AU722241B2 - Ionene polymers as microbicides - Google Patents
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- AU722241B2 AU722241B2 AU78633/98A AU7863398A AU722241B2 AU 722241 B2 AU722241 B2 AU 722241B2 AU 78633/98 A AU78633/98 A AU 78633/98A AU 7863398 A AU7863398 A AU 7863398A AU 722241 B2 AU722241 B2 AU 722241B2
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- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
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Description
t-'/UUIU 28/s'9 Regulation 3.2(2)
AUSTRALIA
Patents Act 1990
ORIGINAL
COMPLETE SPECIFICATION STANDARD PATENT Application Number: Lodged: r r r 11 r 11 r Invention Title: IONENE POLYMERS AS MICROBICIDES The following statement is a full description of this invention, including the best method of performing it known to us 1 Description lonene Polymers As Microbicides This invention relates to methods for the microbicidal control of microorganisms in aqueous systems by treating the system with an effective amount of an ionene polymer.
Particularly, it relates to methods for controlling the growth of species (ssp.) within the bacterial genera Campylobacter, Shigella, Vibrio and Yersinia, and protozoa within the genus Entamoeba in aqueous systems such as potable water, sewage and other nonmarine surface water. This invention also relates to methods for controlling the growth of the bacteria Mycobacterium bovis, Salmonella typhi, and the fungus Candida albicans in these nonmarine aqueous systems. This invention further relates to methods for controlling poliovirus in potable water, sewage, and other nonmarine surface water. Methods for controlling the spread of the diseases cholera and polio are also disclosed.
Cholera is endemic in regions of India and Bangladesh, and has spread to other regions of the globe in a series of pandemics. Recent cholera pandemics from the 1960s through the 1980s have involved Africa, the Philippines, Western Europe and Southeast Asia. In the United States, the number of cases of cholera has increased during the past fifteen years. Zinsser Microbiology 566-73 Joklik, H.P.
Willett, D.B. Amos, C.A. Wilfert, eds., 20th ed., 1992).
Cholera struck recently in Latin America, where the epidemic has affected more than half a million people, resulting in the death of tens of thousands of Latin Americans. The S: cholera epidemic that currently plagues Latin America began in Peru in 1990, and has spread at least as far as Brazil, Guatemala, Mexico, and Nicaragua. The Pan American Health Organization acknowledged that "once cholera arrives on a continent, it's likely to remain endemic until we make vast improvements in water and sanitation." Christine Tierney, Central America Suffers Summertime Cholera Surge, Reuter Newswire, Sept. 4, 1992.
2 Vibrio cholerae is the species of the bacterial genus Vibrio, which causes epidemic cholera, and is among the leading causes of other gastrointestinal infections. V.
parahaemolyticus is another Vibrio that causes gastrointestinal infection, and is prevalent in the United States. Other Vibrio ssp. may cause human illnesses that include diarrhea, bloody diarrhea, vomiting, cramps, sepsis and soft tissue infections. For example, V. vulnificus may produce infection in a preexisting wound or ulcer, or may cause primary sepsis that may be accompanied by shock that may be fatal. V. alginolyticus may also infect wounds, cause middle ear infections (otitis media), or cause bacteremia.
S.M. Finegold, W.J. Martin, Diagnostic Microbiology 86-87, 240-46 (6th ed. 1982). Vibrio ssp. also cause disease in fishes, eels, frogs, other vertebrates and invertebrates as well. See 1 Bergey's Manual of Systematic Bacteriology 518- 38 Krieg and J.G. Holt eds. 1984).
Vibrio bacteria are aquatic bacteria distributed throughout the world which often dangerously contaminate aqueous systems and water supplies. Contaminated water supplies pose the most serious source of Vibrio infection, as Vibrio-associated diseases are transmitted almost exclusively by the fecal contamination of water systems and food materials.
In countries lacking adequate potable water purification facilities, illness is often caused by drinking water contaminated with the bacteria. The drinking of contaminated water is the primary cause of the current cholera pandemics.
In developed countries, Vibrio-associated illness is more often caused by the eating of contaminated seafood or shellfish. The contamination results from releasing inadequately treated sewage into the marine environment.
For example, ingestion of raw oysters contaminated with V. vulnificus may lead to septicemia in as little as twentyfour hours. Thus, the major defense in the control of 3 Vibrio-associated illness is the maintenance of adequate water purification and adequate sewage treatment systems.
R.Y. Stanier, E.A. Adelberg, J.L. Ingraham, The Microbial World 627-29 (1976).
In addition to Vibrio bacteria, the methods of control disclosed herein can be used to control the growth of other microorganisms known to possess the potential to cause waterborne diseases. Members of the genus Campylobacter are bacteria pathogenic for humans and other mammals.
Campylobacter is a major cause of diarrhea in adults and children, causing diarrhea as frequently as do Salmonella and Shigella.
Fever, thrombophlebitis, bacteremia, septic or reactive arthritis, endocarditis, meningoencephalitis, pericarditis, pleuropulminary infection, cholecystitis, diarrhea and septic abortion may be caused by C. fetus subspecies jejuni, or C. fetus ss. intestinalis infection. Contaminated water is an important vehicle of infection. S.M. Finegold, W.J.
Martin, Diagnostic Microbiology 280-81 (6th ed. 1982).
Enteropathogenic Escherichia coli are responsible for outbreaks of diarrhea in infants and newborns, and diarrhea, including "traveler's diarrhea", in adults. E. coli may be invasive and toxin-producing, causing sometimes fatal infections, such as cystitis, pyelitis, pyelonephritis, appendicitis, peritonitis, gallbladder infection, septicemia, meningitis and endocarditis. Finegold Martin, at 84-85, 222.
Mycobacterium bovis, like M. tuberculosis, M. africanum, "i M. ulcerans, and M. leprae, is a strict pathogen. M. bovis is a significant pathogen throughout much of the world, causing tuberculosis, primarily in cattle. Finegold Martin, at 351-52.
