CN117625607A - miR-CM3 of Phellinus linteus and application thereof - Google Patents
miR-CM3 of Phellinus linteus and application thereof Download PDFInfo
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- CN117625607A CN117625607A CN202311502403.1A CN202311502403A CN117625607A CN 117625607 A CN117625607 A CN 117625607A CN 202311502403 A CN202311502403 A CN 202311502403A CN 117625607 A CN117625607 A CN 117625607A
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- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
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Abstract
The invention belongs to the field of biotechnology and medicine, relates to the separation and identification of miR-CM3 from Phellinus linteus, and particularly relates to application of miR-CM 3. The miR-CM3 has a nucleotide sequence shown as SEQ ID NO.2 and has good anti-inflammatory activity. The miR-CM3 can resist inflammatory response induced by Lipopolysaccharide (LPS) and ultraviolet radiation when applied to skin cells or tissues, and can reduce the expression of inflammatory factors. The invention also provides a skin external preparation containing miR-CM3, and the skin external preparation has an anti-inflammatory effect. Provides a new research direction and development foundation for the development of anti-inflammatory skin care products.
Description
The application is a divisional application of an invention patent application 202111573093.3, the application date of 202111573093.3 is 2021, 12 and 21, the application number is 202111573093.3, and the invention name is: miRNA of Phellinus linteus and application thereof are provided.
Technical field:
the invention belongs to the field of biotechnology and medicine, and relates to the separation and identification of miRNA from phellinus linteus, in particular to miR-CM3 and application thereof.
The background technology is as follows:
skin is the first line of defense of the human body and is most susceptible to damage, inflammation or aging of the skin due to the external environment. When external stimuli occur, such as contact with stimulus sources such as air pollutants, ultraviolet rays, physical injury and the like, the immune system of the skin can start signals, release various inflammatory factors, cause acceleration of blood flow and increase of permeability of blood vessels, and cause inflammatory reactions of the skin, and symptoms can comprise redness, heat, itching, sensitivity, swelling and the like. One of the most pronounced acute effects of ultraviolet light on the skin is the induction of inflammation. UVB induces a cascade of cytokines, vasoactive and neuroactive mediators in the skin that together lead to an inflammatory response and to "sunburn". Many people suffer from skin inflammation due to frequent exposure to different irritants and allergens, which can lead to serious health problems if not treated in time. In modern society, with the continuous understanding of the importance of skin care, the skin care knowledge is increased, skin care has become a daily use, and anti-inflammatory repair products have gradually become one of cosmetics used daily by people. Therefore, the research and development of raw materials and mechanisms of anti-inflammatory skin care products have great practical significance.
Lipopolysaccharide (LPS), which is a component of the outer wall of the cell wall of gram-negative bacteria, is a common endotoxin, and consists mainly of lipid and polysaccharide. It can activate mononuclear macrophages, endothelial cells, epithelial cells and the like through a cell signal transduction system, synthesize and release various cytokines and inflammatory mediators, and further cause a series of inflammatory reactions, leading to the appearance of inflammation. Induction of cellular inflammation using LPS is one of the methods of modeling cellular inflammation. In addition, after ultraviolet irradiation, the number of epidermal cell layers and the thickness of epidermis are increased, more dead skin is formed, and the blockage degree of hair follicles is increased, so that the inflammation of vaccinia is worsened. UV irradiation can simulate sun irritation and build up an inflammatory or aging model.
Phellinus linteus is a typical pharmaceutical fungus and contains compounds such as polysaccharides, polyphenols, and flavonoids. More and more researches show that the phellinus linteus plays a remarkable regulating and controlling role in resisting tumor, protecting liver, reducing inflammatory reaction, controlling blood sugar and the like. For example, the polysaccharide isolated from it can inhibit the expression of various inflammatory factors in cells. In addition, the water-soluble extract thereof plays an immunoregulatory role in atopic dermatitis. Phellinus linteus extract was listed in the catalog of used cosmetic raw materials (2021 edition). Currently, phellinus linteus extracts have been used in various skin care and cosmetic formulations.
microRNA (miRNA) is a class of endogenous non-coding RNA of about 19-25nt in length. miRNA is involved in gene posttranscriptional regulation, can regulate the growth and development of cells and organisms, and is related to human diseases. More and more researches show that exogenous plant miRNAs can regulate the expression of target genes of mammals, so that the cross-border regulation is realized. For example, zhang Chenyu found that miR2911 in honeysuckle can be absorbed by mice, inhibiting viral replication by targeting alphavirus. The miRNA in the phellinus linteus can carry out cross-boundary regulation on human skin cells, and plays an anti-inflammatory role. The method has great potential application value in the research and development of anti-inflammatory skin care products.
The invention comprises the following steps:
the invention aims to provide miRNAs of phellinus linteus, namely miR-CM2, miR-CM3, miR-CM4 and miR-CM5 and application thereof, wherein the miR-CM2, miR-CM3, miR-CM4 and miR-CM5 can reduce the expression of inflammatory factors in an inflammation model, and have potential values in the development and application of anti-inflammatory skin care products.
