WO2011044916A1 - Multipurpose eco-friendly disinfecting composition comprising nano size antibacterial agent - Google Patents

Multipurpose eco-friendly disinfecting composition comprising nano size antibacterial agent Download PDF

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Publication number
WO2011044916A1
WO2011044916A1 PCT/EG2009/000025 EG2009000025W WO2011044916A1 WO 2011044916 A1 WO2011044916 A1 WO 2011044916A1 EG 2009000025 W EG2009000025 W EG 2009000025W WO 2011044916 A1 WO2011044916 A1 WO 2011044916A1
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composition
disinfectant
sub
test
virus
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PCT/EG2009/000025
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French (fr)
Inventor
El Sayed Kamel Morsy Elbaialy
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El Sayed Kamel Morsy Elbaialy
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Priority to PCT/EG2009/000025 priority Critical patent/WO2011044916A1/en
Publication of WO2011044916A1 publication Critical patent/WO2011044916A1/en

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    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01NPRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
    • A01N59/00Biocides, pest repellants or attractants, or plant growth regulators containing elements or inorganic compounds
    • A01N59/12Iodine, e.g. iodophors; Compounds thereof
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01NPRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
    • A01N31/00Biocides, pest repellants or attractants, or plant growth regulators containing organic oxygen or sulfur compounds
    • A01N31/02Acyclic compounds
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01NPRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
    • A01N37/00Biocides, pest repellants or attractants, or plant growth regulators containing organic compounds containing a carbon atom having three bonds to hetero atoms with at the most two bonds to halogen, e.g. carboxylic acids
    • A01N37/16Biocides, pest repellants or attractants, or plant growth regulators containing organic compounds containing a carbon atom having three bonds to hetero atoms with at the most two bonds to halogen, e.g. carboxylic acids containing the group; Thio analogues thereof
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01NPRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
    • A01N37/00Biocides, pest repellants or attractants, or plant growth regulators containing organic compounds containing a carbon atom having three bonds to hetero atoms with at the most two bonds to halogen, e.g. carboxylic acids
    • A01N37/36Biocides, pest repellants or attractants, or plant growth regulators containing organic compounds containing a carbon atom having three bonds to hetero atoms with at the most two bonds to halogen, e.g. carboxylic acids containing at least one carboxylic group or a thio analogue, or a derivative thereof, and a singly bound oxygen or sulfur atom attached to the same carbon skeleton, this oxygen or sulfur atom not being a member of a carboxylic group or of a thio analogue, or of a derivative thereof, e.g. hydroxy-carboxylic acids
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01NPRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
    • A01N59/00Biocides, pest repellants or attractants, or plant growth regulators containing elements or inorganic compounds
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01NPRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
    • A01N59/00Biocides, pest repellants or attractants, or plant growth regulators containing elements or inorganic compounds
    • A01N59/16Heavy metals; Compounds thereof
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01NPRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
    • A01N65/00Biocides, pest repellants or attractants, or plant growth regulators containing material from algae, lichens, bryophyta, multi-cellular fungi or plants, or extracts thereof
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01NPRESERVATION OF BODIES OF HUMANS OR ANIMALS OR PLANTS OR PARTS THEREOF; BIOCIDES, e.g. AS DISINFECTANTS, AS PESTICIDES OR AS HERBICIDES; PEST REPELLANTS OR ATTRACTANTS; PLANT GROWTH REGULATORS
    • A01N65/00Biocides, pest repellants or attractants, or plant growth regulators containing material from algae, lichens, bryophyta, multi-cellular fungi or plants, or extracts thereof
    • A01N65/08Magnoliopsida [dicotyledons]
    • A01N65/36Rutaceae [Rue family], e.g. lime, orange, lemon, corktree or pricklyash