Opportunistic in nature, Pseudomonas aeruginosa may infect burn or wound sites, or the urinary or lower respiratory tracts of immunocompromised hosts. Infection may result in serious septicemia. Finegold Martin, at 249, 253.
4 Salmonella spp. cause food poisoning, resulting in nausea, vomiting, diarrhea and sometimes-fatal septicemia.
S. typhi is the etiological agent of typhoid fever. Finegold Martin, at 204-06.
Shigella spp., including S. dysenteriae, are common waterborne pathogenic agents, causing bacillary dysentery as well as bacteremia and pneumonia. In the United States and Canada, S. sonnei and S. flexneri have become the most common etiological agents in bacillary dysentery. Finegold Martin, at 219-221.
Staphylococcus aureus causes one of the most common types of food poisoning. Additionally, various skin infections and more serious diseases, such as toxic shock syndrome, septicemia, meningitis and pneumonia may result from S. aureus infection. Finegold Martin, at 165-66.
Bacteria of the genus Yersinia are also pathogens. Y.
enterocolitica is an enteric pathogen. Infection with this microorganism causes severe diarrhea, gastroenteritis and other types of infections such as bacteremia, peritonitis, cholecystis, visceral abscesses, and mesenteric :.lymphadenitis. Septicemia with 50% mortality has been reported. Y. pestis is the etiologic agent of bubonic, pneumonic, and septicemic plague in humans. Finegold Martin, at 230-31.
Candida albicans is a yeast-like fungus that causes acute or subacute infection called candidiasis. -The yeast may cause lesions in the mouth, esophagus, genitourinary tract, skin, nails, bronchi, lungs and other organs in S..immunocompromised hosts. Bloodstream infection, endocarditis, and meningitis caused by Candida has been reported. Finegold Martin, at 429-30.
Entamoeba histolytica is a parasitic amoeba that infects the cecum and large bowel of humans, primates, other mammals and birds. E. histolytica may penetrate the epithelial tissues of the colon, causing ulceration symptomatic of amoebic dysentery. The amoeba may spread from the colon to the liver via the portal bloodstream and produce abscesses 5 (hepatic amebiasis). In a fraction of these cases, the amoebas may spread to other organs, such as lungs, brain, kidney, skin, and frequently be fatal. Stedman's Medical Dictionary 643 (25th ed. 1990). E. hartmanni and E. coli are more rarely associated with disease in humans. Finegold Martin, at 497-508.
Giardia intestinalis and G. lambia parasitize the small intestine of many mammals, including man. Infection with Giardia (giardiasis) may cause diarrhea, abdominal pain, nausea, anorexia, malaise, fatigue, unexplained eosinophilia, dyspepsia and occasionally malabsorption in humans.
Stedman's Medical Dictionary, at 515; Finegold Martin, at 497, 508-515.
Poliovirus causes acute viral disease (poliomyelitis) sporadically and in epidemics. The disease is endemic in most warm-weather countries throughout the world. Often waterborne, poliovirus may cause minor illness characterized by fever, sore throat, headache, and vomiting, often accompanied by stiffness of the neck and back.
Importantly, poliovirus may cause major illness involving the central nervous system causing paralysis of one or more limbs. Additionally, one form of poliovirus infection (acute bulbar poliomyelitis) affects the brain stem, motor cortex, and medulla oblongata, causing dysfunction of the swallowing mechanism, and respiratory and circulatory distress. Dorland's Illustrated Medical Dictionary 1045 (26th ed. 1981).
This invention provides a method of controlling the above referenced diseases caused by these microorganisms by controlling the growth of these microorganisms in aqueous systems, such as potable water, sewage water, and nonmarine surface water.
An object of this invention is to provide a method for the microbicidal control of unwanted, disease-causing microorganisms in aqueous systems such as potable water, sewage and other nonmarine surface water.
A second object of the invention is to provide methods for controlling microorganisms within the bacterial genera, Vibrio in aqueous systems such as potable water, sewage and other nonmarine surface water.
A further object is to provide a method for controlling the spread of the diseases caused by the microorganisms discussed above, such as cholera.
Other objects and advantages of the invention will be set forth in the description which follows, and in part will be apparent from the description, or may be learned by practice of the invention.
To achieve the above objects, and in accordance with the purpose of the invention as embodied and broadly described herein, there are provided: A method for controlling the growth of at least one microorganism selected from Vibrio spp., in an aqueous system susceptible to the growth of said microorganism and in recognized need of said control comprising the step of adding to said aqueous system an ionene polymer in an amount 15 effective to control the growth at least one microorganism wherein said aqueous system is selected from potable water, sewage, and other nonmarine surface water and said ionene polymer comprises a repeating unit of the formula I:
R
3 o A B (1) wherein R 2
R
3 and R 4 are each methyl.
A is -CH 2
CH
2 0CH 2 or -CH 2
CH(OH)CH
2 B is -CH 2
CH
2 and
X
2 is 2CI and wherein the molecular weight of said ionene polymer ranges from 1,000 to 5,000.
A method for controlling the growth of at least one microorganism selected from Vibrio spp. in an aqueous system susceptible to the growth of said microorganism and in recognized need of said control comprising the step of adding to said aqueous system an ionene polymer in an amount effective to control the growth of said at least one microorganism wherein said aqueous system is selected from potable water, sewage, and other nonmarine surface water and said ionene polymer comprises a repeating unit of formula n:
R
A- N (II)
R
2 10 wherein R' and R 2 are each methyl; A is -CH 2
CH(OH)CH
2 and X is CI; and wherein the molecular weight of said ionene polymer ranges from 2,000 to 500,000.
A method for controlling the spread of cholera transmitted from an aqueous system comprising the step of adding to said aqueous system in recognized need of said control, for the purpose of controlling the spread of cholera, an amount of ionene polymer effective in controlling the growth of at least one microorganism selected from Vibrio spp. wherein said aqueous system is selected from potable water, sewage, and other nonmarine surface water and said ionene polymer comprises a repeating unit of formula I: RI
R
A B 2
R
4 wherein R 1
R
2
R
3 and R 4 are each methyl.