One of the technical schemes provided by the invention is miRNA from Phellinus linteus, which is miR-CM2, miR-CM3, miR-CM4 or miR-CM5 respectively;
the miR-CM2 has a nucleotide sequence shown in SEQ ID NO. 1;
the miR-CM3 has a nucleotide sequence shown as SEQ ID NO. 2;
the miR-CM4 has a nucleotide sequence shown in SEQ ID NO. 3;
the miR-CM5 has a nucleotide sequence shown as SEQ ID NO. 4;
further, the precursor sequence MIR-CM2 of the miR-CM2 has a nucleotide sequence shown in SEQ ID NO. 5;
further, the precursor sequence MIR-CM3 of the miR-CM3 has a nucleotide sequence shown in SEQ ID NO. 6;
further, the precursor sequence MIR-CM4 of the miR-CM4 has a nucleotide sequence shown in SEQ ID NO. 7;
further, the precursor sequence MIR-CM5 of the miR-CM5 has a nucleotide sequence shown in SEQ ID NO. 8;
further, the DNA encoding the precursor sequence MIR-CM2 has a nucleotide sequence shown as SEQ ID NO. 9;
further, the DNA encoding the precursor sequence MIR-CM3 has a nucleotide sequence shown in SEQ ID NO. 10;
further, the DNA encoding the precursor sequence MIR-CM4 has a nucleotide sequence shown as SEQ ID NO. 11;
further, the DNA encoding the precursor sequence MIR-CM5 has the nucleotide sequence shown in SEQ ID NO. 12.
The second technical scheme provided by the invention is application of miR-CM2, miR-CM3, miR-CM4 or miR-CM5;
further, the use is the use of miR-CM2, miR-CM3, miR-CM4 or miR-CM5 in skin care products, cosmetics or cosmetic products, and in the preparation of products for preventing or treating photoaging, in particular in the preparation of anti-inflammatory products.
The third technical scheme provided by the invention is a skin external preparation containing the miR-CM2, miR-CM3, miR-CM4 or miR-CM5;
further, the skin external agent includes, but is not limited to, a skin care product, a cosmetic, an application agent, or the like;
the coating agent comprises, but is not limited to, oil agent, water agent, ointment or gel agent and the like;
further, the addition amount of miR-CM2, miR-CM3, miR-CM4 or miR-CM5 in the skin external agent is 0.2-5% (weight percentage);
further, the external preparation for skin is in the form of at least one of water, essence, gel, emulsion, skin base solution or cream;
further, an emulsion containing miR-CM2 comprises the following components (in percentage by weight): 0.01-0.05% of EDTA disodium, 2-5% of glycerol, 0.05-0.2% of xanthan gum, 0.1-0.3% of p-hydroxyacetophenone, 0.5-3% of Montanov L-emulsifier, 0.5-3% of ARLACEL170 emulsifier, 0.1-0.5% of glycerol stearate, 0.5-3% of cetostearyl alcohol, 2-6% of caprylic/capric triglyceride, 0.5-3% of polydimethylsiloxane, 0.1-0.5% of methyl propylene glycol, 0.5-3% of polyethyleneimine-1500, 0.5-3% of sodium hyaluronate, 0.2-5% of miR-CM and the balance deionized water;
furthermore, miR-CM2 added into the emulsion can be a single-stranded nucleic acid molecule or a double-stranded nucleic acid molecule; the single-stranded nucleic acid molecule is a nucleic acid molecule synthesized according to the nucleotide sequence in SEQ ID NO. 1; the double-stranded nucleic acid molecule is synthesized according to the nucleotide sequence in SEQ ID NO.1 and the complementary sequence thereof;
further, an emulsion containing miR-CM3 comprises the following components (in percentage by weight): 0.01-0.05% of EDTA disodium, 2-5% of glycerol, 0.05-0.2% of xanthan gum, 0.1-0.3% of p-hydroxyacetophenone, 0.5-3% of Montanov L-emulsifier, 0.5-3% of ARLACEL170 emulsifier, 0.1-0.5% of glycerol stearate, 0.5-3% of cetostearyl alcohol, 2-6% of caprylic/capric triglyceride, 0.5-3% of polydimethylsiloxane, 0.1-0.5% of methyl propylene glycol, 0.5-3% of polyethyleneimine-1500, 0.5-3% of sodium hyaluronate, 0.2-5% of miR-CM and the balance deionized water;
furthermore, miR-CM3 added into the emulsion can be a single-stranded nucleic acid molecule or a double-stranded nucleic acid molecule; the single-stranded nucleic acid molecule is a nucleic acid molecule synthesized according to the nucleotide sequence in SEQ ID NO. 2; the double-stranded nucleic acid molecule is synthesized according to the nucleotide sequence in SEQ ID NO.2 and the complementary sequence thereof;
