CN113881088B - Use of non-releasing antimicrobial adhesive coating in antibacterial packaging material - Google Patents

Use of non-releasing antimicrobial adhesive coating in antibacterial packaging material Download PDF

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CN113881088B
CN113881088B CN202010556984.7A CN202010556984A CN113881088B CN 113881088 B CN113881088 B CN 113881088B CN 202010556984 A CN202010556984 A CN 202010556984A CN 113881088 B CN113881088 B CN 113881088B
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packaging material
coating
photoinitiator
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borneol
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CN113881088A (en
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王兴
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Beijing University of Chemical Technology
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    • C08J7/00Chemical treatment or coating of shaped articles made of macromolecular substances
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    • C08J7/0427Coating with only one layer of a composition containing a polymer binder
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    • C08J2323/00Characterised by the use of homopolymers or copolymers of unsaturated aliphatic hydrocarbons having only one carbon-to-carbon double bond; Derivatives of such polymers
    • C08J2323/02Characterised by the use of homopolymers or copolymers of unsaturated aliphatic hydrocarbons having only one carbon-to-carbon double bond; Derivatives of such polymers not modified by chemical after treatment
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    • C08J2333/00Characterised by the use of homopolymers or copolymers of compounds having one or more unsaturated aliphatic radicals, each having only one carbon-to-carbon double bond, and only one being terminated by only one carboxyl radical, or of salts, anhydrides, esters, amides, imides, or nitriles thereof; Derivatives of such polymers
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Abstract

The invention relates to an application of a non-release antimicrobial adhesive coating in an antimicrobial packaging material, wherein the coating mainly comprises a copolymer of two monomers of Bornyl Acrylate (BA) and polyethylene glycol diacrylate (PEGDA) to construct an amphiphilic stereochemical antimicrobial polymer coating, and the coating has good antimicrobial adhesion. The preparation method of the coating mainly comprises the following steps: the first step is to fix the photoinitiator on the surface of the packaging material, and the second step is to graft and copolymerize monomers by surface free radical initiated polymerization. The preparation method of the coating is simple, and the obtained grafted coating is safe and stable; the advantages of the polyacrylate bornyl ester and the polyethylene glycol diacrylate can be fully exerted, and the adhesion of microorganisms is synergistically prevented; the coating is applied to the modification of the surface of a packaging material, and can ensure the smooth structure of a grafted coating.

Description

Application of non-release type antimicrobial adhesion coating in antibacterial packaging material
Technical Field
The invention belongs to the field of biological materials, and particularly relates to application of a non-release antimicrobial adhesive coating in an antibacterial packaging material.
Background
The polymer film or sheet is widely applied to the life and industrial production of people, such as agriculture, food, medical treatment, chemical industry and the like. However, these polymers do not have the function of resisting microbial adhesion, provide a medium for adhesion and transmission of microorganisms, seriously affect the production efficiency and threaten the health of human beings. These problems of microbial contamination have been receiving attention from many researchers in recent years, and it is important to impart anti-microbial adhesion properties by modifying the surface of a polymer without damaging the internal structure of the polymer.
The preparation method of the conventional high-molecular antibacterial material mainly comprises two steps: one method is to add antibacterial components such as filling nano particles and adding antibacterial agents in the preparation process, and the method has high stability of film formation, but simultaneously, the difficulty of the production process is often increased, and the problem of low utilization rate of the antibacterial components exists; the other method is to load the antibacterial component on the surface after the polymer is processed and formed, which can improve the utilization rate of the antibacterial component, but has the problem that the durability of the antibacterial effect is poor as the antibacterial component is released.
For example, the antibacterial surface has wide application and value in the field of packaging, and the invention of application No. 201911306293 discloses an antibacterial food packaging bag, which mainly contains nano silver micro powder and essential oil micro powder as antibacterial components and has good thermal stability, antifouling property and mechanical property. The invention of application No. 201822229981 discloses a high-molecular packaging material with antibacterial and deodorizing effects, wherein a medicament filling layer is arranged on the packaging material, so that the breeding of bacteria is reduced. The antibacterial packaging materials all have the problems that along with the release of antibacterial ingredients, the durability of the antibacterial effect is exposed, even the released antibacterial ingredients influence the food safety and the like. In addition, it is difficult to combine the resistance to fungi and bacteria with the conventional antibacterial materials. Therefore, the production of packaging materials with highly effective and stable non-releasing anti-microbial adhesion coatings has been an important goal of research and development in the industry.
In recent years, methods for introducing functional groups through ultraviolet light-assisted surface modification have attracted the interest of researchers.
In 1996, poplar and Ranby invented a "two-step" living photografting method for polymers, under the condition of ultraviolet irradiation, a photoinitiator Benzophenone (BP) can abstract H atoms of C-H bonds on the surface of a substrate, so that surface free radicals are generated to initiate polymerization, the growth of a graft chain is realized, and terminal free radicals can be coupled with semipinacol free radicals generated by reduction of BP, so that controllable living surface grafting polymerization is realized (Macromolecules, 1996, 29, 3308). Later, young and Yi et al found that Isopropyl Thioxanthone (ITX) with a structure similar to benzophenone also had similar properties and achieved grafting of polymeric substrates in the visible range. The ultraviolet light-initiated surface technology is comprehensively described in "photoinitiation and surface modification" (polymer chemistry, 2001, chemical industry publishers) of Yangtai, beijing university of chemical industry, and all vinyl monomers suitable for the method, such as acrylic acid, acrylate, acrylamide and the like, and photosensitizers suitable for the method, such as benzophenone, anthrone and the like, are pointed out. The invention with application numbers of 200310100364 and 200710146564 optimizes the method and achieves the purpose of modifying the surfaces of various high polymer materials.
The invention of application No. 201410081985 discloses an antibacterial material of cellulose composite borneol, which uses borneol molecules to esterify and modify the macromolecular structure of cellulose, thereby achieving the purpose of resisting microbial adhesion. The method is simple and easy to implement, and has good antibacterial performance. The invention of application No. 201910411303 discloses the use of borneol as a surface modification component of a textile, which is first surface modified with an aminosilicone and then the aldehyde benzoic acid borneol is bonded to the surface of the textile. The invention can obtain stable and safe antimicrobial adhesion textile and has good anti-adhesion effect on fungi and bacteria.
At present, the research on the antimicrobial performance of the borneol only stays in that the substrate is modified by using the borneol alone and has obvious antibacterial effect, but the antibacterial performance of the surface of the modified material cannot be realized by carrying out photoinitiated polymerization on the acrylate monomer of the borneol (see a comparative example).
In addition, the modification method of the aforementioned patent is limited to groups with high reactivity, and the operation steps are relatively complicated, which results in unnecessary waste of resources in the production process. The active light grafting method can reduce the dosage of functional monomers, realize the application of most polymers in the field of antimicrobial adhesion, and has important significance for production and life.
Disclosure of Invention
The invention aims to provide an application of a non-release type antimicrobial adhesive coating in an antibacterial packaging material, and the non-release type antimicrobial adhesive coating mainly composed of a copolymer of borneol acrylate and polyethylene glycol diacrylate is modified on the surface of the packaging material to obtain the packaging material with the non-release type antimicrobial adhesive coating, and the packaging material has excellent and lasting antibacterial performance.
The invention provides an application of a non-release antimicrobial adhesive coating in an antibacterial packaging material, which comprises grafting acrylic borneol ester and polyethylene glycol diacrylate onto the surface of the packaging material in a manner that a photoinitiator generates surface free radicals to copolymerize to form the non-release antimicrobial adhesive coating, so as to obtain the packaging material with the non-release antimicrobial adhesive coating; wherein, the polymer forming the non-release type antimicrobial adhesive coating is formed by copolymerizing two monomers of borneol acrylate and polyethylene glycol diacrylate, and the molecular structure is shown as the formula (I):
Figure BDA0002543624410000031
in the formula (I), n is the number of the repeating units of the polymer and takes the value of a positive integer;
the packaging material is preferably a food packaging material, which comprises a food packaging film, a packaging bag or a packaging box, and the material of the packaging material comprises Polyethylene (PE), polypropylene (PP), biaxially oriented polypropylene (OPP), polyvinyl chloride (PVC), EVA plastic or PO plastic.
In the invention, the borneol acrylate is one or more of L-borneol acrylate, D-borneol acrylate and Iso-borneol acrylate.
