METHOD FOR DETERMINING TOXIC SUBSTANCES BY PLANT GEL AGAR COAGULATING

FIELD OF THE INVENTION

The present invention relates to a method for rapid determination of toxicity substance, in particular to a method for determining whether a sample is toxic by a plant gel agar coagulating. This method can reduce the use of animal or cell experiments, not only for the purpose of protecting the animal, also for reducing the cost of drugs, food or cosmetics in the toxicity test.

BACKGROUND OF THE INVENTION

According to the existing domestic and foreign regulations, for the safety of the human body, health food, new raw materials, drug-containing cosmetics, medical equipment and pharmaceuticals are required to have different toxicological assessment according to the different raw materials, such as acute toxicity experiments, eye irritation experiments, skin irritation experiments, etc. The aforementioned experiment is not only need to spend lots of money for animal experiments, but also sacrifice the lives of many animals.

In addition, the EU has banned the use of animals for cosmetics testing since March 2009, and EU regulations for cosmetics sales have been more regulated since 2013 to prohibit the use of animals as a cosmetic for toxic safety experiments. Cosmetics companies and academic organization are actively engaged in non-animal safety testing methods for cosmetics toxicity. The current developed methods mainly focus on cytotoxicity testing as a cosmetic safety indicator.

The aforementioned cytotoxicity as a cosmetic test indicator, although the animal has been avoided as a cosmetic toxicity safety test the subject of the missing, the culture cells still need to use a lot of serum and to consume a lot of time to observe the toxicity test results. Generally, the research and development cost is still too much for most manufacturers.

Accordingly, to develop a simple and rapid toxicity test method for reducing animal and cytotoxicity test and solving the lack of the existing technology, the relevant technical areas are currently urgently need to solve the problem.

SUMMARY OF THE INVENTION

In general, gelation refers to the branching of macromolecular chains that form a non-liquid colloid through a gradually increasing branching process, which depends on the structure and conformation of the starting material. And such polymer materials are known as “sol” due to the multi-branched water-soluble branch. The “infinite polymerization” structure is referred to as “gel” or “network”, because the gelation link process is accompanied by a gradual increase in the size of the branched polymer and a decrease in solubility. The transition from a limited branched polymer to an infinite polymeric structure is referred to as a “sol-gel transition” (or “gelation”). The different types of gelation mechanisms can be generated by physical linking (physical gelation) or by chemical attachment (chemical gelation). The physical hydrogel is formed by the intermolecular electrostatic force (ionic action), hydrogen bond and hydrophobic interaction, with the characteristics of change (reversibility).

In view of the above, the present invention provides a rapid and simple method for the determining toxic substances by measuring the coagulating time of plant gel agar coagulation to determine whether the sample affects the chemical bond, and further determining whether the sample has biological toxicity. Therefore, the use of animal or cell experiments can be reduced, not only for the purpose of protecting the animal, but also for reducing the cost of the drug, food or cosmetic test

Thus, the present invention provides a rapid and simple method for determining toxic substances by plant gel agar coagulating, which includes: step (1) preparing an agar and a sample, then heating the agar to be completely dissolved to form a hot agar solution; step (2) mixing the hot agar solution and the sample in a carrier to form a mixture; and step (3) cooling the mixture at room temperature to 25° C. during a time duration, wherein the time duration is coagulation time, and the cut-off time of the coagulation time is at 15 minutes to determine the cytotoxicity of the sample; Wherein the agar concentration of the hot agar solution is between 1-6% (w/w) and the volume of the hot agar solution is 1 mL to 250 mL; When the coagulating time is greater than the cut-off time, the sample is classified as a toxic substance; when the solidification time is greater than the cut-off time, the sample is classified as not a toxic substance.

The “irritation” is defined as the destruction of the cell membrane, cytoplasm, and organism, resulting in cell disintegration and necrosis. This disintegration necrosis is usually related to the destruction of the whole cell structure caused by foreign matter, such as structural damage to the constituent cytochemical composition.

In one embodiment of the present invention, the plant gel material is selected from agar.

Preferably, in one embodiment of the invention, the sample may be, for example, a drug, a food, or a cosmetic.