further, an emulsion containing miR-CM4 comprises the following components (in percentage by weight): 0.01-0.05% of EDTA disodium, 2-5% of glycerol, 0.05-0.2% of xanthan gum, 0.1-0.3% of p-hydroxyacetophenone, 0.5-3% of Montanov L-emulsifier, 0.5-3% of ARLACEL170 emulsifier, 0.1-0.5% of glycerol stearate, 0.5-3% of cetostearyl alcohol, 2-6% of caprylic/capric triglyceride, 0.5-3% of polydimethylsiloxane, 0.1-0.5% of methyl propylene glycol, 0.5-3% of polyethyleneimine-1500, 0.5-3% of sodium hyaluronate, 0.2-5% of miR-CM and the balance deionized water;
furthermore, miR-CM4 added into the emulsion can be a single-stranded nucleic acid molecule or a double-stranded nucleic acid molecule; the single-stranded nucleic acid molecule is a nucleic acid molecule synthesized according to the nucleotide sequence in SEQ ID NO. 3; the double-stranded nucleic acid molecule is synthesized according to the nucleotide sequence in SEQ ID NO.3 and the complementary sequence thereof;
further, an emulsion containing miR-CM5 comprises the following components (in percentage by weight): 0.01-0.05% of EDTA disodium, 2-5% of glycerol, 0.05-0.2% of xanthan gum, 0.1-0.3% of p-hydroxyacetophenone, 0.5-3% of Montanov L-emulsifier, 0.5-3% of ARLACEL170 emulsifier, 0.1-0.5% of glycerol stearate, 0.5-3% of cetostearyl alcohol, 2-6% of caprylic/capric triglyceride, 0.5-3% of polydimethylsiloxane, 0.1-0.5% of methyl propylene glycol, 0.5-3% of polyethyleneimine-1500, 0.5-3% of sodium hyaluronate, 0.2-5% of miR-CM and the balance deionized water;
furthermore, miR-CM5 added into the emulsion can be a single-stranded nucleic acid molecule or a double-stranded nucleic acid molecule; the single-stranded nucleic acid molecule is a nucleic acid molecule synthesized according to the nucleotide sequence in SEQ ID NO. 4; the double-stranded nucleic acid molecule is synthesized according to the nucleotide sequence in SEQ ID NO.4 and the complementary sequence thereof;
preferably, the addition amount of miR-CM2 (or miR-CM3 or miR-CM4 or miR-CM 5) is 0.5-1%;
preferably, the emulsion containing miR-CM2 (or miR-CM3 or miR-CM4 or miR-CM 5) comprises the following components (in weight percent): EDTA disodium 0.03%, glycerol 4%, xanthan gum 0.1%, p-hydroxyacetophenone 0.2%, montanov L-emulsifier 1%, ARLACEL170 emulsifier 1%, glyceryl stearate 0.3%, cetostearyl alcohol 1%, caprylic/capric triglyceride 4%, polydimethylsiloxane 1%, methyl propylene glycol 0.35%, polyethylene imine-1500 1%, sodium hyaluronate 1%, miR-CM2 (or miR-CM3 or miR-CM4 or miR-CM 5) 0.75%, and the balance deionized water.
The fourth technical scheme provided by the invention is the application of the skin external preparation containing miR-CM2, miR-CM3, miR-CM4 or miR-CM5, in particular the application of the emulsion containing miR-CM2, miR-CM3, miR-CM4 or miR-CM5, and the emulsion can resist ultraviolet-induced inflammation and reduce the increase of the thickness of epidermis caused by ultraviolet irradiation.
The invention has the beneficial effects that:
the invention screens out a novel phellinus linteus miRNA (miR-CM 2, miR-CM3, miR-CM4 and miR-CM 5) and precursors thereof, namely MIR-CM2, MIR-CM3, MIR-CM4 and MIR-CM5. The miR-CM2/CM3/CM4/CM5 has good anti-inflammatory activity, and the miR-CM2/CM3/CM4/CM5 is applied to skin cells or tissues, so that the anti-inflammatory effect induced by Lipopolysaccharide (LPS) and ultraviolet irradiation can be resisted, and the expression of inflammatory factors is reduced.
The invention provides a formula of a basic skin care product containing miR-CM2, miR-CM3, miR-CM4 or miR-CM5, and the basic skin care product has an anti-inflammatory effect. Provides a new research direction and development foundation for the development of anti-inflammatory skin care products.
The miR-CM2, miR-CM3, miR-CM4 or miR-CM5 disclosed by the invention can provide a mechanism support for research of anti-inflammatory skin care products of phellinus linteus extracts, and a wider space is provided for research and development of the anti-inflammatory skin care products.
Description of the drawings:
FIG. 1 is a secondary structure of precursor MiR-CM2, miR-CM3, miR-CM4 and MiR-CM5 of miR-CM2, miR-CM3, miR-CM4 and miR-CM5.
FIG. 2 is a graph showing the protective effects of miR-CM2, miR-CM3, miR-CM4 and miR-CM5 on skin cells under LPS stimulation.