A is -CH 2
CHOCH
2 or -CH 2
CH(OH)CH
2 B is -CH 2
CH
2 and
X
2 is 2CI1 and wherein the molecular weight of said ionene polymer ranges from 1,000 to 5,000.
A method for controlling the spread of cholera transmitted from an aqueous system comprising the step of adding to said aqueous system in recognized need thereof, for the purpose of controlling the spread of cholera, and amount of ionene polymer effective in controlling the growth of at least one microorganism selected from Vibrio spp., wherein said aqueous system is selected from potable water, sewage, and other nonmarine surface water, and said ionene polymer comprises a repeating unit of the formula (II).
R
2 9 wherein R 1 and R 2 are each methyl; A is -CH 2
CH(OH)CH
2 and X is CI'; and wherein the molecular weight of said ionene polymer ranges from 2,000 to 500,000.
In a first embodiment, the invention relates to a method for controlling the growth of at least one microorganism in an aqueous system susceptible to the growth of the microorganism where the aqueous system is in recognized need of such control. The method comprises the step of adding to the aqueous system an ionene polymer in an amount effective to control the growth at least one microorganism selected from Vibrio spp. The aqueous 9 system may be selected from potable water, sewage, and other nonmarine surface water.
As discussed above, microorganisms selected from Vibrio spp. are known to cause diseases in humans as well as other mammals by contaminating the water supply. According to this invention, ionene polymers can be effective in controlling the growth of such microorganisms in aqueous systems and, thus, can be effective in controlling the spread of diseases caused by these microorganisms. Specifically, ionene polymers are shown below to be effective in the control of Vibrio cholerae and Vibrio parahaemolyticus.
In the methods of this invention, an ionene polymer is used in an !olii amount effective to accomplish the purpose of the particular method, i.e, to o. .o control the growth of at least one microorganism. According to the present invention, control, for example, of the growth or spread of at least one 15 microorganism, means either the inhibition of the growth of a microorganism within the aqueous system or the reduction of the population of a microorganism to an acceptable level. Such control also includes the maintenance of the population of a microorganism in an aqueous system at or below an acceptable level, including zero growth.
o 20 The needs of the particular aqueous system determine what amount of ionene polymer will be required to achieve the desired level of control. The concentration of the ionene polymer in a given aqueous system may be, for example, less than or equal to 50 ppm, and preferably less than or equal to ppm. More preferably, the concentration varies from 1 ppm to 10 ppm and most preferably, the ionene polymer is present in the aqueous system at a concentration of approximately 5 ppm.
The methods of the invention are directed to the control of waterborne, disease-causing microorganisms. Thus, the disclosed methods can be employed in any aqueous system which is susceptible to the growth of such microorganisms.
Of particular concern are those aqueous systems that frequently come into contact with humans and other mammals, including livestock, and which can spread the disease-causing microorganism. These aqueous systems include, but are not limited to, potable water, sewage, and other nonmarine surface water such as ponds, lakes, streams, rivers, industrial cooling or contaminant ponds.
The invention also relates to a method of controlling the spread of cholera transmitted from aqueous systems. This method comprises the step of adding to an aqueous system in recognized need thereof, for the purpose of controlling the spread of cholera, an amount of ionene polymer effective in controlling the growth of Vibrio species. The aqueous system includes those discussed above. Specifically contemplated are those aqueous systems selected from potable water, sewage, and other nonmarine surface water as :ii discussed above.
.i Each of the above methods employs at least one ionene polymer to control the growth of the unwanted, disease causing microorganism in an :15 aqueous system. lonene polymers or polymeric quaternary ammonium 00 0 compounds, cationic polymers containing quaternary nitrogens in the polymer backbone (also known as polymeric quats or polyquats), belong to a S well-known class of compounds.
lonene polymers have been reported to possess biological activity.
oo 20 See, A. Rembaum, Biological Activity of lonene Polymers, Applied Polymer Symposium No. 22, 299-317 (1973).
lonene polymers have a variety of uses in aqueous systems such as microbicides, bactericides, algicides, sanitizers, and disinfectants. U.S. Patent Nos. 3,874,870, 3,898,336, 3,931,319, 4,027,020, 4,054,542, 4,089,977, 4,111,679, 4,506,081, 4,581,058, 4,778,813, 4,970,211, 5,051,124, and 5,093,078, the disclosures of all of which are specifically incorporated by reference herein, give various examples of these polymers and their uses.
lonene polymers have also been used to inhibit surface adhesion of bacteria and algae, U.S. Patent No. 5,128,100, the disclosure of which is specifically incorporated by reference herein. However, ionene polymers have heretofore not been known to be useful for controlling the growth of microorganisms such as Vibrio in aqueous systems. It is thus believed that 11 the uses claimed herein for ionene polymers are novel and are not suggested by any heretofore known uses.
lonene polymers may be classified according to the repeating unit found in the polymer. This repeating unit results from the reactants used to make the ionene polymer.
A first type of ionene polymer comprises the repeating unit of formula I.
R
R
A N B N*(I) R2• R4 X 2 20 In this formula, preferably, R 1
R
2
R
3 and R 4 are all methyl or ethyl.
The group is preferably -CH 2
CH
2 0CCH 2 or -CH 2
CH(OH)CH
2 The group is preferably -CH2CH 2 The counter ion, X 2 is 2CI. lonene polymers having trihalide counter ions are described in U.S. Patent No. 3,778,476. The disclosure of that patent 25 is incorporated herein by reference.
The ionene polymers having the repeating unit of formula I may be prepared by a number of known methods. One method is to react a diamine of the formula R 1
R
2
N-B-NR'R
2 with a dihalide of the formula X-A-X. lonene polymers having this repeating unit and methods for their preparation are, for example, described in U.S. Patents Nos. 3,874,870, 3,931,319, 4,025,627, 4,027,020, 4,506,870 and 5,093,078; the disclosures of which are incorporated herein by reference. The biological activity of ionene polymers having the repeating unit of formula I is also described in these patents.