In the invention, the molecular weight of the polyethylene glycol diacrylate is 200-1000.
According to the invention, the non-releasing antimicrobial adhesive coating is capable of preventing the adhesion of fungi and bacteria; preferably, the molar ratio of the acrylic borneol ester to the polyethylene glycol diacrylate in the non-release antimicrobial adhesive coating layer is (0.3-3) to 1; further preferably, the molar fraction of the bornyl acrylate in the non-releasing antimicrobial adhesive coating is 0.25 to 0.75.
In the present invention, the photoinitiator comprises benzophenone and/or isopropyl thioxanthone.
According to some embodiments of the invention, the application comprises,
step C, dispersing a photoinitiator solution on the surface of the packaging material, and performing illumination, washing and drying in a nitrogen atmosphere to obtain the packaging material with the surface modified by the photoinitiator;
d, dispersing the mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer on the surface of the packaging material of which the surface is modified by the photoinitiator, and performing illumination, washing and drying in nitrogen atmosphere to prepare the packaging material of which the surface is provided with the non-release antimicrobial adhesive coating;
wherein the surface of the packaging material comprises an inner surface of the packaging material and an outer surface of the packaging material, preferably the outer surface of the packaging material.
According to some embodiments of the invention, the photoinitiator solution is obtained by dissolving a photoinitiator in acetone, vortexing, sonicating, and then purging with nitrogen to remove oxygen; preferably, the concentration of the photoinitiator solution is 0.1-0.5g/mL; further preferably, the photoinitiator comprises benzophenone and/or isopropyl thioxanthone.
According to other embodiments of the present invention, the mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer is obtained by dissolving the borneol acrylate monomer and the polyethylene glycol diacrylate monomer in acetone, performing vortex treatment, performing ultrasonic treatment, and then introducing nitrogen to remove oxygen; preferably, in the mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer, the molar ratio of the borneol acrylate to the polyethylene glycol diacrylate is (0.3-3) to 1; further preferably, the concentration of the mixed solution of the bornyl acrylate monomer and the polyethylene glycol diacrylate monomer is 50% to 80% (v/v).
In the invention, the light source is a 200-1000W high-pressure mercury lamp, and the illumination time is 5-10min.
In some embodiments of the invention, in step C, the washing comprises soaking with an ethanol solution at room temperature for 5-10h;
in other embodiments of the present invention, in step D, the washing comprises soaking with dichloromethane and ethanol solution sequentially for 5-10h at room temperature, and ultrasound is performed for 20-30min after each soaking.
According to the invention, in step C, the packaging material is a pretreated packaging material; further preferably, the pretreatment method of the packaging material comprises soaking in ethanol for 10 hours, performing ultrasonic treatment for 30min, washing with ethanol, and performing vacuum drying.
The present invention also provides a packaging material having a non-releasing antimicrobial adhesive coating on its surface, which is obtained in the above-mentioned applications.
The invention provides an application of a non-release antimicrobial adhesive coating in an antibacterial packaging material, wherein the main component of the non-release antimicrobial adhesive coating is formed by a copolymer of two monomers, namely, acrylic borneol ester (BA) and polyethylene glycol diacrylate (PEGDA), an amphiphilic stereochemical antibacterial high polymer coating is constructed, and the coating has good antimicrobial adhesion. The preparation method of the coating mainly comprises the following steps: firstly, preparing a monomer and a photoinitiator into a solution with a certain concentration, then carrying out two-step modification on the packaging material by using a photo-grafting method, fixing the photoinitiator on the surface of the packaging material in the first step, and carrying out surface free radical initiated polymerization on the monomer in the second step to realize grafting. The preparation method is simple, and the obtained grafted coating is safe and stable; the advantages of the polyacrylate bornyl ester and the polyethylene glycol diacrylate can be fully exerted, and the adhesion of microorganisms is synergistically prevented; the coating is applied to surface modification of packaging materials, and can ensure that the grafted coating has a smooth structure.
Drawings
The invention is described in further detail below with reference to the attached drawing figures:
FIG. 1 shows the molecular structure of the polymer constituting the non-release type antimicrobial adhesive coating layer.
FIG. 2 is a scanning electron micrograph of a grafted PBA-PPEGDA coating on the surface of a polypropylene film of example 2.
FIG. 3 is a schematic view showing a flow of preparing a non-release type anti-microbial adhesive coating layer according to the present invention.
FIG. 4 is a graph comparing the results of fungal (Aspergillus niger) contamination of the surface of the hollow white package sample of example 5 with a package sample grafted with a PBA-PPEGDA coating.
FIG. 5 is a graph comparing the plate count results of the number of bacteria (Staphylococcus aureus) adhered to the surface of the hollow white packaging bag sample of example 5 and the surface of the packaging bag sample grafted with the PBA-PPEGDA coating.
Detailed Description
In order that the invention may be readily understood, a more particular description thereof will be rendered by reference to the appended drawings. However, before the present invention is described in detail, it is to be understood that this invention is not limited to particular embodiments described. It is also to be understood that the terminology used herein is for the purpose of describing particular embodiments only, and is not intended to be limiting.
Where a range of values is provided, it is understood that each intervening value, to the extent that there is no stated or intervening value in that stated range, to the extent that there is no such intervening value, is encompassed within the invention. The upper and lower limits of these smaller ranges may independently be included in the smaller ranges, and are also encompassed within the invention, subject to any specifically excluded limit in the stated range. Where a specified range includes one or both of the limits, ranges excluding either or both of those included limits are also included in the invention.
I. Term(s) for
The terms "about," "substantially," and "primarily," when used in conjunction with a range of components, concentrations, temperatures, or other physical or chemical properties or characteristics, as used herein, cover variations that may exist in the upper and/or lower limits of the range for the property or characteristic, including variations due to, for example, rounding, measurement, or other statistical variations. As used herein, numerical values associated with amounts, weights, and the like, are defined as "about" as all numerical values for each particular value plus or minus 1%. For example, the term "about 10%" should be understood to mean "9% to 11%".
II. Detailed description of the preferred embodiments
As described above, in the two methods for preparing the polymer antibacterial material, the antibacterial component is added in the preparation process, the difficulty of the production process is high, and the utilization rate of the antibacterial component is not high; after the polymer is processed and formed, the antibacterial component is loaded on the surface, so that the problems that the antibacterial component is released, the effect durability is poor, even the released antibacterial component influences the food safety and the like exist. In addition, it is difficult to combine the resistance to fungi and bacteria with the conventional antibacterial materials.
At present, the research on the antimicrobial performance of the borneol only stays in that the borneol is used alone to modify a base material, although the borneol has a remarkable antibacterial effect, the antibacterial performance of the surface of a grafting material cannot be realized by carrying out photoinitiated polymerization on an acrylate monomer of the borneol. The existing grafting method is limited to groups with high reactivity, and the operation steps are relatively complex, which can lead to unnecessary resource waste in the production process.
In view of the above, the present inventors have conducted extensive studies on a highly efficient and stable non-release type anti-microbial adhesion coating layer and a method for preparing the same. The invention researches and designs and discovers that the borneol-based non-release antibacterial polymer coating can be prepared by grafting the borneol acrylate and the polyethylene glycol diacrylate on the surface of the high polymer material and copolymerizing the borneol acrylate and the polyethylene glycol diacrylate, and the coating mainly comprises a copolymer of the borneol acrylate and the polyethylene glycol diacrylate and has good antibacterial performance. The present inventors have applied this non-releasing antimicrobial polymer coating to packaging materials to obtain the present invention.
The application of the non-release type antimicrobial adhesive coating in the antibacterial packaging material can be understood as a method for grafting the non-release type antimicrobial adhesive coating on the surface of the packaging material, and the method comprises the steps of grafting the borneol acrylate and the polyethylene glycol diacrylate on the surface of the packaging material in a mode of generating surface free radicals through a photoinitiator to form the non-release type antimicrobial adhesive coating through copolymerization, so as to obtain the packaging material with the non-release type antimicrobial adhesive coating; wherein, the polymer forming the non-release type antimicrobial adhesive coating is formed by copolymerizing two monomers of bornyl acrylate and polyethylene glycol diacrylate, and the molecular structure is shown as the formula (I) (shown in figure 1):
Figure BDA0002543624410000061
in the formula (I), n is the number of repeating units of the polymer and is a positive integer;
the preferred food package material of packaging material, it includes that the material is food packaging film, wrapping bag or packing carton of Polyethylene (PE), polypropylene (PP), biaxial stretching polypropylene (OPP), polyvinyl chloride (PVC), EVA plastics or PO plastics, just packaging material's surface includes packaging material's internal surface and packaging material's surface, preferably packaging material's surface.
