WO2011003179A1 - Healthcare facility disinfecting process and system with oxygen/ozone mixture - Google Patents

Healthcare facility disinfecting process and system with oxygen/ozone mixture Download PDF

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Publication number
WO2011003179A1
WO2011003179A1 PCT/CA2010/000998 CA2010000998W WO2011003179A1 WO 2011003179 A1 WO2011003179 A1 WO 2011003179A1 CA 2010000998 W CA2010000998 W CA 2010000998W WO 2011003179 A1 WO2011003179 A1 WO 2011003179A1
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WO
WIPO (PCT)
Prior art keywords
ozone
room
oxygen
atmosphere
hydrogen peroxide
Prior art date
Application number
PCT/CA2010/000998
Other languages
French (fr)
Inventor
Michael Edward Shannon
Original Assignee
Medizone International Inc.
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Priority to IN963DEN2012 priority Critical patent/IN2012DN00963A/en
Priority to CN201080030657.2A priority patent/CN102481383B/en
Application filed by Medizone International Inc. filed Critical Medizone International Inc.
Priority to CA2735739A priority patent/CA2735739C/en
Priority to SG2011095767A priority patent/SG176977A1/en
Priority to EP10796611.1A priority patent/EP2451489B1/en
Priority to BR112012000384A priority patent/BR112012000384B1/en
Priority to MX2012000302A priority patent/MX344243B/en
Priority to JP2012518702A priority patent/JP2012531979A/en
Priority to EP10842789.9A priority patent/EP2525838B1/en
Priority to CA2785850A priority patent/CA2785850A1/en
Priority to PCT/CA2010/001364 priority patent/WO2011085466A1/en
Priority to US13/522,685 priority patent/US8636951B2/en
Publication of WO2011003179A1 publication Critical patent/WO2011003179A1/en
Priority to US13/343,403 priority patent/US8551399B2/en
Priority to HK13106264.1A priority patent/HK1178468A1/en
Priority to US14/046,535 priority patent/US9616145B2/en

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Classifications

    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61LMETHODS OR APPARATUS FOR STERILISING MATERIALS OR OBJECTS IN GENERAL; DISINFECTION, STERILISATION OR DEODORISATION OF AIR; CHEMICAL ASPECTS OF BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES; MATERIALS FOR BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES
    • A61L2/00Methods or apparatus for disinfecting or sterilising materials or objects other than foodstuffs or contact lenses; Accessories therefor
    • A61L2/16Methods or apparatus for disinfecting or sterilising materials or objects other than foodstuffs or contact lenses; Accessories therefor using chemical substances
    • A61L2/20Gaseous substances, e.g. vapours
    • A61L2/202Ozone
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61LMETHODS OR APPARATUS FOR STERILISING MATERIALS OR OBJECTS IN GENERAL; DISINFECTION, STERILISATION OR DEODORISATION OF AIR; CHEMICAL ASPECTS OF BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES; MATERIALS FOR BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES
    • A61L2/00Methods or apparatus for disinfecting or sterilising materials or objects other than foodstuffs or contact lenses; Accessories therefor
    • A61L2/16Methods or apparatus for disinfecting or sterilising materials or objects other than foodstuffs or contact lenses; Accessories therefor using chemical substances
    • A61L2/20Gaseous substances, e.g. vapours
    • A61L2/208Hydrogen peroxide
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61LMETHODS OR APPARATUS FOR STERILISING MATERIALS OR OBJECTS IN GENERAL; DISINFECTION, STERILISATION OR DEODORISATION OF AIR; CHEMICAL ASPECTS OF BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES; MATERIALS FOR BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES
    • A61L2202/00Aspects relating to methods or apparatus for disinfecting or sterilising materials or objects
    • A61L2202/10Apparatus features
    • A61L2202/11Apparatus for generating biocidal substances, e.g. vaporisers, UV lamps
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61LMETHODS OR APPARATUS FOR STERILISING MATERIALS OR OBJECTS IN GENERAL; DISINFECTION, STERILISATION OR DEODORISATION OF AIR; CHEMICAL ASPECTS OF BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES; MATERIALS FOR BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES
    • A61L2202/00Aspects relating to methods or apparatus for disinfecting or sterilising materials or objects
    • A61L2202/10Apparatus features
    • A61L2202/13Biocide decomposition means, e.g. catalysts, sorbents
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61LMETHODS OR APPARATUS FOR STERILISING MATERIALS OR OBJECTS IN GENERAL; DISINFECTION, STERILISATION OR DEODORISATION OF AIR; CHEMICAL ASPECTS OF BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES; MATERIALS FOR BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES
    • A61L2202/00Aspects relating to methods or apparatus for disinfecting or sterilising materials or objects
    • A61L2202/10Apparatus features
    • A61L2202/14Means for controlling sterilisation processes, data processing, presentation and storage means, e.g. sensors, controllers, programs
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61LMETHODS OR APPARATUS FOR STERILISING MATERIALS OR OBJECTS IN GENERAL; DISINFECTION, STERILISATION OR DEODORISATION OF AIR; CHEMICAL ASPECTS OF BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES; MATERIALS FOR BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES
    • A61L2202/00Aspects relating to methods or apparatus for disinfecting or sterilising materials or objects
    • A61L2202/20Targets to be treated
    • A61L2202/25Rooms in buildings, passenger compartments