A second type of ionene polymer comprises the repeating unit of formula II:
RA
A (ID In this formula II, the definitions of R 1
R
2 and A are the same as those defined above for formula I. X is the monovalent counter ion, CI.
The ionene polymers having the repeating unit of formula I may be prepared by known methods. One method is to react an amine of the formula
R'R
2 N with a haloepoxide such as epichlorohydrin. lonene polymers having the repeating unit of formula II are, for example, described in U.S. Patents Nos. 4,111,679 and 5,051,124, the disclosures of which are incorporated herein by reference. The biological activity of ionene polymers having the repeating unit of formula II is also described in these patents.
*9 9 13- A third type of ionene polymer comprises a repeating unit of formula III: R-
CU
3
CU
3 I I wherein R is N- Q- or I C3I H 2
CU
3
CH
2
CU
2
CU
3
CH
2 -CH2-\ Q is -(CUR' -CH 2
-CU=CU-CH
2
-CH
2
-CH
2
-O-CH
2 -CH2-,
-CU
2
-CH(OH)-CH
2 Or H 0 H I OH -(CHR)n- CH2-Hand I IRliii B'ren ndpisdependentlyHvaryCfromN2Ntor1;ec Ii ineednl hyroe or aIoe ly rop -i divalent R coneXotomnvln one oso whereainc candgp inpenenl varyp Rom 2n to 12; eoahenti diatcounter ion, twlfo monvalent counter ions or a fato 14 of a polyvalent counter ion sufficient to balance the cationic charge in the group B'.
Preferably, R' is hydrogen or a C 1
-C
4 alkyl; n is 2-6 and p is 2-6. Most preferably, R' is hydrogen or methyl, n is 3 and p is 2. Preferred counter ions, X2 and X are the same as those discussed above in formulae I and II.
The polymers of formula III are derived from bis(dialkylaminoalkyl) ureas, which are also known as urea diamines, by known methods. Ionene polymers of the formula III, methods of their preparation, and their biological activities are, for example, described in U.S. Patent No.
4,506,081; the disclosure of which is incorporated here by reference.
Ionene polymers comprising the repeating units of formulae I, II, and III may also be cross-linked with primary, secondary or other polyfunctional amines using means known in the art. Ionene polymers can be cross-linked either through the quaternary nitrogen atom or through another functional group attached to the polymer backbone or to a side chain.
Cross-linked ionene polymers, prepared using crosslinking coreactants, are disclosed in U.S. Patent No.
3,738,945 and Reissue U.S. Patent No. 28,808, the disclosures .of which are incorporated here by reference. The Reissue Patent describes the cross-linking of ionene polymers prepared by the reaction of dimethylamine and epichlorohydrin. The cross-linking coreactants listed are ammonia, primary amines, alkylenediamines, polyglycolamines, piperazines, heteroaromatic diamines and aromatic diamines.
U.S. Patent No. 5,051,124, the disclosure of which is incorporated herein by reference, describes cross-linked ionene polymers resulting from the reaction of dimethylamine, a polyfunctional amine, and epichlorohydrin. Methods of i inhibiting the growth of microorganisms using such crosslinked ionene polymers are also described.
15 Other examples of various cross-linked ionene polymers and their properties are provided in U.S. Patent Nos.
3,894,946, 3,894,947, 3,930,877, 4,104,161, 4,164,521, 4,147,627, 4,166,041, 4,606,773, and 4,769,155. The disclosures of each of these patents is incorporated herein by reference.
The ionene polymers comprising the repeating units of formulae I, II, or III may also be capped, have a specific end group. Capping may be achieved by means known in the art. For example, an excess of either reactant used to make the ionene polymer can be employed to provide a capping group. Alternatively, a calculated quantity of a monofunctional tertiary amine or monofunctional substituted or unsubstituted alkyl halide can be reacted with an ionene polymer to obtain a capped ionene polymer. Ionene polymers can be capped at one or both ends. Capped ionene polymers and their microbicidal properties are described in U.S.
Patents Nos. 3,931,319 and 5,093,078, the disclosures of each of these patents is incorporated herein by reference.
Among the ionene polymers discussed above, a particularly preferred ionene polymer having a repeating unit of formula I is poly[oxyethylene(dimethyliminio)ethylene(dimethyliminio)ethylene 1 2 3 4 dichloride. In this ionene polymer, R R R and R are 2each methyl, A is -CH2CH2OCH2CH 2 B is -CH 2
CH
2 and X 2 is 2C1", and the average molecular weight is 1,000-5,000. This ionene polymer is available from Buckman Laboratories, Inc.
of Memphis, Tennessee as Busan® 77 product, a 60% aqueous dispersion of the polymer, or WSCPO product, a 60% aqueous dispersion of the polymer. Busan® 77 and WSCPO are biocides used primarily in aqueous systems, including metalworking fluids for microorganism control.
Another particularly preferred ionene polymer having a repeating unit of formula I, also available from Buckman Laboratories, Inc. as Busane 79 product, or WSCP II product 1 2 3 4 is the ioneno polymer where R R R and R are each methyl, A is -CH 2 CH(OH)CH2-, B is -CH 2
CH
2 and X 2 is 2C1.
methyl, A is -CH2CH(OH)CH2-, B is -CH2CH-, and X is 2Cl 16 This ionene polymer is a reaction product of tetramethyl-1,2-ethanediamine, with (chloromethyl)-oxirane, and has a 1,000-5,000 average molecular weight. The polymer product BusanO 79 or WSCPII product is a 60% aqueous solution of the polymer.
Preferred ionene polymers having the repeating unit of formula II are those where R 1 and R 2 are each methyl, A is
CH
2
CH(OH)CH
2 and X- is Cl-. Busan® 1055 product is a aqueous dispersion of such an ionene polymer obtained as a reaction product of dimethylamine with (chloromethyl)oxirane having a 2,000-10,000 average molecular weight.
Busan® 1157 product is a 50% aqueous dispersion of the ionene polymer having the repeating unit of formula II, obtained as a reaction product of dimethylamine with epichlorohydrin, cross-linked with-ethylenediamine, where R 1 and R 2 are each methyl, A is -CH 2
CH(OH)CH
2 and X- is Cl-.