In other words, because the smallest unit of organism is cell, and cells contain a variety of life molecules formed by a variety of chemical bonding composition. Thus, the observation of life molecules disintegration of the degree of injury can be replaced by observation of the degree of chemical bond damage to be used as a toxicity indicator

In this way, the method of the present invention can quickly detect whether the sample is a toxic substance that affects cells or organisms. Even if the toxic substance is difficult to pass through the cell membrane or the cytotoxicity can be detected by long-term observation, it is still detectable through the method of present invention. Furthermore, the method of the present invention does not require the use of cell or animal experiments, thereby significantly reducing the cost of toxicity testing.

The present invention can be applied to the clinical trial design and management system, the IRB review operating system, the information system of the contract research institution (CRO), etc., which can support designing the clinical trial protocols under the regulation of clinical trial review unit Good Clinical Practice (GCP).

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 is a flow chart of the steps of the preferred embodiment of the present invention;

FIG. 2 is an analysis of the different concentrations of p-methylaminophenol sulfate and coagulation time of the present invention; p-Methylaminophenol Sulfate concentration increases the agglomeration time of agarose gel. 0 is the control group without adding p-Methylaminophenol Sulfate;

FIG. 3 shows the different concentrations of p-phenylenediamine (PPD) and the coagulation time of the present invention. The increase of PPD concentration affects coagulation time of agar gel. 0 is the control group without adding p-Phenylenediamine;

FIG. 4 shows the different concentrations of 2-aminophenol (2-Aminophenol) and the coagulation time of the present invention; the increase in the concentration of 2-Aminophenol affects the agglomeration time of agar. 0 is the control group without adding 2-Aminophenol;

FIG. 5 shows the different concentrations of Ammonium Lauryl Sulfate (ALS) and the coagulation time of the present invention. The increase of ALS concentration affects the agglomeration time of agar. 0 is the control group without adding ALS;

FIG. 6 is an analysis of the different concentrations of 3-aminophenol (3-Aminophenol) and coagulation time of the present invention. 3-Aminophenol concentration increased the agglomeration time of agar. 0 is the control group without adding 3-Aminophenol.

DETAILED DESCRIPTION OF THE INVENTION

The present invention is tested by different concentrations or different contents of cosmetic materials (samples). Wherein the cosmetic raw materials (samples) are selected from the group consisting of Ammonium Lauryl Sulfate, Butyl Paraben, Disodium Lauroamphodiacate, Monoethanolamine, Glycerin, Hydrogen Peroxide, Hydroxy Ethyl Cellulose, Lysine hydrochloride, methyl p-hydroxybenzate, Methylchloroisothiazolinone, Butylene glycol, p-Methylaminophenol Sulfate, Polyethylene Glycol, Polyquaternium-7, p-phenylenediamine Resorcinol, Salicylic Acid, 2-Aminophenol, 3-Aminophenol, Sodium Sulfide-9-Hydrate Squalane, Tocopherol Acetate, Trisodium Citrate Dihydrate, Isopropyl Myristate and Lactic Acid.

In one of the embodiment of the present invention, the plant gel material is selected from agar.

In one of the embodiment of the present invention is, for sample, but not limited to, a drug, a food, or a cosmetic.

The agar concentration of the present invention is, for example, but not limited to 1%, 2%, 3%, 4%, 5%, 6%. (w/w)

The agar volume of the present invention is from 1 ml (mL) to 250 ml (mL), for example, but not limited to 1 ml, 2 ml, 3 ml, 4 ml, 5 ml, 6 ml, 7 ml, 8 ml, 9 ml, 10 ml, 50 ml, 100 ml, 150 ml, 200 ml, 250 ml.

The coagulation time of the plant gel in the present invention, in particular the coagulation time of the agar gel.

The agar gel solution is dissolved as a clear solution from room temperature to 25° C. The agar gel solution is operated in the carrier, such as a bottle, or a test tube, and about 30°-60° (such as 45°) of the vertical plane of the ground. The coagulation time is defined when the agar gel solution does not flow.