FIG. 3 is a graph showing the expression of inflammatory factors (IL-1β, IL-6, TNF- α, NF- κB) when miR-CM2, miR-CM3, miR-CM4 or miR-CM5 is applied to skin cells.
In each bar graph of fig. 2 and 3, the following steps are sequentially performed from left to right: ctrl group, LPS group, lps+mir-CM2, lps+mir-CM3 group, lps+mir-CM4 group, lps+mir-CM5 group.
FIG. 4 variation in skin epidermis thickness before and after application of miR-CM2, miR-CM3, miR-CM4 or miR-CM5 skin care products in mouse skin;
wherein, the left side is HE staining of the skin of the mouse; the right is the corresponding skin thickness statistical graph.
Detailed Description
The technical solutions of the present invention will be clearly and completely described below with reference to the drawings in the embodiments of the present invention, and it is apparent that the described embodiments are only some embodiments of the present invention, not all embodiments. All other embodiments, which can be made by those skilled in the art based on the embodiments of the invention without making any inventive effort, are intended to be within the scope of the invention.
The experimental procedures in the following examples, unless otherwise specified, are conventional in the art. The materials, reagents and the like used, unless otherwise specified, are all commercially available.
In the present invention, miR represents miRNA;
in the present invention, miR-CM2/CM3/CM4/CM5 represents "miR-CM2, miR-CM3, miR-CM4 or miR-CM5";
phellinus linteus (Phellinus linteus) used in the present invention is purchased from North Nanopsis (BNCC), strain number BNCC109781.
Example 1 screening and identification of miRNAs
1. Preparation of samples
The extraction of the RNA sample may be from a lysate of Phellinus linteus or from an exosome of Phellinus linteus. For lysates: cutting Phellinus linteus in PBS under high pressure, and centrifuging at high speed to obtain supernatant, which is lysate of Phellinus linteus. For exosomes: the exosome of Phellinus linteus is obtained by homogenizing Phellinus linteus, and centrifuging at differential speed. The dead cells were removed by first centrifugation at 3000 Xg for 30 minutes, the supernatant was collected and centrifuged at 10000 Xg for 60 minutes to remove cell debris. The resulting supernatant was further centrifuged at 150000Xg for 90 minutes, and the exosomes (pellet) were suspended in PBS buffer.
RNA extraction and quality detection
Total RNA from the exosome samples was extracted using Trizol (Siemens, america) method. Detecting the integrity of RNA by agarose gel electrophoresis, wherein the electrophoresis shows that 28S and 18S bands are clear and have no degradation; detecting the concentration and purity of RNA by using an ultra-micro spectrophotometer (Tiangen, background), wherein the OD260/280 value is between 1.8 and 2.2, and the OD260/230 is more than or equal to 2.0, which indicates that the purity of the RNA is qualified. The concentration of the RNA sample is more than or equal to 200 ng/. Mu.L, and the total amount is more than or equal to 2. Mu.g. The RNA preliminary detection quality is qualified, so that the construction of a downstream high-quality small RNA-seq library is ensured. Further quality control and miRNA sequencing were performed.
3. Library construction:
the qualified RNA is used for constructing a miRNA library, a proper amount of total RNA is taken for joint connection reaction, a phosphate group is arranged at the 5 'end of the mature miRNA, the 3' end is hydroxyl, the structure is different from other RNA, and under the action of T4 RNA ligase 2 and T4 RNA ligase, 3 'joints and 5' joints with known sequences are added at the two ends. For RNA with 5 'and 3' linkers attached, cDNA of the first strand is synthesized using reverse transcription complementary to the sequence on the linker. And (3) taking the reaction product of the step as a template, and synthesizing and amplifying a double-chain library of miRNA by using PCR. Isolation of miRNA library with insert size of 22-24nt by polyacrylamide gel electrophoresis. And (5) performing quality inspection and quantitative evaluation on the constructed sequencing library to determine whether the sequencing library is suitable for being put on machine.
4. Sequencing on machine
And diluting the sample which is qualified in quality inspection, and loading the sample according to the corresponding proportion according to the sequencing flux requirements of different samples. The library was sequenced using an Illumina high throughput sequencing platform, a double ended sequencing strategy.
5. Bioinformatic analysis (including novel miRNA prediction and expression analysis)
In order to ensure the quality of information analysis, the original sequencing sequences (raw reads) obtained by sequencing are filtered to obtain clean reads for subsequent analysis. Quality filtration was performed using FASTX-Toolkit software. And carrying out small RNA length distribution statistics on the sequences after quality control, wherein miRNAs are concentrated at 21nt or 22nt. In addition, BLAST comparison is carried out on the sequences after quality control and mature miRNA sequences of corresponding species in the miRBase database, and the sequences are compared with the Rfam database and the reference genome, so that the sequencing result is subjected to preliminary evaluation. The results were annotated for different types of Small RNAs.