In the invention, the borneol acrylate is one or more of L-borneol acrylate, D-borneol acrylate and Iso-borneol acrylate.
In the invention, the molecular weight of the polyethylene glycol diacrylate is 200-1000.
The invention creatively selects the hydrophilic polyethylene glycol diacrylate monomer as the annular complementary molecule to form the antimicrobial adhesion coating with local amphipathy, thereby realizing the effect of synergistically enhancing the antimicrobial adhesion.
In the present invention, the photoinitiator comprises benzophenone and/or isopropyl thioxanthone.
The inventors have conducted antimicrobial adhesion tests on non-releasing antimicrobial adhesion coatings and the results show that:
(1) When the molar ratio of the borneol acrylate to the polyethylene glycol diacrylate in the non-release antimicrobial adhesive coating is (0.3-3) to 1, the coating has excellent anti-adhesive effect on fungi; when the molar fraction of the borneol acrylate is less than 0.25 or more than 0.75, the antifungal adhesion effect is reduced to different degrees; in particular, when bornyl acrylate and polyethylene glycol diacrylate are used alone, a complete antifungal adhesion effect cannot be obtained.
(2) When the molar ratio of the borneol acrylate to the polyethylene glycol diacrylate in the non-release antimicrobial adhesive coating is (0.3-3) to 1, the antibacterial adhesive effect is optimal; in particular, when the bornyl acrylate and the polyethylene glycol diacrylate are used alone, a good anti-bacterial adhesion effect cannot be obtained.
As can be seen from the foregoing, the non-releasing antimicrobial adhesive coating provided by the present invention is effective in inhibiting the adhesion of fungi and bacteria to its surface; preferably, the molar ratio of the acrylic borneol ester to the polyethylene glycol diacrylate in the non-release antimicrobial adhesive coating layer is (0.3-3) to 1; further preferably, the molar fraction of the bornyl acrylate in the non-releasing antimicrobial adhesive coating is 0.25 to 0.75.
The invention realizes the graft modification of the PP or PET packaging material. The antibacterial coating with a cross-linked structure is synthesized in two steps by an ultraviolet light grafting method. The coating is connected with the surface of the packaging material through chemical bonds, and has good stability. The monomer of acrylic acid borneol ester is used as a hydrophobic chain segment and a stereochemical chain segment, and the polyethylene glycol diacrylate is used as a hydrophilic chain segment. The hydrophilic chain segment is polyethylene glycol diacrylate, so that the grafting efficiency and the surface grafting flatness can be ensured, and therefore, the grafted coating with excellent performance can be prepared by adjusting the proportion of the polyethylene glycol diacrylate to the acrylic borneol ester.
From the above, it can be seen that the antimicrobial coating provided by the present invention is a non-release material, which affects the adhesion of microorganisms through the molecular structure of the coating surface, rather than releasing a bactericide, and is a safe and environment-friendly coating. Thus, the use of the non-releasing antimicrobial adhesive coating in the antimicrobial packaging material of the present invention also includes the use of the packaging material with the non-releasing antimicrobial adhesive coating in packaging that requires antimicrobial properties, such as food packaging.
The flow chart of the method for preparing the non-release type antimicrobial adhesive coating on the antibacterial packaging material according to the invention is shown in fig. 3, and as can be seen from fig. 3, the method of the invention grafts the acrylic borneol ester and the polyethylene glycol diacrylate on the surface of the packaging material containing C-H bonds through the photoinitiator, and grafts and copolymerizes the acrylic borneol ester and the polyethylene glycol diacrylate on the surface of the packaging material to form the non-release type antimicrobial adhesive coating.
The technical scheme for preparing the non-release antimicrobial adhesive coating is as follows:
(1) Preparing photoinitiator solution and monomer mixed solution
Dissolving a photoinitiator in acetone, carrying out vortex treatment and ultrasonic treatment, and introducing nitrogen to remove oxygen to obtain a photoinitiator solution; preferably, the concentration of the photoinitiator solution is 0.1-0.5g/mL; further preferably, the photoinitiator comprises benzophenone and/or isopropyl thioxanthone, and even more preferably, the photoinitiator is benzophenone and isopropyl thioxanthone.
Dissolving a borneol acrylate monomer and a polyethylene glycol diacrylate monomer in acetone, performing vortex treatment and ultrasonic treatment, and introducing nitrogen to remove oxygen to obtain a mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer; preferably, in the mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer, the molar ratio of the borneol acrylate to the polyethylene glycol diacrylate is (0.3-3) to 1.
The concentration of the prepared mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer is 50-80% (v/v). This is understood to mean that the total volume of the two monomers, i.e., the borneol acrylate and the polyethylene glycol diacrylate, is a volume percentage of the monomer mixed solution.
(2) Dispersing a photoinitiator solution on the surface of the packaging material, and performing illumination, washing and drying in a nitrogen atmosphere to obtain a photoinitiator modified packaging material;
(3) And D, dispersing the mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer on the surface of the packaging material modified by the photoinitiator, and performing illumination, washing and drying in nitrogen atmosphere to obtain the non-release antimicrobial adhesive coating grafted on the surface of the packaging material, which can also be understood as the packaging material with the non-release antimicrobial adhesive coating grafted on the surface.
In some specific embodiments, in the step (2), benzophenone (BP) and Isopropyl Thioxanthone (ITX) are used as the photoinitiators, the photoinitiators are dispersed and adsorbed on the surface of the packaging material by dipping, coating or spraying, and the packaging material modified by the photoinitiators is obtained by ultraviolet irradiation for a certain time in a nitrogen atmosphere.
In some further specific embodiments, the packaging material is first soaked in ethanol and ultrasonically cleaned of impurities, and vacuum dried for use. And then the prepared photoinitiator solution is subjected to ultrasonic treatment and is bubbled with nitrogen for a period of time, so that oxygen is fully dissolved and removed. Then, the photoinitiator is dispersed and adsorbed on the surface of the packaging material by adopting a dipping or coating or spraying method, and is put into an acetone solution for soaking in a nitrogen atmosphere by ultraviolet irradiation for a period of time to remove the unreacted photoinitiator. And finally, drying the mixture in vacuum to obtain the photoinitiator modified packaging material.
In other further specific embodiments, the acetone monomer mixed solution with a certain concentration is prepared by mixing the borneol acrylate and the polyethylene glycol diacrylate according to different proportions, and then the acetone monomer mixed solution is subjected to ultrasonic treatment and is bubbled with nitrogen for a period of time to fully remove oxygen. Then, the monomer mixed solution is dispersed and adsorbed on the surface of the packaging material of which the surface is modified by the photoinitiator by adopting a dipping, coating or spraying method, the packaging material is irradiated for a period of time by ultraviolet light in nitrogen atmosphere, and the monomer mixed solution is sequentially put into dichloromethane and ethanol solution for soaking and is subjected to ultrasonic treatment to remove the monomer and the homopolymer which are not grafted. Finally, the packaging material is dried in vacuum to obtain the packaging material with the surface grafted with the non-release type antimicrobial adhesive coating.
In some embodiments of the invention, the specific method of preparing the non-releasing antimicrobial adhesive coating is as follows:
1. preparation work
(1) And (3) soaking the packaging material in ethanol for 10h and carrying out ultrasonic treatment for 30min to remove impurities on the surface of the film, and drying to obtain the packaging material to be modified.
(2) Preparing 0.1-0.5g/mL acetone solution from photoinitiator isopropyl thioxanthone and benzophenone according to the molar ratio of (1-5) to 1, and performing ultrasonic treatment, introducing nitrogen and removing oxygen.
(3) Preparing a solution with the molar ratio of the borneol acrylate to the polyethylene glycol diacrylate of (0.3-3) to 1 and the concentration of the monomer solution of 50-80% (volume fraction), and using the borneol acrylate and the polyethylene glycol diacrylate as controls, carrying out ultrasonic treatment, introducing nitrogen and removing oxygen.