Definitions

  • Multipurpose Eco-friendly Disinfecting Composition comprising nano size antibacterial agent.
  • This present invention relates to disinfectants composition and more particularly to an environmentally friendly, non-toxic aqueous disinfectant for specific use against pathogenic bacteria and viruses. Also the invention is directed to a composition containing a hydrogen peroxide, nano antibacterial agent and a reduced amount of surfactant.
  • Hydrogen peroxide is a strong, environmentally friendly, disinfectant with a broad spectrum of antimicrobial activity that has been widely used in the healthcare field.
  • hydrogen peroxide is also a strong oxidizing agent that in high concentrations can damage tissue and damage surfaces such as foodstuff, making them more vulnerable to pathogenic penetration.
  • Essential oils are natural products known to have antimicrobial properties and disinfectant solutions based on essential oils have been formulated, U.S. Pat. No. 6,846,498. However, the potency and spectrum of action of many of these formulations lag behind those exhibited by other antimicrobials. Furthermore, formulations are difficult to make because the oils are not readily misciblc in water.
  • the present invention is directed to disinfectant compositions and their use.
  • the invention provides a disinfectant composition
  • a disinfectant composition comprising hydrogen peroxide (H.sub. 2 0.sub.2), aqueous solution of nano silver or nano gold or combination of nano silver and nano gold, quatemaiy ammonium salt, iodine source, orange terpene oil, pine oil, alcoholic mixture, citrate group, acetic acid or peracetic acid and wetting surfactant was presented.
  • the composition can include varied amounts of each of these ingredients.
  • the orange terpene oil is present in the composition from 5% to 40% v/v
  • the iodine source is present in the composition from 5% to 40% v/v
  • the wetting surfactant is present in the composition from 5% to 50% v/v
  • the distilled or deionized H.sub.20 is present in the composition from 5% to 80% v/v
  • the hydrogen peroxide is present in the composition from 1.5% to 8% Ii.sub.20. sub.2 w/v
  • the composition comprises one half as much wetting agent (e.g. polysorbate) by volume as the combined volume of orange terpene oil.
  • the disinfectant composition comprises 2.5% H.sub.20.sub.2 (15% of a 35% hydrogen peroxide solution), 10% v/v orange terpene oil, 0.05% of nano silver range of 3nm to 25nm particle size, 5% v/v polysorbate 80, 0.03%) v/v benzyl ammonium chloride and 60% v/v distilled water.
  • the disinfectant composition further comprises an antioxidant preservative of H.sub.20.sub.2 such as oil of rosemary.
  • the composition further comprises antimicrobials such as iodine compounds, potassium iodide, povodine iodine, and EDTA.
  • the disinfectant composition can also comprise surfactants, common builders that improve surfactant effectiveness, saponifiers, chelating agents, and/or other solvents.
  • the invention provides a method for disinfecting surfaces comprising applying the composition to the surface.
  • the invention further provides a method for reducing the number of mold spores on a surface.
  • the method comprises contacting the surface containing the mold spores with the composition.
  • the disinfectant described herein is composed of food grade material and comprises hydrogen peroxide (H.sub.20. sub.2), orange terpene oil, iodine source, nano silver, nano gold, or combination of nano silver and nano gold, quaternary ammonium salts, alcohols, citrate group, acetic acid, per acetic acid, a non-ionic emulsifier (e.g. polysorbate 80), and distilled or deionized water (H.sub.20).
  • hydrogen peroxide H.sub.20. sub.2
  • orange terpene oil iodine source
  • nano silver nano gold
  • nano gold or combination of nano silver and nano gold
  • quaternary ammonium salts quaternary ammonium salts
  • alcohols citrate group
  • acetic acid per acetic acid
  • a non-ionic emulsifier e.g. polysorbate 80
  • distilled or deionized water H.sub.20
  • the disinfectant is very potent and, as shown in Example 1 , highly effective at killing microorganisms including, but not limited to, bacteria (gram positive or gram negative), bacterial spores, molds, fungi and viruses such as Salmonella cholerasuis, Staphylococcus aureaus, Pseudomonas aeruginosa, Escherichia coli, Streptococcus pneumonia, and Listeria monocytogenes, Influenza virus, swine flue, and H1N1.
  • the disinfectant composition of the invention over other disinfectants is that it can be composed of entirely food grade materials while maintaining its high degree of potency against bacteria and other microorganisms.
  • the non-toxic components of the composition described herein work synergistically against microorganisms. Not to be bound by theory, it is believed that the orange oil together with the other components weakens the microorganisms (bacteria/fungus/mold spores/viruses) making them more venerable to the H. sub.20. sub.2.
  • the disinfectant composition further comprises oil of rosemary, e.g. CAS Number 8000-25-7.
  • any non-ionic emulsifier can be used in the disinfectant composition of the invention, including, but not limited to, alkyl polyethyleneoxy ethers, alkyl phenol polyethyleneoxy ethers, polyethyleneoxy amines, polyethyleneoxy fatty acids, and alkyl dimethyl amino oxides.
  • the composition comprising hydrogen peroxide (H. sub.20. sub.2), orange terpene oil, a non-ionic emulsifier, and distilled or deionized water (H.sub.20) does not comprise an anionic surfactant or an amphoteric surfactant.
  • the non-ionic emulsifier of the disinfectant composition is polysorbate 80 (CAS Number 9005-65-6).
  • the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5%> v/v orange terpene oil, 2.5% v/v of a 35% 0 wt. % hydrogen peroxide solution (equivalent to 3% of H. sub.20. sub.2), 10%o v/v isopropyl alcohol, 5% v/v ethyl alcohol 2.5%o v/v peracetic acid, 3% citric acid, and 0.5% nano silver of particle size 3nm.
  • the composition can be used at full strength or can be diluted with water. Dilutions can range from 1 : 1 to 1 : 10,000.
  • the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange terpene oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 10% v/v isopropyl alcohol, 5% v/v ethyl alcohol 2.5% v/v acetic acid, 3% citric acid, while the nano silver can be replaced by nano gold, or nano platinum, or nano rhodium, or nano iridium ,or nano palladium where all of the above nano metals have antibiotic, anti viral, antifungal action
  • the disinfectant composition can be formulated, if desired, as a gel, spray, foam, or paste, or as a disinfecting wipe, using standard formulations known in the art as appropriate.
  • the disinfectant composition can be made by mixing the components together using any known means.
  • the components are mixed together sequentially.
  • the components are added in sequence to distilled water in the following order: orange terpene oil, acetic acid, isopropyl alcohol, ethyl alcohol, then polysorbate 80, citric acid, then iodine source compound and finally nano silver solution.
  • hydrogen peroxide is then added and mixed for approximately 10 minutes.
  • the distilled water is kept between 90°C and 100°C to facilitate the emulsification process.
  • the components can be obtained from any source. Preferably food grade components are used.
  • the orange terpene oil can be obtained from Polarome International, Inc. (200 Theodore Conrad Drive, Jersey City, N.J. 07035) (Orange Terpenes, CAS Number 68647-72-3, EINECS Number 232-433-8; the polysorbate 80 can be obtained from Spectrum Chemicals (14422 South San Pedro Street, Gardena, Calif. 90248) and the hydrogen peroxide from Solvay Chemicals Inc. (1632 Haden Road, Houston, Tex. 77015) or from FMC corporation (1735 Market Street Philadelphia, Pa 19103), (Durox.RTM.35%).
  • composition described herein can include multiple surfactants, including, but not limited to nonionic surfactants such as nonylphenol ethoxylate, alcohol ethoxylates, octylphenol ethoxylate, coconut diethanolamide (cocoamide DEA), unspecified nonionic surfactant; anionic surfactants such as linear alkyl benzene sulfonate (dodecylbenzene sulfonate), alcohol sulfates (lauryl sulfates), alcohol ether sulfates (lauryl ether sulfates, laureth sulfates), sodium alkyl polyether sulfonate, alkyl polyglycosides, unspecified anionic surfactant, and soap; amphoteric surfactants such as, alkylbetaine, unspecified amphoteric surfactant; and cationic surfactants such as alkyl dimethyl benzyl ammonium chlorides, unspecified quaternary am
  • composition of the invention can further comprise common builders that improve surfactant effectiveness, saponifiers, chelating agents, and/or other solvents
  • additives include, but are not limited to, acetic acid, hydrochloric acid, citric acid, sodium hydroxide, potassium hydroxide, carbonates sodium carbonate, sodium bicarbonate, pyrophosphates, polyphosphates, phosphate esters, orthophosphates, sodium metasilicate, sodium silicate, ethanolamines, carbonates, silicates, EDTA, STPP, and zeolites/PCA, isopropanol, methanol, ethanol, 2-butoxyethanol, diethylene glycol ethyl ether, diethylene glycol, monomethylether, l-methoxy-2-propanol, 2-2- butoxyethyoxyethanol, d-limonene, pine oil, tall oil, ammonia (ammonium hydroxide), hydrocarbons, propylene glycol, ethylene glycol, or 1,3-proponed
  • quaternary ammonium compounds include, but are not limited to alkyl dimethyl benzyl ammonium chlorides, unspecified quaternary ammonium chlorides or compounds, alkylaryl dimethyl ammonium chloride, dimethyl ethyl benzyl ammonium chloride, ethylbenzene ammonium chloride, didecyl dimethyl ammonium chloride, and octyl dimethyl ammonium chloride.
  • the quaternary ammonium compound is present in the composition at 0.01-1%.
  • Example phenols include, but are not limited to ortho-benzyl parachlorophenol, ortho-phcnylphenol, and para-tertiary-amylphenol.
  • the phenol is present in the composition at 2- 5%.
  • Example alcohols include but are not limited to Isopropyl alcohol and ethanol.
  • sodium hypochlorite is present in the composition from 0.5-5%.
  • antimicrobial agents include, but are not limited to, triclosan, cetyl pyridium chloride, domiphen bromide, zinc compounds, sanguinanine soluble pyrophosphates, fluorides, alexidine, octonidine, EDTA, and the like.
  • the non-toxic nature of the disinfectant described herein allows for its use not only in applications where the harshness of the disinfectant is irrelevant, but also in applications more sensitive in nature, for example when disinfecting skin, treating plants and food stuff, and killing oral microorganisms.
  • the disinfectant described herein is used to sanitize porous or non-porous surfaces. Any surface can be cleaned using the disinfectant of the invention including, but not limited to, leather, wood, metal, plastic, synthetics, and fabrics.
  • the composition of the invention can disinfect surfaces containing bacteria, bacterial spore's fungus, and/or viruses (DNA or RNA viruses).
  • compositions can be used to inactivate vegetative bacteria and bacterial spores upon contact.
  • Bacteria that can be inactivated by the compositions can be gram negative or gram positive bacteria