Novel miRNA prediction and expression analysis. Because the hairpin structure of the miRNA precursor can be used for predicting miRNA, the miRNA can be compared to a genome sequence, the sequences at two sides of the miRNA can be intercepted for predicting the secondary structure of the RNA, and the novel miRNA can be obtained by combining with the information such as the Dicer enzyme binding site, the free energy of the secondary structure and the like. Comparing reads with a reference genome by adopting mirdrep 2 software, and according to the comparison result of the reads and the genome, combining homologous miRNA sequences of related species, such as RNA secondary structures of RNAfold and the like, predicting and identifying new miRNA mature bodies (Star miRNA and material miRNA) and precursor sequences of the species, and counting the expression condition of the new miRNA of each sample.
Through the separation and identification, four novel miRNAs from Phellinus linteus are respectively named as miR-CM2, miR-CM3, miR-CM4 and miR-CM5. The secondary structure is shown in figure 1, and the figures show that stable stem-loop structures similar to miRNA precursors are formed, the mature sequences of the stable stem-loop structures are shown in sequence tables SEQ ID NO. 1-NO. 4, the precursor sequences of the stable stem-loop structures are shown in sequence tables SEQ ID NO. 5-NO. 8, and the encoding genes of the precursor sequences of the stable stem-loop structures are shown in sequence tables SEQ ID NO. 9-NO. 12.
SEQ ID NO.1 (miR-CM 2 mature sequence): uccucaagguuauccgua (18 bp).
SEQ ID NO.2 (miR-CM 3 mature sequence): ccggugcgcucucgacagcc (20 bp).
SEQ ID NO.3 (miR-CM 4 mature sequence): acguguggauccagacggguu (21 bp). SEQ ID NO.4 (miR-CM 5 mature sequence): uauuccauuccguccauccu (20 bp).
Example 2miR-CM 2-CM 5 reduced inflammatory injury of HaCaT cells caused by LPS
CCK8 experiment
1) Preparation of cell samples
Human immortalized epidermal cells (HaCaT cells) were cultured in DMEM (Gibco, U.S.) supplemented with 10% fetal bovine serum (BI, israel) and 100U/mL penicillin streptomycin cocktail (Menlam, china) and at 37℃and 5% CO concentration 2 Growing in an incubator;
and respectively transfecting miR-CM2 miics, miR-CM3 miics, miR-CM4 miics and miR-CM5 miics into the cultured HaCaT cells through Lipo2000 transfection reagent (Siemeaway, U.S.) and pre-protecting for 24 hours. LPS was added to each well (96-well plate) at a final concentration of 1. Mu.g/mL, and CCK8 assay (experimental group) was performed after 6h of stimulation.
Control group (Ctrl group): the normal culture of the human immortalized epidermal cells (HaCaT cells) does not carry out any treatment (without pre-protection and LPS stimulation); the model group (LPS group) was not pre-protected, only LPS stimulated; the experimental group (LPS+miR-CM 2/CM3/CM4/CM5 group) was pre-protected and LPS stimulated.
Transfection protocol: taking a 24-well plate as an example, other culture materials were adjusted for transfection scale with reference to the instructions, all numbers and volumes were calculated per well. Cells were inoculated in 500 μl of antibiotic-free medium and allowed to fuse up to 50% of the time during transfection. The amount of cells per well at the time of transfection was as follows: 20pmol of miR-CM2, miR-CM3, miR-CM4 or miR-CM5 are diluted with 50. Mu.L of Opti-MEM culture medium, respectively, and gently mixed. mu.L of Lipo2000 was diluted in 50. Mu.L of Opti-MEM medium and incubated for 5min at room temperature. The first two solutions were mixed (to make the total volume 100. Mu.L), gently mixed, and left at room temperature for 20 minutes to form 100. Mu.L of transfection solution. mu.L of the transfection solution was added to each well of cells, and the mixture was gently shaken. (the present invention relates to the transfection procedure using this method unless otherwise specified).
miR-CM2, miR-CM3, miR-CM4, miR-CM5, namely miR-CM2 analogue, miR-CM3 analogue, miR-CM4 analogue and miR-CM5 analogue, which are double-stranded sequences, wherein:
miR-CM2 mimics:
the sense strand sequence is: 5'-uccucaagguuauccgua-3' (with miR-CM2, SEQ ID NO. 1);
the antisense strand sequence is: 5'-cggauaaccuugaggauu-3' (SEQ ID NO. 13).
miR-CM3 mimics:
The sense strand sequence is: 5'-ccggugcgcucucgacagcc-3' (with miR-CM3, SEQ ID NO. 2);
the antisense strand sequence is: 5'-cugucgagagcgcaccgguu-3' (SEQ ID NO. 14).
miR-CM4 mimics:
The sense strand sequence is: 5'-acguguggauccagacggguu-3' (with miR-CM4, SEQ ID NO. 3); the antisense strand sequence is: 5'-cccgucuggauccacacguuu-3' (SEQ ID NO. 15).
miR-CM5 mimics:
The sense strand sequence is: 5'-uauuccauuccguccauccu-3' (with miR-CM5, SEQ ID NO. 4);
the antisense strand sequence is: 5'-gauggacggaauggaauauu-3' (SEQ ID NO. 16).