2. The first-step modification preparation process of the packaging material comprises the following steps:
dispersing and adsorbing the photoinitiator on the surface of the packaging material by adopting a dipping or coating or spraying method, preheating for 1min by using a high-pressure mercury lamp, rotationally irradiating the packaging material for 5-10min in a nitrogen atmosphere, taking out the packaging material, soaking the packaging material in an ethanol solution for 5-10h, cleaning, drying, and removing the photoinitiator which is not reacted completely to obtain the packaging material of which the surface is modified by the photoinitiator.
3. The second grafting preparation process of the packaging material comprises the following steps:
dispersing and adsorbing 50-200 mu L of monomer solution on the surface of a packaging material by adopting a dipping or coating or spraying method, preheating for 1min by using a high-pressure mercury lamp, rotationally irradiating the packaging material for 5-10min in a nitrogen atmosphere, sequentially putting the packaging material into dichloromethane solution and ethanol solution, respectively cleaning for 5-10h, performing ultrasonic treatment for 20-30min each time to remove unreacted monomer and homopolymer, and drying to remove a solvent to obtain the packaging material with the non-release antimicrobial coating.
The invention combines the hydrophilic and hydrophobic chain segment with the stereochemical strategy through photo-grafting, is easy to implement, and can be widely applied to various packaging materials with antimicrobial requirements, in particular to food packaging materials.
In the present invention, the reaction efficiency is reflected by the graft ratio, which is calculated by the following formula:
percent grafting (% = [ (mass of membrane after grafting-mass of membrane before grafting)/total mass of monomer put ] × 100%
The bacteriostasis or antibiosis test method of the invention is as follows:
determination of antifungal adhesion properties: cutting the blank substrate material and the substrate material grafted by the non-release antimicrobial adhesive coating into round samples with the diameter of 10.0 +/-0.1 mm, irradiating the round samples for 1 hour on the front and back sides under an ultraviolet lamp, and then co-culturing the round samples with fungi.
Specifically, the membrane with coating side facing upwards is flatly adhered on malt extract agar culture medium, and then 10 μ L of fungus solution [ fungus spore solution containing spore (1-5). Times.10 ] spore (spore solution of fungus) is dripped at a distance of 1-2cm from the material 8 Per mL]Constant temperature at 30 ℃ and relative humidity of 85% +/-5%Culturing for 8 days at constant temperature and humidity, observing and recording the pollution condition of the surface of the substrate material by using a camera. The evaluation standard of the mildew-proof effect is shown in table 1, wherein the coverage area of the mildew on the surface of the control sample is more than 60% (namely, the mildew-proof effect reaches 4 grades), and when the growth of the mildew on the surface of the blank test sample cannot be observed by eyes, the test is judged to be effective, otherwise, the test is invalid.
TABLE 1 evaluation criteria for mold-proofing effects
Figure BDA0002543624410000091
Figure BDA0002543624410000101
Determination of antibacterial adhesion properties: the blank substrate material and the substrate material grafted by the non-release antimicrobial adhesion coating are cut into circular samples with the diameter of 10.0 +/-0.1 mm, and after sterilization treatment by positive and negative irradiation under an ultraviolet lamp for 1 hour, the circular samples are cultured with bacteria.
Specifically, the concentration of bacteria was first set to 10 7 CFU/mL PBS bacterial suspension, immersing blank substrate material and non-release type antimicrobial adhesion coating grafted substrate material into 1mL bacteria with concentration of 10 7 Fully contacting the CFU/mL PBS suspension with the material at the temperature of 4 ℃ for co-culturing for 24 hours, taking out the material, washing the material with sterile physiological saline for three times, finally removing the washing liquid by using filter paper, putting the material into 1.8mL sterile physiological saline, carrying out ultrasonic treatment for 15min, coating a 100 mu L flat plate, culturing for 24 hours at the temperature of 37 +/-2 ℃, counting the colony of the flat plate, and calculating the antibacterial adhesion rate according to the formula (III):
R(%)=[(A-B)/A]×100% (III)
in the formula (III):
r-antibacterial adhesion rate of the sample;
a-surface bacteria adhesion quantity (CFU/mL) after the substrate material and the bacterial liquid react for 24 hours;
and (3) the surface bacteria adhesion quantity (CFU/mL) of the B-non-release type antimicrobial adhesion coating grafted base material after 24h of bacterial liquid action.
Examples
The present invention will be specifically described below with reference to specific examples. The experimental methods described below are, unless otherwise specified, conventional laboratory methods. The experimental materials described below, unless otherwise specified, are commercially available.
The strains for antifungal experiments or antibacterial experiments include:
aspergillus niger (ATCC 16404); staphylococcus aureus (Staphylococcus aureus) (ATCC 25923); wherein the term "ATCC" refers to American Type Culture Collection. All the strains are purchased from China Industrial microorganism strain preservation management center, and each strain is independently used as an experimental strain to carry out antifungal experiment or antibacterial experiment on a sample to be tested.
Malt extract (wort) agar medium used in antifungal experiments, nutrient agar medium used for bacterial count in antibacterial experiments, and TSB medium (trypticase soytone liquid medium) used for preparing bacterial solution were purchased from beijing obozin biotechnology, ltd.
Example 1:
preparing a grafted PBA-PPEGDA coating of a polyacrylonitrile membrane:
(1) Preparation of solutions
Preparation of photoinitiator solution: weighing 4.2300g of isopropyl thioxanthone and 0.6066g of benzophenone in a brown sample bottle, adding 10mL of acetone, vortexing, performing ultrasonic treatment for 20min to fully dissolve the acetone, and finally bubbling the acetone for 20min by using a nitrogen blower (ND 400, hangzhou Ruichi instruments, inc.) to fully remove oxygen to obtain a photoinitiator solution.
Preparation of monomer solution: 2.08mL BA,2.00mL PEGDA (relative molecular weight 200) are mixed evenly (the molar ratio of BAP to PEGDA is 1: 1), 0.8mL of mixed monomer and 0.2mL of acetone are sucked and placed in a brown sample bottle for ultrasonic treatment, and then nitrogen is introduced for deoxygenation for 20min to obtain a monomer solution.
(2) Preparation of photoinitiator modified Polyacrylonitrile membranes
Soaking polyacrylonitrile membrane in ethanol for 10 hr, ultrasonic treating for 30min to remove impurities, washing surface with ethanol, and vacuum drying. The quartz plate is placed on the bottom layer to be used as a support, and the polyacrylonitrile film is covered on the quartz plate. And (3) sucking 100 mu L of photoinitiator solution by using a pipette gun to drop on the surface of the membrane, covering a quartz plate on the membrane, and slightly pressing to remove bubbles to form a liquid interlayer. After preheating by a high-pressure mercury lamp for 1min, placing the obtained reaction device model under the high-pressure mercury lamp for irradiating for 8min. And taking out the model, soaking the model in an acetone solution for 10 hours, putting the model into a vacuum drying oven for drying, and removing the unreacted photoinitiator and solvent to obtain the photoinitiator modified polyacrylonitrile membrane.
(3) Preparation of Polyacrylonitrile film with PBA-PPEGDA coating
And (3) dispersing 100 mu L of monomer solution on the surface of the membrane according to the reaction model in the step (2), irradiating for 8min, sequentially putting the reaction device into dichloromethane solution and ethanol solution, respectively cleaning for 10h, soaking for 30min after each time, performing ultrasonic treatment to remove unreacted monomers and homopolymers, drying and removing a solvent to obtain the polyacrylonitrile membrane with the PBA-PPEGDA coating, wherein the grafting efficiency of the monomers reaches 50%, and the reaction has the advantages of simple operation and high reaction efficiency.
Determination of antifungal adhesion properties:
cutting the polyacrylonitrile membrane with the coating and the ungrafted membrane into a wafer with the diameter of 1cm, irradiating the front side and the back side of the wafer for 1h under an ultraviolet lamp for sterilization, then co-culturing the wafer and aspergillus niger in the same wort agar culture medium, enabling the side of the wafer with the grafting layer to face upwards, dripping 10 mu L of aspergillus niger spore liquid at a position 1-2cm away from the material, and culturing for 8 days to observe the pollution condition of the surface of the material. The result shows that no obvious mildew grows under the magnifier, and the corresponding mildew-proof grade is 0, so that the antifungal adhesive has excellent antifungal adhesive effect.
Comparative example 1: preparation of grafted PBA coating of polyacrylonitrile membrane:
(1) Preparation of solutions
Preparation of photoinitiator solution: weighing 4.2300g of isopropyl thioxanthone and 0.6066g of benzophenone in a brown sample bottle, adding 10mL of acetone, vortexing, performing ultrasonic treatment for 20min to fully dissolve the acetone, and finally bubbling the acetone for 20min by using a nitrogen blower to fully remove oxygen to obtain a photoinitiator solution.