  • compositions can be used to inactivate bacillus, including, without limitation B. anthracis, B. cereus, B. circulans, B. subtilis, and B. megaterium.
  • Compositions of the invention can also be used to inactivate Clostridium, e. g., C. botulinum, C. perfringens, and C. tetani.
  • Other bacteria that can be inactivated by the composition include, but are not limited to, H. influenzae, N. gonorrhoeae, S. agalactiae, S. pneumonia, and S. pyogenes and V. cholerae.
  • Contacting a virus with the composition of the invention can inactivate a virus.
  • compositions on viral agents can be monitored using any suitable means, such as, for example, plaque reduction assay (PRA), cellular enzyme-linked immunosorbent assay (ELISA), P-galactosidase assay, and electron microscopy (EM).
  • PRA plaque reduction assay
  • ELISA cellular enzyme-linked immunosorbent assay
  • EM electron microscopy
  • Viruses which can be inactivated by contact with the composition include, without limitation, virus of the families Baculoviridae, Herpesviridae, Iridoviridae, Poxviridae, "African Swine Fever Viruses," Adenoviridae, Caulimoviridae, Myoviridae, Phycodnaviridae, Tectiviridae, Papovaviridae, Circoviridae, Parvoviridae, Hepadnaviridae, Cystoviridae, Bimaviridae, Reoviridae, Coronaviridae, Flaviviridae, Togaviridae, "Arteri virus,” Astroviridae, Caliciviridae, Picomaviridae, Potyviridae, Retroviridae, Orthomyxoviridae, Filoviridae, Paramyxoviridae, Rhabdoviridae, Arenaviridae, and Bunyaviridae
  • the virus is herpes, pox, papilloma, corona, influenza, hepatitis, Sendai, Sindbis and vaccinia viruses, West Nile, hanta, and viruses which cause the common cold.
  • contacting a fungus with the composition of the invention inactivates the fungus.
  • the fungus is a yeast, such as, for example various species of Candida (e.
  • Candida albicans or filamentous yeast including but not limited to Aspergillus species or dermatophytes such as Trichophyton ubrura, Trichophyton mentagrophytes, Microsporam canis, Microsporum -gypseux, and Epiderophytonfloccosum, and types thereof, as well as others.
  • composition of the invention can also be used for mold remediation for building, equipment, and facilities.
  • molds include, but are not limited to Cladosporium, Fusarium, Alternaria, Curvularia, Aspergillus, and Penicillium.
  • the disinfectant described herein can also be used as an aerosol or spray to eliminate odors, e.g. as a room or fabric deodorizer.
  • the disinfectant described herein is used as a mouthwash to eliminate bad breath and to reduce the presence of oral microorganisms.
  • additional conventional components may be added to the disinfectant of the invention as in mouthwashes of the prior art.
  • softeners such as glycerin may be added to enhance the lubricous mouth feel of the mouthwash as it is used and to provide a refreshing, moist, organoleptic feeling thereafter.
  • Glycerin may be incorporated in amounts of from about 0.05% w/v to about 10.0% w/v, and preferably in an amount of about 5% w/v.
  • Sweeteners such as aspartame or sodium saccharin and the like may be added for better taste in amounts of from about 0.005% w/v to about 1.0% w/v, and preferably in an amount of approximately 0.05% w/v.
  • Other essential oils can be added to alter the flavor.
  • Zinc chloride or other zinc salts e.g. zinc gluconate, zinc sulfate etc., may be added as an astringent for an "antiseptic cleaning" feeling in an amount of from about 0.0025% w/v to about 0.200% w/v.
  • the disinfectant described herein is used in medical applications, such as to clean skin wounds, or skin surfaces.
  • the disinfectant can also be used as a hand sanitizer.
  • the disinfectant is very potent and highly effective at killing microorganisms including, but not limited, to Salmonella cholerasuis, Staphylococcus aureaus, Pseudomonas aeruginosa, Escherichia coli, Streptococcus pneumonia, Listeria monocytogenes and influenza.
  • the disinfectant described herein is used as germicidal for disinfecting/cleaning foodstuff or plant matter.
  • Hydrogen peroxide solutions have also been found to be effective at inhibiting sprouting and rooting of foodstuffs, such as potatoes or other vegetables, thereby extending the shelf life of perishable food stuffs and plant matter.
  • the disinfectant composition can be sprayed directly on plant matter or mixed with soil to discourage infestation with parasitic organisms.
  • the composition is used in the food industry in preventing and treating food contaminated with pathogens.
  • such compositions may be used to reduce or inhibit microbial growth or otherwise abrogate the deleterious effects of microbial contamination of food.
  • the composition can be used to kill bacteria and fungus on poultry eggs, fruit, vegetables, and meat.
  • the inclusion of the compositions of the invention within the food product itself would be effective in killing bacteria that may have been accidentally contaminated meat or poultry.
  • the composition can be included in juice products to prevent growth of certain fungi, which cause contamination and lead to production of mycotoxins.
  • the compositions are applied in food industry acceptable forms such as washes, dips, additives, preservatives, or seasonings.
  • the disinfectant is loaded onto a cleaning wipe.
  • the cleaning wipe upon which the disinfectant composition is loaded thereon, is made of an absorbent/adsorbent material.
  • the cleaning wipe has at least one layer of nonwoven material.
  • Nonlimiting examples of commercially available cleaning wipes that can be used include DuPont 8838, Dexter Z A, Dexter 10180, Dexter M10201, Dexter 8589, Ft. James 836, and Concert STD60LN, and Ahlstrom 4759. All of these cleaning wipes include a blend of polyester and wood pulp.
  • Dexter Ml 0201 also includes rayon, a wood pulp derivative.
  • the loading ratio of the cleaning composition onto the cleaning wipe is about 2-5: 1, and typically about 3-4: 1.
  • the disinfectant composition is loaded onto the cleaning wipe in any number of manufacturing methods. Typically, the cleaning wipe is soaked in the disinfectant composition for a period of time until the desired amount of loading is achieved.
  • the disinfectant composition is packaged in a pressurized gas aerosol can.
  • Common aerosol propellants include butane, isobutene, liquefied natural gas, and propane.
  • the invention provides methods for disinfecting surfaces to inactivate pathogenic organisms comprising contacting a surface with the disinfectant composition of the invention.
  • the step of contacting can involve contacting any substrate, which may be or is suspected to be contaminated, with the composition of the invention.
  • substrate it is meant, without limitation any subject, such as a human or an animal (contact can be in vivo or ex vivo, any article, any surface, or any enclosure.
  • a pathogenic microorganism can be, without limitation, bacteria, a virus, a fungus, a protozoan or a combination thereof.
  • the step of contacting can be performed for any amount of time sufficient to inactivate a microorganism.
  • inactivation occurs within about 5 minutes to about 10 minutes after initial contact.
  • the inactivation may occur over a longer period of time, for example, 5, 10, 15, 20, 25, 30, 60 minutes or longer after administration.
  • compositions can be administered by spraying, fogging, misting, exposure to aerosols, wiping with a wet or saturated cloth or toilette, drenching, immersing.
  • the invention further provides a method for reducing the number of mold spores on a surface.
  • the method comprises contacting the mold spores with the composition comprising hydrogen peroxide (H. sub.20. sub.2), orange terpene oil, iodine source compound, nano silver, citric acid, acetic acid, isopropanol, ethyl alcohol , a non-ionic emulsifier (e.g. polysorbate 80), and distilled or deionized water (H. sub.20).
  • Any mold can be treated using methods of the invention.
  • the germicidal spray composition comprising
  • the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5%> v/v orange oil, 5% v/v of a 35% > wt. % hydrogen peroxide solution (equivalent to 5.35%) of H.sub.20.sub.2), 20% > v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0.05% > pevodine iodine and 1.5% nano silver of particle size 15nm.
  • the analysis was performed per "Germicidal Spray Test", AO AC 17.sup.th edition, 6.3.03, versus Salmonella cholerasuis ATCC 10708, Staphylococcus aureaus ATCC 6538, Pseudomonas aeruginosa ATCC 15442, Escherichia coli ATCC 8739, Streptococcus pneumonia ATCC 49619, and Listeria monocytogenes ATCC 19113. Testing was performed as required by the EPA FIFRA.
  • the AO AC procedure used in this study is a widely known and accepted method for disinfectant evaluation.
  • Microorganisms were grown for 48 h in nutrient broth. Glass slides were then inoculated with the grown culture and the inoculated slides were subsequently exposed to the germicidal spray for 10 minutes (60 microorganism inoculated slides/lot/microorganism were tested). After exposure to the disinfectant, slides were used as inoculates in leethen media and microorganism growth determined. Positive, negative and inhibition controls were performed.
  • Controls included uninoculated containers of leethen broth (media controls) and sterile uninoculated glass slides (negative control), there was no growth; Glass slides inoculated with organism and a sterile glass slide immersed in test disinfectant (inhibition control), there was no growth which indicates that the letheen broth neutralizes the disinfectant; Glass slide inoculated with organism (viability control), there was growth; and Glass slide inoculated with organism (enumerated), >10.sup.6 cfu.
  • the germicidal spray composition comprising
  • the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 20% v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0,05% pevodine iodine and 1.5% nano silver of particle size 15nm. was tested for toxicity according to protocol number X5D050G, which incorporates by reference Northview Standard Operating Procedure 16D-05 and is on file in Northview Pacific Laboratories, Inc. No amendments were made to the protocol.
  • a limit screen test was performed using three female Sprague-Dawley rats, which received an oral limit Dose of 50000 mg/kg of the test article. The animals were observed for mortality, weight change and toxic signs for a two week period. Animals were observed daily and weighed on days 7 and 14.
  • test article was 1 g/ml and shaken before use. Dosing procedure. The dose was administered by means of a gavage needle attached to a hypodermic syringe. The test animals received a 5 mL/kg solution containing the test article. Three rats were dosed on the first day of dosing. Because all three rats survived no further testing was required.
  • the germicidal spray composition comprising hi one embodiment, the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 20% v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0.05% pevodine iodine and 1.5% nano silver of particle size 15nm.
  • the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 20% v/v isopropyl alcohol, 25% v/v