This ionene polymer has a 100,000-500,000 average molecular weight.
Busan® 1155 product is a 50% aqueous dispersion of an ionene polymer having the repeating unit of formula II, where
R
1 and R 2 are each methyl, A is -CH 2
CH(OH)CH
2 X~ is Cl and the ionene polymer is cross-linked with ammonia. This ionene polymer has a molecular weight of approximately 100,000- 500,000.
Busan® 1099 product or Bubond® 65 product is a aqueous dispersion of a cross-linked ionene polymer having 1 2 repeating units of formula II, where R and R are each methyl, A is -CH 2
CH(OH)CH
2 X is Cl-, the cross-linking agent is monomethylamine. This ionene polymer has a molecular weight of approximately 10,000-100,000.
Preferred ionene polymers having the repeating unit of formula III are those where R is a urea diamine and B' is
CH
2
CH(OH)CH
2 and X- is Cl-. BL® 1090 is a 50% aqueous dispersion of the ionene polymer obtained as a reaction S product of N,N'-bis-[l-(3-(dimethylamino)-propyl]urea and epichlorohydrin, such an ionene polymer having a 2,000- 15,000, preferably 3,000-7,000, average molecular weight.
17 Each of the above ionene polymers and products identified by trade name is available from Buckman Laboratories, Inc. of Memphis Tennessee.
The invention will be demonstrates by the following examples, which are intended merely to be illustrative of the present invention and are not limiting.
EXAMPLE 1 Ionene polymers were evaluated for their effectiveness in killing Vibrio cholerae in two levels of water hardness.
The following ionene polymer products were used: Busan® 77, Busan® 79, Busan® 1055, Busan® 1099, and Busan® 1157.
The microbicidal activity of each polymer was tested at AOAC water hardness levels of 300 ppm and 900 ppm which measures calcium and magnesium levels. 300 ppm AOAC corresponds to a level of moderately hard water. 900 ppm indicates extremely hard water, approaching brackishness.
For each ionene polymer product, the following weight/ weight concentrations of the ionene polymer product in the test system were used: 0.0 ppm, 5.0 ppm, 10.0 ppm, and 20.0 ppm. V. cholerae ATCC 14035, GBL 52107, were exposed in aqueous solution supplemented with .01% trypticase soy broth for 24 hours at room temperature. Vibriocide survivors were determined by plate count in alkaline trypticase soy agar.
The results, which are summarized in Tables 1 through 5, show that ionene polymers, when used in accordance with the present invention, provide dramatic reductions in the viability of V. cholerae, as evidence by the decrease in surviving bacteria plated after 24 hours exposure. The complete kill, <10 cfu/ml survivors, at concentrations as low as 5.0 ppm ionene polymer product in AOAC hardness 300 ppm, indicates the effectiveness of ionene polymers against V.
cholerae. The substantial decrease in the level of surviving S V. cholerae in as little as 20 ppm in 4 out of 5 of the polymers at AOAC 900 ppm illustrates the effectiveness of ionene polymers against V. cholerae even in extremely hard water.
18 TABLE 1 BusanO 77 Dose Level, ppm 0 5 10 Bacterial Count (cf u/mi) AQAC 300 ppm 1.4 x 106 <10 <10 AQAC 900 ppm 1.2 x 10 1.2 x 103 9.1 x 102 4.7 x 102 TABLE 2 Busan' 79 Dose Level, ppm 0 5 10 Bacterial Count (cfulml) AQAC 300 ppm 1.4 x 106 <10 <10 AQAC 900 ppm 1.2 x 10 7 2.1 x 10 2.3 x 13 TABLE 3 BusanO 1055 Dose Level, ppm 0 5 10 Bacterial Count (cfu/ml) AQAC 300 ppm 1.4 x 106 <10 <10 AQAC 900 ppm 1.2 x 107 2.0 x 106 1.3 x 105 9.1 x 103 TABLE 4 Busan6~ 1099 Dose Level, ppm 0 5 10 Bacterial Count (cf u/mi) ADAC 300 ppm 1.4 x 106 <10 <10 AQAC 900 ppm 1.2 x 107 6.2 x 105 4.0 x 105 2.5 x 104 #q 19 TABLE Busane 1157 Dose Level, ppm 0 5 10 Bacterial Count (cfu/ml) AOAC 300 ppm 1.4 x 106 <10 <10 AOAC 900 ppm 1.2 x 107 1.2 x 107 1.5 x 106 3.7 x 106 EXAMPLE 2 lonene polymer products Bubonde 65, Busan® 77, Busan® 79 and Busan® 1055 were evaluated for effectiveness in killing the bacteria Campylobacter jejuni, Escherichia coli, Mycobacterium bovis, Pseudomonas aeruginosa, Salmonella typhi, Shigella dysenteriae, Staphylococcus aureus, Vibrio parahaemolyticus ATCC 17802, Yersinia enterocolitica, and the yeast Candida albicans, in deionized water and artificial pond water. Results are shown in Tables 6-9.
Sterile deionized water, pH 7 to 7.5, was supplemented with polymer products at the concentrations of 2.5 ppm, ppm, and 20 ppm.
Artificial pond water consisted of sterile deionized water, sterile salts (350 ppm KC1, 350 ppm CaCI 2 350 ppm NaCI) and 0.01% sterile trypticase soy broth. Polymer products were added to this medium at concentrations of ppm, 10 ppm, and 20 ppm.
Bacteria, except for Campylobacter jejuni and Mycobacterium Bovis, and yeast were cultured in trypticase soy broth for 24-36 hours and seeded into 100 ml of the test solution at a concentration of 10 4 cfu/ml. The bacteria and yeast were contacted with the solution for 18-24 hours at without agitation, then quantitated by standard pour plate methodology in trypticase soy agar.