Please refer to FIG. 1, wherein the present invention relates to a method for rapid determination of toxicity substance, in particular to a method for determining whether a sample is toxic by a plant gel agar coagulating.

Step 1 (S101): preparing a plant gel material and a sample.

Step 2 (S102): mixing the plant gel material and the sample to form a mixture.

Step 3 (S103): measuring the coagulation time of the mixture.

According to the present invention, the change of the gel bonding is equal to the damage of the living tissue and/or the cell structure caused by the sample, thereby causing the biological toxicity and irritation, so as to define the coagulation time.

The term “irritation” is defined as the destruction of the cell membrane, cytoplasm, and organogenesis, which is usually disintegrated and necrotic. This disintegration necrosis is usually related to the destruction of the whole cell structure caused by foreign matter, for example, with the constituent cytochemical composition bonding damage related. In other words, the “irritation” of the present invention may be derived from cell viability and cytotoxicity assays.

In addition, the scope of the present invention may be further illustrated by the following specific examples, but is not intended to limit the scope of the invention in any way.

Example 1:Cell Viability Analysis

The B16-F10 cells (purchased from the Food Industry Development Institute Fellowship Center/National Institutes of Health Cell Bank, ATCC number: CRL-6475) and skin 3T3 cells (purchased from the Food Industry Development Institute Center/National Institutes of Health Cell Bank, ATCC number: CCL-92) to test the toxicity of each sample (IC50; μg/ml).

Furthermore, the MTT reagent can be reduced to purple crystalline formazan by the mitochondrial enzyme of surviving cells, and the crystals are dissolved by DMSO (Dimethyl Sulfoxide). Then the absorbance of OD570 nm was measured, and the color depth is proportional with the number of viable cells. Skin B16-F10 cells and skin 3T3 cells are seeded in 96-well plates with 8×10³per well, and after 3-5 hours the cells are plated on 96-well plates and added to the sample (100 μl per well). After incubation for 24 hours, MTT reagent (MTT 5 mg/ml dissolved in PBS) was reacted for 1 to 2 hours. The culture medium in 96-well dish was blotted with MTT reagent and dissolved in 100 μl of DMSO. The absorbance values are read at a wavelength of 570 nm with an ELISA kit

The IC50 refers to half of the concentration of a drug or substance (inhibitor) that inhibits certain biological procedures (or some of the substances contained in the procedure, such as enzymes, cell receptors, or microorganisms), such as enzymatic reaction, or antigen-antibody reaction. In the cytotoxicity test, a specific concentration of a drug cause cell death by 50% is called 50% inhibition concentration. That means, the ratio of the dead cells and all cells is equal to 50% of the corresponding concentration IC50 value can be used to measure the death inducing ability of drugs, that is, the stronger the ability of the aforementioned drugs to induce death, the lower the value.

Therefore, the present invention obtains data on cytotoxicity IC50 of various cosmetics materials by cell survival analysis, and can be compared with the coagulation time of various cosmetic materials in the different embodiments described later.

Example 2: Evaluate the Effect of Various Cosmetic Materials on Agar Coagulation Time

The agar is extracted from the seaweed, and its polysaccharide body is closely related to the formation of the hydrogen bond during the cooling and coagulation. The invention utilizes a carrier such as a test tube to see the effect of added cosmetic material to the coagulation of agar, so as to assess the toxicity of cosmetic materials. In this example, the present invention further evaluates the relevance of the cosmetic material on agar coagulation time and the cytotoxic IC50.

The agar is prepared as the main application material for the plant gel material of the present invention and a different sample is prepared to test the coagulation time of the 25 samples as described above. For example, the concentrations of agar solutions are 1%, 2%, 3%, 4%, 5%, 6% (w/w). Especially, 3% agar solution is heated to 100° C. to dissolved, and then add 100 ml or 200 ml of agar solution to a bottle or a test tube with various samples (100 ml, or 200 ml) and mixed. Tilt the bottle, or test tube with a relative plane of about 45° to observe whether there is coagulation every 30 seconds, and recorded the cooling and coagulation time from 100° C. to room temperature.

The Equivalence is defined as =Number of Compounds Correctly Identified/Total Number of Compounds Tested.