  • the eyes were examined and graded for ocular reaction at 1, 24, 48, and 72 hours after application of the test substance for corneal ulceration or opacity, inflammation of the iris, or redness and chemosis of the conjunctivae.
  • the results are interpreted according to the Kay and Calandra Method (Kay J. H. & Calandra, J. C, "Interpretation of eye irritation tests", Journal of society of cosmetic chemists, 13:281- 289, 1962).
  • test article was determined to be moderately irritating to eyes of New Zeland Rabbits. All animals remained healthy throughout the study period. There was significant irritation in all 3 animals beginning at the 1 hour scoring and continuing through the 96 hour scoring. The scores all went back to "0", normal scoring, by the 7-day scoring.
  • the germicidal spray composition comprising
  • the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 20% v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0,05% pevodine iodine and 1.5% nano silver of particle size 15nm. was tested for toxicity according to protocol number X5D052G, which incorporates by reference Northview Standard Operating Procedure 16D-07 and is on file in Northview Pacific Laboratories, Inc. No amendments were made to the protocol.
  • the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 20% v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0.05% pevodine iodine and 1.5% nano silver of particle size 15nm. Was tested for virucidal efficacy. MICROBIOTEST INC.
  • the microbiology and virology laboratory 105 Carpenter Drive, Sterling, Va. 20164 performed the tests from Feb. 10, 2005 to Feb. 18, 2005 and all raw data, protocol, protocol modifications, test material records, and the final report, are stored in the archives at MICROBIOTEST INC. (105 Carpenter Drive, Sterling, Va. 20164) or at a controlled facility offsite.
  • the Virucidal Efficacy test was performed as detailed in the following protocol from MICROBIOTEST INC.:
  • Test conditions'. Challenge virus Avian Influenza A virus, Turkey /Wis/66 strain (H9N2), Charles River Laboratories; Host: Embryonated chicken eggs, B&E Eggs; Active ingredient in test product: Hydrogen peroxide; Neutralizer used: Earle's Balanced Salt Solution containing 0.3% Thioglycolic acid and 0.1% Catalase; Contact time: 10 minutes; Contact temperature: Ambient room temperature (22. degree.
  • the test is designed to substantiate virucidal effectiveness claims for a product to be labeled as a virucide. It determines the potential of the test agent to disinfect hard surfaces contaminated with viruses.
  • the test is designed to stimulate consumer use and conforms to EPA Guidelines DIS/TSS-7, November 1981, and follows the procedure outlined in the American Society for Test Materials (ASTM) test method designated E 1053-97.
  • Virus will be dried on a sterile glass Petri dish at ambient temperature. Test agents specified by the sponsor in the miscellaneous section of the protocol will be used to treat the dried virus according to the label claims. After a defined exposure period, the neutralized test agent-virus mixture will be scraped from the surface, neutralized and assayed for the presence of infectious virus.
  • Test, control and reference substances will be supplied by the sponsor of the study.
  • the test agent will be tested as supplied by the sponsor unless directed otherwise. All operations performed on the test agent such as dilution or specialized storage conditions must be specified by the sponsor before initiation of testing.
  • the sponsor assures MICROBIOTEST testing facility management that the test agent has been appropriately tested for identity, strength, purity, stability, and uniformity as applicable. MICROBIOTEST will retain all unused test agents for a period of at least three months after completion of the test, then return them to the sponsor of the study or discard them in a manner that meets the approval of the safety officer.
  • MICROBIOTEST Materials supplied by MICROBIOTEST, including, but not limited to: 1) Challenge virus (requested by the sponsor of the study): Avian Influenza virus. 2) Host: Embryonated chicken eggs. 3) Laboratory equipment and supplies. 4) Media and reagents: Media and reagents relevant to the vims-host system and test agent being tested will be documented in the first project sheet and/or the data pack.
  • Test system identification All Petri dishes, dilution tube racks, and host-containing apparatus will be labeled with virus identification and project number.
  • Experimental design Procedures involved in performance of virucidal studies are described a series of SOPs and logs that are maintained at MICROBIOTEST. The procedures used in different phases of the study will be documented in the data pack.
  • Inoculum preparation Viral stocks are purchased from reputable sources that identify them by scientifically accepted methods and are propagated at MICROBIOTEST. Records are maintained that demonstrate the origin of the virus. The virus stocks are stored at an ultra-low temperature. Frozen viral stocks will be thawed on the day of the test (fresh stock cultures may be used at the discretion of the Study Director).
  • Carrier preparation An aliquot of 0.2 mL of stock virus will be spread, with a cell scraper, over an area of approximately 4 in. sup.2 that has been marked on the underside of pre-sterilized Petri dishes. The virus will be allowed to dry for 30 to 60 minutes at room temperature. The drying time and temperature will be recorded. One carrier will be prepared for each test agent and the plate recovery control. One plate will be prepared for the neutralizer effectiveness control using an appropriate medium.
  • Test agent preparation The agent will be prepared according to the sponsor's directions or proposed label claims.
  • test agent After the carrier(s) are properly prepared, 2.0 mL of the test agent will be added. The plates will remain at the temperature and for the time specified by the sponsor. Following the contact period, the test agent will be neutralized with 2.0 mL of the appropriate neutralizing solution and the mixture will be scraped from the surface of the dish with a cell scraper. This will be considered approximately a one log.sub.10 dilution. If columns are used, each sample will be loaded into separate pre-spun Sephacryl columns. Following passage through columns, the eluate will be removed aseptically and serially diluted. If columns are not used, serial dilutions of neutralized virus-test agent mixture will be prepared in using an appropriate diluent.
  • the agent will be used as the sponsor directs, the volume dispensed will be measured and an equal volume of neutralizer will be used. Following the contact time, the procedure for processing the samples will be the same as described earlier.
  • Viral host culture Two-tenths mL of selected dilutions of the neutralized inoculum/disinfectant mixture will be inoculated intra-allantoically in embryonic eggs and incubated for 5-7 days at 37.+-.2C. Four determinations will be recorded for each dilution of both tests and controls. The eggs will be candled one-day post-inoculation of test and control samples. All dead embryos will be discarded and the data will be recorded.
  • the eggs will be candled and then kept at 2.+-.2C overnight. Afterwards, the allantoic fluid will be harvested and kept at 2.+-.2C until assay. The samples will be assayed for the presence of replicating virus using hemagglutination assay following SOP 1006.1 1 (current version) and the results will be recorded.
  • Neutralizer effectiveness This control will determine if residual active ingredient is present after neutralization. One lot of the test agent will be used for the neutralizer effectiveness control. This control will be processed exactly as the test procedure but instead of viral inoculum, appropriate media will be added. Post neutralization, a 1.0-mL sample will be divided into three portions, using two for toxicity-related controls and the other for neutralizer effectiveness. A 0.5 mL sample will be serially diluted, after which 100 .mu.L of diluted virus will be added to each dilution and held for a period greater than or equal to the contact time. Then these samples will be used to inoculate host embryos as described for the test procedure.
  • Toxicity The toxicity sample, acquired from the neutralizer effectiveness control, will be diluted and have no virus added. Selected dilutions will be inoculated into the host and incubated in the same manner as the rest of the test and control samples. These effects are distinct from virus-specific cytopathic effects, which will be evident in the stock titer and plate recovery control cultures.
  • Toxicity-related viral interference control The test agent may not be effective against the challenge virus yet be toxic to the host employed to detect its infectivity and may inhibit accurate interpretation of the test. To determine the possibility of such interference by residual toxic molecules, host treated with serially diluted neutralized test agent will be infected with a known number of infectious virions. Post-incubation they will be scored and compared with non-treated infected host cells control. This will rule out any possibility of toxicity-related viral interference remaining in the neutralized test agent post-contact time.
  • Plate recovery The carrier used will be prepared as the test. A volume of an appropriate media equivalent to that of the test agent will be added to the dried virus. Post contact time this sample will be treated as the test. This control will determine the relative loss in vims infectivity resulting from drying and neutralization alone. The results from this control will be compared with the test results to confirm recovery of at least four log.sub.lO of infectious virus following drying and neutralization. This titer will be compared with the titers of the test results to reach the acceptable test criteria. When samples are required to pass through the Sephacryl columns, a column titer control (CTC) will be performed by assaying a portion of PRC before passing through the columns to determine the effect on infectious virus titer after passage through the columns.
  • CTC column titer control
  • CTC Column titer control
  • VST Virus stock titer
  • Test agent passes the test if there is complete inactivation of the virus at all dilutions. When toxicity is evident, at least a three-log reduction in titer must be demonstrated beyond the toxic level.
  • Test acceptance criteria The test will be acceptable for evaluation of the test results if the criteria listed below are satisfied. The study director may consider other causes that may affect test reliability and acceptance; a) the infectious virus recovered from the PRC control must be .gtoreq.4-log.sub.10. b) Viral-induced toxicity must be distinguishable from test agent induced toxic effects.
  • Avian Influenza virus was exposed to the germicidal spray composition for 10 minutes at ambient room temperature (22. degree. C). the germicidal spray inactivated Avian Influenza vims, as no virus was detected after exposure. All controls met the criteria for a valid test. Virus was not recovered in the host viability control confirming media sterility and host viability.