Definitions

  • This invention relates to disinfecting systems for use in healthcare facilities, public health facilities and the like, to eliminate or at least to reduce to acceptable levels, microbial residues which are resistant to conventional disinfectant and sterilization systems.
  • Clostridium difficile C. difficile
  • E. coli E. coli
  • Pseudomonas aeruginosa methicillin-resistant Staphylococcus aureus
  • VRE vancomycin-resistant Enterococcus
  • C difficile Of particular concern in this context are the bacteria C difficile and MRSA.
  • C difficile was relatively uncommon, but has now become epidemic in many regions of the world. Indeed, it is now recognized by a growing number of public health officials as a worldwide epidemic (pandemic) with incalculable financial and health implications.
  • MRSA has been identified by the American Academy of Orthopaedic Surgeons as the single biggest concern for surgical procedures, and concurs with recent journal articles that it constitutes a "silent epidemic.” Under current healthcare facility cleaning and sterilizing procedures, both C difficile and MRSA, as well as the aforementioned E.
  • VRE vancomycin-resistant Enterococcus
  • a biofilm is an aggregate of microorganisms in which cells adhere to each other and/or to a surface. They are frequently embedded in a self produced matrix of extracellular polymeric substance (EPS), a polymeric conglomeration generally composed of extracellular DNA, proteins and polysaccharides. Biofilms form on surfaces, e.g. in hospital settings, in the presence of water vapour.
  • EPS extracellular polymeric substance
  • the biofilm grows through a combination of cell division and recruitment. When the biofilm is established, the aggregate cell colonies are apparently increasingly antibiotic resistant. It has also been reported that biofilm bacteria apply chemical weapons to defend themselves against disinfectants and antibiotics (see “Biofilm Bacteria Protect Themselves With Chemical Weapons", Dr. Carsten Matz et. al., Helmholtz Cetre for Infection Research, Brauschweig, reported on lnforniac.com, July 23, 2008).
  • Bacteria living in a biofilm have significantly differently properties from the planktonic form of the same species, as the dense and protected environment of the film allows them to co-operate and interact in various ways.
  • Traditional antibiotic therapy is usually not sufficient to eradicate chronic infections, and one major reason for their persistence seems to be the capability of the bacteria to grow within biofilms that protect them from adverse environmental factors.
  • Chlorinated solutions with and without ammonia are commonly used, but have shown only limited success. To add to this challenge, such solutions cannot be used on electronic devices commonly installed in wards, recovery rooms, operating theaters, etc.
  • Vaporized hydrogen peroxide (VHP) is highly effective when applied to smooth surfaces, but has little or no efficacy on porous materials and fabrics. Moreover, VHP is very damaging to electronic devices.
  • Ozone is known to be a powerful anti-bacterial, anti-fungal and anti-viral agent. For over 100 years, it has been used for water purification. It is known to be effective against Legionella Bacteria, E. coli and pseudomonas populations in such plants.
  • Ozone use in healthcare facilities is, however, problematic. Solutions containing ozone are explosive on warming. Ozone is medically harmful to those exposed to it, causing irritation of eyes and mucous membranes, pulmonary edema, and chronic respiratory disease if low, safe levels of exposure are exceeded. Moreover, it is widely recognized to be an environmental hazard.
  • Canadian Patent Application 2,486,831 Arts et. al. discloses the use of a combination of ozone and UV radiation for decontamination of air in a room such as a mobile isolation unit, a hospital room and the like. The air is caused to flow through a portable unit containing a filter exposed to ozone.
  • the patent contains an experimental account of treating rooms of a residence, effectively treating cladosporium mold spores and penicillium/aspergillus molds in the room air. No details of the precise conditions used are given. There is no demonstration or disclosure of treatment of contaminated surfaces in a room.
  • the present invention provides, from one aspect, an ozone-based disinfection system for rooms and their contents within all healthcare facilities, mobile or stationary, and other critical infrastructure such as schools and government buildings.
  • ozone-containing gases are delivered into and applied to the surfaces and equipment and objects contained within the room.
  • the application can be through simple contact of the gaseous atmosphere with the surfaces, or, in the case of difficult-to-clean surfaces such as drapes, carpets and other fibrous surfaces, it can be by means of a dislodgement system effecting physical agitation of the surface (scrubbing brushes, high pressure jets or the like, sometimes referred to herein as "scrubbing").
  • the ozone-containing gases are applied at controlled concentrations and, in some cases, elevated pressures which have been found to be effective in destroying critical viral, bacterial and fungal pathogens found in environments, including but not limited to the five especially troublesome bacteria Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); and vancomycin-resistant Enterococcus (VRE).
  • C. difficile Clostridium difficile
  • E. coli E. coli
  • Pseudomonas aeruginosa Pseudomonas aeruginosa
  • MRSA methicillin-resistant Staphylococcus aureus
  • VRE vancomycin-resistant Enterococcus
  • the system of the invention also allows an operator to apply the ozone-containing gases at predetermined concentrations of ozone directly to problem surfaces in the room, with a physical agitation action and under pressure where appropriate.
  • the system also includes an ozone-destruct unit for removing residual ozone from the room atmosphere. The whole system is portable, so that it can be moved from room to room as required, and is harmless to equipment contained in the room. Once the sterilization process is completed, the room can be back in medical use within 20 minutes, with its residual atmospheric ozone level at an acceptable 0.04 ppm or less.
  • FIG. 1 of the accompanying drawings is a diagrammatic illustration of an apparatus in accordance with an embodiment of the invention, disposed within a room to be disinfected;
  • Figures 2A and 2B are diagrammatic illustrations of physical agitation systems for use in embodiments of the invention.
  • FIG. 3 is a diagrammatic illustration of an apparatus according to the invention, in portable, transportation mode
  • Figure 4 is a diagrammatic illustration of a test apparatus used to generate some of the test results reported below;
  • Figure 5 is a diagrammatic illustration of the test apparatus used to generate the results reported in Example 10 below.
  • One significant feature of the system according to certain embodiments of the invention is the ability to adjust the pressure of the ozone/oxygen gas mixture being used for disinfection purposes. It has been found that, in many cases, effective disinfection of a room and its contents from bacterial contamination can best be achieved by pressurizing the atmosphere in the room with ozone/oxygen mixture containing from about 10 to about 100 ppm of ozone, to a pressure higher than normal atmospheric pressure, e.g. from about 14.7 psi to about 100 psi. A localized pressurized air jet can also be used, which would obviate the need to raise the overall pressure in the room. Raising the room pressure may require initial sealing of the room prior to the decontamination process. With many rooms where medical procedures are conducted, such as operating theatres, this is a simple process, since such rooms are designed to be substantially sealed when in use for medical procedures. With other rooms, this may require some significant initial preparation.
  • Another, particularly preferred embodiment of the invention utilizes hydrogen peroxide, as well as ozone, in the disinfecting gaseous atmosphere.
  • ozone and hydrogen peroxide increasing the pressure within the room may not be necessary.
  • the particularly troublesome bacteria which are likely to cause nosocomial infections in a hospital environment, namely Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); vancomycin-resistant Enterococcus (VRE), deposit on surfaces in a hospital environment such as stainless steel surfaces, ceramic surfaces and marble surfaces and quickly form a biofilm in which the microorganisms thrive.
  • a process of combating bacteria in an enclosed space within a room and contained in biofilm on surfaces within the room which comprises: creating in the room a disinfecting atmosphere which includes ozone at a concentration of 2 - 350 ppm by weight and hydrogen peroxide at an amount of 0.2 - 10 wt. %, at a relative humidity of at least 60%; exposing the biofilm carrying surfaces having live bacteria therein to the disinfecting atmosphere for a period of at least 30 minutes sufficient for an effective kill of the bacteria in the microfilm; and subsequently removing ozone from the atmosphere, down to 0.04 ppm or less.
  • the disinfecting atmosphere has a relative humidity of at least 65%.
  • Another preferred embodiment provides a process for disinfecting a room and surfaces therein to combat at least one of the microorganisms bacteria Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); vancomycin-resistant Enterococcus (VRE); Bacillus subtilus, and/or anthrax, which comprises exposing the room and surfaces therein to a gaseous atmosphere which includes an effective amount of ozone and an effective amount of hydrogen peroxide, for a period of time which substantially reduces levels of bacteria on the surfaces, and subsequently removing the residual ozone in the room's atmosphere, down to a safe low level.
  • a gaseous atmosphere which includes an effective amount of ozone and an effective amount of hydrogen peroxide
  • the process is particularly effective with or without physical agitation, in disinfection of stainless steel surfaces which abound in medical treatment facilities, and on which bacteria are tenacious and difficult to destroy, due at least in part to their generation of a biofilm on such surfaces.
  • the process is also effective in destroying and deactivating anthrax bacteria, as evidenced by its effectiveness against the well-established anthrax surrogate, Bacillus subtilis.
  • a portable system for rapidly disinfecting rooms, surfaces and equipment therein comprising:
  • an ozone generator for discharging into the room a gaseous mixture including ozone; an ozone controller adapted to control the amount of discharged ozone; a source of hydrogen peroxide for discharging controlled amounts of hydrogen peroxide into the room; means for discharging the hydrogen peroxide and ozone into the room; humidity adjusting means adapted to increase or decrease the relative humidity of the room during treatment; and an ozone remover adapted to destroy ozone, down to a safe level in the room atmosphere for subsequent human utilization.
  • a process for disinfecting a room of a healthcare facility which comprises: introducing into the room a gas mixture which includes ozone and hydrogen peroxide in effective amounts; raising the pressure within the room above atmospheric pressure, or introducing a pressurized gas stream; physically agitating fibrous and porous surfaces within the room while the surfaces are exposed to the pressurized gas stream of hydrogen peroxide and ozone containing atmosphere of relative humidity at least 60%; returning the room to atmospheric pressure; and, removing the residual ozone from the room's atmosphere, down to a safe level.
  • Preferred ozone amounts are from about 20 - 350 parts per million in the treatment gas atmosphere, more preferably 20 - 200, even more preferably 20 - 90 parts per million in the oxygen/ozone gas mixture, and most preferably 35 - 80 ppm ozone.
  • Preferred amounts of hydrogen peroxide are the amounts supplied to the room treatment atmosphere using an aqueous solution containing 0.2 - 10%, more preferably 1 - 5%, hydrogen peroxide. In the description below, the peroxide percentages used are sometimes expressed in terms of these solution percentages. The amounts are chosen so that no serious deleterious effects are suffered by other equipment in the treatment room.
  • the amount of hydrogen peroxide in the disinfecting atmosphere can be calculated from the volume of aqueous hydrogen peroxide evaporated into the disinfecting atmosphere, the volume of the room being disinfected and the concentration of hydrogen peroxide in the starting solution.
  • Times of exposure of the room and its surface to the ozone-containing atmosphere are suitably from 30 minutes to about 120 minutes, preferably from about 60 to about 105 minutes, and most preferably about 90 minutes. These times are constrained to some extent by the need to clear the room of ozone (down to a maximum of 0.04 ppm) following the disinfection phase, and return the room to medical use within a reasonable period of time, with the entire start-to-finish time not exceeding 150 minutes.
  • the ozone removal is an extremely rapid and fully effective process. Both the hydrogen peroxide and the ozone (and any products of interaction between them) should be removed before the room is put back into normal use.
  • the dislodgement system allows penetration of carpet, drape and similar surfaces in the room, to gain access to concealed/sequestered spores and/or colonies of bacteria.
  • the dislodgement system can be manually operated, with operators protected by a hazard suit and mask, or remotely operated or totally automated. It may take the form of one or more outlet jets, with associated manually operable jet pressure controls. It may take the form of a revolving or fixed brush with bristles of appropriate stiffness, alone or in combination with an outlet jet.
  • Any form of dislodgement system effective to disturb the pile of carpet fabrics, upholstery fabrics and the like so as to access the remote parts which might harbor bacterial spores or colonies can be used.
  • the ozone for use in the present invention can be generated by any known means.
  • the apparatus of the invention preferably includes a container of medical grade oxygen.
  • the oxygen container can be a standard, pressurized vessel containing medical grade oxygen, of the type commonly found in medical facilities.
  • Oxygen from this container is fed to an ozone generator, where the oxygen is subjected to electrical discharge, normally with high voltage alternating current, to convert small amounts of the oxygen to ozone and produce a gaseous mixture of oxygen and ozone.
  • the quantity of ozone in the mixture is controllable by adjustment of the voltage of the electrical discharge.
  • Suitable ozone generators are known and available commercially.
  • the relative amounts of ozone generated are relatively small, expressed in parts per million (ppm), but such is the power of ozone as a disinfectant, especially in combination with hydrogen peroxide in accordance with this invention, that such small quantities thereof are all that is required.
  • ozone generation can be used if preferred.
  • Ultraviolet radiation of appropriate wavelength, incident upon oxygen or air is one acceptable alternative.
  • air from the room itself may be fed into the ozone generating unit to supply the required oxygen for conversion to ozone.
  • Other methods of ozone generation which can be used include photocatalytic reactions, cold plasma, etc.
  • the relative humidity of the treatment space should be at least 60% and preferably at least 65%, for effective disinfection. To ensure this, it is preferred to incorporate a humidifier in the system of the invention, using sterile water from an internal system reservoir to adjust and control the humidity of the issuing gas mixture.
  • the adjustable humidifier need only increase the humidity of the space to the desirable level and can be placed in any location within the space.
  • the hydrogen peroxide vapor is suitably applied, in controlled amounts, to the air/water vapor issuing from the humidifier and thus added to the ozone/oxygen containing gas mixture.
  • hydrogen peroxide can be applied to the water used to humidify the target location.
  • Hydrogen peroxide is commercially available as aqueous solutions of standard concentrations of hydrogen peroxide.
  • a standard solution of known peroxide concentration is suitably diluted down by a fixed volume of distilled water.
  • the peroxide load is standardized based on the known volume of water from the peroxide solution required to raise the relative humidity to the desired extent, e.g. from 40 - 80%. From this, the amount of hydrogen peroxide in volume % or ppm by volume introduced into the treatment facility can be calculated.
  • Certain systems according to embodiments of the invention may include a temperature adjuster and controller for the gas mixture.
  • This can be a simple heater/cooler through which either the incident oxygen or the generated oxygen/ozone mixture passes prior to discharge into the room atmosphere. While simple adjustment of the temperature of the room using an external room heating system and thermostat can be effective, it is preferred to adjust the temperature of the issuing gas mixture, for most effective treatment of the carpet and drapery surfaces.
  • the ideal range of temperature for ozone and ozone/hydrogen peroxide decontamination of pathogens is 15 0 C to 30 0 C.
  • the system of the invention also includes an ozone removal unit. Such units are known, and can be purchased commercially for use in the present invention.
  • Suitable ozone removal units are those based on activated carbon as the removal medium. These act very quickly, and do not lead to the formation of hazardous reaction products. The inclusion of such units enables the treated facility to be cleared of ozone and returned to normal use rapidly, an important feature where health care facilities are involved.
  • Other types include systems based on catalysts such as manganese oxide or other metal oxides, which may be heated to remove moisture, thermal destruction in conjunction with other metals including platinum or palladium.
  • Fig. 1 of the accompanying drawings shows a patient room surgical suite 10, closed ready for disinfection by a process according to an embodiment of the invention.
  • the suite is substantially hermetically sealed.
  • a pressurized cylinder 12 of oxygen feeding oxygen gas into a humidifier 14 and thence to an ozone generator 16, which includes electrical discharge plates of variable voltage to adjust the quantity of ozone which is generated.
  • a heater and a pressure controller may be disposed near the entrance to the ozone generator.
