KR101997026B1 - Composition for promoting differentiation or proliferation of natural killer cell comprising sesamolin - Google Patents

Abstract

The present invention relates to a novel use of sesamolin having the activity of promoting differentiation or proliferation of natural killer cells. More specifically, the present invention relates to a novel use of sesamolin for promoting the differentiation or proliferation of natural killer cells comprising sesamolin as an active ingredient The present invention relates to a method for promoting the differentiation or proliferation of natural killer cells, comprising the step of treating a natural killer cell with a composition, a medium composition for differentiation or proliferation of natural killer cells, and sesamolin. Cetamolin according to the present invention is excellent in the activity of promoting the differentiation, proliferation and maturation of natural killer cells, and is capable of easily securing a large number of natural killer cells as a cell therapy agent that targets and kills diseased cells .

Description

TECHNICAL FIELD The present invention relates to a composition for promoting the differentiation or proliferation of natural killer cells comprising ceasaroline as an active ingredient,

The present invention relates to a composition for promoting the differentiation or proliferation of natural killer cells comprising sesamolin as an active ingredient.

Of the cells that make up the immune system, in particular natural killer cells (NK cells), function to remove host cells, bacteria, intracellular parasites or virus-infected host cells without pre-sensitization by the antigen , Rejection of inadequate bone marrow transplantation, and regulation of immune responses in T cells, acting on the first line of the in vivo immune system defense mechanism.

As a result of investigating the ability of NK cells to selectively kill cancer cells, many studies have been conducted. In cancer patients, the number and activity of NK cells in the peripheral blood were decreased compared with those in normal subjects. It is known that the risk of cancer development and metastasis increases if it is lowered. In addition, NK cells play an important role in the innate immune response against host-infected pathogens or cancer cells and the acquired immune response through cytokine secretion. The main mechanism that NK cells use to kill target cells is perforin ) And granzyme B are secreted into the target cells through the immune synapses. The secreted perforin makes a hole in the target cell wall, and the granzyme that enters the target cell through the hole carries the target cell Induce apoptosis.

Thus, NK cells have been shown to play a crucial role in cancer progression, in which cells are transformed into malignant cells, and in the early stages of viral infection. Based on these studies, NK cells using NK cells With the emergence of cell therapy, research on NK cells is actively under way.

On the other hand, in order to effectively utilize NK cells for the treatment of immune cells such as anticancer, a large number of NK cells are required to be secured. However, NK cells are only 5 to 15% of lymphocytes in the blood, even in normal persons, and the number, differentiation and function of NK cells are often lowered in cancer patients, and it is difficult to obtain sufficient cell numbers for treating diseases It is true. In addition, NK cells obtained according to the method of proliferation of existing NK cells have various variations in proliferation rate and cytotoxic activity. Therefore, new NK cell proliferation, differentiation, or maturation methods are strongly needed for securing a large amount of NK cells that maintain the therapeutic activity of diseases such as sufficient tumor cell killing ability.

Thus, the present invention has been completed by constructing a method for securing a large amount of NK cells by first confirming that ceasaroline has an activity of promoting differentiation, proliferation and maturation of NK cells.

Korean Patent No. 10-1283634

Accordingly, an object of the present invention is to provide a composition for promoting the differentiation or proliferation of natural killer cells, which comprises sesamolin as an active ingredient.

Another object of the present invention is to provide a medium composition for the differentiation or proliferation of natural killer cells comprising sesamolin as an active ingredient.

Another object of the present invention is to provide a method for promoting the differentiation or proliferation of natural killer cells, which comprises treating sesamolin to natural killer cells.

In order to achieve the above object, the present invention provides a composition for promoting the differentiation or proliferation of natural killer cells, comprising sesamolin as an active ingredient.

In one embodiment of the present invention, the sesamolin may be one that increases the expression of CD56, CD107a and NKG2D in naturally occurring kill cells.

In addition, the present invention provides a medium composition for differentiation or proliferation of natural killer cells comprising sesamolin as an active ingredient.

In one embodiment of the present invention, the ceasaroline may be contained in an amount of 10 to 100 μg / ml.