Abstract

Non-toxic environmentally friendly, healthily safe, a highly potent aqueous disinfectant is disclosed for specific use as prevention against contamination by potentially pathogenic bacteria and virus. Applications of the disinfectant include, but are not limited to, uses as a mouthwash, skin cleanser, or as a germicidal for disinfecting surfaces such as foodstuff, plant matter, leather, wood, metal, plastic, fabrics, and medical surgical masks. Also the disinfectant formulation could be applied for human skin care as disinfecting gel. Methods for using the disinfectant composition of the invention are also provided. The disinfectant comprises hydrogen peroxide, nano silver, nano gold, orange terpene oil, pine oil, quaternary ammonium salts, iodine source, alcoholic mixture, citrate group, and wetting surfactant. The aqueous disinfectant has been shown to be very effective at eliminating standard indicator organisms such as staphylococcus aureus, salmonella cholerasuis, pseudomonas aeruginosa, swine flue, HlNl virus. The product of the invention is completely natural and non-toxic to adults and children even if swallowed. The inventive compositions also optionally comprise additional ingredients, and are therefore suitable for a wide variety of personal, home and industrial care purposes.

Description

Multipurpose Eco-friendly Disinfecting Composition comprising nano size antibacterial agent.
TECHNICAL FILED:
This present invention relates to disinfectants composition and more particularly to an environmentally friendly, non-toxic aqueous disinfectant for specific use against pathogenic bacteria and viruses. Also the invention is directed to a composition containing a hydrogen peroxide, nano antibacterial agent and a reduced amount of surfactant.
BACKGROUND OF THE ART :
A number of products have been developed for the purpose of disinfecting and cleaning. However, most of these products contain toxic, poisonous ingredients that are detrimental to the environment and to the human health.
Hydrogen peroxide is a strong, environmentally friendly, disinfectant with a broad spectrum of antimicrobial activity that has been widely used in the healthcare field. Unfortunately, hydrogen peroxide is also a strong oxidizing agent that in high concentrations can damage tissue and damage surfaces such as foodstuff, making them more vulnerable to pathogenic penetration.
Essential oils, are natural products known to have antimicrobial properties and disinfectant solutions based on essential oils have been formulated, U.S. Pat. No. 6,846,498. However, the potency and spectrum of action of many of these formulations lag behind those exhibited by other antimicrobials. Furthermore, formulations are difficult to make because the oils are not readily misciblc in water.
DISCLOSURE OF THE INVENTION :
The present invention is directed to disinfectant compositions and their use.
The invention provides a disinfectant composition comprising hydrogen peroxide (H.sub.20.sub.2), aqueous solution of nano silver or nano gold or combination of nano silver and nano gold, quatemaiy ammonium salt, iodine source, orange terpene oil, pine oil, alcoholic mixture, citrate group, acetic acid or peracetic acid and wetting surfactant was presented. The composition can include varied amounts of each of these ingredients. In one embodiment, the orange terpene oil is present in the composition from 5% to 40% v/v, the iodine source is present in the composition from 5% to 40% v/v, the wetting surfactant is present in the composition from 5% to 50% v/v, the distilled or deionized H.sub.20 is present in the composition from 5% to 80% v/v and the hydrogen peroxide is present in the composition from 1.5% to 8% Ii.sub.20. sub.2 w/v hi another embodiment, the composition comprises one half as much wetting agent (e.g. polysorbate) by volume as the combined volume of orange terpene oil. In one preferred embodiment the disinfectant composition comprises 2.5% H.sub.20.sub.2 (15% of a 35% hydrogen peroxide solution), 10% v/v orange terpene oil, 0.05% of nano silver range of 3nm to 25nm particle size, 5% v/v polysorbate 80, 0.03%) v/v benzyl ammonium chloride and 60% v/v distilled water.
In one embodiment, the disinfectant composition further comprises an antioxidant preservative of H.sub.20.sub.2 such as oil of rosemary.
In one embodiment, the composition further comprises antimicrobials such as iodine compounds, potassium iodide, povodine iodine, and EDTA. In addition, the disinfectant composition can also comprise surfactants, common builders that improve surfactant effectiveness, saponifiers, chelating agents, and/or other solvents. The invention provides a method for disinfecting surfaces comprising applying the composition to the surface.
The invention further provides a method for reducing the number of mold spores on a surface. The method comprises contacting the surface containing the mold spores with the composition.
Detailed Description .'
A highly potent non-toxic, environmentally friendly, disinfectant that can be used for a wide breadth of applications was discovered by our company R&D sector. The disinfectant described herein is composed of food grade material and comprises hydrogen peroxide (H.sub.20. sub.2), orange terpene oil, iodine source, nano silver, nano gold, or combination of nano silver and nano gold, quaternary ammonium salts, alcohols, citrate group, acetic acid, per acetic acid, a non-ionic emulsifier (e.g. polysorbate 80), and distilled or deionized water (H.sub.20). The disinfectant is very potent and, as shown in Example 1 , highly effective at killing microorganisms including, but not limited to, bacteria (gram positive or gram negative), bacterial spores, molds, fungi and viruses such as Salmonella cholerasuis, Staphylococcus aureaus, Pseudomonas aeruginosa, Escherichia coli, Streptococcus pneumonia, and Listeria monocytogenes, Influenza virus, swine flue, and H1N1.
An advantage of the disinfectant composition of the invention over other disinfectants is that it can be composed of entirely food grade materials while maintaining its high degree of potency against bacteria and other microorganisms. The non-toxic components of the composition described herein work synergistically against microorganisms. Not to be bound by theory, it is believed that the orange oil together with the other components weakens the microorganisms (bacteria/fungus/mold spores/viruses) making them more venerable to the H. sub.20. sub.2. In one embodiment, the disinfectant composition further comprises oil of rosemary, e.g. CAS Number 8000-25-7.
Any non-ionic emulsifier can be used in the disinfectant composition of the invention, including, but not limited to, alkyl polyethyleneoxy ethers, alkyl phenol polyethyleneoxy ethers, polyethyleneoxy amines, polyethyleneoxy fatty acids, and alkyl dimethyl amino oxides. In another embodiment, the composition comprising hydrogen peroxide (H. sub.20. sub.2), orange terpene oil, a non-ionic emulsifier, and distilled or deionized water (H.sub.20) does not comprise an anionic surfactant or an amphoteric surfactant.
In one embodiment, the non-ionic emulsifier of the disinfectant composition is polysorbate 80 (CAS Number 9005-65-6).
In one embodiment, the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5%> v/v orange terpene oil, 2.5% v/v of a 35%0 wt. % hydrogen peroxide solution (equivalent to 3% of H. sub.20. sub.2), 10%o v/v isopropyl alcohol, 5% v/v ethyl alcohol 2.5%o v/v peracetic acid, 3% citric acid, and 0.5% nano silver of particle size 3nm. The composition can be used at full strength or can be diluted with water. Dilutions can range from 1 : 1 to 1 : 10,000.
In one embodiment, the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange terpene oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 10% v/v isopropyl alcohol, 5% v/v ethyl alcohol 2.5% v/v acetic acid, 3% citric acid, while the nano silver can be replaced by nano gold, or nano platinum, or nano rhodium, or nano iridium ,or nano palladium where all of the above nano metals have antibiotic, anti viral, antifungal action The disinfectant composition can be formulated, if desired, as a gel, spray, foam, or paste, or as a disinfecting wipe, using standard formulations known in the art as appropriate.
The disinfectant composition can be made by mixing the components together using any known means. Preferably the components are mixed together sequentially. For example, the components are added in sequence to distilled water in the following order: orange terpene oil, acetic acid, isopropyl alcohol, ethyl alcohol, then polysorbate 80, citric acid, then iodine source compound and finally nano silver solution. While being mixed at moderate speed, hydrogen peroxide is then added and mixed for approximately 10 minutes. In one preferred embodiment, the distilled water is kept between 90°C and 100°C to facilitate the emulsification process.
The components can be obtained from any source. Preferably food grade components are used. As an example source, the orange terpene oil can be obtained from Polarome International, Inc. (200 Theodore Conrad Drive, Jersey City, N.J. 07035) (Orange Terpenes, CAS Number 68647-72-3, EINECS Number 232-433-8; the polysorbate 80 can be obtained from Spectrum Chemicals (14422 South San Pedro Street, Gardena, Calif. 90248) and the hydrogen peroxide from Solvay Chemicals Inc. (1632 Haden Road, Houston, Tex. 77015) or from FMC corporation (1735 Market Street Philadelphia, Pa 19103), (Durox.RTM.35%).
While it is preferable to use only food grade components in the composition, other non-food grade components can also be added.
The composition described herein can include multiple surfactants, including, but not limited to nonionic surfactants such as nonylphenol ethoxylate, alcohol ethoxylates, octylphenol ethoxylate, coconut diethanolamide (cocoamide DEA), unspecified nonionic surfactant; anionic surfactants such as linear alkyl benzene sulfonate (dodecylbenzene sulfonate), alcohol sulfates (lauryl sulfates), alcohol ether sulfates (lauryl ether sulfates, laureth sulfates), sodium alkyl polyether sulfonate, alkyl polyglycosides, unspecified anionic surfactant, and soap; amphoteric surfactants such as, alkylbetaine, unspecified amphoteric surfactant; and cationic surfactants such as alkyl dimethyl benzyl ammonium chlorides, unspecified quaternary ammonium chlorides or compounds, alkylaryl dimethyl ammonium chloride, dimethyl ethyl benzyl ammonium chloride, ethylbenzene ammonium chloride, didecyl dimethyl ammonium chloride, octyl dimethyl ammonium chloride. The composition of the invention can further comprise common builders that improve surfactant effectiveness, saponifiers, chelating agents, and/or other solvents, examples of such additives include, but are not limited to, acetic acid, hydrochloric acid, citric acid, sodium hydroxide, potassium hydroxide, carbonates sodium carbonate, sodium bicarbonate, pyrophosphates, polyphosphates, phosphate esters, orthophosphates, sodium metasilicate, sodium silicate, ethanolamines, carbonates, silicates, EDTA, STPP, and zeolites/PCA, isopropanol, methanol, ethanol, 2-butoxyethanol, diethylene glycol ethyl ether, diethylene glycol, monomethylether, l-methoxy-2-propanol, 2-2- butoxyethyoxyethanol, d-limonene, pine oil, tall oil, ammonia (ammonium hydroxide), hydrocarbons, propylene glycol, ethylene glycol, or 1,3-proponediol.
Although not necessary, it is possible to employ other antimicrobial agents in the composition of this invention, for example quaternary ammonium compounds, phenols, alcohols, sodium hypochlorite, pine oil or other known antimicrobial oils. Examples of quaternary ammonium compounds include, but are not limited to alkyl dimethyl benzyl ammonium chlorides, unspecified quaternary ammonium chlorides or compounds, alkylaryl dimethyl ammonium chloride, dimethyl ethyl benzyl ammonium chloride, ethylbenzene ammonium chloride, didecyl dimethyl ammonium chloride, and octyl dimethyl ammonium chloride. Preferably the quaternary ammonium compound is present in the composition at 0.01-1%. Example phenols include, but are not limited to ortho-benzyl parachlorophenol, ortho-phcnylphenol, and para-tertiary-amylphenol. Preferably the phenol is present in the composition at 2- 5%. Example alcohols include but are not limited to Isopropyl alcohol and ethanol. Preferably, sodium hypochlorite is present in the composition from 0.5-5%. Other exemplary antimicrobial agents include, but are not limited to, triclosan, cetyl pyridium chloride, domiphen bromide, zinc compounds, sanguinanine soluble pyrophosphates, fluorides, alexidine, octonidine, EDTA, and the like.
The non-toxic nature of the disinfectant described herein allows for its use not only in applications where the harshness of the disinfectant is irrelevant, but also in applications more sensitive in nature, for example when disinfecting skin, treating plants and food stuff, and killing oral microorganisms.
In one embodiment, the disinfectant described herein is used to sanitize porous or non-porous surfaces. Any surface can be cleaned using the disinfectant of the invention including, but not limited to, leather, wood, metal, plastic, synthetics, and fabrics. The composition of the invention can disinfect surfaces containing bacteria, bacterial spore's fungus, and/or viruses (DNA or RNA viruses).
The compositions can be used to inactivate vegetative bacteria and bacterial spores upon contact. Bacteria that can be inactivated by the compositions can be gram negative or gram positive bacteria, gram negative bacteria include, for example and without limitation, Vibrio, Salmonella, Shigella, pseudomonas, Escherichia, Klebsiella, Proteus, Enterobacter, Serratia, Moraxella, Legionella, Bordetella, Gardnerella, Haemophilus, Neisseria, Brucella, Yersinia, Pasteurella, Bacteroids, and Helicobacter gram positive bacteria include, for example, and without limitation, Bacillus, Clostridium, Arthrobacter, Micrococcus, Staphylococcus, Streptococcus, Listeria, Corynebacteria, Planococcus, Mycobacterium, Nocardia, Rhodococcus, Andacidfast bacilli such as Mycobacterium. In one embodiment the compositions can be used to inactivate bacillus, including, without limitation B. anthracis, B. cereus, B. circulans, B. subtilis, and B. megaterium. Compositions of the invention can also be used to inactivate Clostridium, e. g., C. botulinum, C. perfringens, and C. tetani. Other bacteria that can be inactivated by the composition include, but are not limited to, H. influenzae, N. gonorrhoeae, S. agalactiae, S. pneumonia, and S. pyogenes and V. cholerae.