2) Cell viability assay
Cell viability was measured using Cell Counting Kit-8 (CCK-8) (APExBIO, USA).
Mu.l of CCK-8 solution was added to each well of the 96-well plate. The plates were placed in an incubator for 1 hour. Absorbance at 450nm was measured using an enzyme-labeled instrument. The more the cells proliferate, the darker the color; the more cytotoxic the more light the colour.
As can be seen from fig. 2, 1 μg/ml of LPS stimulation significantly reduced the cell viability of HaCaT cells, reducing the survival rate of HaCaT cells. And the pre-protection of miR-CM2, miR-CM3, miR-CM4 or miR-CM5 obviously improves the reduction of the activity of HaCaT cells caused by LPS of 1 mu g/ml. The result shows that the pre-protection of miR-CM2, miR-CM3, miR-CM4 or miR-CM5 can reduce the damage degree of cells and reduce the decrease of the cell viability in the inflammatory damage of the cells caused by LPS treatment.
2. Real-time fluorescent quantitative PCR detection of gene expression
1) Preparation of cell samples
Preparation of cell samples was performed as in example 2, step 1.
2) Extraction of Total RNA
Total RNA was extracted from the samples by Trizol (Siemens, USA) method. The integrity and purity of the RNA samples were checked as in example 1, step 2.
3) Reverse transcription
cDNA was synthesized by reverse transcription using Hifair III 1st Strand cDNA Synthesis SuperMix for qPCR (gDNA digester plus) (next holy, shanghai) kit. The removal of genomic residual genomic DNA and reverse transcription system was as follows:
the following mixture was prepared in an RNase-free centrifuge tube, and gently swirled and mixed. Incubate at 42℃for 2min.
Preparation of reverse transcription reaction System (20. Mu.L System)
25 ℃ for 5min;55 ℃ for 15min;85 ℃ for 5min. The obtained cDNA was stored at-20 ℃.
4) qPCR experiment
qPCR was performed using Hieff UNICON Universal Blue qPCR SYBR Green Master Mix (next holy, shanghai).
The primers used for detection were as follows:
IL-1. Beta. Upstream primer: CCACAGACCTTCCAGGAGAATG (SEQ ID NO. 17); IL-1 beta downstream primer: GTGCAGTTCAGTGATCGTACAGG (SEQ ID NO. 18).
IL-6 upstream primer: AGACAGCCACTCACCTCTTCAG (SEQ ID NO. 19);
IL-6 downstream primer: TTCTGCCAGTGCCTCTTTGCTG (SEQ ID NO. 20).
TNF- α upstream primer: CTCTTCTGCCTGCTGCACTTTG (SEQ ID NO. 21); TNF-alpha downstream primer: ATGGGCTACAGGCTTGTCACTC (SEQ ID NO. 22).
NF-. Kappa.B upstream primer: GCAGCACTACTTCTTGACCACC (SEQ ID NO. 23); NF-. Kappa.B downstream primer: TCTGCTCCTGAGCATTGACGTC (SEQ ID NO. 24).
Adopts beta-actin as an internal reference gene:
beta-actin upstream primer: CACCATTGGCAATGAGCGGTTC (SEQ ID NO. 25); beta-actin downstream primer: AGGTCTTTGCGGATGTCCACGT (SEQ ID NO. 26).
cDNA stock was diluted 4-fold and qPCR reaction system (20. Mu.l) was prepared on ice:
after thoroughly mixing, 20. Mu.L of the reaction solution was sucked into the reaction well, the heat-sealing film was sealed, and the mixture was centrifuged briefly. Detection was performed on a PCR instrument. qPCR reaction procedure was as follows: a pre-denaturation stage, 95 ℃ for 2 min;40 cyclic stages (including denaturation, annealing/extension), denaturation 95 ℃,10s, annealing/extension 60 ℃,30s; melting curve phase (instrument default settings); experimental data were obtained for subsequent results analysis.
Experiments were repeated at least three times. The relative expression of each inflammatory factor is calculated by taking reference genes as references. The results (FIG. 3) show that the relative expression levels of inflammatory factors of HaCaT cells pre-protected by transfection of miR-CM2, miR-CM3, miR-CM4 or miR-CM5 are lower than those of LPS stimulated groups to different degrees. The miR-CM2, miR-CM3, miR-CM4 or miR-CM5 pre-protection is indicated to reduce the increase of inflammatory factors caused by LPS stimulation and reduce inflammatory response.
The result shows that the pre-protection of miR-CM2, miR-CM3, miR-CM4 or miR-CM5 can reduce the inflammatory damage of HaCaT cells caused by LPS.