Campylobacter jejuni growth was quantitated by spread plate technigue on Chocolate Agar, and incubated at 37 0 C in a BBL "Campy Pack" for 48 hours. Mycobacterium bovis growth 20 Campylobacter jejuni growth was quantitated by spread plate technique on Chocolate Agar, and incubated at 37°C in a BBL "Campy Pack" for 48 hours. Mycobacterium bovis growth was quantitated by membrane filtration and cultivated in Glucose Base broth at 35 0 C for 28 days.
TABLE 6 Microbicidal Activity of BubondO Dose Level, ppm Bacterial Count (cfu/ml) Campylobacter jejuni Deionized Water Artificial Pond Water Escherichia coli Deionized Water Artificial Pond Water Pseudomonas aeruginosa Deionized Water Artificial Pond Water Salmonella typhi Deionized Water Artificial Pond Water Shigella dysenteriae Deionized Water Artificial Pond Water Staphylococcus aureus Deionized Water Artificial Pond Water Vibrio parahaemolyticus Deionized Water Artificial Pond Water Yersinia enterocolitica Deionized Water Artificial Pond Water Mycobacterium bovis Deionized Water Artificial Pond Water Yeast Count Candida albicans Deionized Water Artificial Pond Water 0 1.0 x 104 1.0 x 104 2.5 <10
NT
5
NT
<10 1.0 x 10 4 5.0 x 10 3
NT
1.0 x 105 NT 3.0 x 10 4 1.0 x 104 1.0 x 105 <10
NT
1.0 x 104 3.1 x 104 1.0 x 105 NT 9. 9. 9 9 i 9 9 9 9999 9.
9* 9 9 99 9 1.0 x 104 1.0 x 104 1.0 x 10 6 1.0 x 104 1.0 x 106 1.0 x 105 1.0 x 104 1.0 x 104 28 28 1.0 x 104 1.0 x 104 <10
NT
<10
NT
<10
NT
<10
NT
<1
NT
<10
NT
NT
210
NT
1.6 x 104
NT
<10
NT
<10
NT
600
NT
<10
NT
9
NT
<10 10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 470 <10 <10 750 <10 <10 NT Not tested 21 TABLE 7 Microbicidal Activity of BusanO 77 Dose Level, ppm Bacterial Count (cfu/ml) Campylobacter jejuni Deionized Water Artificial Pond Water Escherichia coli Deionized Water Artificial Pond Water Pseudomonas aeruginosa Deionized Water Artificial Pond Water Salmonella typhi Deionized Water Artificial Pond Water Shigella dysenteriae Deionized Water Artificial Pond Water Staphylococcus aureus Deionized Water Artificial Pond Water Vibrio parahaemolyticus Deionized Water Artificial Pond Water Yersinia enterocolitica Deionized Water Artificial Pond Water Mycobacterium bovis Deionized Water Artificial Pond Water Yeast Count Candida albicans Deionized Water Artificial Pond Water 0 1.0 x 104 1.0 x 104 1.0 x 104 1.0 x 105 1.0 x 104 1.0 x 105 1.0 x 104 1.0 x 105 1.0 x 104 1.0 x 104 1.0 x 106 1.0 x 104 1.0 x 106 1.0 x 105 1.0 x 104 1.0 x 104 28 28 1.0 x 104 1.0 x 104 2.5 <10
NT
<10
NT
<10
NT
50
NT
<10
NT
<10
NT
700
NT
<10
NT
<1
NT
<10
NT
NT
<10
NT
<10
NT
810
NT
620
NT
<10
NT
<10
NT
2.1 x 103
NT
<10
NT
9
NT
40 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 570 <10 <10 5 <10 <10 NT Not tested 22 TABLE 8 Microbicidal Activity of Busane 79 Dose Level, ppm Bacterial Count (cfu/ml) Campylobacter jejuni Deionized Water Artificial Pond Water Escherichia coli Deionized Water Artificial Pond Water Pseudomonas aeruginosa Deionized Water Artificial Pond Water Salmonella typhi Deionized Water Artificial Pond Water Shigella dysenteriae Deionized Water Artificial Pond Water Staphylococcus aureus Deionized Water Artificial Pond Water Vibrio parahaemolyticus Deionized Water Artificial Pond Water Yersinia enterocolitica Deionized Water Artificial Pond Water Mycobacterium bovis Deionized Water Artificial Pond Water Yeast Count Candida albicans Deionized Water Artificial Pond Water 0 1.0 x 104 1.0 x 104 2.5 <10
NT
1.0 x 10 4 2.1 x 10 1.0 x 10 5
NT
1.0 x 104 1.0 x 10 5 1.0 x 10 4 1.0 x 105 1.0 x 104 1.0 x 104 1.0 x 106 1.0 x 104 1.0 x 106 1.0 x 105 1.0 x 104 1.0 x 104 28 28 1.0 x 104 1.0 x 104 <10
NT
<10
NT
<10
NT
<10
NT
<10
NT
<10
NT
5
NT
<10
NT
5
NT
<10 4 NT <10
NT
<10
NT
<10
NT
<10
NT
<10
NT
1.05 x 103
NT
<10
NT
1
NT
<10 10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 450 <10 <10
S
.5 f..
*0
S
<10 <10 NT Not tested 23 TABLE 9 Microbicidal Activity of Busan® 1055 Dose Level, ppm Bacterial Count (cfu/ml) Campylobacter jejuni Deionized Water Artificial Pond Water Escherichia coli Deionized Water Artificial Pond Water Pseudomonas aeruginosa Deionized Water Artificial Pond Water Salmonella typhi Deionized Water Artificial Pond Water Shigella dysenteriae Deionized Water Artificial Pond Water Staphylococcus aureus Deionized Water Artificial Pond Water Vibrio parahaemolyticus Deionized Water Artificial Pond Water Yersinia enterocolitica Deionized Water Artificial Pond Water Mycobacterium bovis Deionized Water Artificial Pond Water Yeast Count Candida albicans Deionized Water Artificial Pond Water 0 1.0 x 10 4 1.0 x 104 1.0 x 104 1.0 x 105 1.0 x 104 1.0 x 10 5 1.0 x 104 1.0 x 105 1.0 x 104 1.0 x 10 4 1.0 x 106 1.0 x 104 2.5 <10
NT
<10
NT
<10
NT
<10
NT
<10
NT
2.9 x 10
NT
<10
NT
<10
NT
NT
NT
<10
NT
5
NT
<10
NT
<10
NT
<10
NT
<10
NT
<10 14 NT <10
NT
3.1 x 10 2
NT
<10
NT
NT
NT
<10 10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10 <10
NT
<.001 <10 <10 <.001
NT
1.0 1.0 x 106 x 105 9 9 9 9 9 9 9 9*~ St.