Preparation of monomer solution: 0.8mL of BA and 0.2mL of acetone are mixed and placed in a brown sample bottle for ultrasonic treatment, and then nitrogen is introduced for deoxygenation for 20min to obtain a monomer solution (the molar ratio of BAP to PEGDA is 1: 0).
(2) Preparation of photoinitiator-modified Polyacrylonitrile membranes
Soaking polyacrylonitrile membrane in ethanol for 10 hr, ultrasonic treating for 30min to remove impurities, washing surface with ethanol, and vacuum drying. And putting the quartz plate on the bottom layer as a support, and covering the polyacrylonitrile film on the quartz plate. And (3) sucking 100 mu L of photoinitiator solution by using a pipette gun to drop on the surface of the membrane, covering a quartz plate on the membrane, and slightly pressing to remove bubbles to form a liquid interlayer. After preheating by a high-pressure mercury lamp for 1min, the obtained reaction device model is placed under the high-pressure mercury lamp to irradiate for 8min. And taking out the model, soaking the model in an acetone solution for 10 hours, putting the model into a vacuum drying oven for drying, and removing the unreacted photoinitiator and solvent to obtain the photoinitiator modified polyacrylonitrile membrane.
(3) Preparation of Polyacrylonitrile membranes with PBA coatings
And (3) dispersing 100 mu L of monomer solution on the surface of the membrane according to the reaction model in the step (2), irradiating for 8min, putting the reaction device into dichloromethane solution, cleaning for 10h, soaking, performing ultrasonic treatment for 30min to remove unreacted monomers and homopolymers, drying and removing the solvent to obtain the polyacrylonitrile membrane with the PBA coating, wherein the grafting efficiency of the monomers is 1.6%.
Determination of antifungal adhesion properties:
cutting the polyacrylonitrile membrane with the coating and the ungrafted membrane into round sheets with the diameter of 1cm, irradiating the round sheets on the front and back sides for 1h under an ultraviolet lamp for sterilization, then co-culturing the round sheets and aspergillus niger in the same wort agar culture medium, enabling the side of the membrane with the grafted layer to face upwards, dropwise adding 10 mu L of aspergillus niger spore solution at a position 1-2cm away from the material, and culturing for 8 days to observe the pollution condition of the surface of the material. The results show that the mould coverage on the surface of the sample is 27.3%, corresponding to mould proof grade 2, it fails to achieve a complete antifungal adhesion effect.
Comparative example 2:
preparation of a grafted PPEGDA coating of a polyacrylonitrile membrane:
(1) Preparation of solutions
Preparation of photoinitiator solution: weighing 4.2300g of isopropyl thioxanthone and 0.6066g of benzophenone in a brown sample bottle, adding 10mL of acetone, carrying out vortex, carrying out ultrasonic treatment for 20min to fully dissolve the acetone, and finally carrying out bubbling for 20min by using a nitrogen blower to fully remove oxygen to obtain a photoinitiator solution.
Preparation of monomer solution: 0.8mL of PEGDA (relative molecular weight 200) and 0.2mL of acetone were mixed and placed in a brown sample bottle for sonication, followed by purging with nitrogen for 20min to obtain a monomer solution (mole ratio of BAP to PEGDA is 0: 1).
(2) Preparation of photoinitiator modified polyacrylonitrile membrane the polyacrylonitrile membrane is soaked in ethanol for 10h, and is ultrasonically treated for 30min to remove impurities, the surface is washed with ethanol, and vacuum drying is carried out. The quartz plate is placed on the bottom layer to be used as a support, and the polyacrylonitrile film is covered on the quartz plate. And (3) sucking 100 mu L of photoinitiator solution by using a pipette gun to drop on the surface of the membrane, covering a layer of quartz plate above the membrane, and slightly pressing to remove bubbles to form a liquid interlayer. After preheating by a high-pressure mercury lamp for 1min, the obtained reaction device model is placed under the high-pressure mercury lamp to irradiate for 8min. And taking out the model, soaking the model in an acetone solution for 10 hours, putting the model into a vacuum drying oven for drying, and removing the unreacted photoinitiator and solvent to obtain the photoinitiator modified polyacrylonitrile membrane.
(3) Preparation of Polyacrylonitrile Membrane with PPEGDA coating
And (3) dispersing 100 mu L of monomer solution on the surface of the membrane according to the reaction model in the step (2), irradiating for 8min, putting the reaction device into ethanol solution, cleaning for 10h, soaking, performing ultrasonic treatment for 30min to remove unreacted monomers and homopolymers, drying and removing the solvent to obtain the polyacrylonitrile membrane with the PPEGDA coating, wherein the grafting efficiency of the monomers is 53%.
Determination of antifungal adhesion properties:
cutting the polyacrylonitrile membrane with the coating and the ungrafted membrane into a wafer with the diameter of 1cm, irradiating the front side and the back side of the wafer for 1h under an ultraviolet lamp for sterilization, then co-culturing the wafer and aspergillus niger in the same wort agar culture medium, enabling the side of the wafer with the grafting layer to face upwards, dripping 10 mu L of aspergillus niger spore liquid at a position 1-2cm away from the material, and culturing for 8 days to observe the pollution condition of the surface of the material. The mold coverage on the sample surface was 3.9%, corresponding to mold resistance rating 1, which failed to fully exhibit the antifungal adhesion effect.
Example 2: preparation of grafted PBA-PPEGDA coating of polyethylene film:
(1) Preparation of solutions
Preparation of photoinitiator solution: weighing 2.5400g of isopropyl thioxanthone and 1.8220g of benzophenone in a brown sample bottle, adding 10mL of acetone, carrying out vortex, carrying out ultrasonic treatment for 20min to fully dissolve the acetone, and finally carrying out bubbling for 20min by using a nitrogen blower to fully remove oxygen to obtain a photoinitiator solution.
Preparation of monomer solution: 2.08mLBA,4.00mLPEGDA (relative molecular weight of 400) were mixed (mole ratio of BAP to PEGDA was 1: 1), 0.65mL of mixed monomer and 0.35mL of acetone were sucked and put in a brown sample bottle for ultrasonic treatment, and then nitrogen was introduced to remove oxygen for 20min, to obtain a monomer solution.
(2) Preparation of photoinitiator modified polyethylene film
Soaking polyethylene film in acetone for 10 hr, ultrasonic treating for 30min to remove impurities, washing surface with acetone, and vacuum drying. The quartz plate is placed on the bottom layer to be used as a support, and the quartz plate is covered with a polyethylene film. And (3) sucking 100 mu L of photoinitiator solution by using a pipette gun to drop on the surface of the membrane, covering a quartz plate on the membrane, and slightly pressing to remove bubbles to form a liquid interlayer. After preheating by a high-pressure mercury lamp for 1min, the obtained reaction device model is placed under the high-pressure mercury lamp to irradiate for 8min. And taking out the model, soaking the model in an acetone solution for 10 hours, putting the model into a vacuum drying oven for drying, and removing the unreacted photoinitiator and solvent to obtain the photoinitiator modified polyethylene film.
(3) Preparation of polyethylene film with PBA-PPEGDA coating
And (3) dispersing 100 mu L of monomer solution on the surface of the membrane according to the reaction model in the step (2), irradiating for 8min, sequentially putting the reaction device into dichloromethane solution and ethanol solution, respectively cleaning for 10h, performing ultrasonic treatment for 30min after each soaking to remove unreacted monomers and homopolymers, and drying to remove the solvent to obtain the polyethylene membrane with the single-sided PBA-PPEGDA coating.
Grafting is carried out on one side of the ungrafted coating layer according to the same mode to obtain the polyethylene film with the double-sided PBA-PPEGDA coating layer, and the grafting efficiency of the monomer is 94.6%. The reaction has the advantages of simple operation and high reaction efficiency.
The PBA-PPEGDA coating obtained is observed by a scanning electron microscope (Hitachi S-4700 scanning electron microscope, hitachi, japan) and the result is shown in figure 2, so that an obvious grafting layer structure can be observed, which indicates that the PBA-PPEGDA coating is successfully synthesized.