Example 3 miR-CM2, miR-CM3, miR-CM4 or miR-CM5 skin care emulsion reduces the thickness of epidermis in skin inflammation of mice caused by ultraviolet irradiation
1) Preparation of miR-CM2, miR-CM3, miR-CM4 or miR-CM5 skin care emulsion
The formula of the miR-CM2 skin care emulsion comprises the following components: calculated according to the weight percentage, EDTA disodium 0.03%, glycerin 4%, xanthan gum 0.1%, p-hydroxyacetophenone 0.2%, montanov L-emulsifier 1%, ARLACEL170 emulsifier 1%, glycerol stearate 0.3%, cetostearyl alcohol 1%, caprylic/capric triglyceride 4%, polydimethylsiloxane 1%, methyl propylene glycol 0.35%, polyethyleneimine-1500% 1%, sodium hyaluronate 1%, miR-CM2 0.75%, and the balance deionized water.
The composition of the miR-CM3 skin care emulsion is the same as that of the miR-CM2 skin care emulsion, and miR-CM2 is replaced by miR-CM 3;
the composition of the miR-CM4 skin care emulsion is the same as that of the miR-CM2 skin care emulsion, and miR-CM2 is replaced by miR-CM 4;
the composition of the miR-CM5 skin care emulsion is the same as that of the miR-CM2 skin care emulsion, and miR-CM2 is replaced by miR-CM5;
according to the above formula, the preparation method comprises the following steps:
firstly, mixing EDTA disodium, glycerol, xanthan gum, p-hydroxyacetophenone, montanov L-emulsifier, ARLACEL170 emulsifier, glycerol stearate, cetostearyl alcohol, caprylic/capric triglyceride, polydimethylsiloxane, methyl propylene glycol and water in advance for emulsification to obtain emulsion;
then, pre-mixing polyethyleneimine-1500 and sodium hyaluronate into a solution, adding miR-CM2 (or miR-CM3 or miR-CM4 or miR-CM5, wherein the miR-CM2, miR-CM3, miR-CM4 and miR-CM5 are nucleic acid molecules obtained by synthesis according to nucleotide sequences shown in sequence tables SEQ ID NO.1, SEQ ID NO.2, SEQ ID NO.3 and SEQ ID NO. 4) into the solution, gently mixing, and standing for 25min to obtain a mixed solution containing miR-CM2 (or miR-CM3 or miR-CM4 or miR-CM 5);
and finally, adding the mixed solution containing miR-CM2 (or miR-CM3 or miR-CM4 or miR-CM 5) into the emulsion obtained by pre-mixing and emulsifying at the temperature below 40 ℃ to obtain the miR-CM2 (or miR-CM3 or miR-CM4 or miR-CM 5) skin care emulsion.
2) Establishment of mouse photoaging model
Kunming mice (females, 6-8 weeks) were randomly divided into seven groups (n=5, 1 control group, 4 experimental group, 1 model group 1, 1 model group 2), and back dehairing treatment. Normal feeding of mice in each group; wherein the control group was not given any treatment; experiment group, model group 1 and model group 2 were subjected to ultraviolet irradiation (UVA irradiation)The frequency is three times per week, and the dosage is 8J/cm 2 For 4 weeks), the four skin care emulsions prepared in the step 1) are respectively applied for treatment after each irradiation of the experimental group; after each irradiation of model group 2, a basic skin care emulsion without miR-CM2/CM3/CM4/CM5 is given (the preparation method is the same as step 1), and only miR-CM2/CM3/CM4/CM5 components are removed for smearing treatment; model group 1 was irradiated with ultraviolet light alone and no treatment was given. All mice were euthanized after 4 weeks. Back skin tissue was collected and fixed in formalin.
3) HE staining
Tissues were dehydrated and embedded in paraffin according to standard procedures. Sections were obtained at 4 μm thickness and stained using Hematoxylin Eosin (HE) staining kit (soribao, beijing).
Hematoxylin-Eosin staining (HE staining) is the most basic staining method in pathological routine tableting. Hematoxylin dye solution is alkaline, and mainly causes chromatin in nuclei and ribosomes in cytoplasm to be purple blue; eosin is an acid dye that primarily reds the cytoplasmic and extracellular matrix components.
Paraffin sections were dewaxed in xylene 2 times for 5-10min each. Gradient ethanol (100%, 95%, 85%, 75%) was rehydrated, 3min per gradient. Distilled water for 2min. Hematoxylin dye liquor is used for dyeing for 2-20min (the specific time is adjusted according to the dyeing result and experimental requirements), and the flooding is removed by washing with distilled water. Differentiation liquid is differentiated for 3min, and is washed for 2 times with tap water for 2min each time. Placing in eosin dye solution for 30s-2min, washing with distilled water for 2-3s, and rapidly dehydrating. Gradient ethanol (75% ethanol, 85% ethanol, 95% ethanol, and 100% ethanol) was used for each rinse for 2-3s. Washing with 100% ethanol for 1min, and observing with a mirror after xylene is transparent for 1min each time.