5 9 9 *55e *9 *C 9 1.0 x 104 1.0 x 104 28 28 1.0 x 104 1.0 x 104 NT Not tested EXAMPLE 3 Ionene polymer products Bubond* 65, Busan® 77, Busano 79 and Busan® 1055 were evaluated for effectiveness in killing the protozoan Entamoeba histolytica ATCC 30922 GBL Lab. No.
42409.
24 Effectiveness of thess polymer products was tested in deionized water and artificial pond water as described in Example 2. The concentration of Entamoeba trophozoites in the inoculum was 320/mi. Entamoeba were enumerated, as shown in Tables 10-13, by direct microscopic observation of motility in a hemocytometer counting chamber at 400x.
TABLE Microbicidal Activity of Bubond® Dose Level, ppm 0 2.5 5 10 Number of Motile Organisms/ml Entamoeba histolytica Deionized Water 768 <1 NT <1 <1 Artificial Pond Water 1086 NT <1 <1 <1 TABLE 11 Microbicidal Activity of Busan® 77 Dose Level, ppm 0 2.5 5 10 Number of Motile Organisms/ml Entamoeba histolytica Deionized Water 768 <1 NT <1 <1 Artificial Pond Water 1086 NT <1 <1 <1 TABLE 12 Microbicidal Activity of Busane 79 Dose Level, ppm 0 2.5 5 10 Number of Motile Organisms/ml Entamoeba histolytica Deionized Water 768 <1 NT <1 <1 Artificial Pond Water 1086 NT <1 <1 <1 0e es
S
0 S 0S 0@ 0 000S es 0O 0O
S.
00
S
0S 0O 0
S
*0@ @0 OS S 0S
OOS
25 FTBLE 13 Microbicidal Activity of BusanO 1055 Dose Level, ppm 0 2.5 5 10 Number of Motile Organisms/mi Entamoeba hi stolyti ca Deionized Water 768 <1 NT <1 <1 Artificial Pond Water 1086 NT <1 <1 <1 The concentration (ppm, of the ionene polymer product in the test system) of BubondO 65, Busans 77, BusanO 79 and BusanO 1055 required to kill at least 99.9% of the tested pathogenic microorganisms is summarized in Tables 14-17.
TAB3LE 14 Microbicidal Activity of BubondO t/c Microorganism Bacteria: Campylobacter jejuni Escher-ichia coi Mycobacteri urn bovi s Pseudomona s a eru gin osa Salmonella typhi Shigella dysenteriae Staphylococcus a ureus Vibri a paraha emolyti cus Yersinia en terocoli tica Yeast: Candida albi cans Protozoa (trophozoites): Entamoeba histolytica Concentrations (ppm) Deionized Water Artificial Pond Water 26 TABLE Microbicidal Activity of BusanO 77 microorganism Bacteria: Campylobacter jejuni Escherlchla coi mycoba cter urn bovi 5 Pseudomona s aeruginosa Salmonella typhi Shigella dysenteriae Staphylococcus a ureus Vibrlo parahaemolyticus Yersinia enterocoli tica Yeast: Can dicia albi cans Protozoa (trophozoites): Ent amoeba his tolytica Concentrations (ppm) Deionized Water Artificial Pond Water TABLE 16 Microbicidal Activity of BusanO 79 4*
I'
Microorganism Bacteria: Campylobacter jejuni Escherichia coi Mycoba cteriurn bo vi a Pseudomonas a erug.Lnosa Salmonella typhi Shigella dysenteriae Staphylococcus aureus VI bri a parahaemolyticus Yersinla enterocoli tica Yeast: Candida albi cans Protozoa (trophozoites): Ent amoeba histoiytica Concentrations (ppm) Deionized Water Artificial Pond Water 27 TABLE 17 Microbicidal Activity of Busane 1055 Concentrations (ppm) Microorganism Deionized Water Artificial Pond Water Bacteria: Campylobacter jejuni 2.5 Escherichia coli 2.5 Mycobacterium bovis 2.5 Pseudomonas aeruginosa 2.5 Salmonella typhi 2.5 Shigella dysenteriae 2.5 Staphylococcus aureus 10 Vibrio parahaemolyticus 2.5 Yersinia enterocolitica 2.5 Yeast: Candida albicans 2.5 Protozoa (trophozoites): Entamoeba histolytica 2.5 EXAMPLE 4 Ionene polymer products Bubond® 65, Busane 77, Busan® 79 and Busan® 1055, were evaluated for effectiveness against poliovirus.
0.3 ml of poliovirus Type 1, maintained as a stock solution (of greater than or equal to 10 TC ID 50 in EMEM containing 5% calf serum was added to 100 ml of the test solutions described in Example 2. Virus viability was quantitated by calculation of the TC ID 50 (the average of one Tissue Culture Infectious Dose for of the test units.) The virus (0.1 ml per well) was cultivated in Hep-2 cells for 5 days at 37°C, 8-10% CO 2 Virus growth, as shown in Tables 18-21, was established by microscopic observation of cytopathic effect to the cell monolayer.