Determination of antifungal adhesion properties:
cutting the blank polyethylene film and the polyethylene film modified by the non-release antimicrobial adhesive composite coating into round samples with the diameter of 10.0 +/-0.1 mm, irradiating the round samples for 1 hour on the front and back sides under an ultraviolet lamp for sterilization, and then culturing the round samples and fungi for 8 days to observe the pollution condition of the surface of the material. The surface of the modified film has no obvious mildew growth, and the modified film has an excellent antifungal adhesion effect corresponding to the mildew-proof grade 0.
Determination of antibacterial adhesion properties:
cutting the polyethylene film with the coating and the polyethylene film without grafting into round pieces with the diameter of 1cm, irradiating the round pieces on the front and back sides under an ultraviolet lamp for 1h for sterilization, and then co-culturing with staphylococcus aureus. Firstly, staphylococcus aureus 10 is prepared 7 And (3) immersing 1mL of PBS bacterial suspension in the CFU/mL bacterial suspension, fully contacting the materials at 4 ℃ for co-culture for 24 hours, taking out the materials, washing the materials with sterile normal saline for three times, removing a washing liquid by using filter paper, placing the materials in 1.8mL of sterile normal saline, carrying out ultrasonic treatment for 15 minutes, coating a 100 mu L plate, culturing for 24 hours at 37 ℃, and calculating the colony number of the plate. The antibacterial adhesion rate to staphylococcus aureus is 99.89%.
Comparative example 3:
preparation of grafted PBA coating of polyethylene film:
(1) Preparation of solutions
Preparation of photoinitiator solution: weighing 2.5400g of isopropyl thioxanthone and 1.8220g of benzophenone in a brown sample bottle, adding 10mL of acetone, carrying out vortex, carrying out ultrasonic treatment for 20min to fully dissolve the acetone, and finally carrying out bubbling for 20min by using a nitrogen blower to fully remove oxygen to obtain a photoinitiator solution.
Preparation of monomer solution: 0.65mL BA and 0.35mL acetone were mixed and placed in a brown sample bottle for sonication, followed by purging with nitrogen for 20min to obtain a monomer solution (BAP to PEGDA molar ratio of 1: 0).
(2) Preparation of photoinitiator modified polyethylene film
Soaking polyethylene film in acetone for 10 hr, ultrasonic treating for 30min to remove impurities, washing surface with acetone, and vacuum drying. And placing the quartz plate on a bottom layer for supporting, and covering a polyethylene film on the quartz plate. And (3) sucking 100 mu L of photoinitiator solution by using a pipette gun to drop on the surface of the membrane, covering a layer of quartz plate above the membrane, and slightly pressing to remove bubbles to form a liquid interlayer. After preheating by a high-pressure mercury lamp for 1min, the obtained reaction device model is placed under the high-pressure mercury lamp to irradiate for 8min. And taking out the model, soaking the model in an acetone solution for 10 hours, putting the model into a vacuum drying oven for drying, and removing the unreacted photoinitiator and solvent to obtain the photoinitiator modified polyethylene film.
(3) Preparation of polyethylene film with PBA coating
And (3) dispersing 100 mu L of monomer solution on the surface of the film according to the reaction model in the step (2), irradiating for 8min, putting the reaction device into dichloromethane solution, cleaning for 10h, soaking, performing ultrasonic treatment for 30min to remove unreacted monomers and homopolymers, and drying to remove the solvent to obtain the polyethylene film with the single-sided PBA coating.
Grafting is carried out on one side of the ungrafted coating layer according to the same mode to obtain the polyethylene film with the double-sided PBA coating layer, and the grafting efficiency of the monomer is 30.0%.
Determination of antifungal adhesion properties:
cutting blank polyethylene film and polyethylene film modified by PBA coating into round samples with diameter of 10.0 +/-0.1 mm, irradiating the round samples for 1 hour on the front and back sides under an ultraviolet lamp for sterilization, and co-culturing the round samples with fungi for 8 days to observe the pollution condition of the material surface. Mildew is observed on both the blank film and the polyethylene film modified by the PBA coating, and the complete antifungal adhesion effect cannot be achieved corresponding to the mildew-proof grade 1.
Determination of antibacterial adhesion properties:
cutting the polyethylene film with the coating and the polyethylene film without grafting into round pieces with the diameter of 1cm, irradiating the round pieces on the front and back sides under an ultraviolet lamp for 1h for sterilization, and then co-culturing with staphylococcus aureus. Firstly, the concentration of staphylococcus aureus is set to be 10 7 And (3) immersing 1mL of PBS bacterial suspension into the material, fully contacting the material at 4 ℃ for co-culturing for 24h, taking out the material, washing the material with sterile physiological saline for three times, removing a washing liquid by using filter paper, placing the material in 1.8mL of sterile physiological saline, carrying out ultrasonic treatment for 15min, coating a 100 mu L plate, culturing for 24h at 37 ℃, and calculating the colony number of the plate.
The result shows that the polyethylene film with the grafted coating layer has a certain antibacterial adhesion effect, but the antibacterial adhesion effect is poor, and the antibacterial adhesion rate to staphylococcus aureus is 84.3%.
Comparative example 4:
preparation of grafted PEGDA coating of polyethylene film:
(1) Solution preparation photoinitiator solution preparation: weighing 2.5400g of isopropyl thioxanthone and 1.8220g of benzophenone in a brown sample bottle, then adding 10mL of acetone, carrying out vortex, carrying out ultrasonic treatment for 20min to fully dissolve the acetone, and finally carrying out bubbling with a nitrogen blower for 20min to fully remove oxygen to obtain a photoinitiator solution.
Preparation of monomer solution: 0.65mL of PEGDA (relative molecular weight 400) and 0.35mL of acetone were mixed and placed in a brown sample bottle for sonication, followed by purging with nitrogen for 20min to obtain a monomer solution (mole ratio of BAP to PEGDA is 0: 1).
(2) Preparation of photoinitiator modified polyethylene film
Soaking polyethylene film in acetone for 10 hr, ultrasonic treating for 30min to remove impurities, washing surface with acetone, and vacuum drying. And placing the quartz plate on a bottom layer for supporting, and covering a polyethylene film on the quartz plate. And (3) sucking 100 mu L of photoinitiator solution by using a pipette gun to drop on the surface of the membrane, covering a quartz plate on the membrane, and slightly pressing to remove bubbles to form a liquid interlayer. After preheating by a high-pressure mercury lamp for 1min, the obtained reaction device model is placed under the high-pressure mercury lamp to irradiate for 8min. And taking out the model, soaking the model in an acetone solution for 10 hours, putting the model into a vacuum drying oven for drying, and removing the unreacted photoinitiator and solvent to obtain the photoinitiator modified polyethylene film.
(3) Preparation of polyethylene film with PPEGDA coating
And (3) dispersing 100 mu L of monomer solution on the surface of the film according to the reaction model in the step (2), irradiating for 8min, putting the reaction device into ethanol solution, cleaning for 10h, soaking, performing ultrasonic treatment for 30min to remove unreacted monomers and homopolymers, and drying to remove the solvent to obtain the polyethylene film with the single-side PEGDA coating.
The grafting was carried out in the same manner on the side of the ungrafted coating, obtaining a polyethylene film with a double-sided PPEGDA coating, the grafting efficiency of the monomer being 93.4%.
Determination of antifungal adhesion properties:
cutting the blank polyethylene film and the polyethylene film modified by the PPEGDA coating into round samples with the diameter of 10.0 +/-0.1 mm, irradiating the round samples for 1 hour on the front and back sides under an ultraviolet lamp for sterilization, and then culturing the round samples and fungi for 8 days to observe the pollution condition on the surface of the material. Mildew is observed on both the blank film and the polyethylene film modified by the PPEGDA coating, and the complete antifungal adhesion effect cannot be achieved corresponding to the mildew-proof grade 1.
Determination of antibacterial adhesion properties:
cutting the polyethylene film with the coating and the polyethylene film without grafting into round pieces with the diameter of 1cm, irradiating the round pieces on the front and back sides under an ultraviolet lamp for 1h for sterilization, and then co-culturing with staphylococcus aureus. Firstly, the concentration of staphylococcus aureus is set to be 10 7 Immersing 1mL of PBS bacterial suspension in the CFU/mL bacterial suspension, fully contacting the material at 4 ℃ for co-culturing for 24h, taking out the material, washing with sterile physiological saline for three times, removing the washing liquid by using filter paper, placing in 1.8mL of sterile physiological saline, and carrying out ultrasonic treatment for 15 hmin, take 100. Mu.L plate coating, culture at 37 ℃ for 24h, count plate colony. The antibacterial adhesion rate to staphylococcus aureus is 86.1%.