The Sensitivity is defined as =Number of Irritants Correctly Identified/Total Number of Irritants (samples of irritated samples/all irritating samples).

The Specificity is defined as =Number of Non-Irritants Correctly Identified/Total Number of Non-Irritants (all non-irritating samples/all non-irritating samples).

The False positive rate is defined as =Number of Non-Irritants Classified as Irritants/Total Number of Compounds Tested (no irritating sample is detected as irritant/all samples).

False Negative Rate is defined as =Number of Irritants Classified as Non-Irritants/Total Number of Compounds Tested (irritated samples are measured as non-irritating/all samples).

TABLE 1

the relevance of the cosmetic material on agar coagulation time and the

cytotoxic IC50

Parameters 1
B16-F10
3T3

Equivalence (%)
92.0 (23/25)
92.0 (23/25)

Sensitivity (%)
100 (9/9)
100 (8/8)

Specificity (%)
87.5 (14/16)
82.35 (14/17)

The False positive rate (%)
0 (0/25)
0 (0/25)

False Negative Rate (%)
8.0 (2/25)
12 (3/25)

The parameters 1 in Table 1 refer to the classification of samples with 5% (w/w) concentration. When the cosmetic material at 3% agar, the coagulation time is greater than 15 minutes as the determination point of toxicity (cytotoxicity IC50 less than 250 μg/ml).

TABLE 2

the effect of cosmetic materials on the coagulation time of agar and cytotoxicity (1)

Agar
B16-F10
Skin cell 3T3

concentration %
coagulation
cytotoxicity
Cytotoxicity

Name 1
(w/w)
time (min)
IC₅₀: μg/ml
IC₅₀: μg/ml

AmmoniumLauryl
0
13.234 ± 0.188
53.7
57

Sulfate
1
16.444 ± 0.477

5
18.811 ± 0.987

10
28.372 ± 1.287

15
39.572 ± 1.077

Disodium
0
13.234 ± 0.188
72.8
55.6

Lauroamphodiacetate
1
14.356 ± 0.097

5
20.422 ± 0.106

10
43.333 ± 0.112

15
87.784 ± 0.176

Hydrogen Peroxide
0
13.234 ± 0.188
48.9
63.7

1
18.406 ± 0.121

5
30.544 ± 0.139

10
91.139 ± 0.257

17.5
>1440

Methylchloroisothiazolinone
0
13.234 ± 0.188
58
36.5

0.5
47.582 ± 0.103

1
97.514 ± 0.103

5
420.550 ± 0.073

7
>1440

p-Methylaminophenol
0
13.234 ± 0.188
2.46
2.93

Sulfate
1
15.478 ± 0.320

5
21.428 ± 0.887

10
32.489 ± 0.792

20
56.917 ± 0.932

30
88.311 ± 2.173

p-Phenylenediamine
0
13.234 ± 0.188
29.9
89.6

1
16.245 ± 0.468

5
22.189 ± 0.782

10
27.500 ± 1.073

20
39.489 ± 1.572

30
52.689 ± 1.982

Resorcinol
0
13.234 ± 0.188
4929.1
9858.2

1
32.821 ± 0.082

5
238.511 ± 0.101

10
>4320

20
>4320

30
>4320

2-Aminophenol
0
13.234 ± 0.188
39.34
41.2

1
15.231 ± 0.196

5
20.35 ± 0.678

10
29.44 ± 1.082

20
44.339 ± 0.972

30
61.421 ± 1.362

3-Aminophenol
0
13.234 ± 0.188
126.5
307.8

1
16.489 ± 0.475

5
20.455 ± 0.968

10
24.478 ± 1.280

20
43.671 ± 0.886

30
67.444 ± 1.687

sodium
0
13.234 ± 0.188
4187.1
>10000

Sulfide-9-Hydrate
0.5
109.250 ± 0.101

1
>1440

5
>1440

10
>1440

20
>1440

30
>1440

Lactic acid
0
13.234 ± 0.188
66
30.483

1
18.299 ± 0.078

5
23.378 ± 0.091

10
43.302 ± 0.099

20
253.306 ± 0.124

30
>1440

The names in Table 2 above refer to the samples and cosmetics that agar coagulation time is greater than 15 minutes when the concentration (w/w) is 5%.

