR OBTAINING AN EXTRACT OF ALGAE|ES201930478A| ES2796961B2|2019-05-30|2019-05-30|METHOD FOR OBTAINING AN EXTRACT OF ALGAE|
    PCT/ES2020/070292| WO2020260734A1|2019-05-30|2020-05-08|Method for obtaining an algae extract|
    CONC2021/0017298A| CO2021017298A2|2019-05-30|2021-12-16|Method for obtaining an algae extract|
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