Example 3:
preparation of grafted PBA-PPEGDA coating of polyethylene terephthalate film:
(1) Solution preparation of photoinitiator solution: weighing 0.84g of isopropyl thioxanthone and 3.0333g of benzophenone in a brown sample bottle, adding 10mL of acetone, performing vortex and ultrasonic treatment for 20min to fully dissolve the acetone, and finally bubbling the acetone for 20min by using a nitrogen blower to fully remove oxygen to obtain a photoinitiator solution.
Preparation of monomer solution: 1.56mLBA and 2.50mLPEGDA (relative molecular weight 1000) are mixed (the molar ratio of BAP to PEGDA is 3: 1), dissolved uniformly by ultrasonic, 0.5mL of mixed monomer and 0.5mL of acetone are absorbed and placed in a brown sample bottle for ultrasonic treatment, and then nitrogen is introduced to remove oxygen for 20min, so that a monomer solution is obtained.
(2) Preparation of photoinitiator modified polyethylene terephthalate film
Soaking polyethylene terephthalate film in ethanol for 10h, performing ultrasonic treatment for 30min to remove impurities, washing the surface with ethanol, and vacuum drying. And placing a quartz plate on a bottom layer for supporting, and covering a polyethylene terephthalate film on the quartz plate. And (3) sucking 100 mu L of photoinitiator solution by using a pipette gun to drop on the surface of the membrane, covering a quartz plate on the membrane, and slightly pressing to remove bubbles to form a liquid interlayer. After preheating by a high-pressure mercury lamp for 1min, placing the obtained reaction device model under the high-pressure mercury lamp for irradiating for 5min. And taking out the model, soaking the model in an acetone solution for 5 hours, putting the model into a vacuum drying oven for drying, and removing the photoinitiator and the solvent which are not reacted completely to obtain the photoinitiator modified polyethylene terephthalate film.
(3) Preparation of polyethylene terephthalate film with PBA-PPEGDA coating
Dispersing 100 mu L of monomer solution on the surface of the membrane according to the reaction model in the step (2), irradiating for 5min, sequentially putting the reaction device into dichloromethane solution and ethanol solution, respectively cleaning for 5h, soaking and then performing ultrasonic treatment for 20min to remove unreacted monomers and homopolymers, drying and removing the solvent to obtain the polyethylene terephthalate membrane with the PBA-PPEGDA coating, wherein the grafting efficiency of the monomers reaches 90%, and the reaction has the advantages of simple operation and high reaction efficiency.
Determination of antifungal adhesion properties:
cutting the polyethylene terephthalate film with the coating and the ungrafted film into a circular sheet with the diameter of 1cm, irradiating the circular sheet with ultraviolet lamps for 1 hour on the front side and the back side for sterilization, co-culturing the circular sheet and aspergillus niger in the same wort agar culture medium, enabling the side of the circular sheet with the grafting layer to face upwards, placing the circular sheet at a position 1-2cm away from the center of a culture dish, dropwise adding 10 mu L of aspergillus niger spore solution into the center of the culture dish, and culturing for 8 days to observe the pollution condition of the surface of the material. The result reaches the mildew-proof grade of 0, and the antifungal adhesive has excellent antifungal adhesion effect.
Example 4: preparation of grafted PBA-PPEGDA coating of polypropylene film:
(1) Solution preparation:
preparation of photoinitiator solution: weighing 0.6600g of isopropyl thioxanthone and 0.3400g of benzophenone in a brown sample bottle, adding 10mL of acetone, carrying out vortex, carrying out ultrasonic treatment for 20min to fully dissolve the acetone, and finally carrying out bubbling for 20min by using a nitrogen blower to fully remove oxygen to obtain a photoinitiator solution.
Preparation of monomer solution: 1.04mLBA,3.00mLPEGDA (relative molecular weight 200) are mixed uniformly (the molar ratio of BAP to PEGDA is 1: 3), 0.8mL of mixed monomer and 0.2mL of acetone are sucked and placed in a brown sample bottle for ultrasonic treatment, and then nitrogen is introduced to remove oxygen for 20min, so as to obtain a monomer solution.
(2) Preparation of photoinitiator-modified Polyacrylonitrile membranes
Soaking the polypropylene film in ethanol for 10h, performing ultrasonic treatment for 30min to remove impurities, washing the surface with ethanol, and vacuum drying. The quartz plate is placed on the bottom layer to be used as a support, and the quartz plate is covered with a polypropylene film. And (3) sucking 100 mu L of photoinitiator solution by using a pipette gun to drop on the surface of the membrane, covering a layer of quartz plate above the membrane, and slightly pressing to remove bubbles to form a liquid interlayer. After preheating by a high-pressure mercury lamp for 1min, placing the obtained reaction device model under the high-pressure mercury lamp for irradiating for 10min. And taking out the model, soaking the model in an acetone solution for 8 hours, putting the model into a vacuum drying oven for drying, and removing the unreacted photoinitiator and solvent to obtain the photoinitiator modified polypropylene film.
(3) Preparation of Polyacrylonitrile Membrane with PBA-PPEGDA coating
And (3) dispersing 100 mu L of monomer solution on the surface of the membrane according to the reaction model in the step (2), irradiating for 10min, sequentially putting the reaction device into dichloromethane solution and ethanol solution, respectively cleaning for 8h, soaking each time, and then performing ultrasonic treatment for 25min to remove unreacted monomers and homopolymers, and drying to remove the solvent to obtain the polypropylene membrane with the PBA-PPEGDA coating. After the reaction, it was observed that the monomer remained without any liquid and was completely graft-fixed to the surface of the substrate. The reaction has the advantages of simple operation and high reaction efficiency.
Determination of antifungal adhesion properties:
cutting the polypropylene film with the coating and the ungrafted film into round pieces with the diameter of 1cm, irradiating the round pieces for 1h under an ultraviolet lamp for sterilization treatment, then co-culturing the round pieces with the aspergillus niger in the same wort agar culture medium, enabling the side of the membrane with the grafting layer to face upwards, placing the membrane at a position 1-2cm away from the center of a culture dish, then dropwise adding 10 mu L of aspergillus niger spore liquid into the center of the culture dish, and culturing for 8 days to observe the pollution condition of the surface of the material. The result reaches the mildew-proof grade of 0, and the antifungal adhesive has excellent antifungal adhesion effect.
Example 5:
packaging bag with surface grafted PBA-PPEGDA coating
(1) Solution preparation:
preparation of photoinitiator solution: weighing 4.2300g of isopropyl thioxanthone and 0.6066g of benzophenone in a brown sample bottle, adding 10mL of acetone, carrying out vortex, carrying out ultrasonic treatment for 20min to fully dissolve the acetone, and finally carrying out bubbling for 20min by using a nitrogen blower to fully remove oxygen to obtain a photoinitiator solution.
Preparation of monomer solution: after 2.08mL BA and 2.00mL PEGDA (relative molecular weight 200) are mixed uniformly, 0.8mL of mixed monomer and 0.2mL of acetone are sucked and placed in a brown sample bottle for ultrasonic treatment, and then nitrogen is introduced to remove oxygen for 20min, so that monomer solution is obtained.
(2) Preparation of photoinitiator modified packaging bag
Soaking the packaging bag in ethanol for 10h, removing impurities by ultrasonic treatment for 30min, washing the surface with ethanol, and vacuum drying. And (3) putting the packaging bag into a photoinitiator solution for dipping, so that the photoinitiator is adsorbed on the surface of the packaging bag. Preheating by a high-pressure mercury lamp for 1min, rotationally irradiating the packaging bag for 8min in nitrogen atmosphere, taking out the packaging bag, and soaking the packaging bag in an acetone solution for 10h to obtain the photoinitiator modified packaging bag.
(3) Packaging bag with surface grafted PBA-PPEGDA coating
And (3) dipping the packaging bag in the monomer solution according to the mode of the step (2), preheating by a high-pressure mercury lamp for 1min, rotationally irradiating the packaging bag for 8min in a nitrogen atmosphere, taking out the packaging bag, sequentially putting the packaging bag in a dichloromethane solution and an ethanol solution, respectively cleaning for 10h, performing ultrasonic treatment for 30min after each soaking, removing unreacted monomers and homopolymers, and drying to remove a solvent to obtain the packaging bag with the PBA-PPEGDA coating. After the reaction, it was observed that the monomer remained without being present in the form of a liquid and was completely graft-fixed to the surface of the substrate. The reaction has the advantages of simple operation and high reaction efficiency.