In addition, the present invention provides a method for promoting the differentiation or proliferation of natural killer cells, comprising treating sesamolin to natural killer cells.

In one embodiment of the present invention, the sesamolin may be treated with the natural killer cells at a concentration of 10 to 100 μg / ml and then cultured for 24 to 72 hours.

The present invention relates to a novel use of sesamolin having the activity of promoting the differentiation or proliferation of natural killer cells. The present invention provides a novel use of sesamolin for promoting the differentiation, proliferation and maturation of natural killer cells, It is possible to obtain a large number of natural killer cells having the function of a cell therapy agent that can be targeted and treated.

FIG. 1 shows the results of confirming the cytotoxicity of sesamolin after treatment of natural killer cells with the concentration of sesamolin.
FIG. 2 shows the results of measuring the degree of CD56 expression, which is a cell differentiation marker, through flow cytometry to determine whether or not cell differentiation of natural killer cells is promoted by treatment with sesamolin.
3A shows the results of an analysis of the degree of increase in the expression of CD107a, a cell maturation factor, in a natural killer cell according to the sesamolin treatment by a flow cytometer,
FIG. 3B shows the results of flow cytometry analysis of the degree of increase in the expression of NKG2D, a cell maturation factor, in natural killer cells following treatment with sesamolin.
Fig. 4 shows the results of analyzing the cytotoxic capacity-enhancing effect of natural killer cells by treatment with sesamolin.

The present invention is characterized by providing a novel use of sesamolin having the activity of promoting differentiation or proliferation of natural killer cells.

Natural killer (NK) is a primary line of defense against infection or cancer cells, and is a circulating lymphocyte in the blood. By stimulating secretory proinflammatory cytokines and cytotoxicity, natural killer cells eliminate infected cells or metastasized cells in the body.

Therefore, in order to effectively use the natural killer cells having the therapeutic effect of the disease as a cell therapy agent, a large number of natural killer cells are required, but it is difficult to obtain a sufficient number of cells because the natural killer cells are present in a small amount in the lymphocytes in the blood. In addition, in order to treat cells using natural killer cells, it is necessary to cultivate the cells in vitro, and it is necessary to optimize the extracellular differentiation conditions of natural killer cells.

In this respect, it has been confirmed that the present invention can effectively assure the differentiation, proliferation or maturation of natural killer cells when treated with natural killer cells, as a method for securing a large number of natural killer cells.

Accordingly, the present invention can provide a composition for promoting the differentiation or proliferation of natural killer cells comprising sesamolin as an active ingredient.

On the other hand, it is known that sesamolin has an antioxidant activity as one of the unique components of sesame oil, and no research on other functions has been reported. Thus, the present invention firstly clarified the function of ceasaroline to affect the differentiation and proliferation of NK cells.

The term " promoting the proliferation of natural killer cells " in the present invention means that the number of natural killer cells is increased in vivo or in vitro in pure killer natural killer cells , Which means that the natural killer cell proliferating ability is increased when the sesamolin is treated in comparison with the control group not treated with ceasaroline.

In vivo, natural killer cells undergo differentiation in the bone marrow, and the microenvironment of bone marrow is essential for the differentiation of natural killer cells. Natural killer cells are characterized by sequential acquisition of various surface molecules as they undergo differentiation processes.

In one embodiment of the present invention, the expression of CD56, CD107a and NKG2D, which are differentiation and maturation markers of natural killer cells, was confirmed in order to confirm the differentiation and maturation promoting ability of natural killer cells by the sesamolin treatment.

Therefore, in the present invention, the term " promoting the differentiation of natural killer cells " means promoting the differentiation from the precursor state of natural killer cells into mature natural killer cells, and also means increasing the activity of mature natural killer cells. Specifically, it means that the differentiation of natural killer cells is increased when treated with ceasaroline compared with the control without treatment with sesamolin.

The activity of the natural killer cell means that the action of the function of the natural killer cell described above occurs or increases, and refers to the ability to detect and kill or kill an infectious cell, nonspecific infectious pathogen, cancer cell, and the like.

The present invention also provides a medium composition for the differentiation or proliferation of natural killer cells comprising sesamolin as an active ingredient.