Contacting a virus with the composition of the invention can inactivate a virus.
The effect of compositions on viral agents can be monitored using any suitable means, such as, for example, plaque reduction assay (PRA), cellular enzyme-linked immunosorbent assay (ELISA), P-galactosidase assay, and electron microscopy (EM). Viruses which can be inactivated by contact with the composition include, without limitation, virus of the families Baculoviridae, Herpesviridae, Iridoviridae, Poxviridae, "African Swine Fever Viruses," Adenoviridae, Caulimoviridae, Myoviridae, Phycodnaviridae, Tectiviridae, Papovaviridae, Circoviridae, Parvoviridae, Hepadnaviridae, Cystoviridae, Bimaviridae, Reoviridae, Coronaviridae, Flaviviridae, Togaviridae, "Arteri virus," Astroviridae, Caliciviridae, Picomaviridae, Potyviridae, Retroviridae, Orthomyxoviridae, Filoviridae, Paramyxoviridae, Rhabdoviridae, Arenaviridae, and Bunyaviridae.
In one embodiment, the virus is herpes, pox, papilloma, corona, influenza, hepatitis, Sendai, sindbis and vaccinia viruses, West Nile, hanta, and viruses which cause the common cold. In yet another embodiment, contacting a fungus with the composition of the invention inactivates the fungus. In one embodiment, the fungus is a yeast, such as, for example various species of Candida (e. g., Candida albicans) or filamentous yeast including but not limited to Aspergillus species or dermatophytes such as Trichophyton ubrura, Trichophyton mentagrophytes, Microsporam canis, Microsporum -gypseux, and Epiderophytonfloccosum, and types thereof, as well as others.
The composition of the invention can also be used for mold remediation for building, equipment, and facilities. Examples of molds include, but are not limited to Cladosporium, Fusarium, Alternaria, Curvularia, Aspergillus, and Penicillium.
The disinfectant described herein can also be used as an aerosol or spray to eliminate odors, e.g. as a room or fabric deodorizer.
In one embodiment, the disinfectant described herein is used as a mouthwash to eliminate bad breath and to reduce the presence of oral microorganisms. Although not necessary, additional conventional components may be added to the disinfectant of the invention as in mouthwashes of the prior art. For example, softeners such as glycerin may be added to enhance the lubricous mouth feel of the mouthwash as it is used and to provide a refreshing, moist, organoleptic feeling thereafter. Glycerin may be incorporated in amounts of from about 0.05% w/v to about 10.0% w/v, and preferably in an amount of about 5% w/v. Sweeteners such as aspartame or sodium saccharin and the like may be added for better taste in amounts of from about 0.005% w/v to about 1.0% w/v, and preferably in an amount of approximately 0.05% w/v. Other essential oils can be added to alter the flavor. Zinc chloride or other zinc salts e.g. zinc gluconate, zinc sulfate etc., may be added as an astringent for an "antiseptic cleaning" feeling in an amount of from about 0.0025% w/v to about 0.200% w/v. hi one embodiment, the disinfectant described herein is used in medical applications, such as to clean skin wounds, or skin surfaces. The disinfectant can also be used as a hand sanitizer. The disinfectant is very potent and highly effective at killing microorganisms including, but not limited, to Salmonella cholerasuis, Staphylococcus aureaus, Pseudomonas aeruginosa, Escherichia coli, Streptococcus pneumonia, Listeria monocytogenes and influenza.
In one embodiment, the disinfectant described herein is used as germicidal for disinfecting/cleaning foodstuff or plant matter. Hydrogen peroxide solutions have also been found to be effective at inhibiting sprouting and rooting of foodstuffs, such as potatoes or other vegetables, thereby extending the shelf life of perishable food stuffs and plant matter. The disinfectant composition can be sprayed directly on plant matter or mixed with soil to discourage infestation with parasitic organisms.
In one embodiment, the composition is used in the food industry in preventing and treating food contaminated with pathogens. Thus, such compositions may be used to reduce or inhibit microbial growth or otherwise abrogate the deleterious effects of microbial contamination of food. For example, the composition can be used to kill bacteria and fungus on poultry eggs, fruit, vegetables, and meat. Also, the inclusion of the compositions of the invention within the food product itself would be effective in killing bacteria that may have been accidentally contaminated meat or poultry. The composition can be included in juice products to prevent growth of certain fungi, which cause contamination and lead to production of mycotoxins. For these applications, the compositions are applied in food industry acceptable forms such as washes, dips, additives, preservatives, or seasonings. The use of media and agents for additives, preservatives, and seasonings that are acceptable in food industry is well known in the art. Except insofar as any conventional additives, preservatives and seasonings are incompatible with the disinfectant composition of the invention, their use in preventing or treating food born microbes and their toxic products is contemplated. Supplementary active ingredients may also be incorporated into the compositions.
In one embodiment the disinfectant is loaded onto a cleaning wipe. The cleaning wipe, upon which the disinfectant composition is loaded thereon, is made of an absorbent/adsorbent material. Typically, the cleaning wipe has at least one layer of nonwoven material. Nonlimiting examples of commercially available cleaning wipes that can be used include DuPont 8838, Dexter Z A, Dexter 10180, Dexter M10201, Dexter 8589, Ft. James 836, and Concert STD60LN, and Ahlstrom 4759. All of these cleaning wipes include a blend of polyester and wood pulp. Dexter Ml 0201 also includes rayon, a wood pulp derivative. The loading ratio of the cleaning composition onto the cleaning wipe is about 2-5: 1, and typically about 3-4: 1. The disinfectant composition is loaded onto the cleaning wipe in any number of manufacturing methods. Typically, the cleaning wipe is soaked in the disinfectant composition for a period of time until the desired amount of loading is achieved.
In one embodiment, the disinfectant composition is packaged in a pressurized gas aerosol can. Common aerosol propellants include butane, isobutene, liquefied natural gas, and propane. The invention provides methods for disinfecting surfaces to inactivate pathogenic organisms comprising contacting a surface with the disinfectant composition of the invention. The step of contacting can involve contacting any substrate, which may be or is suspected to be contaminated, with the composition of the invention. By substrate it is meant, without limitation any subject, such as a human or an animal (contact can be in vivo or ex vivo, any article, any surface, or any enclosure. A pathogenic microorganism can be, without limitation, bacteria, a virus, a fungus, a protozoan or a combination thereof.
The step of contacting can be performed for any amount of time sufficient to inactivate a microorganism. In one embodiment, inactivation occurs within about 5 minutes to about 10 minutes after initial contact. However, it is understood that when the emulsions are used in a therapeutic context and applied topically or systemically, the inactivation may occur over a longer period of time, for example, 5, 10, 15, 20, 25, 30, 60 minutes or longer after administration.
The step of contacting can be performed using any appropriate means of application. For example, compositions can be administered by spraying, fogging, misting, exposure to aerosols, wiping with a wet or saturated cloth or toilette, drenching, immersing.
The invention further provides a method for reducing the number of mold spores on a surface. The method comprises contacting the mold spores with the composition comprising hydrogen peroxide (H. sub.20. sub.2), orange terpene oil, iodine source compound, nano silver, citric acid, acetic acid, isopropanol, ethyl alcohol , a non-ionic emulsifier (e.g. polysorbate 80), and distilled or deionized water (H. sub.20). Any mold can be treated using methods of the invention.
EXAMPLES
Example I :
Efficacy:
Methods:
The germicidal spray composition comprising In one embodiment, the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5%> v/v orange oil, 5% v/v of a 35%> wt. % hydrogen peroxide solution (equivalent to 5.35%) of H.sub.20.sub.2), 20%> v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0.05%> pevodine iodine and 1.5% nano silver of particle size 15nm. was tested for its ability to kill Salmonella cholerasuis, Staphylococcus aureaus, Pseudomonas aeruginosa, Escherichia coli, Streptococcus pneumonia, and Listeria monocytogenes. Three lots were tested, one being at least greater than 120 days old.
The analysis was performed per "Germicidal Spray Test", AO AC 17.sup.th edition, 6.3.03, versus Salmonella cholerasuis ATCC 10708, Staphylococcus aureaus ATCC 6538, Pseudomonas aeruginosa ATCC 15442, Escherichia coli ATCC 8739, Streptococcus pneumonia ATCC 49619, and Listeria monocytogenes ATCC 19113. Testing was performed as required by the EPA FIFRA. The AO AC procedure used in this study is a widely known and accepted method for disinfectant evaluation.
Microorganisms were grown for 48 h in nutrient broth. Glass slides were then inoculated with the grown culture and the inoculated slides were subsequently exposed to the germicidal spray for 10 minutes (60 microorganism inoculated slides/lot/microorganism were tested). After exposure to the disinfectant, slides were used as inoculates in leethen media and microorganism growth determined. Positive, negative and inhibition controls were performed.
Results
All organisms tested were found to be susceptible to the disinfectant. Absolutely no growth was observed in media that was inoculated with the organism slides which were exposed to disinfectant. Controls included uninoculated containers of leethen broth (media controls) and sterile uninoculated glass slides (negative control), there was no growth; Glass slides inoculated with organism and a sterile glass slide immersed in test disinfectant (inhibition control), there was no growth which indicates that the letheen broth neutralizes the disinfectant; Glass slide inoculated with organism (viability control), there was growth; and Glass slide inoculated with organism (enumerated), >10.sup.6 cfu.
Example II:
EPA Acute Oral Toxicity
Methods
The germicidal spray composition comprising In one embodiment, the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 20% v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0,05% pevodine iodine and 1.5% nano silver of particle size 15nm. was tested for toxicity according to protocol number X5D050G, which incorporates by reference Northview Standard Operating Procedure 16D-05 and is on file in Northview Pacific Laboratories, Inc. No amendments were made to the protocol.
A limit screen test was performed using three female Sprague-Dawley rats, which received an oral limit Dose of 50000 mg/kg of the test article. The animals were observed for mortality, weight change and toxic signs for a two week period. Animals were observed daily and weighed on days 7 and 14.
Animal preparation. The animals were fasted overnight before dose administration. During fasting they continued to receive water ad libitum. Food was withheld until four hours after dosing in order to facilitate gastrointestinal absorption of the test article.
Sample preparation. The density of the test article was 1 g/ml and shaken before use. Dosing procedure. The dose was administered by means of a gavage needle attached to a hypodermic syringe. The test animals received a 5 mL/kg solution containing the test article. Three rats were dosed on the first day of dosing. Because all three rats survived no further testing was required.
Results
A single oral administration of germicidal spray product at a limit dose of 5000 mg/kg produced no mortalities. The clinical observations are summarized in FIG. 1. All animals gained weight during the test period and no abnormalities upon necropsy were observed.
Example III:
EPA Primary Eye Irritation Test:
Method
The germicidal spray composition comprising hi one embodiment, the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 20% v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0.05% pevodine iodine and 1.5% nano silver of particle size 15nm. was tested for toxicity according to protocol number X5D051G, which incorporates by reference Northview Standard Operating Procedure 16D-08 and is on file in Northview Pacific Laboratories, Inc. No amendments were made to the protocol. Six New Zeland Rabbits were used. On the day prior to dosing the rabbit's eyes were examined using flourescein sodium opthamalic strips and ultraviolet light. Only rabbits without eye defects or irritation were used. A. 100 ul volume of test material was introduced into the conjuctival sac of the right eye of each rabbit. The left eye remained untreated. The treated eye was washed out with physiological saline 24 hours after dosing.
The eyes were examined and graded for ocular reaction at 1, 24, 48, and 72 hours after application of the test substance for corneal ulceration or opacity, inflammation of the iris, or redness and chemosis of the conjunctivae. The results are interpreted according to the Kay and Calandra Method (Kay J. H. & Calandra, J. C, "Interpretation of eye irritation tests", Journal of society of cosmetic chemists, 13:281- 289, 1962).
Results