  • Output of oxygen/ozone gas mixture is via room outlets 18, 20 to the atmosphere of the suite 10, and via wands 22A and/or 22B to a dislodgement means in the form of scrubbing brushes 24A and 24B mounted on the outlet ends of the respective wands 22A, 22B.
  • the heater, the pressure controller, the voltage supplied to the ozone generator 16 and the humidity level supplied by the humidifier 14 are all controlled and adjusted from an external control panel 26 via respective electrical connections 28, 30, 32 and 34.
  • Also disposed within the suite is an oscillating fan 34 and an ozone destruct filter unit 36.
  • a container of aqueous hydrogen peroxide solution 19 and associated air blower 21 which, during operation, blows vaporized hydrogen peroxide in controlled amounts into discharge wand 22A and 22B to mix with the output of ozone/oxygen therein.
  • the amount of hydrogen peroxide being supplied is controlled by adjustment of the blower 21 through a connection thereof to the control panel 26.
  • hydrogen peroxide can be supplied from generator 19 to the humidifier 14.
  • Figs. 2A and 2B of the accompanying drawings show in more detail forms of dislodgement means 24A and 24B for use in the present invention, attached to the outlet, discharge ends of respective wands 22.
  • the dislodgement means 24A has a jet outlet nozzle 38A at its extremity, and a generally circular plate 40 mounted on the wand 22A near the discharge end.
  • the wand 22A passes through a central aperture 42 in a plate 40.
  • the plate 40 has brush bristles 46A mounted on its lower surface, arranged in two arcs around the jet outlet nozzle 38A and protruding downwardly to an extent just beyond the extent of outlet from nozzle 38A.
  • oxygen/ozone gas mixture or oxygen/ozone/hydrogen peroxide gas mixture issues from nozzle 38A at relatively high pressure, and can be directed by the operator holding the wand to a carpet surface area while at the same time the operator scrubs the carpet surface area with the bristles 46A.
  • Fig 2B shows an alternative but essentially similar arrangement, in which plate 40 is replaced by a wheeled platform 44 carrying two rotary brushes 46B and three jet outlets 38B for the oxygen/ozone/hydrogen peroxide delivery at pressure, located forwardly of the rotary brushes 46B.
  • FIG. 3 of the accompanying drawings illustrates the portability of a system according to the invention. Parts are numbered as in Fig. 1 .
  • a 4-wheeled cart 48 is provided, on which all the component parts of the system can be loaded for ease of transportation from one room to another.
  • the instrumentation and control panel can be disconnected for transportation, and re-connected and disposed outside when the apparatus is placed in another room for use as shown in Fig. 1 .
  • the cart 48 is removed while the system is in use, but is loaded with the components after use, either for transportation to another room or for storage.
  • the operation of the system will be readily apparent from the preceding description of its component parts and their inter-connection.
  • the cart 48 carrying the component parts is wheeled into the room 10 to be disinfected, and the parts are distributed around the room and connected together as illustrated in Fig. 1 .
  • An operator wearing a hazard suit and other appropriate protective clothing enters the room and holds the wand 22.
  • the room is sealed.
  • Conditions of treatment are set on the control panel 26, and the apparatus is switched on so that oxygen/ozone/hydrogen peroxide gas mixture at controlled ozone concentration, hydrogen peroxide concentration, relative humidity, temperature and elevated pressure issues from jet nozzle 38.
  • the operator applies the jetted gas mixture to the carpet surfaces, drapery surfaces and other absorbent surfaces in the room, scrubbing the surfaces at the same time with the bristles 46.
  • the room becomes pressurized above atmospheric pressure, due to the introduction of the oxygen/ozone gas mixture. Pressure is continually monitored by the control panel 26 to ensure safe working conditions for the operator, as well as the temperature, humidity and ozone concentration in the room. Smooth surfaces in the room may not need the action of the dislodgement means, but are satisfactorily disinfected by contact with the atmosphere in the room, especially when hydrogen peroxide and ozone are used in combination.
  • the oscillating fan 34 is operated throughout the procedure, to circulate the oxygen/ozone mixture throughout the room.
  • the hydrogen peroxide supply (if used), the oxygen supply and ozone generator are switched off. Then the ozone destruct filter is operated, sucking in the ozone-containing gases, destroying the ozone and issuing pure oxygen from it.
  • the room can now be opened, the apparatus disconnected and loaded on the cart 48, and the room put back to its normal use.
  • Inoculum was prepared by performing a series of serial dilutions of 0.9 ml 0.85 NaCI broth with 0.1 ml of original 0.5 McFarland inoculum (6 x 10 fold) to give solutions of 10 "1 , 10 '2 , 10 '3 , 10 ' 4 , 10 5 , 10 "6 and 10 "7 cfu/mL
  • Organisms were plated out in triplicate, 0.1 ml of each solution being spread over the surface of Columbia sheep's blood agar plates. Two sets of plates (12 plates per organism) were subjected to ozone/oxygen exposure at preselected concentrations of ozone (ppm), humidity and temperature conditions in the illustrated apparatus. The other sets of 2 were treated as controls, with no ozone exposure, but kept at room temperature.
  • ppm concentrations of ozone
  • Fig. 4 For ozone exposure, the apparatus generally illustrated in Fig. 4 was used.
  • test plates were mounted inside a disinfection chamber 60, the upstream end 62 of which had an ozone inlet port 64, a hydrogen peroxide vapor inlet port 65 (which in Examples 1 - 9 described below was blocked), and a water vapor inlet port 66.
  • a cylinder 68 of pressurized medical grade oxygen was provided, feeding oxygen to an ozone generator 70, equipped with alternating current electrical plates to which variable voltage could be supplied via input control 72.
  • the output of oxygen/ozone mixed gas from the ozone generator 70 was fed to the ozone inlet port 64 of the disinfection chamber 60.
  • a water vapor humidifier 74 supplied water vapor to inlet port 66.
  • the disinfection chamber 60 also contained a heater/cooler (not shown), a temperature sensor 76, a pressure sensor 78, a humidity sensor 80 and an ozone sensor 82, connected electrically via respective lines 84, 86, 88 and 90 to a control panel and monitor 92, connected to feed back to the oxygen cylinder 68 to control flow for pressure adjustment purposes, to the ozone generator 70 to control and adjust the ozone quantity, to the water vapor humidifier 74 to control and adjust relative humidity in the disinfection chamber 60, and to the heater/cooler to control and adjust the temperature in the chamber.
  • These parameters were all pre-set on the control panel to desired values and automatically re-adjusted themselves to these values as the experiments progressed.
  • An ozone destruct filter 94 was connected to the downstream end 96 of the disinfection chamber 60 at outlet port 98, to destroy ozone issuing from the chamber 60 at the end of the experiment. Gases were circulated within the chamber 60, and expelled therefrom at the termination of the experiment, using a fan 100 mounted therein. After placing the test plates in the chamber 60, it is sealed until the end of each experiment.
  • the control plates and the ozone treated plates were placed in an incubator at the same time.
  • the plate counts were read through a microscope, and the numbers of colony forming units on each plate was counted.
  • the spores are aerotolerant.
  • Example 1 The experiment of example 1 was repeated using the same bacterial strain, but exposing the test plates in the chamber to 50 ppm ozone in oxygen, at 2O 0 C and 80% relative humidity.
  • Example 1 The experiment of Example 1 was repeated, except for using as test organism P. aeruginosa ATCC 27853. The same conditions of ozone exposure, dilution, incubation and testing were used. On the test plates, active colony counts of 1 1 and 18 were found at 10 ⁇ 2 dilution, and active colony counts of 5 and 27 were found at 10 ⁇ 3 dilution. At higher dilutions, there were no detectable colonies. In contrast, the control, non-ozone exposed plates showed colonies too numerous to count, at all dilutions up to and including 10 ⁇ 6 . A 2.8 log reduction was achieved (7.9 log to 5.1 log).
  • Example 3 The experiment of Example 3 was repeated, using the same test organism, but treating the test samples in the chamber with ozone/oxygen gas mixture containing 50 ppm ozone, at 80% humidity, for 90 minutes. By the same recovery and test procedures, it was determined that the control plates had cfus too numerous to count.
  • Example 3 The experiment of Example 3 was repeated but using Enterrococcus faecalis (high level vancomycin resistant) Clinical Strain 80269 as the test organism, with 90 minute exposure to ozone/oxygen mixture of 35 ppm ozone, at 21 0 C and 80% relative humidity.
  • the eluates from control plates (duplicated) had cfu counts of too numerous to count at dilution 10 ⁇ 2 , 10 ⁇ 3 and 10 ⁇ 4 ; cfu counts of 402 and 346 at dilution 10 ⁇ 5 ; cfu counts of 35 and 25 at dilution 10 ⁇ 6 ; and cfu counts of 14 and at dilution 10 ⁇ 7 .
  • Example 5 The experiment of Example 5 was repeated using the same VRE Clinical Strain as the test organism, but with 90 minute exposure to ozone/oxygen mixture of 50 ppm ozone, at 20 0 C and 80% relative humidity.
  • the eluates from control plates (duplicated) had cfu counts of too numerous to count at dilution 10 ⁇ 2 , 10 "3 and 10 ⁇ 4 ; cfu counts of 369 and 359 at dilution 10 ⁇ 5 ; cfu counts of 46 and 46 at dilution 10 ⁇ 6 ; and cfu counts of 9 and 2 at dilution 10 ⁇ 7 .
  • the eluates from the test plates gave cfu counts of 50 at dilution 10 ⁇ 2 ; cfu counts of less than 30 at dilution 10 ⁇ 3 ; and cfu counts of 0 at higher dilutions 10 ⁇ 5 .
  • Example 3 The experiment of Example 3 was repeated but using E. CoIi Strain ATCC 25922 as the test organism, with 90 minute exposure to ozone/oxygen mixture of 35 ppm ozone, at 21 0 C and 80% relative humidity.
  • the eluates from control plates (duplicated) had cfu counts of too numerous to count at dilution 10 '2 , 10 '3 and 10 '4 ; cfu counts of greater than 300 at dilution 10 '5 ; cfu counts of 95 and 66 at dilution 10 ⁇ 6 ; and cfu counts of 3 and 10 at dilution 10 ⁇ 7 .
  • the eluates from the test plates gave cfu counts of 43 and 38 at dilution 10 ⁇ 2 ; cfu counts of 25 and 1 at dilution 10 ⁇ 3 ; 6 and 15 at dilution 10 4 ; cfu counts of 3 and 10 at dilution 10 5 ; and cfu counts of 0 at higher dilutions.
  • Example 7 The experiment of Example 7 was repeated was repeated using the same E. CoIi Strain ATCC 25922 as the test organism, but with a 90 minute exposure to ozone/oxygen mixture of 50 ppm ozone, at 20 0 C and 80% relative humidity.
  • the eluates from control plates (duplicated) had cfu counts too numerous to count at dilution 10 ⁇ 2 , 10 "3 and 10 ⁇ 4 ; cfu counts of 563 and 350 at dilution 10 ⁇ 5 ; cfu counts of 74 and 87 at dilution 10 ⁇ 6 ; and cfu counts of 7 and 7 at dilution 10 ⁇ 7 .
  • the eluates from the test plates gave cfu counts of 13 and 28 at dilution 10 ⁇ 2 ; cfu counts of 8 and 7 at dilution 10 ⁇ 3 ; cfu counts of 7 and 5 at dilution 10 ⁇ 4 ; and 0 at all other, higher dilutions.
  • C. difficile clinical strain nontoxigenic #135, Queens University Medical School, Springfield, Canada
  • C. difficile strains anaerobic condition requirements, for example
  • the C. difficile strain was streaked on 12-20 pre-reduced Brucella blood agar plates and incubated anaerobically for 48 hours at 35 0 C. Each plate was flooded with 5 ml of sterile distilled water and the bacterial colonies gently scraped from the agar surface with a plastic sterile bacteriological loop. The resulting bacterial suspension was mixed and allowed to rest at room temperature in a sealed tube for 20 minutes to permit the osmotic lysis of the vegetative forms of the bacteria. The bacterial suspension was centrifuged at 3,000 x gravity for 20 minutes to pellet the spores and remaining bacterial cells.
  • the supernatant was discarded and the pellet re- suspended in 5 - 7 millilitres of sterile distilled water and mixed vigorously to re-suspend the spores and remaining bacterial cells.
  • the above steps were repeated three times to produce a pellet consisting of C, difficile spores.
  • the final suspension was placed in a heating block at 70 0 C for 20 minutes.
  • the spores were stored in 100% ethanol at 4 0 C. This preparation yielded approximately 1 .5 x 10 5 cfu/ml of spores. Gram stain of the spore preparation confirmed that the suspension consists of spores with very few vegetative cells.
  • Test plates were given a 90 minute exposure to ozone/oxygen mixture of 35 ppm ozone, at 21 0 C and 80% relative humidity. The subsequent incubation was for 48 hours under anaerobic conditions.
  • the eluates from control plates (duplicated) had cfu counts of 1 13 and 50 at dilution 10 "2 and 10 and 10 at dilution 10 ⁇ 3 ; whereas the eluates from the test plates showed no cfus at any dilution tested.
  • FIG. 5 An apparatus as diagrammatically illustrated in the accompanying Fig. 5 was used.
  • a chamber 100 closed while the experiments were in progress, contained near one end a frame 102 holding a layer (disc) 104 of fibrous drape material (sterile cotton gauze), impregnated with MRSA and dried so that a biofilm formed. Ozone rich atmosphere is fed into the chamber.
  • An electrical fan 106 with rotary blades 108 was disposed 3 cm from the gauze, so as to blow gases within the chamber through the gauze at high velocity, to cause physical agitation of the gauze.
  • a dish 1 10 containing an exposed, similarly impregnated gauze 1 12 was disposed near the other end of the chamber 100, so that it was exposed to essentially static atmosphere in the chamber.
  • Test bacteria namely Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa (PAU); Methicillin-Resistant Staphylococcus aureus (MRSA); Vancomycin-Resistant Enterococcus (VRE); were prepared as described for the previous experiments (see Example 1 for the preparation of the aerobic bacteria, Example 9 for the preparation of C. difficile).
  • Bacillus subtilis (the surrogate for anthrax) was prepared analogously to the preparation of C. difficile, except that the bacteria was grown on Columbia sheep's blood agar plates incubated for 18 - 24 hours in room air at 35 0 C. They were separately cultured on plates for 24 hours.
  • Some of the plates were subjected to ozone/oxygen exposure using ozone 80 ppm, 42 - 80% humidity and room temperature of about 22 0 C, for a period of 90 minutes, in the illustrated apparatus, as controls. Additional controls had no ozone or hydrogen peroxide treatment, but were prepared and exposed in the same way.
  • test plates were mounted inside the disinfection chamber 60, and treated with ozone and water vapor as previously described, but additionally using hydrogen peroxide supplied as a vapor to the chamber via port 65.
  • the disinfection chamber 60 also contained the same heater/cooler system and sensors previously described.
  • Plates treated according to the invention were exposed to 80 ppm ozone and gaseous hydrogen peroxide from a 1 % or a 3% aqueous solution, air being blown through the aqueous solution in the illustrated apparatus to create the gaseous hydrogen peroxide. Other conditions and exposure times were kept the same.
  • the stainless steel discs were vigorously mixed in 10 ml of sterile 0.85% saline using a vortex mixer at high speed for 60 seconds to elute off all surviving viable bacteria or spores.
  • the eluted suspension containing both living and dead bacteria, is serially diluted 10 fold in sterile 0.85% saline and the diluted bacteria were quantitatively plated onto Columbia sheep's blood agar plates for the aerobic bacteria or Brucella anaerobic blood agar plates for C. difficile, incubated under appropriate conditions, in triplicate so as to determine the original inoculum concentration.
  • the survivor colony counts were logarithmically transformed and the geometric mean calculated.
  • the agar plates after exposure were cultivated in an incubator for 24 hours. The plates were then stained, examined through a microscope, and the numbers of colony forming units on each plate was counted.
  • Tables 3, 4, 5, 6, 7 and 8 below provide a summary of experiments, whereby combinations of ozone, H 2 O 2 , humidity and exposure time were evaluated in terms of the ability to eliminate the following bacteria when artificially applied as a biofilm onto non-porous surfaces such as stainless steel discs: E. coli; Pseudomonas aeruginosa (PAU); Bacillus subtilis (the surrogate for anthrax). Clostridium difficile (C. difficile); Vancomycin-Resistant Enterococcus (VRE); and Methicillin-Resistant Staphylococcus aureus (MRSA), same strains as before.
  • the steel discs for testing and the agar plates for testing were prepared exposed and tested as described in the previous Example, with exposure conditions shown in the Tables below. In some cases, indicated as “chamber”, the tests were conducted as described in Example 10 and with an apparatus generally as illustrated in Fig. 4. In other cases indicated as "room”, the tests were conducted by exposing the disks and plates in a closed room, as generally illustrated in Fig. 1 .
  • one aspect of the invention is a process for disinfecting a room, which comprises introducing into the room an oxygen/ozone gas mixture, raising the pressure within the room above atmospheric pressure, physically agitating fibrous and porous surfaces within the room while the surfaces are exposed to the ozone containing atmosphere of relative humidity at least 65%, returning the room to atmospheric pressure, and removing the residual ozone from the room's atmosphere, down to a maximum level of 0.04 ppm.
  • Another aspect of the invention is a portable system for disinfecting rooms and surfaces therein with ozone, comprising an oxygen container, an ozone generator fed with medical grade oxygen from the oxygen container and discharging a mixture of oxygen and ozone, an ozone controller adapted to control the proportion of ozone in the mixture of oxygen and ozone, a discharge tube to receive the mixture of oxygen and ozone from the ozone generator, the discharge tube having an outlet end, a physical agitation system at the outlet end of the discharge tube, for physical agitation of surfaces with oxygen/ozone mixture issuing therefrom, pressure adjusting means connected to the ozone generator arranged to adjust the pressure of the oxygen/ozone mixture discharged by the physical agitation system and the oxygen/ozone gas pressure in the room under treatment, temperature adjusting means connected to the ozone generator arranged to adjust the temperature of the oxygen/ozone mixture discharged by the physical agitation system, humidity adjusting means adapted to humidify the treatment location to a relative humidity not less than 65%, and an ozone