The medium composition of the present invention can be used by adding ceasaroline to a basic medium used for culturing a normal natural killer cell. The term " basic medium " used in the present invention is a culture medium for animal cells, which basically includes inorganic salts, carbon sources, amino acids, bovine serum albumin (BSA) And may include all of the medium. Particularly preferably, the culture medium contains NaCl, KCl and NaHCO3 as inorganic salts, and includes glucose, sodium pyruvate and calcium lactate as a carbon source, and includes essential amino acids and non-essential amino acids including glutamine as amino acids , Other trace elements and buffers as cofactors, and the like.

More preferably, the medium may also comprise an antibiotic. As a preferred embodiment, the basic medium may include various commercially-known mediums for animal cell culture such as DMEM (Dulbecco's Modified Eagle's Medium), EDM (Endothelial differentiation medium), MEM (Minimal Essential Medium), BME Medium Eagle, RPMI1640, F-10, F-12, α-Minimal Essential Medium, G-MEM and Iscove's Modified Dulbecco's Medium. But is not limited thereto.

Further, the present invention provides a method for promoting the differentiation or proliferation of natural killer cells, comprising treating sesamolin to natural killer cells.

The above-mentioned " treatment with natural killer cells " includes direct injection into tissues containing natural killer cells, blood, serum or the like, or addition of natural killer cells purely isolated in vitro to the culture medium before or during culturing. By treating the above-mentioned sesamolin with natural killer cells, the effect of proliferation and differentiation of natural killer cells by treatment with sesamolin can be further increased.

Generally, there are two ways of propagating natural killer cells. One of them is a method of purely isolating natural killer cells, followed by appropriate stimulation using feeder cells. In another method, peripheral blood lymphocytes (PBL) or peripheral blood lymphocytes There is a method of selectively extracting natural killer cells from peripheral blood mononuclear cells (PBMC) to obtain relatively many natural killer cells. However, since the natural killer cells obtained by the conventional method have low cell killing ability and are not only pure natural killer cells but also T cells, there is a tendency that T cells which recognize self and non-self by self-MHC molecules There is a problem in that it is limited to self-implantation unless cells are removed.

However, the natural killer cells treated with the sesamolin according to the present invention can significantly increase the proliferation of the natural killer cells by a simple method of treating only the sesamolin, and the natural killer cells treated with the sesamolin have excellent cell kill ability Were confirmed through experiments.

The method of treating the natural killer cells according to the present invention is carried out by treating the natural killer cell itself or the culture solution of the cell with 10 to 100 μg / ml of sesamolin for 24 to 72 hours .

When the concentration is less than 10 μg / ml, there is a problem that the proliferation and differentiation effects of natural killer cells can not be derived. On the other hand, treatment of more than 100 μg / ml may cause toxicity to the natural killer cell itself , There is also an uneconomical problem in that a better effect is not induced.

In addition, according to the method of the present invention, it is possible to obtain a large number of mature natural killer cells in which proliferation and differentiation have sufficiently progressed within a short period of 24 to 72 hours by treating with sesamolin, thereby enhancing the production efficiency of natural killer cells.

Hereinafter, the present invention will be described in more detail with reference to Examples. These examples are for further illustrating the present invention, and the scope of the present invention is not limited to these examples.

< Example  1>

Cesar Moline  Check cytotoxicity

In order to confirm the cytotoxicity of sesamolin, the natural killer cell (NK cell) was treated with ceasaroline for each concentration and cultured for 72 hours, and the cytotoxicity was analyzed by cell viability measurement.

As a result, as shown in Fig. 1, it was found that the cell survival rate did not significantly change in the sesamolin-free treatment group and the treatment group.

Therefore, it was confirmed that ceasaroline did not induce toxicity to cells and was stable in cells.

< Example  2>

Cesar Moline Natural killer cell  Identification of cell differentiation increasing activity

In order to analyze the effect of sesamolin on the cell differentiation of natural killer cells, NK precursor cells in vitro were treated with ceasaroline (10 μg / ml, 20 μg / ml, 40 μg / ml) The expression of CD56, a factor for confirming the differentiation of cells, was analyzed by flow cytometry.