based on the Kay and Calandra method of classifying eye irritation properties, the test article was determined to be moderately irritating to eyes of New Zeland Rabbits. All animals remained healthy throughout the study period. There was significant irritation in all 3 animals beginning at the 1 hour scoring and continuing through the 96 hour scoring. The scores all went back to "0", normal scoring, by the 7-day scoring.
Example IV:
EPA Primary Dermal Irritation Test:
Method
The germicidal spray composition comprising In one embodiment, the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 20% v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0,05% pevodine iodine and 1.5% nano silver of particle size 15nm. was tested for toxicity according to protocol number X5D052G, which incorporates by reference Northview Standard Operating Procedure 16D-07 and is on file in Northview Pacific Laboratories, Inc. No amendments were made to the protocol.
Three New Zealand White rabbits were used. One day prior to dosing, the hair on each animal's back was removed with clippers. A one inch square gauze patch containing a 0.5 mL volume of the test article was applied to the shaved skin on each animal. The patch was held in place with surgical tape. After application the trunli of each animal was wrapped with gauze to prevent the animal from disturbing the test patch. During an exposure period of 4 hours, the animal was not restrained in any way. After the exposure period, the patch was removed and test article residues were gently rinsed off with a non-irritating solvent, water. The dosing sites were reexamined and scored 30-60 minutes, 24, 48, and 72 hours after unwrapping. Additional scores were recorded 7 and 14 days after unwrapping to determine the time course of resolution for any irritation that persisted.
The animals were observed for mortality, signs of ill health, or reaction to treatment. Results
On the day of patch removal, all three animals exhibited slight erythema (score of 1 ) at the 30-60 minute scoring and one animal (38383) had slight erythema to the 48 hour scoring. There were no irritation responses observed at the 72 hour observation for any of the animals. All animals remained healthy throughout the study period. The test article was slightly irritating to the skin of three test animals.
Example V:
Virucidal Efficacy of the Composition of the Invention:
Method
The germicidal spray composition In one embodiment, the disinfectant is a composition that comprises 60% v/v distilled water, 10% v/v polysorbate 80, 5% v/v orange oil, 5% v/v of a 35% wt. % hydrogen peroxide solution (equivalent to 5.35% of H.sub.20.sub.2), 20% v/v isopropyl alcohol, 25% v/v ethyl alcohol 2.5% v/v per acetic acid, 3% citric acid, 0.05% pevodine iodine and 1.5% nano silver of particle size 15nm. Was tested for virucidal efficacy. MICROBIOTEST INC. (the microbiology and virology laboratory 105 Carpenter Drive, Sterling, Va. 20164) performed the tests from Feb. 10, 2005 to Feb. 18, 2005 and all raw data, protocol, protocol modifications, test material records, and the final report, are stored in the archives at MICROBIOTEST INC. (105 Carpenter Drive, Sterling, Va. 20164) or at a controlled facility offsite. The Virucidal Efficacy test was performed as detailed in the following protocol from MICROBIOTEST INC.:
Protocol for Virucidal Efficacy Test
Test conditions'. Challenge virus: Avian Influenza A virus, Turkey /Wis/66 strain (H9N2), Charles River Laboratories; Host: Embryonated chicken eggs, B&E Eggs; Active ingredient in test product: Hydrogen peroxide; Neutralizer used: Earle's Balanced Salt Solution containing 0.3% Thioglycolic acid and 0.1% Catalase; Contact time: 10 minutes; Contact temperature: Ambient room temperature (22. degree. C); Dilution: Ready to use as received; Media and reagents :Earle's Balanced Salt Solution, Earle's Balanced Salt Solution containing 0.3% Thioglycolic acid and 0.1% Catalase, Sephacryl S-1000, Chicken red blood cells, Phosphate Buffered Saline containing 0.5% fetal bovine serum, Phosphate Buffered Saline
Objective: The test is designed to substantiate virucidal effectiveness claims for a product to be labeled as a virucide. It determines the potential of the test agent to disinfect hard surfaces contaminated with viruses. The test is designed to stimulate consumer use and conforms to EPA Guidelines DIS/TSS-7, November 1981, and follows the procedure outlined in the American Society for Test Materials (ASTM) test method designated E 1053-97.
Testing conditions: Virus will be dried on a sterile glass Petri dish at ambient temperature. Test agents specified by the sponsor in the miscellaneous section of the protocol will be used to treat the dried virus according to the label claims. After a defined exposure period, the neutralized test agent-virus mixture will be scraped from the surface, neutralized and assayed for the presence of infectious virus.
Materials: Test, control and reference substances will be supplied by the sponsor of the study. The test agent will be tested as supplied by the sponsor unless directed otherwise. All operations performed on the test agent such as dilution or specialized storage conditions must be specified by the sponsor before initiation of testing. The sponsor assures MICROBIOTEST testing facility management that the test agent has been appropriately tested for identity, strength, purity, stability, and uniformity as applicable. MICROBIOTEST will retain all unused test agents for a period of at least three months after completion of the test, then return them to the sponsor of the study or discard them in a manner that meets the approval of the safety officer.
Materials supplied by MICROBIOTEST, including, but not limited to: 1) Challenge virus (requested by the sponsor of the study): Avian Influenza virus. 2) Host: Embryonated chicken eggs. 3) Laboratory equipment and supplies. 4) Media and reagents: Media and reagents relevant to the vims-host system and test agent being tested will be documented in the first project sheet and/or the data pack.
Test system identification: All Petri dishes, dilution tube racks, and host-containing apparatus will be labeled with virus identification and project number. Experimental design: Procedures involved in performance of virucidal studies are described a series of SOPs and logs that are maintained at MICROBIOTEST. The procedures used in different phases of the study will be documented in the data pack. Inoculum preparation: Viral stocks are purchased from reputable sources that identify them by scientifically accepted methods and are propagated at MICROBIOTEST. Records are maintained that demonstrate the origin of the virus. The virus stocks are stored at an ultra-low temperature. Frozen viral stocks will be thawed on the day of the test (fresh stock cultures may be used at the discretion of the Study Director). Carrier preparation: An aliquot of 0.2 mL of stock virus will be spread, with a cell scraper, over an area of approximately 4 in. sup.2 that has been marked on the underside of pre-sterilized Petri dishes. The virus will be allowed to dry for 30 to 60 minutes at room temperature. The drying time and temperature will be recorded. One carrier will be prepared for each test agent and the plate recovery control. One plate will be prepared for the neutralizer effectiveness control using an appropriate medium.
Test agent preparation: The agent will be prepared according to the sponsor's directions or proposed label claims.
Test: After the carrier(s) are properly prepared, 2.0 mL of the test agent will be added. The plates will remain at the temperature and for the time specified by the sponsor. Following the contact period, the test agent will be neutralized with 2.0 mL of the appropriate neutralizing solution and the mixture will be scraped from the surface of the dish with a cell scraper. This will be considered approximately a one log.sub.10 dilution. If columns are used, each sample will be loaded into separate pre-spun Sephacryl columns. Following passage through columns, the eluate will be removed aseptically and serially diluted. If columns are not used, serial dilutions of neutralized virus-test agent mixture will be prepared in using an appropriate diluent. For spray type agents, the agent will be used as the sponsor directs, the volume dispensed will be measured and an equal volume of neutralizer will be used. Following the contact time, the procedure for processing the samples will be the same as described earlier. Viral host culture: Two-tenths mL of selected dilutions of the neutralized inoculum/disinfectant mixture will be inoculated intra-allantoically in embryonic eggs and incubated for 5-7 days at 37.+-.2C. Four determinations will be recorded for each dilution of both tests and controls. The eggs will be candled one-day post-inoculation of test and control samples. All dead embryos will be discarded and the data will be recorded. Following completion of the incubation period, the eggs will be candled and then kept at 2.+-.2C overnight. Afterwards, the allantoic fluid will be harvested and kept at 2.+-.2C until assay. The samples will be assayed for the presence of replicating virus using hemagglutination assay following SOP 1006.1 1 (current version) and the results will be recorded.
Controls
Neutralizer effectiveness (NE): This control will determine if residual active ingredient is present after neutralization. One lot of the test agent will be used for the neutralizer effectiveness control. This control will be processed exactly as the test procedure but instead of viral inoculum, appropriate media will be added. Post neutralization, a 1.0-mL sample will be divided into three portions, using two for toxicity-related controls and the other for neutralizer effectiveness. A 0.5 mL sample will be serially diluted, after which 100 .mu.L of diluted virus will be added to each dilution and held for a period greater than or equal to the contact time. Then these samples will be used to inoculate host embryos as described for the test procedure. Toxicity (TX): The toxicity sample, acquired from the neutralizer effectiveness control, will be diluted and have no virus added. Selected dilutions will be inoculated into the host and incubated in the same manner as the rest of the test and control samples. These effects are distinct from virus-specific cytopathic effects, which will be evident in the stock titer and plate recovery control cultures.
Toxicity-related viral interference control: The test agent may not be effective against the challenge virus yet be toxic to the host employed to detect its infectivity and may inhibit accurate interpretation of the test. To determine the possibility of such interference by residual toxic molecules, host treated with serially diluted neutralized test agent will be infected with a known number of infectious virions. Post-incubation they will be scored and compared with non-treated infected host cells control. This will rule out any possibility of toxicity-related viral interference remaining in the neutralized test agent post-contact time.
Plate recovery (PRC): The carrier used will be prepared as the test. A volume of an appropriate media equivalent to that of the test agent will be added to the dried virus. Post contact time this sample will be treated as the test. This control will determine the relative loss in vims infectivity resulting from drying and neutralization alone. The results from this control will be compared with the test results to confirm recovery of at least four log.sub.lO of infectious virus following drying and neutralization. This titer will be compared with the titers of the test results to reach the acceptable test criteria. When samples are required to pass through the Sephacryl columns, a column titer control (CTC) will be performed by assaying a portion of PRC before passing through the columns to determine the effect on infectious virus titer after passage through the columns.
Column titer control (CTC): This control will be performed to determine any effects the columns may have on infectious virus titer. It will only be performed if columns are used in the study. The sample for this control will be acquired from a portion of the PRC, prior to passing through the columns, and will be serially diluted in an appropriate media. It will then be processed in the same manner as the test.
Virus stock titer (VST): In order to verify the virus stock titer, al aliquot of the virus inoculum will be serially diluted in an appropriate media and processed, as well as assayed as described for the test.
(HVC) Eggs for Clarification: Four eggs will be inoculated with an appropriate media during the incubation phase of the study. This control will demonstrate that cells remain viable throughout the course of the assay period. In addition, it will confirm the sterility of the media employed throughout the assay period.
Calculation: The 50% embryo infectious/lethal dose per mL (EFD/ELD.sub.50/mL) will be determined using the method of Reed and Muench, Am. J. of Hyg. 1938, 27:493. The test results will be reported as the reduction of the virus titer due to treatment with test agent expressed as log.sub.10.
Product evaluation criteria: According to the regulatory agencies, the test agent passes the test if there is complete inactivation of the virus at all dilutions. When toxicity is evident, at least a three-log reduction in titer must be demonstrated beyond the toxic level. Test acceptance criteria: The test will be acceptable for evaluation of the test results if the criteria listed below are satisfied. The study director may consider other causes that may affect test reliability and acceptance; a) the infectious virus recovered from the PRC control must be .gtoreq.4-log.sub.10. b) Viral-induced toxicity must be distinguishable from test agent induced toxic effects.
Results
Avian Influenza virus was exposed to the germicidal spray composition for 10 minutes at ambient room temperature (22. degree. C). the germicidal spray inactivated Avian Influenza vims, as no virus was detected after exposure. All controls met the criteria for a valid test. Virus was not recovered in the host viability control confirming media sterility and host viability.