The skin structure is mainly divided into three layers: epidermis, dermis, and subcutaneous tissue. HE staining can stain various components of tissue cells for comprehensive visualization of tissue architecture. Skin tissue is subjected to HE staining, so that a tissue structure staining picture of the skin can be easily obtained and used for judging various skin indexes, such as epidermis thickness. HE staining results were used to calculate skin thickness by imageJ software, and the statistics are shown on the right side of fig. 4.
The control group corresponds to the Ctrl group in fig. 4.
Experimental groups correspond to those in fig. 4: UV+miR-CM2 group, UV+miR-CM3 group, UV+miR-CM4 group and UV+miR-CM5 group.
Model set 1 corresponds to the UV set in fig. 4.
Model set 2 corresponds to the uv+ base emulsion set in fig. 4.
As a result (shown in fig. 4), it was found that after UV irradiation, the skin thickness of model group 1 (i.e., UV group in fig. 4) was significantly increased compared to the skin thickness of control group (i.e., ctrl group in fig. 4), indicating that the modeling of the mouse photoaging model was successful. And the skin thickness of the model group 1 is not significantly different from that of the model group 2 (namely, the UV+ basic emulsion group in fig. 4), which indicates that the emulsion coated with the miR-CM2/CM3/CM4/CM5 component cannot protect the skin of the mice against the increase of the skin thickness caused by ultraviolet irradiation, while the miR-CM2, miR-CM3, miR-CM4 or miR-CM5 skin-care emulsion protection (namely, the UV+miR-CM2 group, the UV+miR-CM3 group, the UV+miR-CM4 group and the UV+miR-CM5 group in fig. 4) can resist the increase of the skin thickness caused by ultraviolet irradiation, which indicates that the miR-CM2, miR-CM3, miR-CM4 or miR-CM5 skin-care emulsion can significantly inhibit skin inflammation caused by ultraviolet irradiation, reduce the skin thickness of the skin of the treated group and reduce skin irregular proliferation caused by inflammation caused by ultraviolet irradiation.
The foregoing description of the preferred embodiments of the invention is not intended to be limiting, but rather is intended to cover all modifications, equivalents, alternatives, and improvements that fall within the spirit and scope of the invention.
Claims (8)
1. miRNA from phellinus linteus is characterized by specifically comprising miR-CM3, wherein the nucleotide sequence of the miRNA is shown in SEQ ID NO. 2: ccggugcgcucucgacagcc.
2. A miRNA from Phellinus linteus as set forth in claim 1,
the precursor sequence MIR-CM3 of miR-CM3 has a nucleotide sequence shown in SEQ ID NO. 6: cccuugguugucuaccguucauaaaaucggguuggcuugagcuaggguagagcgcagcacuucugcuggauc cggugcgcucucgacagcccuuaaaagaccaaggua.
The DNA of the coding precursor sequence MIR-CM3 has a nucleotide sequence shown in SEQ ID NO. 10.
3. The analogue of miRNA from Phellinus linteus of claim 1,
the miR-CM3 analogues are miR-CM3 mimics:
the sense strand sequence is: 5'-ccggugcgcucucgacagcc-3', as shown in SEQ ID NO. 2;
the antisense strand sequence is: 5'-cugucgagagcgcaccgguu-3' as shown in SEQ ID NO. 14.
4. The use of a miRNA from phellinus linteus or an analogue of claim 3, according to claim 1, characterized by the use of miR-CM3 or an analogue thereof for the preparation of a product for preventing or treating skin inflammation.
5. The external preparation for skin containing miR-CM3 according to claim 1, wherein the content of miR-CM3 in the external preparation for skin is 0.2% -5%.
6. The external skin preparation of claim 5, wherein an emulsion comprising miR-CM3 comprises the following components: 0.01-0.05% of EDTA disodium, 2-5% of glycerol, 0.05-0.2% of xanthan gum, 0.1-0.3% of p-hydroxyacetophenone, 0.5-3% of Montanov L-emulsifier, 0.5-3% of ARLACEL170 emulsifier, 0.1-0.5% of glycerol stearate, 0.5-3% of cetostearyl alcohol, 2-6% of caprylic/capric triglyceride, 0.5-3% of polydimethylsiloxane, 0.1-0.5% of methyl propylene glycol, 0.5-3% of polyethyleneimine-1500, 0.5-3% of sodium hyaluronate, 0.2-5% of miR-CM and the balance deionized water.
7. The external preparation for skin according to claim 6, comprising the following components: EDTA disodium 0.03%, glycerol 4%, xanthan gum 0.1%, p-hydroxyacetophenone 0.2%, montanov L-emulsifier 1%, ARLACEL170 emulsifier 1%, glyceryl stearate 0.3%, cetostearyl alcohol 1%, caprylic/capric triglyceride 4%, polydimethylsiloxane 1%, methyl propylene glycol 0.35%, polyethyleneimine-1500 1%, sodium hyaluronate 1%, miR-CM 3.75%, and deionized water in balance.
8. Use of the external preparation for skin according to any one of claims 5 to 7.
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