TABLE 3

the effect of cosmetic materials on the coagulation time of agar and cytotoxicity (2)

Agar
B16-F10
Skin cell 3T3

concentration %
coagulation time
cytotoxicity
Cytotoxicity

Name 2
(w/w)
(min)
IC₅₀: μg/ml
IC₅₀: μg/ml

Butyl Paraben
0
13.234 ± 0.188
>10000
3564.7

1
13.186 ± 0.080

5
13.210 ± 0.079

10
13.182 ± 0.076

20
13.141 ± 0.050

30
13.238 ± 0.107

Monoethanolamine
0
13.234 ± 0.188
3646.4
>10000

1
13.193 ± 0.067

5
13.251 ± 0.077

10
13.296 ± 0.066

20
13.345 ± 0.088

30
13.354 ± 0.083

Glycerin
0
13.234 ± 0.188
>10000
>10000

1
13.220 ± 0.081

5
13.228 ± 0.053

10
13.333 ± 0.087

20
13.265 ± 0.067

30
13.322 ± 0.091

Hydroxy Ethyl
0
13.234 ± 0.188
>10000
4207.8

Cellulose
1
13.17 ± 0.060

5
13.216 ± 0.089

10
13.216 ± 0.087

20
13.193 ± 0.064

30
13.219 ± 0.093

Lysine
0
13.234 ± 0.188
4377.3
>10000

hydrochloride
1
13.241 ± 0.080

5
13.198 ± 0.077

10
13.238 ± 0.100

20
13.254 ± 0.119

30
13.286 ± 0.147

methyl
0
13.234 ± 0.188
4853.9
>10000

p-hydroxybenzate
1
13.230 ± 0.084

5
13.197 ± 0.066

10
13.242 ± 0.087

20
13.208 ± 0.100

30
13.203 ± 0.090

Butylene Glycol
0
13.234 ± 0.188
>10000
7323.7

1
13.252 ± 0.100

5
13.304 ± 0.077

10
14.489 ± 0.082

20
15.539 ± 0.101

30
15.688 ± 0.088

Polyethylene Glycol
0
13.234 ± 0.188
>10000
>10000

1
13.194 ± 0.077

5
13.221 ± 0.091

10
13.249 ± 0.098

20
13.160 ± 0.072

30
13.210 ± 0.072

Polyquaternium-7
0
13.234 ± 0.188
>10000
>10000

1
13.213 ± 0.081

5
13.229 ± 0.070

Salicylic Acid
0
13.234 ± 0.188
413.7
1388.2

1
13.210 ± 0.087

5
13.221 ± 0.091

10
13.144 ± 0.068

20
13.219 ± 0.093

30
13.184 ± 0.063

Squalane
0
13.234 ± 0.188
5423.2
>10000

1
13.260 ± 0.068

5
13.199 ± 0.073

10
13.276 ± 0.081

20
13.254 ± 0.077

30
13.305 ± 0.097

Tocopherol Acetate
0
13.234 ± 0.188
>10000
>10000

1
13.200 ± 0.080

5
13.209 ± 0.079

10
13.185 ± 0.072

20
13.167 ± 0.066

30
13.192 ± 0.071

Trisodium Citrate
0
13.234 ± 0.188
3335.4
>10000

Dihydrate
1
13.122 ± 0.020

5
13.194 ± 0.048

10
13.185 ± 0.048

20
13.24 ± 0.069

30
13.246 ± 0.072

Isopropyl Myristate
0
13.234 ± 0.188
>10000
>10000

1
13.153 ± 0.056

5
13.186 ± 0.069

10
13.185 ± 0.066

20
13.172 ± 0.065

30
13.206 ± 0.087

The names in Table 3 above refer to the samples and cosmetics that agar coagulation time is greater than 15 minutes when the concentration (w/w) is 5%.