Abstract

A system and process for disinfecting rooms such as health care facility rooms with oxygen/ozone mixture is described, which is effective to combat "superbugs" such as Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); and vancomycin-resistant Enterococcus (VRE). In preferred embodiments, hydrogen peroxide is additionally used. The system and process is effective to destroy bacteria deposited on surfaces as biofilm, and, accompanied by physical agitation such as jet nozzle outlets, is effective to disinfect carpet, drapery and similar absorbent and porous surfaces.

Description

HEALTHCARE FACILITY DISINFECTING PROCESS AND SYSTEM WITH
OXYGEN/OZONE MIXTURE
FIELD OF THE INVENTION
This invention relates to disinfecting systems for use in healthcare facilities, public health facilities and the like, to eliminate or at least to reduce to acceptable levels, microbial residues which are resistant to conventional disinfectant and sterilization systems.
BACKGROUND OF THE INVENTION
Despite intensive preventive efforts over the past several years in hospital and other healthcare facilities, the incidence of life threatening infections caused by a growing array of antibiotic resistant bacteria (sometimes referred to as "superbugs") has grown significantly and is now posing a serious problem for medical staff world wide. According to an editorial in the journal "Science" (July 2008), the number of deaths in 2006 attributable to bacterial infections in healthcare facilities in the United States exceeded the U.S. death toll attributed to HIV/AIDS in the same year, and probably result in as many as 70,000 deaths per year in the United States. This is despite the best efforts of healthcare personnel properly to clean their facilities and the equipment contained therein.
The major causative agents (bacteria) for hospital-based infections (nocosomial infections) are Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); and vancomycin-resistant Enterococcus (VRE).
Approximately 5% of all acute care hospitalizations in the U.S. develop a nosocomial infection with an incidence rate of five infections per thousand patient days, and an added expenditure in excess of $4.5 billion (Wentzel R, Edmond M D, "The Impact of Hospital Acquired Blood Stream Infections," Emerg. Inf. Dis., Mar-April 2001:7(174)). When this rate is applied to the 35 million patients admitted to 7,000 acute-care institutions in the U.S., it is estimated that there are more than 2 million cases per year. Nocosomial infections are estimated to double, at least, the mortality and morbidity risks of any admitted patient.
The significant, and growing, incidence of antibiotic resistant bacteria in healthcare facilities has been termed by some as a "Silent Epidemic". On the international scene, a World Health Organization survey of 55 hospitals in 14 countries representing four WHO regions (Europe, Eastern Mediterranean, South-East Asia and Western Pacific) reported that an average of 8.7% of hospital patients had nocosomial infections. The WHO estimates that, at any time, over 1 .4 million people worldwide suffer from infection acquired in hospital.
Of particular concern in this context are the bacteria C difficile and MRSA. Until recently, C difficile was relatively uncommon, but has now become epidemic in many regions of the world. Indeed, it is now recognized by a growing number of public health officials as a worldwide epidemic (pandemic) with incalculable financial and health implications. MRSA has been identified by the American Academy of Orthopaedic Surgeons as the single biggest concern for surgical procedures, and concurs with recent journal articles that it constitutes a "silent epidemic." Under current healthcare facility cleaning and sterilizing procedures, both C difficile and MRSA, as well as the aforementioned E. coli; Pseudomonas aeruginosa; and vancomycin-resistant Enterococcus (VRE), are ineffectively treated and subsequently removed, so that colonies of these pathogens accumulate in healthcare facilities, especially on porous surfaces such as carpets and drapes.
Attempts to combat and kill nosocomial infections caused by bacteria such as Pseudomonas aeruginosa and Staphylococcus aureus are hampered by the fact that the bacteria grow within biofilms that protect them from adverse environmental factors. A biofilm is an aggregate of microorganisms in which cells adhere to each other and/or to a surface. They are frequently embedded in a self produced matrix of extracellular polymeric substance (EPS), a polymeric conglomeration generally composed of extracellular DNA, proteins and polysaccharides. Biofilms form on surfaces, e.g. in hospital settings, in the presence of water vapour.
Free floating microorganisms in planktonic (single cell) mode attach to a surface, and if not immediately removed, will anchor themselves more permanently to the surface. These first colonists provide more diverse adhesion sites for the arrival of other cells, thus beginning to build a matrix that holds the biofilm together and provides additional anchoring sites for arriving cells. The biofilm grows through a combination of cell division and recruitment. When the biofilm is established, the aggregate cell colonies are apparently increasingly antibiotic resistant. It has also been reported that biofilm bacteria apply chemical weapons to defend themselves against disinfectants and antibiotics (see "Biofilm Bacteria Protect Themselves With Chemical Weapons", Dr. Carsten Matz et. al., Helmholtz Cetre for Infection Research, Brauschweig, reported on lnforniac.com, July 23, 2008).
Bacteria living in a biofilm have significantly differently properties from the planktonic form of the same species, as the dense and protected environment of the film allows them to co-operate and interact in various ways. Traditional antibiotic therapy is usually not sufficient to eradicate chronic infections, and one major reason for their persistence seems to be the capability of the bacteria to grow within biofilms that protect them from adverse environmental factors.
Also of growing concern are threatened bioterrorist and warfare attacks using potentially lethal bacteria. Some of the deadliest bacteria, for example anthrax, are highly resistant to conventional sterilization agents and treatments. Contamination of public facilities with such bacteria constitutes a significant threat to human life with residual amounts of such bacteria being almost impossible to remove using current methods. BRIEF REFERENCE TO THE PRIOR ART.
Current procedures for the sanitization of hospitals and other healthcare facilities have become increasingly ineffective, resulting in the accumulation of deadly bacteria throughout the facilities. Rising costs of the provision of healthcare in most if not all countries militate against spending more than the minimum time and effort on cleaning and sterilizing procedures.
Chlorinated solutions with and without ammonia are commonly used, but have shown only limited success. To add to this challenge, such solutions cannot be used on electronic devices commonly installed in wards, recovery rooms, operating theaters, etc.
Vaporized hydrogen peroxide (VHP) is highly effective when applied to smooth surfaces, but has little or no efficacy on porous materials and fabrics. Moreover, VHP is very damaging to electronic devices.
Once a non-medical surface such as carpet, drapery, bedding, porous material in ceilings and the like become impregnated with highly resistant pathogens, especially spore formers such as C difficile, they cannot be effectively disinfected using currently available agents and processes.
Ozone is known to be a powerful anti-bacterial, anti-fungal and anti-viral agent. For over 100 years, it has been used for water purification. It is known to be effective against Legionella Bacteria, E. coli and pseudomonas populations in such plants.
Ozone use in healthcare facilities is, however, problematic. Solutions containing ozone are explosive on warming. Ozone is medically harmful to those exposed to it, causing irritation of eyes and mucous membranes, pulmonary edema, and chronic respiratory disease if low, safe levels of exposure are exceeded. Moreover, it is widely recognized to be an environmental hazard. Canadian Patent Application 2,486,831 Arts et. al., discloses the use of a combination of ozone and UV radiation for decontamination of air in a room such as a mobile isolation unit, a hospital room and the like. The air is caused to flow through a portable unit containing a filter exposed to ozone.
U.S. Patent 7,404,624 Cumberland et.al., issued August 5, 2008, describes methods for abating allergens, pathogens, odours and volatile organic compounds in air, using an atmosphere having specific combinations of ozone concentration, hydrogen peroxide concentrations, temperature and humidity delivered over a specified period of time. The patent contains an experimental account of treating rooms of a residence, effectively treating cladosporium mold spores and penicillium/aspergillus molds in the room air. No details of the precise conditions used are given. There is no demonstration or disclosure of treatment of contaminated surfaces in a room. The general disclosure of the patent states that selected conditions of ozone concentration, hydrogen peroxide, humidity and temperature are highly effective in killing airborne molds and fungi at ozone concentrations below 6 - 9 ppm, but the precise conditions used are not disclosed. In general, the patent teaches use in an atmosphere of 2 - 10 ppm ozone, hydrogen peroxide which is 75% - 150% by weight of the atmospheric ozone concentration, at a temperature of 15 - 27°C and time 0.5 - 3 hours. Many other airborne pathogens, including bacteria, are said to be treatable by this method, but no experimental evidence is offered.
There is thus a need for an effective but inexpensive system for disinfecting rooms of healthcare facilities, including all the contents therein. Such a system should drastically reduce (99.999% or greater) the amounts of at least the five aforementioned bacteria in all contaminated spaces to be of clinical and public health value. Furthermore, this level of microbial decontamination must be achieved such that the space is only removed from healthcare use for a minimum period of time, while remaining safe and harmless with respect to electronic and other equipment in the room. Accordingly, the decontamination process should not require that the space in question be emptied of its contents while the system is operated.
SUMMARY OF THE INVENTION
The present invention provides, from one aspect, an ozone-based disinfection system for rooms and their contents within all healthcare facilities, mobile or stationary, and other critical infrastructure such as schools and government buildings. Using such a system, ozone-containing gases are delivered into and applied to the surfaces and equipment and objects contained within the room. The application can be through simple contact of the gaseous atmosphere with the surfaces, or, in the case of difficult-to-clean surfaces such as drapes, carpets and other fibrous surfaces, it can be by means of a dislodgement system effecting physical agitation of the surface (scrubbing brushes, high pressure jets or the like, sometimes referred to herein as "scrubbing"). The ozone-containing gases are applied at controlled concentrations and, in some cases, elevated pressures which have been found to be effective in destroying critical viral, bacterial and fungal pathogens found in environments, including but not limited to the five especially troublesome bacteria Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); and vancomycin-resistant Enterococcus (VRE).
In addition to effectively eliminating aerosolized pathogens within a given space, the system of the invention also allows an operator to apply the ozone-containing gases at predetermined concentrations of ozone directly to problem surfaces in the room, with a physical agitation action and under pressure where appropriate. The system also includes an ozone-destruct unit for removing residual ozone from the room atmosphere. The whole system is portable, so that it can be moved from room to room as required, and is harmless to equipment contained in the room. Once the sterilization process is completed, the room can be back in medical use within 20 minutes, with its residual atmospheric ozone level at an acceptable 0.04 ppm or less.
BRIEF REFERENCE TO THE DRAWINGS
Figure 1 of the accompanying drawings is a diagrammatic illustration of an apparatus in accordance with an embodiment of the invention, disposed within a room to be disinfected;
Figures 2A and 2B are diagrammatic illustrations of physical agitation systems for use in embodiments of the invention;
Figure 3 is a diagrammatic illustration of an apparatus according to the invention, in portable, transportation mode;
Figure 4 is a diagrammatic illustration of a test apparatus used to generate some of the test results reported below;
Figure 5 is a diagrammatic illustration of the test apparatus used to generate the results reported in Example 10 below.
THE PREFERRED EMBODIMENTS
One significant feature of the system according to certain embodiments of the invention is the ability to adjust the pressure of the ozone/oxygen gas mixture being used for disinfection purposes. It has been found that, in many cases, effective disinfection of a room and its contents from bacterial contamination can best be achieved by pressurizing the atmosphere in the room with ozone/oxygen mixture containing from about 10 to about 100 ppm of ozone, to a pressure higher than normal atmospheric pressure, e.g. from about 14.7 psi to about 100 psi. A localized pressurized air jet can also be used, which would obviate the need to raise the overall pressure in the room. Raising the room pressure may require initial sealing of the room prior to the decontamination process. With many rooms where medical procedures are conducted, such as operating theatres, this is a simple process, since such rooms are designed to be substantially sealed when in use for medical procedures. With other rooms, this may require some significant initial preparation.
Another, particularly preferred embodiment of the invention utilizes hydrogen peroxide, as well as ozone, in the disinfecting gaseous atmosphere. When using ozone and hydrogen peroxide, increasing the pressure within the room may not be necessary. The particularly troublesome bacteria which are likely to cause nosocomial infections in a hospital environment, namely Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); vancomycin-resistant Enterococcus (VRE), deposit on surfaces in a hospital environment such as stainless steel surfaces, ceramic surfaces and marble surfaces and quickly form a biofilm in which the microorganisms thrive. Treatment with the combination of hydrogen peroxide and ozone, at appropriate humidity, according to this preferred aspect of the invention, destroys the bacteria in the biofilm, either by chemically attacking the biofilm to expose the microorganisms to the biocidal action of the ozone and hydrogen peroxide, or by interference of the bacterial cells' activity in the biofilm by the ozone/hydrogen peroxide combination employed, or by a combination of these, possibly with other, mechanisms.
Thus according to this preferred embodiment of the present invention, from one aspect, there is provided a process of combating bacteria in an enclosed space within a room and contained in biofilm on surfaces within the room, which comprises: creating in the room a disinfecting atmosphere which includes ozone at a concentration of 2 - 350 ppm by weight and hydrogen peroxide at an amount of 0.2 - 10 wt. %, at a relative humidity of at least 60%; exposing the biofilm carrying surfaces having live bacteria therein to the disinfecting atmosphere for a period of at least 30 minutes sufficient for an effective kill of the bacteria in the microfilm; and subsequently removing ozone from the atmosphere, down to 0.04 ppm or less.
Preferably the disinfecting atmosphere has a relative humidity of at least 65%.
Another preferred embodiment provides a process for disinfecting a room and surfaces therein to combat at least one of the microorganisms bacteria Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); vancomycin-resistant Enterococcus (VRE); Bacillus subtilus, and/or anthrax, which comprises exposing the room and surfaces therein to a gaseous atmosphere which includes an effective amount of ozone and an effective amount of hydrogen peroxide, for a period of time which substantially reduces levels of bacteria on the surfaces, and subsequently removing the residual ozone in the room's atmosphere, down to a safe low level.
The process is particularly effective with or without physical agitation, in disinfection of stainless steel surfaces which abound in medical treatment facilities, and on which bacteria are tenacious and difficult to destroy, due at least in part to their generation of a biofilm on such surfaces. The process is also effective in destroying and deactivating anthrax bacteria, as evidenced by its effectiveness against the well-established anthrax surrogate, Bacillus subtilis.
According to another aspect of this embodiment, there is also provided a portable system for rapidly disinfecting rooms, surfaces and equipment therein, comprising:
an ozone generator for discharging into the room a gaseous mixture including ozone; an ozone controller adapted to control the amount of discharged ozone; a source of hydrogen peroxide for discharging controlled amounts of hydrogen peroxide into the room; means for discharging the hydrogen peroxide and ozone into the room; humidity adjusting means adapted to increase or decrease the relative humidity of the room during treatment; and an ozone remover adapted to destroy ozone, down to a safe level in the room atmosphere for subsequent human utilization.