Claims

Claims
1. A disinfectant composition comprising hydrogen peroxide (H. sub.20. sub.2), orange terpene oil, nano silver, nano gold, or combination of nano silver and nano gold, quaternary ammonium salt, iodine source, a non-ionic emulsifier, and distilled or deionized water (H.sub.20).
2. The composition of claim 1, wherein the orange terpene oil is present in the composition from 5% to 40% v/v, the iodine is present in the composition from 5% to 40%) v/v, the non-ionic emulsifier is present in the composition from 5% to 50% v/v, the distilled or deionized H. sub.20 is present in the composition from 5% to 80%o v/v and the hydrogen peroxide is present in the composition from 1.5% to 8% w/v H. sub.20. sub.2, nano metal is present from 0.01 to 0.15%.
3. The disinfectant composition of claim 1, wherein the non-ionic emulsifier is polysorbate 80.
4. The composition of claim 1, wherein the composition comprises 5.25% w/v H.sub.20.sub.2, 10% v/v orange terpene oil, 5% v/v povidone iodine, 10% v/v polysorbate 80, 0.05% nano silver of particle size 3 nm and 60% v/v distilled water.
5. The disinfectant composition of claim 1, further comprising oil of rosemary.
6. The disinfectant composition of claim 1 , further comprising an antimicrobial agent such as benzyl ammonium chloride.
7. The disinfectant composition of claim 1, further comprising a surfactant.
8. The composition of claim 1, wherein the composition is formulated as a gel, or a spray, or a paste, or a disinfecting wipe.
9. A method for disinfecting a surface comprising contacting a surface with the disinfectant composition of claim 1.
10. A method for reducing the number of mold spores on a surface comprising contacting the mold spores with a disinfectant composition of claim 1.
PCT/EG2009/000025 2009-10-14 2009-10-14 Multipurpose eco-friendly disinfecting composition comprising nano size antibacterial agent WO2011044916A1 (en)

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Cited By (13)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN102531134A (en) * 2011-12-26 2012-07-04 溧阳市澳谷信息科技有限公司 Method for using orange peel cooking liquid to eliminate Microcystis aeruginosa in water body
WO2013107475A1 (en) * 2012-01-16 2013-07-25 Wilo Se Use of an aqueous composition, made of an optionally organically coated nano metal powder of at least one element from group ib of the transition metals or an alloy of said elements with one another and optionally hydrogen peroxide, as a biocide
CN103385804A (en) * 2013-07-24 2013-11-13 阎昭良 Nano-silver mouth wash for preventing and treating oral diseases and preparation method thereof
EP2731432A2 (en) * 2011-07-14 2014-05-21 Ecolab USA Inc. Deodorization of peracids
US9084421B2 (en) 2011-07-14 2015-07-21 Ecolab Usa Inc. Deodorization of peracids
US20150305343A1 (en) * 2014-04-28 2015-10-29 American Sterilizer Company Process and composition for killing spores
CN108391673A (en) * 2018-03-01 2018-08-14 北京中科东亚纳米材料科技有限公司 A kind of preparation method of nano silver/quaternary ammonium salt compound disinfectant
EP3415009A1 (en) * 2017-06-12 2018-12-19 Wilbert Hygiene GmbH Disinfection wipe
WO2019075176A3 (en) * 2017-10-11 2019-06-06 Markesbery Blue Pearl LLC Methods and systems for sequential delivery of aqueous peracid compositions
US10603396B2 (en) 2016-05-26 2020-03-31 Markesbery Blue Pearl LLC Methods and system for disinfection
US11425911B2 (en) 2017-05-25 2022-08-30 Markesbery Blue Pearl LLC Method for disinfection of items and spaces
RU2788728C1 (en) * 2022-01-17 2023-01-24 Георгий Александрович Фролов Composition with long-lasting biocidal effect and the composition mouthwash
EP3973778A4 (en) * 2019-05-23 2023-07-05 Elves Chemical Co., Ltd. Freeze-resistant disinfectant composition and preparation method therefor

Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO1996006644A1 (en) * 1994-08-30 1996-03-07 Allergan, Inc. Contact lens disinfecting compositions and methods employing terpenes
US20060051430A1 (en) * 2004-09-07 2006-03-09 Arata Andrew B Silver dihydrogen citrate compositions
WO2006074117A2 (en) * 2005-01-05 2006-07-13 Robert Holladay Silver/water, silver gels and silver-based compositions; and methods for making and using the same
US20080166437A1 (en) * 2007-01-04 2008-07-10 Rosskopf Erin N Methods of reducing pests and treating gastrointestinal nematode infections
US20090312279A1 (en) * 2005-12-23 2009-12-17 Sterilex Technologies, Llc Antimicrobial compositions

Patent Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO1996006644A1 (en) * 1994-08-30 1996-03-07 Allergan, Inc. Contact lens disinfecting compositions and methods employing terpenes
US20060051430A1 (en) * 2004-09-07 2006-03-09 Arata Andrew B Silver dihydrogen citrate compositions
WO2006074117A2 (en) * 2005-01-05 2006-07-13 Robert Holladay Silver/water, silver gels and silver-based compositions; and methods for making and using the same
US20090312279A1 (en) * 2005-12-23 2009-12-17 Sterilex Technologies, Llc Antimicrobial compositions
US20080166437A1 (en) * 2007-01-04 2008-07-10 Rosskopf Erin N Methods of reducing pests and treating gastrointestinal nematode infections

Cited By (16)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JP2017075195A (en) * 2011-07-14 2017-04-20 エコラボ ユーエスエー インコーポレイティド Deodorization of peracids
EP2731432A4 (en) * 2011-07-14 2014-12-17 Ecolab Usa Inc Deodorization of peracids
JP2014522857A (en) * 2011-07-14 2014-09-08 エコラボ ユーエスエー インコーポレイティド Peracid deodorization
EP2731432A2 (en) * 2011-07-14 2014-05-21 Ecolab USA Inc. Deodorization of peracids
US9084421B2 (en) 2011-07-14 2015-07-21 Ecolab Usa Inc. Deodorization of peracids
CN102531134A (en) * 2011-12-26 2012-07-04 溧阳市澳谷信息科技有限公司 Method for using orange peel cooking liquid to eliminate Microcystis aeruginosa in water body
WO2013107475A1 (en) * 2012-01-16 2013-07-25 Wilo Se Use of an aqueous composition, made of an optionally organically coated nano metal powder of at least one element from group ib of the transition metals or an alloy of said elements with one another and optionally hydrogen peroxide, as a biocide
CN103385804A (en) * 2013-07-24 2013-11-13 阎昭良 Nano-silver mouth wash for preventing and treating oral diseases and preparation method thereof
US20150305343A1 (en) * 2014-04-28 2015-10-29 American Sterilizer Company Process and composition for killing spores
US10603396B2 (en) 2016-05-26 2020-03-31 Markesbery Blue Pearl LLC Methods and system for disinfection
US11425911B2 (en) 2017-05-25 2022-08-30 Markesbery Blue Pearl LLC Method for disinfection of items and spaces
EP3415009A1 (en) * 2017-06-12 2018-12-19 Wilbert Hygiene GmbH Disinfection wipe
WO2019075176A3 (en) * 2017-10-11 2019-06-06 Markesbery Blue Pearl LLC Methods and systems for sequential delivery of aqueous peracid compositions
CN108391673A (en) * 2018-03-01 2018-08-14 北京中科东亚纳米材料科技有限公司 A kind of preparation method of nano silver/quaternary ammonium salt compound disinfectant
EP3973778A4 (en) * 2019-05-23 2023-07-05 Elves Chemical Co., Ltd. Freeze-resistant disinfectant composition and preparation method therefor
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