As shown in FIG. 2, in the NK cells treated with the ceasaroline of the present invention, the number of CD56-expressing cells was larger than that of the untreated control, and the degree of expression of CD56 .

These results indicate that the sesamolin of the present invention has an activity of promoting the differentiation of natural killer cells.

< Example  3>

Cesar Moline Natural killer cell  Identification of cell maturation promoting activity

In order to analyze whether cytosmolin affects the cell maturation of natural killer cells, the present inventors also examined whether the degree of expression of CD107a and NKG2D, which are cell maturation factors (markers), was measured by flow cytometry Respectively.

As a result, as shown in Figs. 3A and 3B, it was found that the number of cells expressing CD107a and NKG2D was increased on the surface of NK cells depending on the treatment concentration of sesamolin. Therefore, the inventors of the present invention have found that the sesamolin of the present invention can promote not only the differentiation of natural killer cells but also the cell maturation.

< Example  4>

To Sesamolin  by Natural killer cell Diseased cell Kill ability  Confirm

It was confirmed that when the sesamolin was treated with NK (natural killer cells), the cell differentiation and cell maturation of NK cells could be promoted through the above examples. Therefore, the present inventors conducted the following experiment to determine whether natural killer cells promoted differentiation and maturation by treatment with sesamolin can enhance the killing ability of diseased cells. First, as shown in the following table, each test group was treated with different amounts of ceasaroline, and the cytotoxicity of cancer cells by NK cells was analyzed as cytotoxicity.

Experimental group Experimental group Processing contents Group A (20 / / ml, 40 / / ml) for NK cells, and treated with sesamolin Group B (20 / / ml, 40 / / ml) was added to NK cells, Group C Treatment with sesamolin (40 μg / ml), NK cells treated with sesamolin (20 μg / ml, 40 μg / ml)

As a result, as shown in Fig. 4, the group treated with sesamolin in both the cancer cells and the natural killer cells was superior to the group treated with the sesamolin only in the cancer cells or natural killer cells, . In addition, the effect of increasing the killing ability of natural killer cells was found to be increased in proportion to the treatment concentration of sesamolin.

< Example  5>

To Sesamolin  by Natural killer cell  Confirm cell proliferation activity

Further, in order to confirm that the sesamolin of the present invention has an activity of promoting the proliferation of natural killer cells, the natural killer cells used in the above example were treated with the sesamolin of the present invention by concentration (10 μg / ml , 20 ㎍ / ml, 40 ㎍ / ml), and the degree of cell proliferation was measured using the CFSE dividing method. As a control group, a group not treated with sesamolin was used. CFSE dilution is a method to identify cell proliferation by labeling the protein in the cell with a fluorescent substance and then dividing the fluorescence-labeled proteins into two halves when the cell division (nuclear division and cytoplasmic division) divides the stem cells into two daughter cells. Cells were treated with 5 μM CFSE for 10 min at 37 ° C, reacted, washed three times with PBS buffer, and then the fluorescence intensity was measured using CFSE-labeled natural killer cells using a FACScalibur. Respectively.

As a result, the natural killer cell proliferation was markedly increased in the group treated with sesamolin compared to the untreated group, and it was confirmed that more cell division occurred depending on the concentration of sesamolin treatment, Molluscan induce and promote the proliferation of natural killer cells.

The present invention has been described with reference to the preferred embodiments. It will be understood by those skilled in the art that various changes in form and details may be made therein without departing from the spirit and scope of the invention as defined by the appended claims. Therefore, the disclosed embodiments should be considered in an illustrative rather than a restrictive sense. The scope of the present invention is defined by the appended claims rather than by the foregoing description, and all differences within the scope of equivalents thereof should be construed as being included in the present invention.

Claims (6)

delete delete A medium composition for promoting proliferation of natural killer cells, comprising sesamolin as an active ingredient. The method of claim 3,
Wherein the ceasaroline is contained at 10 to 100 占 퐂 / ml. A method for promoting the proliferation of natural killer cells in vitro, comprising treating sesamolin with natural killer cells. 6. The method of claim 5,
Wherein said sesamolin is treated with said natural killer cells at a concentration of 10 to 100 占 퐂 / ml and then cultured for 24 to 72 hours.

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