It is sometimes beneficial, to increase the effectiveness and shorten the duration of the process, to operate at elevated pressure, even when using both ozone and hydrogen peroxide in the disinfecting gas. Thus, according to another aspect of the present invention, there is provided a process for disinfecting a room of a healthcare facility, which comprises: introducing into the room a gas mixture which includes ozone and hydrogen peroxide in effective amounts; raising the pressure within the room above atmospheric pressure, or introducing a pressurized gas stream; physically agitating fibrous and porous surfaces within the room while the surfaces are exposed to the pressurized gas stream of hydrogen peroxide and ozone containing atmosphere of relative humidity at least 60%; returning the room to atmospheric pressure; and, removing the residual ozone from the room's atmosphere, down to a safe level. Preferred ozone amounts are from about 20 - 350 parts per million in the treatment gas atmosphere, more preferably 20 - 200, even more preferably 20 - 90 parts per million in the oxygen/ozone gas mixture, and most preferably 35 - 80 ppm ozone. Preferred amounts of hydrogen peroxide are the amounts supplied to the room treatment atmosphere using an aqueous solution containing 0.2 - 10%, more preferably 1 - 5%, hydrogen peroxide. In the description below, the peroxide percentages used are sometimes expressed in terms of these solution percentages. The amounts are chosen so that no serious deleterious effects are suffered by other equipment in the treatment room. The amount of hydrogen peroxide in the disinfecting atmosphere can be calculated from the volume of aqueous hydrogen peroxide evaporated into the disinfecting atmosphere, the volume of the room being disinfected and the concentration of hydrogen peroxide in the starting solution. Times of exposure of the room and its surface to the ozone-containing atmosphere are suitably from 30 minutes to about 120 minutes, preferably from about 60 to about 105 minutes, and most preferably about 90 minutes. These times are constrained to some extent by the need to clear the room of ozone (down to a maximum of 0.04 ppm) following the disinfection phase, and return the room to medical use within a reasonable period of time, with the entire start-to-finish time not exceeding 150 minutes. The ozone removal is an extremely rapid and fully effective process. Both the hydrogen peroxide and the ozone (and any products of interaction between them) should be removed before the room is put back into normal use.
Another significant feature of preferred embodiments of the present invention is the provision of a dislodgement system at the outlet end of the discharge. The dislodgement system allows penetration of carpet, drape and similar surfaces in the room, to gain access to concealed/sequestered spores and/or colonies of bacteria. The dislodgement system can be manually operated, with operators protected by a hazard suit and mask, or remotely operated or totally automated. It may take the form of one or more outlet jets, with associated manually operable jet pressure controls. It may take the form of a revolving or fixed brush with bristles of appropriate stiffness, alone or in combination with an outlet jet. Any form of dislodgement system effective to disturb the pile of carpet fabrics, upholstery fabrics and the like so as to access the remote parts which might harbor bacterial spores or colonies can be used. This includes non-physical applications such as air jets, ultrasonic energy, radio-frequency energy and electromagnetic waves, for example, capable of causing physical disruption and which result in micro-physical movements of fibrous surfaces.
The ozone for use in the present invention can be generated by any known means. In the case of corona or other electrical discharge generation from oxygen, the apparatus of the invention preferably includes a container of medical grade oxygen. The oxygen container can be a standard, pressurized vessel containing medical grade oxygen, of the type commonly found in medical facilities. Oxygen from this container is fed to an ozone generator, where the oxygen is subjected to electrical discharge, normally with high voltage alternating current, to convert small amounts of the oxygen to ozone and produce a gaseous mixture of oxygen and ozone. The quantity of ozone in the mixture is controllable by adjustment of the voltage of the electrical discharge. Suitable ozone generators are known and available commercially. The relative amounts of ozone generated are relatively small, expressed in parts per million (ppm), but such is the power of ozone as a disinfectant, especially in combination with hydrogen peroxide in accordance with this invention, that such small quantities thereof are all that is required.
Alternative forms of ozone generation can be used if preferred. Ultraviolet radiation of appropriate wavelength, incident upon oxygen or air, is one acceptable alternative. In such a system, air from the room itself may be fed into the ozone generating unit to supply the required oxygen for conversion to ozone. Other methods of ozone generation which can be used include photocatalytic reactions, cold plasma, etc. The relative humidity of the treatment space should be at least 60% and preferably at least 65%, for effective disinfection. To ensure this, it is preferred to incorporate a humidifier in the system of the invention, using sterile water from an internal system reservoir to adjust and control the humidity of the issuing gas mixture. In this way, desirable humidity for most effective disinfection is achieved at the point of discharge where dislodgement of a carpet or drapery surface can take place. The adjustable humidifier need only increase the humidity of the space to the desirable level and can be placed in any location within the space. When using hydrogen peroxide in addition to ozone, the hydrogen peroxide vapor is suitably applied, in controlled amounts, to the air/water vapor issuing from the humidifier and thus added to the ozone/oxygen containing gas mixture. Alternatively, hydrogen peroxide can be applied to the water used to humidify the target location. Hydrogen peroxide is commercially available as aqueous solutions of standard concentrations of hydrogen peroxide. For use in embodiments of the present invention, a standard solution of known peroxide concentration is suitably diluted down by a fixed volume of distilled water. The peroxide load is standardized based on the known volume of water from the peroxide solution required to raise the relative humidity to the desired extent, e.g. from 40 - 80%. From this, the amount of hydrogen peroxide in volume % or ppm by volume introduced into the treatment facility can be calculated.
Certain systems according to embodiments of the invention may include a temperature adjuster and controller for the gas mixture. This can be a simple heater/cooler through which either the incident oxygen or the generated oxygen/ozone mixture passes prior to discharge into the room atmosphere. While simple adjustment of the temperature of the room using an external room heating system and thermostat can be effective, it is preferred to adjust the temperature of the issuing gas mixture, for most effective treatment of the carpet and drapery surfaces. The ideal range of temperature for ozone and ozone/hydrogen peroxide decontamination of pathogens is 150C to 300C. The system of the invention also includes an ozone removal unit. Such units are known, and can be purchased commercially for use in the present invention. Depending on the volume of the room atmosphere and the capacity of the ozone removal unit, more than one such unit may be incorporated in the system of the invention. Suitable ozone removal units are those based on activated carbon as the removal medium. These act very quickly, and do not lead to the formation of hazardous reaction products. The inclusion of such units enables the treated facility to be cleared of ozone and returned to normal use rapidly, an important feature where health care facilities are involved. Other types include systems based on catalysts such as manganese oxide or other metal oxides, which may be heated to remove moisture, thermal destruction in conjunction with other metals including platinum or palladium.
Fig. 1 of the accompanying drawings shows a patient room surgical suite 10, closed ready for disinfection by a process according to an embodiment of the invention. The suite is substantially hermetically sealed. Inside the suite is a pressurized cylinder 12 of oxygen, feeding oxygen gas into a humidifier 14 and thence to an ozone generator 16, which includes electrical discharge plates of variable voltage to adjust the quantity of ozone which is generated. A heater and a pressure controller (not shown) may be disposed near the entrance to the ozone generator. Output of oxygen/ozone gas mixture is via room outlets 18, 20 to the atmosphere of the suite 10, and via wands 22A and/or 22B to a dislodgement means in the form of scrubbing brushes 24A and 24B mounted on the outlet ends of the respective wands 22A, 22B. The heater, the pressure controller, the voltage supplied to the ozone generator 16 and the humidity level supplied by the humidifier 14 are all controlled and adjusted from an external control panel 26 via respective electrical connections 28, 30, 32 and 34. Also disposed within the suite is an oscillating fan 34 and an ozone destruct filter unit 36.
Disposed within the suite 10 is a container of aqueous hydrogen peroxide solution 19 and associated air blower 21 which, during operation, blows vaporized hydrogen peroxide in controlled amounts into discharge wand 22A and 22B to mix with the output of ozone/oxygen therein. The amount of hydrogen peroxide being supplied is controlled by adjustment of the blower 21 through a connection thereof to the control panel 26. In an alternative arrangement, hydrogen peroxide can be supplied from generator 19 to the humidifier 14.
Figs. 2A and 2B of the accompanying drawings show in more detail forms of dislodgement means 24A and 24B for use in the present invention, attached to the outlet, discharge ends of respective wands 22. The dislodgement means 24A has a jet outlet nozzle 38A at its extremity, and a generally circular plate 40 mounted on the wand 22A near the discharge end. The wand 22A passes through a central aperture 42 in a plate 40. The plate 40 has brush bristles 46A mounted on its lower surface, arranged in two arcs around the jet outlet nozzle 38A and protruding downwardly to an extent just beyond the extent of outlet from nozzle 38A. In use, oxygen/ozone gas mixture or oxygen/ozone/hydrogen peroxide gas mixture issues from nozzle 38A at relatively high pressure, and can be directed by the operator holding the wand to a carpet surface area while at the same time the operator scrubs the carpet surface area with the bristles 46A.
Fig 2B shows an alternative but essentially similar arrangement, in which plate 40 is replaced by a wheeled platform 44 carrying two rotary brushes 46B and three jet outlets 38B for the oxygen/ozone/hydrogen peroxide delivery at pressure, located forwardly of the rotary brushes 46B.
Figure 3 of the accompanying drawings illustrates the portability of a system according to the invention. Parts are numbered as in Fig. 1 . A 4-wheeled cart 48 is provided, on which all the component parts of the system can be loaded for ease of transportation from one room to another. The instrumentation and control panel can be disconnected for transportation, and re-connected and disposed outside when the apparatus is placed in another room for use as shown in Fig. 1 . The cart 48 is removed while the system is in use, but is loaded with the components after use, either for transportation to another room or for storage.
The operation of the system will be readily apparent from the preceding description of its component parts and their inter-connection. The cart 48 carrying the component parts is wheeled into the room 10 to be disinfected, and the parts are distributed around the room and connected together as illustrated in Fig. 1 . An operator wearing a hazard suit and other appropriate protective clothing enters the room and holds the wand 22. The room is sealed. Conditions of treatment are set on the control panel 26, and the apparatus is switched on so that oxygen/ozone/hydrogen peroxide gas mixture at controlled ozone concentration, hydrogen peroxide concentration, relative humidity, temperature and elevated pressure issues from jet nozzle 38. The operator applies the jetted gas mixture to the carpet surfaces, drapery surfaces and other absorbent surfaces in the room, scrubbing the surfaces at the same time with the bristles 46. The room becomes pressurized above atmospheric pressure, due to the introduction of the oxygen/ozone gas mixture. Pressure is continually monitored by the control panel 26 to ensure safe working conditions for the operator, as well as the temperature, humidity and ozone concentration in the room. Smooth surfaces in the room may not need the action of the dislodgement means, but are satisfactorily disinfected by contact with the atmosphere in the room, especially when hydrogen peroxide and ozone are used in combination. The oscillating fan 34 is operated throughout the procedure, to circulate the oxygen/ozone mixture throughout the room.
After a pre-set time of the procedure, and after all the appropriate, absorbent surfaces have been scrubbed, a time not normally exceeding 90 minutes, the hydrogen peroxide supply (if used), the oxygen supply and ozone generator are switched off. Then the ozone destruct filter is operated, sucking in the ozone-containing gases, destroying the ozone and issuing pure oxygen from it. The room can now be opened, the apparatus disconnected and loaded on the cart 48, and the room put back to its normal use.
EXPERIMENTAL EXAMPLES
Effective and optimum conditions for use in the present invention were determined using a laboratory apparatus as generally illustrated in Fig. 4 of the accompanying drawings.
A single pure colony of each aerobic test bacteria, namely E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); and vancomycin-resistant Enterococcus (VRE) was inoculated to a Columbia agar plate with 5% sheep's blood. They were incubated at 350C in room air for 18 - 24 hours. From the plate, 4-5 isolated colonies were selected, and suspended in tryptic soy broth to achieve a 0.5 McFarland turbidity standard (1 .5 x10 8 cfu/ml) measured using a spectrophotometer. Inoculum was prepared by performing a series of serial dilutions of 0.9 ml 0.85 NaCI broth with 0.1 ml of original 0.5 McFarland inoculum (6 x 10 fold) to give solutions of 10"1, 10'2, 10'3, 10' 4, 10 5, 10"6 and 10"7 cfu/mL
Organisms were plated out in triplicate, 0.1 ml of each solution being spread over the surface of Columbia sheep's blood agar plates. Two sets of plates (12 plates per organism) were subjected to ozone/oxygen exposure at preselected concentrations of ozone (ppm), humidity and temperature conditions in the illustrated apparatus. The other sets of 2 were treated as controls, with no ozone exposure, but kept at room temperature.
For ozone exposure, the apparatus generally illustrated in Fig. 4 was used.
The test plates were mounted inside a disinfection chamber 60, the upstream end 62 of which had an ozone inlet port 64, a hydrogen peroxide vapor inlet port 65 (which in Examples 1 - 9 described below was blocked), and a water vapor inlet port 66. A cylinder 68 of pressurized medical grade oxygen was provided, feeding oxygen to an ozone generator 70, equipped with alternating current electrical plates to which variable voltage could be supplied via input control 72. The output of oxygen/ozone mixed gas from the ozone generator 70 was fed to the ozone inlet port 64 of the disinfection chamber 60. A water vapor humidifier 74 supplied water vapor to inlet port 66. The disinfection chamber 60 also contained a heater/cooler (not shown), a temperature sensor 76, a pressure sensor 78, a humidity sensor 80 and an ozone sensor 82, connected electrically via respective lines 84, 86, 88 and 90 to a control panel and monitor 92, connected to feed back to the oxygen cylinder 68 to control flow for pressure adjustment purposes, to the ozone generator 70 to control and adjust the ozone quantity, to the water vapor humidifier 74 to control and adjust relative humidity in the disinfection chamber 60, and to the heater/cooler to control and adjust the temperature in the chamber. These parameters were all pre-set on the control panel to desired values and automatically re-adjusted themselves to these values as the experiments progressed.
An ozone destruct filter 94 was connected to the downstream end 96 of the disinfection chamber 60 at outlet port 98, to destroy ozone issuing from the chamber 60 at the end of the experiment. Gases were circulated within the chamber 60, and expelled therefrom at the termination of the experiment, using a fan 100 mounted therein. After placing the test plates in the chamber 60, it is sealed until the end of each experiment.
The control plates and the ozone treated plates were placed in an incubator at the same time. The plate counts were read through a microscope, and the numbers of colony forming units on each plate was counted. The spores are aerotolerant.
EXAMPLE 1
A series of tests as described above was conducted on MRSA ATCC 33592. The microorganism-bearing dishes were exposed in the chamber to an oxygen/ozone mixed atmosphere containing 80 ppm ozone, for 90 minutes at 200C and 85% relative humidity. Duplicate test plates were run. 10 μl_ volume aliquots washed off the plates were serially diluted with inoculum, to final dilution factors 10~2, 10~3, 10~4, 10~5, 10~6 and 10~7. Control plates, not subjected to ozone exposure, were prepared, and the plates incubated for 24 hours as described. The surfaces of the agar plates were eluted to remove the bacterial colonies, and the eluates plated out for examination under a microscope.
Counting of the active, reproducing colonies of bacteria in the eluate compositions, under a microscope, revealed that the eluates from control plates at dilutions 10~2, had 19 and 1 1 cfus (duplicate plates), and no cfus from plates of higher dilution, whereas the experimental, ozone-exposed plates yielded compositions exhibiting no cfus at any of the tested dilutions. A 3.35 log reduction was achieved (8.3 log to 4.9 log).
EXAMPLE 2
The experiment of example 1 was repeated using the same bacterial strain, but exposing the test plates in the chamber to 50 ppm ozone in oxygen, at 2O0C and 80% relative humidity.
Counting of the active, reproducing colonies of bacteria in the eluate compositions, under a microscope, revealed that the eluates from control plates at dilutions 10~2, had 374, 415, 414 and 423 cfus (quadruplicated plates), 33, 35, 38 and 37cfus from control plates at dilutions 10~3, had 4, 1 , 2 and 2 cfus at dilution 10~4 and no cfus at higher dilutions. Those from the eluates of treated plates revealed 27, 1 1 , 42 and 58 active cfus at dilutions 10~2, 3, 1 , 3 and 5 cfus at dilution 10~3 (quadruplicate plates), and no cfus from plates of higher dilution.
EXAMPLE 3
The experiment of Example 1 was repeated, except for using as test organism P. aeruginosa ATCC 27853. The same conditions of ozone exposure, dilution, incubation and testing were used. On the test plates, active colony counts of 1 1 and 18 were found at 10~2 dilution, and active colony counts of 5 and 27 were found at 10~3 dilution. At higher dilutions, there were no detectable colonies. In contrast, the control, non-ozone exposed plates showed colonies too numerous to count, at all dilutions up to and including 10~6. A 2.8 log reduction was achieved (7.9 log to 5.1 log).