Determination of antifungal adhesion properties:
cutting the blank packaging bag and the non-release antimicrobial adhesive composite coating modified packaging bag into round samples with the diameter of 10.0 +/-0.1 mm, irradiating the front and back surfaces of the round samples for 1 hour under an ultraviolet lamp for sterilization, and then co-culturing the round samples with fungi for 8 days to observe the pollution condition of the surface of the material. The results show that the surface of the packaging bag sample grafted by the PBA-PPEGDA coating has no obvious mildew growth under a magnifying glass, and has an excellent antifungal adhesion effect corresponding to the mildew-proof grade of 0 (see figure 4).
Determination of antibacterial adhesion properties:
cutting the coating packaging bag and the unmodified packaging bag into round pieces with the diameter of 1cm, irradiating the round pieces on the front side and the back side under an ultraviolet lamp for 1 hour for sterilization, and then co-culturing with staphylococcus aureus. Firstly, staphylococcus aureus 10 is prepared 7 PBS bacteria of CFU/mLSuspending, taking 1mL of bacterial suspension, immersing the material, fully contacting the material at 4 ℃ for co-culturing for 24h, taking out the material, washing the material with sterile normal saline for three times, finally removing the washing liquid by using filter paper, placing the material in 1.8mL of sterile normal saline, carrying out ultrasonic treatment for 15min, taking 100 mu L of plate for coating, culturing for 24h at 37 ℃, and calculating the colony number of the plate. The results showed that the antibacterial adhesion rate of the non-release type antimicrobial adhesion coating modified packaging bag to staphylococcus aureus was 99.63% (see fig. 5).
It should be noted that the above-mentioned embodiments are only for explaining the present invention, and do not constitute any limitation to the present invention. The present invention has been described with reference to exemplary embodiments, but the words which have been used herein are words of description and illustration, rather than words of limitation. The invention can be modified, as prescribed, within the scope of the claims and without departing from the scope and spirit of the invention. Although the invention has been described herein with reference to particular means, materials and embodiments, the invention is not intended to be limited to the particulars disclosed herein, but rather extends to all other methods and applications having the same functionality.

Claims (11)

1. The application of the non-release type antimicrobial adhesive coating in the antibacterial packaging material comprises grafting the borneol acrylate and the polyethylene glycol diacrylate onto the surface of the packaging material in a mode that the photoinitiator generates surface free radicals to be copolymerized to form the non-release type antimicrobial adhesive coating, so as to obtain the packaging material with the non-release type antimicrobial adhesive coating; wherein, the polymer forming the non-release type antimicrobial adhesive coating is formed by copolymerizing two monomers of acrylic borneol ester and polyethylene glycol diacrylate, and the molecular structure is shown as the formula (I):
Figure FDA0003881094040000011
in the formula (I), n is the number of repeating units of the polymer and takes the value of a positive integer;
the packaging material is a food packaging material and comprises a food packaging film, a packaging bag or a packaging box, and the material of the packaging material comprises polyethylene, polypropylene, biaxially oriented polypropylene, polyvinyl chloride, EVA (ethylene vinyl acetate) plastics or PO (polyethylene oxide) plastics;
the non-releasing antimicrobial adhesion coating is capable of preventing fungal and bacterial adhesion; the molar ratio of the acrylic borneol ester to the polyethylene glycol diacrylate in the non-release antimicrobial adhesive coating is (0.3-3): 1; the mole fraction of the bornyl acrylate in the non-releasing antimicrobial adhesive coating is 0.25-0.75.
2. The use of claim 1, wherein the borneol acrylate is one or more of L-borneol acrylate, D-borneol acrylate and Iso-borneol acrylate; and/or the molecular weight of the polyethylene glycol diacrylate is 200-1000.
3. Use according to claim 1, wherein the photoinitiator comprises benzophenone and/or isopropylthioxanthone.
4. The use according to any one of claims 1-3, characterized in that the use comprises,
step C, dispersing a photoinitiator solution on the surface of the packaging material, and performing illumination, washing and drying in a nitrogen atmosphere to obtain the packaging material with the surface modified by the photoinitiator;
d, dispersing the mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer on the surface of the packaging material of which the surface is modified by the photoinitiator, and performing illumination, washing and drying in nitrogen atmosphere to prepare the packaging material of which the surface is provided with the non-release antimicrobial adhesive coating;
wherein the surface of the packaging material comprises an inner surface of the packaging material and an outer surface of the packaging material.
5. Use according to claim 4, wherein the surface of the packaging material is the outer surface of the packaging material.
6. The use according to claim 4, wherein the photoinitiator solution is obtained by dissolving a photoinitiator in acetone, vortexing, sonicating, and then deoxygenating by introducing nitrogen; the concentration of the photoinitiator solution is 0.1-0.5g/mL; the photoinitiator comprises benzophenone and/or isopropyl thioxanthone.
7. The use according to claim 4, wherein the mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer is obtained by dissolving the borneol acrylate monomer and the polyethylene glycol diacrylate monomer in acetone, performing vortex treatment and ultrasonic treatment, and then introducing nitrogen to remove oxygen; in the mixed solution of the borneol acrylate monomer and the polyethylene glycol diacrylate monomer, the molar ratio of the borneol acrylate to the polyethylene glycol diacrylate is (0.3-3) to 1; the concentration of the mixed solution of the acrylic borneol ester monomer and the polyethylene glycol diacrylate monomer is 50-80% (v/v).
8. The use according to claim 4,
the light source for illumination is a 200-1000W high-pressure mercury lamp, and the illumination time is 5-10min;
and/or, in step C, the washing comprises soaking with an ethanol solution at room temperature for 5-10h;
and/or, in the step D, the washing comprises soaking for 5-10 hours at room temperature by using dichloromethane and ethanol solution in sequence, and performing ultrasonic treatment for 20-30min after each soaking.
9. Use according to any one of claims 5 to 7,
the light source for illumination is a 200-1000W high-pressure mercury lamp, and the illumination time is 5-10min;
and/or, in step C, the washing comprises soaking with an ethanol solution at room temperature for 5-10h;
and/or, in the step D, the washing comprises soaking for 5-10 hours at room temperature by using dichloromethane and ethanol solution in sequence, and performing ultrasonic treatment for 20-30min after each soaking.
10. Use according to claim 4, wherein in step C the packaging material is a pre-treated packaging material; the pretreatment method of the packaging material comprises the steps of sequentially soaking in ethanol for 10 hours, carrying out ultrasonic treatment for 30min, then washing with ethanol, and carrying out vacuum drying.
11. Use according to any one of claims 5-8, characterized in that in step C the packaging material is a pre-treated packaging material; the pretreatment method of the packaging material comprises the steps of sequentially soaking in ethanol for 10 hours, carrying out ultrasonic treatment for 30min, then washing with ethanol, and carrying out vacuum drying.
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Citations (4)

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Publication number Priority date Publication date Assignee Title
US6358557B1 (en) * 1999-09-10 2002-03-19 Sts Biopolymers, Inc. Graft polymerization of substrate surfaces
CN103881010A (en) * 2014-03-07 2014-06-25 北京化工大学 Borneol-based macromolecule antibacterial material
CN109023923A (en) * 2018-07-09 2018-12-18 合肥洁诺医疗用品有限公司 It is a kind of to protect the preparation method for taking non-woven fabrics
CN109529128A (en) * 2018-11-30 2019-03-29 中国科学院长春应用化学研究所 A kind of anti-infective coating and preparation method thereof

Patent Citations (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US6358557B1 (en) * 1999-09-10 2002-03-19 Sts Biopolymers, Inc. Graft polymerization of substrate surfaces
CN103881010A (en) * 2014-03-07 2014-06-25 北京化工大学 Borneol-based macromolecule antibacterial material
CN109023923A (en) * 2018-07-09 2018-12-18 合肥洁诺医疗用品有限公司 It is a kind of to protect the preparation method for taking non-woven fabrics
CN109529128A (en) * 2018-11-30 2019-03-29 中国科学院长春应用化学研究所 A kind of anti-infective coating and preparation method thereof

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