28 T A LE 18 Nicrobicidal Activity of BubondO 65 Against Poliovirus Dose Level, ppm 0 2.5 5 10 TC ID 50 Deionized Water 105.5 104.7 NT 10. 10 5 3 Artificial Pond Water 104. NT 10. 10. 104.0 TABLE 19 Microbicida. Activity of Busane 77 Against Poliovirus Dose Level, ppm 0 2.5 5 10 TC ID 50 Deionized Water 10 5 -5 10. NT 10. Artificial Pond Water 104.0 NT 10. 10. TABLE Microbicidal Activity of BusanO 79 Against Poliovirus Dose Level, ppm 0 2.5 5 10 TC ID 50 Deionized Water 155 045 NT 10- 104.3 Artificial Pond Water 10 4 0 NT 104.0 104.3 TABLE 21 Microbicidal Activity of BusanO 1055 Against Poliovirus Dose Level, ppm 0 2.5 5 10 TC ID 50 Deionized Water 105. 15. NT 10. 104.7 Artificial Pond Water 104.0 NT 10. 104.7 10 3 .7 "ocanprises/ccmprising" when used in this specification is taken to specify the presence of stated features, integers, steps or ccinponents but does not preclude the presence or addition of one or more other features, integers, steps, canponents or groups thereof.
*4 a a a a
Claims (7)
1. The method for controlling the growth of at least one microorganism selected from Vibrio spp., in an aqueous system susceptible to the growth of said microorganism and in recognized need of said control comprising the step of adding to said aqueous system an ionene polymer in an amount effective to control the growth at least one microorganism wherein said aqueous system is selected from potable water, sewage, and other nonmarine surface water and said ionene polymer comprises a repeating unit of the formula I: 0 *A is -CH2CH2OCH 2 or-CHCH(OH)CH2- B is -CHCH and X 2 is 2C1 and wherein the molecular weight of said ionene polymer ranges from 1,000 to 5,000.
2. The method of claim 1 wherein said Vibrio bacteria is Vibrio cholerae.
3. The method of claim 1 wherein the Vibrio bacteria is Vibrio parahaemolyticus.
4. The method of claim 1 wherein the concentration of said ionene polymer is said potable water is 5 ppm.
A method for controlling the growth of at least one microorganism selected from Vibrio supp. in an aqueous system susceptible to the growth of said microorganism and in recognized need of said control comprising the step of adding to said aqueous system an ionene polymer in an amount effective to control the growth of said at least one microorganism wherein said aqueous system is selected from potable water, sewage, and other nonmarine surface water and said ionene polymer comprises a repeating unit of formula II: R A m wherein R' and R 2 are each methyl; 2 X is CI; and wherein the molecular weight of said ionene polymer ranges from 2,000 to 500,000.
6. A method for controlling the spread of cholera transmitted from an aqueous system comprising the step of adding to said aqueous system in recognized need thereof, for the purpose of controlling the spread of cholera, and amount of ionene polymer effective in controlling the growth of at least one microorganism selected from Vibrio spp., wherein said aqueous system is selected from potable water, sewage, and other nonmarine surface water, and said ionene polymer comprises a repeating unit of the formula R' (I) wherein R 1 and R 2 are each methyl; A is -CH 2 CH(OH)CH 2 and X is CI; and wherein the molecular weight of said ionene polymer ranges from 2,000 to 500,000.
7. A method of controlling the spread of cholera transmitted from an aqueous system comprising the step of adding to said aqueous system in recognized need of said control, for the purpose of controlling the spread of cholera, an amount of ionene polymer effective in controlling the growth of at least one microorganism selected from Vibrio spp. Wherein said aqueous system is selected from potable water, sewage, and other nonmarine surface water and said ionene polymer comprises a repeating unit of formula I: 0* RR R 0* B R X wherein R' R 2 R and R 4 are each methyl. 0 A is -CH2CH20CH 2 or -CH2CH(OH)CH-; 11 B is -CH 2 CH 2 and X 2 is 2CI and wherein the molecular weight of said ionene polymer ranges from 1,000 to 5,000. DATED this 4th day of April 2000 BUCKMAN LABORATORIES INTERNATIONAL, INC. WATERMARK PATENT TRADEMARK ATTORNEYS 290 BURWOOD ROAD HAWTHORN VICTORIA 3122 AUSTRALIA Case: P11423AU00 IAS/CLR/BPR
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| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| AU78633/98A AU722241B2 (en) | 1993-03-05 | 1998-07-31 | Ionene polymers as microbicides |
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US027097 | 1993-03-05 | ||
| AU62999/94A AU6299994A (en) | 1993-03-05 | 1994-03-04 | Ionene polymers as microbicides |
| AU78633/98A AU722241B2 (en) | 1993-03-05 | 1998-07-31 | Ionene polymers as microbicides |
Related Parent Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU62999/94A Division AU6299994A (en) | 1993-03-05 | 1994-03-04 | Ionene polymers as microbicides |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| AU7863398A AU7863398A (en) | 1998-10-01 |
| AU722241B2 true AU722241B2 (en) | 2000-07-27 |
Family
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| AU (1) | AU722241B2 (en) |
Citations (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US4111679A (en) * | 1977-08-17 | 1978-09-05 | Chemed Corporation | Polyquaternary compounds for the control of microbiological growth |
| GB2126579A (en) * | 1982-09-02 | 1984-03-28 | Buckman Labor Inc | Polymeric quaternary ammonium substituted ureas |
| US5093078A (en) * | 1989-02-10 | 1992-03-03 | Buckman Laboratories International, Inc. | Novel polymeric quaternary ammonium trihalides and use of polymeric quaternary ammonium trihalides as microbicides, sanitizers and disinfectants |
-
1998
- 1998-07-31 AU AU78633/98A patent/AU722241B2/en not_active Ceased
Patent Citations (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US4111679A (en) * | 1977-08-17 | 1978-09-05 | Chemed Corporation | Polyquaternary compounds for the control of microbiological growth |
| GB2126579A (en) * | 1982-09-02 | 1984-03-28 | Buckman Labor Inc | Polymeric quaternary ammonium substituted ureas |
| US5093078A (en) * | 1989-02-10 | 1992-03-03 | Buckman Laboratories International, Inc. | Novel polymeric quaternary ammonium trihalides and use of polymeric quaternary ammonium trihalides as microbicides, sanitizers and disinfectants |
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| AU7863398A (en) | 1998-10-01 |
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