EXAMPLE 4
The experiment of Example 3 was repeated, using the same test organism, but treating the test samples in the chamber with ozone/oxygen gas mixture containing 50 ppm ozone, at 80% humidity, for 90 minutes. By the same recovery and test procedures, it was determined that the control plates had cfus too numerous to count. The test plates, run in duplicate, had cfu counts of 212 and 183 at dilution 10'2; counts of 13 and 50 at dilution 10'3; and no cfus at higher dilutions.
EXAMPLE 5
The experiment of Example 3 was repeated but using Enterrococcus faecalis (high level vancomycin resistant) Clinical Strain 80269 as the test organism, with 90 minute exposure to ozone/oxygen mixture of 35 ppm ozone, at 21 0C and 80% relative humidity. The eluates from control plates (duplicated) had cfu counts of too numerous to count at dilution 10~2 , 10~3 and 10~4 ; cfu counts of 402 and 346 at dilution 10~5; cfu counts of 35 and 25 at dilution 10~6; and cfu counts of 14 and at dilution 10~7. In contrast, the eluates from the test plates (duplicates) gave cfu counts of 78 and 29 at dilution 10~2 ; cfu counts of 47 and 6 at dilution 10~3; 1 12 and 50 at dilution 10~4 ; cfu counts of 0 and 1 at dilution 10~5 ; cfu counts of 1 and 0 at dilution 10~6; and cfu counts of 0 and 1 at dilution 10~7. A 2.95 log reduction was achieved (7.7 log to 4.7 log). EXAMPLE 6
The experiment of Example 5 was repeated using the same VRE Clinical Strain as the test organism, but with 90 minute exposure to ozone/oxygen mixture of 50 ppm ozone, at 200C and 80% relative humidity. The eluates from control plates (duplicated) had cfu counts of too numerous to count at dilution 10~2 , 10"3 and 10~4 ; cfu counts of 369 and 359 at dilution 10~5; cfu counts of 46 and 46 at dilution 10~6; and cfu counts of 9 and 2 at dilution 10~7. In contrast, the eluates from the test plates (duplicates) gave cfu counts of 50 at dilution 10~2; cfu counts of less than 30 at dilution 10~3; and cfu counts of 0 at higher dilutions 10~5.
EXAMPLE 7
The experiment of Example 3 was repeated but using E. CoIi Strain ATCC 25922 as the test organism, with 90 minute exposure to ozone/oxygen mixture of 35 ppm ozone, at 21 0C and 80% relative humidity. The eluates from control plates (duplicated) had cfu counts of too numerous to count at dilution 10'2, 10'3 and 10'4; cfu counts of greater than 300 at dilution 10'5; cfu counts of 95 and 66 at dilution 10~6; and cfu counts of 3 and 10 at dilution 10~7. In contrast, the eluates from the test plates (duplicates) gave cfu counts of 43 and 38 at dilution 10~2; cfu counts of 25 and 1 at dilution 10~3; 6 and 15 at dilution 104; cfu counts of 3 and 10 at dilution 10 5; and cfu counts of 0 at higher dilutions.
A 3.22 log reduction (7.8 log to 4.6 log) was achieved. EXAMPLE 8
The experiment of Example 7 was repeated was repeated using the same E. CoIi Strain ATCC 25922 as the test organism, but with a 90 minute exposure to ozone/oxygen mixture of 50 ppm ozone, at 200C and 80% relative humidity. The eluates from control plates (duplicated) had cfu counts too numerous to count at dilution 10~2, 10"3 and 10~4; cfu counts of 563 and 350 at dilution 10~5; cfu counts of 74 and 87 at dilution 10~6; and cfu counts of 7 and 7 at dilution 10~7. In contrast, the eluates from the test plates (duplicates) gave cfu counts of 13 and 28 at dilution 10~2 ; cfu counts of 8 and 7 at dilution 10~3; cfu counts of 7 and 5 at dilution 10~4 ; and 0 at all other, higher dilutions.
EXAMPLE 9
A strain of C. difficile (clinical strain nontoxigenic #135, Queens University Medical School, Kingston, Ontario, Canada) was also used as a test organism, but owing to the well-known difficulties with growing C. difficile strains (anaerobic condition requirements, for example), a somewhat different preparatory method was adopted.
The C. difficile strain was streaked on 12-20 pre-reduced Brucella blood agar plates and incubated anaerobically for 48 hours at 350C. Each plate was flooded with 5 ml of sterile distilled water and the bacterial colonies gently scraped from the agar surface with a plastic sterile bacteriological loop. The resulting bacterial suspension was mixed and allowed to rest at room temperature in a sealed tube for 20 minutes to permit the osmotic lysis of the vegetative forms of the bacteria. The bacterial suspension was centrifuged at 3,000 x gravity for 20 minutes to pellet the spores and remaining bacterial cells. The supernatant was discarded and the pellet re- suspended in 5 - 7 millilitres of sterile distilled water and mixed vigorously to re-suspend the spores and remaining bacterial cells. The above steps were repeated three times to produce a pellet consisting of C, difficile spores. To kill any remaining vegetative bacteria, the final suspension was placed in a heating block at 700C for 20 minutes. The spores were stored in 100% ethanol at 40C. This preparation yielded approximately 1 .5 x 105 cfu/ml of spores. Gram stain of the spore preparation confirmed that the suspension consists of spores with very few vegetative cells.
Serial 10 fold dilutions of the spore suspension in sterile 0.85% NaCI were conducted as previously described, and then inoculation was conducted by spreading 0.1 ml of each dilution over the surface of BAK agar plates. The yield of C. difficile spores was about 6 x 104 -2 x 106 cfu/ml. Some plates were exposed to ozone in the illustrated apparatus as previously described, others were kept as controls.
Test plates were given a 90 minute exposure to ozone/oxygen mixture of 35 ppm ozone, at 21 0C and 80% relative humidity. The subsequent incubation was for 48 hours under anaerobic conditions. The eluates from control plates (duplicated) had cfu counts of 1 13 and 50 at dilution 10"2 and 10 and 10 at dilution 10~3; whereas the eluates from the test plates showed no cfus at any dilution tested.
A 4 log reduction (4 log to zero) was achieved. EXAMPLE 10
Experiments conducted to simulate the problems commonly faced in most modern hospitals related to decontaminating textiles such as carpets and drapes have clearly demonstrated the superior efficacy of direct pressurized air flow over a more static gaseous environment. An apparatus as diagrammatically illustrated in the accompanying Fig. 5 was used. A chamber 100, closed while the experiments were in progress, contained near one end a frame 102 holding a layer (disc) 104 of fibrous drape material (sterile cotton gauze), impregnated with MRSA and dried so that a biofilm formed. Ozone rich atmosphere is fed into the chamber. An electrical fan 106 with rotary blades 108 was disposed 3 cm from the gauze, so as to blow gases within the chamber through the gauze at high velocity, to cause physical agitation of the gauze. A dish 1 10 containing an exposed, similarly impregnated gauze 1 12 was disposed near the other end of the chamber 100, so that it was exposed to essentially static atmosphere in the chamber. A control gauze, which was similarly impregnated but received no treatment, was also evaluated. The results are reported in Table 1 below. In Table 1 , columns A, B, C and D are the results at 10 fold serial dilutions, obtained by standard procedure. Results measured on gauzes subjected to physical agitation are recorded as "direct". Those on the gauzes in essentially static atmosphere are recorded as "indirect".
In all instances, the combination of 80 ppm ozone and 1 % H2O2 at a relative humidity of 80% with an exposure time of 30 minutes proved superior to all other combinations including 1 % H2O2 with no ozone and 80 ppm ozone with no H2O2. In these experiments the methodology utilized with respect to microbiological procedures was the same as that described above for other experiments. Accordingly it has been concluded that in order to achieve a 6-7 log bacterial kill in hospital environments wherein carpets and other textiles are commonly found, an ozone/H2O2 pressure applicator or physical agitator is essential. Based on the experiments provided and other research, the incremental improvement in bacterial kill achievable through a pressure applicator is in the order of 2 - 3 logs (100 - 1000 x greater).
Figure imgf000027_0001
EXAMPLE 11
Test bacteria, namely Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa (PAU); Methicillin-Resistant Staphylococcus aureus (MRSA); Vancomycin-Resistant Enterococcus (VRE); were prepared as described for the previous experiments (see Example 1 for the preparation of the aerobic bacteria, Example 9 for the preparation of C. difficile). Bacillus subtilis (the surrogate for anthrax) was prepared analogously to the preparation of C. difficile, except that the bacteria was grown on Columbia sheep's blood agar plates incubated for 18 - 24 hours in room air at 350C. They were separately cultured on plates for 24 hours. From the plate, 4-5 isolated colonies were selected, and suspended in 0.85 NaCI to achieve a 0.5 McFarland turbidity standard (1 .5 x10 8 cfu/ml) measured using a spectrophotometer. Inoculum was prepared by performing a series of serial dilutions of 0.9 ml 0.85 NaCI broth with 0.1 ml of original 0.5 McFarland inoculum (6x10 fold) to give solutions of 10"\ 10~2, 10 ~3 , 10 "4 , 10 "5 , 10 "6 and 10 "7 cfu/mL Organisms were plated out in triplicate, as previously described, 0.1 ml of each solution being spread over the surface of Columbia sheep's blood agar (in respect of the aerobic bacteria) or Brucella anaerobic blood agar plates (in respect of C. difficile and B. subtilis) on plates, or on stainless steel plates. On agar, the bacteria maintain planktonic mode. On steel plates, biofilms containing the bacteria form.
For the experiments on steel plates, 40 microlitres of the original inoculum as prepared above was placed onto the surface of a series of 1 cm diameter stainless steel discs. These were allowed to dry in a biological safety cabinet for approximately 45 minutes until the inoculum spots were dry. The steel discs were placed in a sterile Petri dish to facilitate their transfer to the test chamber. Once dry, the lid of the Petri dish was placed over the discs, and they were carefully transferred to the treatment location where they were exposed to the ozone test conditions. Appropriate numbers of control discs are left covered in the biological safety cabinet, and not exposed to the ozone test conditions.
Some of the plates were subjected to ozone/oxygen exposure using ozone 80 ppm, 42 - 80% humidity and room temperature of about 220C, for a period of 90 minutes, in the illustrated apparatus, as controls. Additional controls had no ozone or hydrogen peroxide treatment, but were prepared and exposed in the same way.
With reference to Fig. 4, the test plates were mounted inside the disinfection chamber 60, and treated with ozone and water vapor as previously described, but additionally using hydrogen peroxide supplied as a vapor to the chamber via port 65. The disinfection chamber 60 also contained the same heater/cooler system and sensors previously described.
Plates treated according to the invention were exposed to 80 ppm ozone and gaseous hydrogen peroxide from a 1 % or a 3% aqueous solution, air being blown through the aqueous solution in the illustrated apparatus to create the gaseous hydrogen peroxide. Other conditions and exposure times were kept the same.
Immediately after the exposure to the test conditions, and similarly for the unexposed control discs, the stainless steel discs were vigorously mixed in 10 ml of sterile 0.85% saline using a vortex mixer at high speed for 60 seconds to elute off all surviving viable bacteria or spores. The eluted suspension, containing both living and dead bacteria, is serially diluted 10 fold in sterile 0.85% saline and the diluted bacteria were quantitatively plated onto Columbia sheep's blood agar plates for the aerobic bacteria or Brucella anaerobic blood agar plates for C. difficile, incubated under appropriate conditions, in triplicate so as to determine the original inoculum concentration. The survivor colony counts were logarithmically transformed and the geometric mean calculated. The difference between the bacterial counts of the unexposed controls and the exposed test discs yielded the logarithmic reduction in bacteria under the test conditions. If this procedure results in no growth, 100% of the bacteria within the biofilm have been killed by exposure to the ozone/hydrogen peroxide.
The agar plates after exposure were cultivated in an incubator for 24 hours. The plates were then stained, examined through a microscope, and the numbers of colony forming units on each plate was counted.
The results are reported in Table 2 below, as 10 fold reductions in live bacteria on the agar plate or the steel plate, in comparison with the starting plate prior to any exposure. Thus a value of 1 means a 10 fold or one log reduction relative to the control samples which is not considered a significant effect. A value of 5 means a 5 log or 99.999% reduction in live bacteria was achieved, enough to be termed "full disinfection", for practical purposes. A value of 6 means a 6 log or 99.9999% reduction in live bacteria was achieved which is defined internationally (CDC) as "sterilization". The bacterial strains were as reported in the previous experiments. The Bacillus subtilis was ATCC 19659 spores.
TABLE 2
Figure imgf000030_0001
EXAMPLE 12
Tables 3, 4, 5, 6, 7 and 8 below provide a summary of experiments, whereby combinations of ozone, H2O2, humidity and exposure time were evaluated in terms of the ability to eliminate the following bacteria when artificially applied as a biofilm onto non-porous surfaces such as stainless steel discs: E. coli; Pseudomonas aeruginosa (PAU); Bacillus subtilis (the surrogate for anthrax). Clostridium difficile (C. difficile); Vancomycin-Resistant Enterococcus (VRE); and Methicillin-Resistant Staphylococcus aureus (MRSA), same strains as before.
The steel discs for testing and the agar plates for testing were prepared exposed and tested as described in the previous Example, with exposure conditions shown in the Tables below. In some cases, indicated as "chamber", the tests were conducted as described in Example 10 and with an apparatus generally as illustrated in Fig. 4. In other cases indicated as "room", the tests were conducted by exposing the disks and plates in a closed room, as generally illustrated in Fig. 1 .
The below Tables of results also report a period of post exposure (PEEP), in minutes, which is the time interval between the ozone/peroxide exposure termination and the start of the procedure for determining the results. This simulates real practice in disinfecting hospital rooms and similar environments, where bacteria, after disinfectant treatment, die over a period of time. To allow for this, it is preferred that at least 25 minutes should elapse from the time the ozone/hydrogen peroxide exposure terminates before the disinfected room is put back into normal service.
Figure imgf000032_0001
Figure imgf000033_0001
Figure imgf000034_0001
Figure imgf000035_0001
Figure imgf000036_0001
Figure imgf000037_0001
Figure imgf000038_0001
Figure imgf000039_0001
Figure imgf000040_0001
Figure imgf000041_0001
Figure imgf000042_0001
Figure imgf000043_0001
Figure imgf000044_0001
The findings with respect to Bacillus subtilis clearly indicate that 80 ppm ozone, 1 % H2O2 at 80% relative humidity produces a 6 log (+) reduction when these aerobic spores are exposed for 90 minutes. Given the uniqueness of this bacteria and the fact that it is routinely used as a surrogate for anthrax, the above combination of treatment parameters renders this device highly effective in a bioterrorism countermeasures scenario.
The findings with respect to Pseudomonas aeruginosa show definitely that 80 ppm ozone, 1 %H2O2 at 80 % relative humidity with an exposure time of 25 minutes produces a 100% kill (7 + logs). The same findings were observed when biofilms of E. CoIi samples on stainless steel discs were exposed for 25 minutes to a combination of 80 ppm ozone, 1 % H2O2 at a relative humidity of 80%.
With respect to Clostridium difficile and vancomycin resistant Enterrococcus, the same combination of 80 ppm ozone, 1 % H2O2 and 80% relative humidity proved highly effective in achieving 100% elimination of bacteria in biofilms placed on a stainless steel surface and exposed for 45 minutes.
The results summarized in Table 8 above clearly demonstrates that the same combination of 80 ppm ozone, 1 % H2O2 and 80% relative humidity achieves 100% kill (6+ log reduction) when biofilms of MRSA were exposed for 30 minutes.
Conclusion
The data provided in the above Tables clearly demonstrate that the process according to the invention is capable of completely eliminating bacteria contained within biofilm preparations on a non-porous hardened surface such as stainless steel. Although small adjustments in the time of exposure are necessary for the common pathogens found in hospital settings (25 - 45 minutes), Bacillus subtilis and therefore its cousin anthrax require almost twice the exposure time, but these pathogens are of little concern to hospitals.
Thus one aspect of the invention is a process for disinfecting a room, which comprises introducing into the room an oxygen/ozone gas mixture, raising the pressure within the room above atmospheric pressure, physically agitating fibrous and porous surfaces within the room while the surfaces are exposed to the ozone containing atmosphere of relative humidity at least 65%, returning the room to atmospheric pressure, and removing the residual ozone from the room's atmosphere, down to a maximum level of 0.04 ppm.
Another aspect of the invention is a portable system for disinfecting rooms and surfaces therein with ozone, comprising an oxygen container, an ozone generator fed with medical grade oxygen from the oxygen container and discharging a mixture of oxygen and ozone, an ozone controller adapted to control the proportion of ozone in the mixture of oxygen and ozone, a discharge tube to receive the mixture of oxygen and ozone from the ozone generator, the discharge tube having an outlet end, a physical agitation system at the outlet end of the discharge tube, for physical agitation of surfaces with oxygen/ozone mixture issuing therefrom, pressure adjusting means connected to the ozone generator arranged to adjust the pressure of the oxygen/ozone mixture discharged by the physical agitation system and the oxygen/ozone gas pressure in the room under treatment, temperature adjusting means connected to the ozone generator arranged to adjust the temperature of the oxygen/ozone mixture discharged by the physical agitation system, humidity adjusting means adapted to humidify the treatment location to a relative humidity not less than 65%, and an ozone remover adapted to receive oxygen/ozone mixture from the environment of use of the discharge tube and to remove ozone from the mixture.