In addition, the present invention also relies on the concentration-dependent relationship in the agar coagulation time for various cosmetic materials of different concentrations. Please refer to FIG. 2, which is the different agar coagulation with different types of cosmetics. With the increase in the concentration of p-Methylaminophenol Sulfate, the agar coagulation time is significantly longer and statistically significant (“*” Represents the control group p<0.05 compared to the control group p<0.05; “**” Represents the control group p<0.01 compared to the control group p<0.05); (the data is expressed in mean±SEM, where the triple test in FIG. 2; Data are represented as the mean±SEM; N=3∘*p<0.05 compared with control; **p<0.01 compared with control.)

Refer to FIG. 3, with the increase in the concentration of p-phenylenediamine, the agar coagulation time is significantly longer and statistically significant; (the data is expressed in mean±SEM, where the triple test in FIG. 3; Data are represented as the mean±SEM; N=3∘*p<0.05 compared with control; **p<0.01 compared with control.)

Refer to FIG. 4, with the increase in the concentration of 2-Aminophenol, the agar coagulation time is significantly longer and statistically significant; (the data is expressed in mean±SEM, where the triple test in FIG. 4; Data are represented as the mean±SEM; N=3∘*p<0.05 compared with control; **p<0.01 compared with control.)

Refer to FIG. 5, with the increase in the concentration of Ammonium Lauryl Sulfate, the agar coagulation time is significantly longer and statistically significant; (the data is expressed in mean±SEM, where the triple test in FIG. 5; Data are represented as the mean±SEM; N=3∘*p<0.05 compared with control; **p<0.01 compared with control.)

Refer to FIG. 6, with the increase in the concentration of 3-Aminophenol, the agar coagulation time is significantly longer and statistically significant; (the data is expressed in mean±SEM, where the triple test in FIG. 6; Data are represented as the mean±SEM; N=3∘* p<0.05 compared with control; **p<0.01 compared with control.)

In other words, the results of Table 2, Table 3, FIGS. 2 to 6 show that the agar coagulation time and toxicity of the tested cosmetic materials are in a concentration-dependent relationship.

In summary, the agar coagulation time is measured with samples and compared with B16-F10 cells and 3T3 cytotoxicity. As shown in Tables 2 to 3, if the higher the toxic substance content of sample, the longer the agar coagulation time than the control group will be measured. For example, the sample of the toxic substance is mixed with the agar of the present invention and the agar coagulation time is more than 15 minutes.

In other words, the present invention is tested for agar coagulation time and compared with cell survival analysis experiments to verify that the cosmetic materials and samples are “not harmful to skin.” Such as Butyl Paraben, Glycerin, Hydroxy Ethyl Cellulose, Lysine hydrochloride, Polyethylene Glycol, Polyquaternium-7 and Trisodium Citrate Dihydrate.

In addition, the present invention is tested for agar coagulation time and compared with cell survival analysis experiments to verify the cosmetic materials and samples are “harmful to skin.” Such as Ammonium Lauryl Sulfate, Disodium Lauroamphodiacate, Hydrogen Peroxide, Methylchloroisothiazolinone, P-Methylaminophenol Sulfate, p-Phenylenediamine, Resorcinol, 2-Aminophenol, 3-Aminophenol, Sodium Sulfide-9-Hydrate and Lactic acid.

Accordingly, the present invention provides a method for rapid determination of toxicity substance. In particular, a method for determining whether a sample is toxic by a plant agar coagulating. The method can reduce the use of animal or cell experiments, not only for the purpose of protecting the animal, also for reducing the cost of drugs, food or cosmetics in the toxicity test. More particularly, a method for rapidly and easily detecting a toxic substance by agar curing, not only in the range of about 15 to about 60 minutes, such as cosmetics, food, drugs and other samples, but also the above samples can contain harmful substances against the biological substances, and thus can include such as cosmetics and other samples to determine whether it contains excessive toxic substances.

Although the present invention has been described in terms of specific embodiments and examples, it will be appreciated that the embodiments disclosed herein are for illustrative purposes only and various modifications and alterations might be made by those skilled in the art without departing from the spirit and scope of the invention as set forth in the following claims.

METHOD FOR DETERMINING TOXIC SUBSTANCES BY PLANT GEL AGAR COAGULATING

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