Claims

WHAT IS CLAIMED IS:
1 . A process of combating bacteria in an enclosed space within a room and contained in biofilm on surfaces within the room, which comprises: creating in the room a disinfecting atmosphere which includes ozone at a concentration of 2 - 350 ppm by weight and hydrogen peroxide at an amount of 0.2 - 10 wt. %, at a relative humidity of at least 60%; exposing the biofilm carrying surfaces having live bacteria therein to the disinfecting atmosphere for a period of at least 30 minutes sufficient for an effective kill of the bacteria in the microfilm; and subsequently removing ozone from the atmosphere, down to 0,04 ppm or less.
2. The process of claim 1 1 wherein the time of exposure is from about 30 minutes to about 120 minutes.
3. The process of claim 1 or claim 2 wherein the ozone concentration in the disinfecting atmosphere is from 20 to 200 ppm.
4. The process of claim 3 wherein the ozone concentration in the disinfecting atmosphere is from 35 - 100 ppm.
5. The process of any preceding claim wherein the hydrogen peroxide amount is from 0.5 - 10 %.
6. The process of claim 5 wherein the hydrogen peroxide amount in the disinfecting atmosphere is from 1 - 5 %.
7. The process of any preceding claim wherein the bacteria being combated are Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); vancomycin-resistant Enterococcus (VRE); or combinations of two or more of said bacteria.
8. The process of any of claims 1 -6 wherein the bacteria being treated is Bacillus subtilis or anthrax, or a combination thereof.
9. The process of any preceding claim including the additional step of subjecting porous and fibrous surfaces within the room to physical agitation while exposed to the disinfecting atmosphere.
10. The process of claim 9 wherein the physical agitation is conducted with application of bristles.
1 1 . The process of claim 9 wherein the physical agitation is conducted with application of air pressure jets.
12. The process of claim 9 wherein the physical agitation is conducted with application of ultrasonic energy, radio-frequency energy or electromagnetic waves, capable of causing physical disruption.
13. The process of any preceding claim wherein the biofilm carrying surfaces are exposed to a localized stream of the disinfecting atmosphere.
14. The process of any preceding claim wherein the pressure of the disinfecting atmosphere when the biofilm carrying surfaces are exposed thereto is above atmospheric pressure.
15. The process of claim 14 wherein the pressure of the disinfecting atmosphere is from 14.7 to 100 psi.
16. A process for disinfecting a room and surfaces therein, which comprises: introducing into the room an oxygen/ozone gas mixture; raising the pressure within the room above atmospheric pressure; physically agitating fibrous and porous surfaces within the room while the surfaces are exposed to the ozone containing atmosphere at a relative humidity of at least 70%; returning the room to atmospheric pressure, and removing the residual ozone from the room's atmosphere, down to a maximum level of 0.04 ppm.
17. The process of claim 16 wherein the ozone is delivered to the room atmosphere as a mixed oxygen/ozone gas, with the ozone present in an approximate amount of 10 - 100 ppm.
18. The process of claim 17 wherein the ozone is delivered to the room atmosphere as a mixed oxygen/ozone gas, with the ozone present in an approximate amount of 30 - 90 ppm.
19. The process of claim 18 wherein the ozone is delivered to the room atmosphere as a mixed oxygen/ozone gas, with the ozone present in an approximate amount of 35 - 80 ppm.
20. The process of any of claims 16 - 19 wherein the pressure within the room is raised to between 14.7 psi and 100 psi.
21 . The process of any of claims 16 - 20 wherein the room and its surfaces are exposed to the oxygen/ozone mixture for a period of from about 45 to 120 minutes.
22. The process of claim 21 wherein the room and its surfaces are exposed to the oxygen/ozone mixture for a period of from about 60 to 105 minutes.
23. The process of any of claims 16 - 22 applied to disinfection of at least one of the bacteria Clostridium difficile (C. difficile); E. coli; Pseudomonas aeruginosa; methicillin-resistant Staphylococcus aureus (MRSA); and vancomycin-resistant Enterococcus (VRE).
24. The process of any of claims 16 - 23 which additionally includes introduction into the room of an effective amount of hydrogen peroxide.
25 A portable system for disinfecting rooms and surfaces therein with ozone, comprising: an ozone generator discharging a mixture of oxygen and ozone; an ozone controller adapted to control the proportion of ozone in the mixture of oxygen and ozone; a discharge tube to receive the mixture of oxygen and ozone from the ozone generator, the discharge tube having an outlet end; a physical agitation system at the outlet end of the discharge tube, for physically agitating surfaces with oxygen/ozone mixture issuing therefrom; pressure adjusting means connected to the ozone generator arranged to adjust the pressure of the oxygen/ozone mixture discharged by the physical agitation system and the oxygen/ozone gas pressure in the room under treatment; temperature adjusting means connected to the ozone generator arranged to adjust the temperature of the oxygen/ozone mixture discharged by the scrubbing system; humidity adjusting means adapted to humidify the treatment location to a relative humidity of at least 65%; and an ozone remover adapted to receive oxygen/ozone mixture from the environment of use of the discharge tube and to remove ozone from the mixture.
26. The system of claim 25 wherein the humidity adjusting means is a humidifier interposed between the ozone generator and the oxygen container, with input from the oxygen container and output to the ozone generator.
27. The system of claim 25 or claim 26 wherein the ozone generator is fed with medical grade oxygen and the ozone controller is electrical discharge plates disposed within the ozone generator, adapted to supply variable, controlled voltage to the oxygen gas supplied thereto.
28. The system of any of claims 25 - 27 wherein the physical agitation system comprises at least one jet nozzle outlet.
29. The system of claim 28 wherein the physical agitation system further includes bristles disposed adjacent to the jet nozzle outlet and protruding slightly below the discharge end thereof.
30. The system of any of claims 25 - 29 wherein the ozone generator includes at least one oxygen/ozone outlet to the room in addition to the discharge tube.
31 . The system of any of claims 25 - 30 further including a wheeled cart for loading and transportation of the system.
32. A portable system for disinfecting rooms, surfaces and equipment therein, comprising: an ozone generator for discharging into the room a gaseous mixture including ozone; an ozone controller adapted to control the amount of discharged ozone ; a source of hydrogen peroxide for discharging controlled amounts of hydrogen peroxide into the room; means for discharging the hydrogen peroxide and ozone into the room; humidity adjusting means adapted to increase or decrease the relative humidity of the room during treatment; and an ozone remover adapted to destroy ozone, down to a safe level in the room atmosphere for subsequent human utilization.
33. The system of claim 32 wherein the means for discharging the hydrogen peroxide and ozone into the room includes a discharge wand having an outlet end.
34. The system of claim 33 wherein the outlet end of the discharge wand includes a dislodgement system for agitating and disturbing surfaces to which it is applied.
35. The system of claim 34 wherein the dislodgement system is a jet nozzle outlet.
36. The system of claim 34 or claim 35 wherein the dislodgement system includes bristles for scrubbing action.
37. The system of any of claims 32 - 36 wherein the means for discharging hydrogen peroxide gas and ozone further includes an outlet which bypasses the wand.
38. The system of any of claims 32 - 37 further including a wheeled cart for loading and transportation of the system.
PCT/CA2010/000998 2009-07-06 2010-07-05 Healthcare facility disinfecting process and system with oxygen/ozone mixture WO2011003179A1 (en)

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MX2012000302A MX344243B (en) 2009-07-06 2010-07-05 Healthcare facility disinfecting process and system with oxygen/ozone mixture.
JP2012518702A JP2012531979A (en) 2009-07-06 2010-07-05 Process and system for disinfecting medical facilities using a mixture of oxygen / ozone
CA2735739A CA2735739C (en) 2009-07-06 2010-07-05 Healthcare facility disinfecting process and system with oxygen/ozone mixture
CN201080030657.2A CN102481383B (en) 2009-07-06 2010-07-05 To sterilize with oxygen/ozone mixture the method and system in health care place
EP10796611.1A EP2451489B1 (en) 2009-07-06 2010-07-05 Healthcare facility disinfecting process and system with oxygen/ozone mixture
BR112012000384A BR112012000384B1 (en) 2009-07-06 2010-07-05 oxygen / ozone mixture health care facility process and disinfection system
SG2011095767A SG176977A1 (en) 2009-07-06 2010-07-05 Healthcare facility disinfecting process and system with oxygen/ozone mixture
IN963DEN2012 IN2012DN00963A (en) 2009-07-06 2010-07-05
CA2785850A CA2785850A1 (en) 2010-01-18 2010-09-08 Bio-terrorism counteraction using ozone and hydrogen peroxide
EP10842789.9A EP2525838B1 (en) 2010-01-18 2010-09-08 Bio-terrorism counteraction using ozone and hydrogen peroxide
PCT/CA2010/001364 WO2011085466A1 (en) 2010-01-18 2010-09-08 Bio-terrorism counteraction using ozone and hydrogen peroxide
US13/522,685 US8636951B2 (en) 2010-01-18 2010-09-08 Bio-terrorism counteraction using ozone and hydrogen peroxide
US13/343,403 US8551399B2 (en) 2009-07-06 2012-01-04 Healthcare facility disinfecting system
HK13106264.1A HK1178468A1 (en) 2010-01-18 2013-05-27 Bio-terrorism counteraction using ozone and hydrogen peroxide
US14/046,535 US9616145B2 (en) 2009-07-06 2013-10-04 Healthcare facility disinfecting system

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Cited By (18)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2011085466A1 (en) 2010-01-18 2011-07-21 Medizone International Inc. Bio-terrorism counteraction using ozone and hydrogen peroxide
WO2012031366A1 (en) * 2010-09-08 2012-03-15 Medizone International Inc. Food-handling facility disinfection treatment
WO2012031365A1 (en) * 2010-09-08 2012-03-15 Medizone International Inc. Combating insect infestations
WO2012031364A1 (en) * 2010-09-08 2012-03-15 Medizone International Inc. Sports equipment and facility disinfection
WO2012037678A1 (en) * 2010-09-20 2012-03-29 Medizone International Inc. Process for sterilization of air spaces and surfaces using advanced oxidation stress
JP2013158701A (en) * 2012-02-03 2013-08-19 Ihi Shibaura Machinery Corp Oxidation treatment system
JP2013158702A (en) * 2012-02-03 2013-08-19 Ihi Shibaura Machinery Corp Oxidation treatment system
JP2013158699A (en) * 2012-02-03 2013-08-19 Ihi Shibaura Machinery Corp Oxidation treatment method, and oxidation treatment system
US8551399B2 (en) 2009-07-06 2013-10-08 Medizone International, Inc. Healthcare facility disinfecting system
JP2014023596A (en) * 2012-07-25 2014-02-06 Ihi Corp Sterilizer
US9616145B2 (en) 2009-07-06 2017-04-11 Medizone International, Inc. Healthcare facility disinfecting system
USRE47582E1 (en) 2009-07-28 2019-08-27 Sterifre Medical, Inc. Free radical sterilization system and method
WO2020073075A1 (en) * 2018-10-10 2020-04-16 Wellkleen Pty Ltd Sterilisation device
US11253620B2 (en) 2016-06-17 2022-02-22 Sterifre Medical, Inc. Sterilization, disinfection, sanitization, decontamination, and therapeutic devices, systems, and methods
WO2022060723A1 (en) * 2020-09-15 2022-03-24 DD SterOZone LLC Apparatus and methods for trioxidane disinfection
US11344643B2 (en) 2017-10-25 2022-05-31 Sterifre Medical, Inc. Devices, systems, and methods for sterilization, disinfection, sanitization and decontamination
IT202000030941A1 (en) * 2020-12-15 2022-06-15 Kros Way Srls SYSTEM AND METHOD OF DISINFECTION AND FIXED OR MOBILE DECONTAMINATION
RU2802662C1 (en) * 2023-01-11 2023-08-30 Федеральное государственное бюджетное образовательное учреждение высшего образования "Оренбургский государственный медицинский университет" Министерства здравоохранения Российской Федерации Method for pseudomonas aeruginosa biofilm destruction by a combination of ozone with hydrogen peroxide

Families Citing this family (21)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
AU2012242611B2 (en) * 2011-04-15 2016-05-19 Samuel Richard Trapani Room sterilization method and system
US9339572B2 (en) 2013-03-15 2016-05-17 EP Technologies LLC Methods and solutions for killing or deactivating spores
WO2015048903A1 (en) * 2013-10-04 2015-04-09 Medizone International Inc. Healthcare facility disinfecting system
WO2015168768A1 (en) 2014-05-05 2015-11-12 Sanuvox Technologies Inc. Room decontamination system, method and controller
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US11000613B1 (en) 2016-08-15 2021-05-11 Synergy Med Global Design Solutions, Llc Transportable self-sterilizing clinical environment
US10071177B1 (en) 2016-08-15 2018-09-11 Synergy Med Global Design Solutions, Llc Hospital and operating room designs and sterilization methods
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US10342246B2 (en) 2016-09-09 2019-07-09 Quail Systems, Llc Ozone generator, system, and methods for retrofit of enclosed and air-conditioned environments
CA3038956C (en) * 2016-10-19 2023-12-19 Christopher Alexander CORSETTI Sanitization system
US10692704B2 (en) 2016-11-10 2020-06-23 Gojo Industries Inc. Methods and systems for generating plasma activated liquid
WO2020050864A1 (en) * 2018-09-09 2020-03-12 SYNERGY MED GLOBAL DESIGN SOLUTIONS, LLC (a Delaware LLC) Designs and sterilization methods for hospital and operating rooms
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JP7264328B1 (en) 2022-09-07 2023-04-25 日本空調サービス株式会社 Space decontamination method and space decontamination device

Citations (8)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US5904901A (en) 1996-01-22 1999-05-18 Duskin Co., Ltd. Deodorization/odor-removal/disinfection method and deodorization/odor-removal/disinfection apparatus
CA2486831A1 (en) 2002-05-20 2004-02-05 Theodore A. M. Arts Air decontamination devices
WO2005060385A2 (en) * 2003-12-10 2005-07-07 Steris Inc. Ozone enhanced vaporized hydrogen peroxide decontamination method and system
US20060104858A1 (en) 2003-01-06 2006-05-18 Potember Richard S Hydroxyl free radical-induced decontamination of airborne spores, viruses and bacteria in a dynamic system
US20070008205A1 (en) 2005-07-06 2007-01-11 Aldrich Robert C Laser pulse counter
US20070086913A1 (en) 2004-11-11 2007-04-19 Ajt & Associates, Inc. Ozone Disinfection Apparatus
US7407624B2 (en) 2002-04-16 2008-08-05 Prompt Care, Inc. Method for abatement of allergens, pathogens and volatile organic compounds
US20090263499A1 (en) * 2008-04-18 2009-10-22 Ethicon, Inc. Area decontamination via low-level concentration of germicidal agent

Family Cites Families (11)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US5316741A (en) * 1991-05-30 1994-05-31 Zontec Inc. Ozone generator
US5972196A (en) * 1995-06-07 1999-10-26 Lynntech, Inc. Electrochemical production of ozone and hydrogen peroxide
JPH0960931A (en) * 1995-08-30 1997-03-04 Takuma Co Ltd Ultrasonic wave humidifying and sterilizing device
US6045846A (en) * 1998-12-18 2000-04-04 Dionex Corporation Produce sterilization
JP2001129062A (en) * 1999-11-04 2001-05-15 Mitsubishi Electric Corp Method and apparatus for disinfecting floor surface
CH700121B1 (en) * 2002-07-02 2010-06-30 Skan Ag Method and device for decontamination of a clean room.
US7071152B2 (en) 2003-05-30 2006-07-04 Steris Inc. Cleaning and decontamination formula for surfaces contaminated with prion-infected material
CN102008359B (en) * 2005-05-03 2013-08-21 乌尔特里奥公司 Oral hygiene devices employing an acoustic waveguide
JP4954993B2 (en) * 2005-07-07 2012-06-20 ステリス インコーポレイテッド Indoor decontamination using hydrogen peroxide vapor
US20070119699A1 (en) * 2005-11-30 2007-05-31 Airocare, Inc. Apparatus and method for sanitizing air and spaces
BR112012000384B1 (en) 2009-07-06 2018-07-17 Medizone Int Inc oxygen / ozone mixture health care facility process and disinfection system

Patent Citations (8)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US5904901A (en) 1996-01-22 1999-05-18 Duskin Co., Ltd. Deodorization/odor-removal/disinfection method and deodorization/odor-removal/disinfection apparatus
US7407624B2 (en) 2002-04-16 2008-08-05 Prompt Care, Inc. Method for abatement of allergens, pathogens and volatile organic compounds
CA2486831A1 (en) 2002-05-20 2004-02-05 Theodore A. M. Arts Air decontamination devices
US20060104858A1 (en) 2003-01-06 2006-05-18 Potember Richard S Hydroxyl free radical-induced decontamination of airborne spores, viruses and bacteria in a dynamic system
WO2005060385A2 (en) * 2003-12-10 2005-07-07 Steris Inc. Ozone enhanced vaporized hydrogen peroxide decontamination method and system
US20070086913A1 (en) 2004-11-11 2007-04-19 Ajt & Associates, Inc. Ozone Disinfection Apparatus
US20070008205A1 (en) 2005-07-06 2007-01-11 Aldrich Robert C Laser pulse counter
US20090263499A1 (en) * 2008-04-18 2009-10-22 Ethicon, Inc. Area decontamination via low-level concentration of germicidal agent

Non-Patent Citations (4)

* Cited by examiner, † Cited by third party
Title
DR. CARSTEN MATZ: "Biofilm Bacteria Protect Themselves With Chemical Weapons", HELMHOLTZ CETRE FOR INFECTION RESEARCH, BRAUSCHWEIG, 23 July 2008 (2008-07-23)
SCIENCE, July 2008 (2008-07-01)
See also references of EP2451489A4 *
WENTZEL R; EDMOND M D: "The Impact of Hospital Acquired Blood Stream Infections", EMERG. INF. DIS., vol. 7, no. 174, April 2011 (2011-04-01)

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US8551399B2 (en) 2009-07-06 2013-10-08 Medizone International, Inc. Healthcare facility disinfecting system
USRE49474E1 (en) 2009-07-28 2023-03-28 Sterifre Medical, Inc. Free radical sterilization system and method
USRE47582E1 (en) 2009-07-28 2019-08-27 Sterifre Medical, Inc. Free radical sterilization system and method
WO2011085466A1 (en) 2010-01-18 2011-07-21 Medizone International Inc. Bio-terrorism counteraction using ozone and hydrogen peroxide
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US8636951B2 (en) 2010-01-18 2014-01-28 Medizone International, Inc. Bio-terrorism counteraction using ozone and hydrogen peroxide
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US9616144B2 (en) 2010-09-08 2017-04-11 Medizone International Inc. Food-handling facility disinfection treatment
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US8992829B2 (en) 2010-09-08 2015-03-31 Medizone International Inc. Sports equipment and facility disinfection
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US11253620B2 (en) 2016-06-17 2022-02-22 Sterifre Medical, Inc. Sterilization, disinfection, sanitization, decontamination, and therapeutic devices, systems, and methods
US11344643B2 (en) 2017-10-25 2022-05-31 Sterifre Medical, Inc. Devices, systems, and methods for sterilization, disinfection, sanitization and decontamination
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RU2802662C1 (en) * 2023-01-11 2023-08-30 Федеральное государственное бюджетное образовательное учреждение высшего образования "Оренбургский государственный медицинский университет" Министерства здравоохранения Российской Федерации Method for pseudomonas aeruginosa biofilm destruction by a combination of ozone with hydrogen peroxide

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CA2735739A1 (en) 2011-01-13

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