[go: up one dir, main page]

WO1982002322A1 - Meat spoilage inhibiting process - Google Patents

Meat spoilage inhibiting process Download PDF

Info

Publication number
WO1982002322A1
WO1982002322A1 PCT/US1981/000033 US8100033W WO8202322A1 WO 1982002322 A1 WO1982002322 A1 WO 1982002322A1 US 8100033 W US8100033 W US 8100033W WO 8202322 A1 WO8202322 A1 WO 8202322A1
Authority
WO
WIPO (PCT)
Prior art keywords
meat
spoilage
solution
ppm
chlorine dioxide
Prior art date
Legal status (The legal status 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 status listed.)
Ceased
Application number
PCT/US1981/000033
Other languages
French (fr)
Inventor
Kent S Barta
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Individual
Original Assignee
Individual
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
Application filed by Individual filed Critical Individual
Priority to AU72226/81A priority Critical patent/AU7222681A/en
Priority to EP81901410A priority patent/EP0069120A1/en
Priority to PCT/US1981/000033 priority patent/WO1982002322A1/en
Publication of WO1982002322A1 publication Critical patent/WO1982002322A1/en
Anticipated expiration legal-status Critical
Ceased legal-status Critical Current

Links

Classifications

    • AHUMAN NECESSITIES
    • A23FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
    • A23BPRESERVATION OF FOODS, FOODSTUFFS OR NON-ALCOHOLIC BEVERAGES; CHEMICAL RIPENING OF FRUIT OR VEGETABLES
    • A23B4/00Preservation of meat, sausages, fish or fish products
    • A23B4/26Apparatus for preserving using liquids ; Processes therefor
    • AHUMAN NECESSITIES
    • A23FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
    • A23BPRESERVATION OF FOODS, FOODSTUFFS OR NON-ALCOHOLIC BEVERAGES; CHEMICAL RIPENING OF FRUIT OR VEGETABLES
    • A23B4/00Preservation of meat, sausages, fish or fish products
    • A23B4/06Freezing; Subsequent thawing; Cooling
    • A23B4/08Freezing; Subsequent thawing; Cooling with addition of chemicals or treatment with chemicals before or during cooling, e.g. in the form of an ice coating or frozen block
    • AHUMAN NECESSITIES
    • A23FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
    • A23BPRESERVATION OF FOODS, FOODSTUFFS OR NON-ALCOHOLIC BEVERAGES; CHEMICAL RIPENING OF FRUIT OR VEGETABLES
    • A23B4/00Preservation of meat, sausages, fish or fish products
    • A23B4/14Preserving with chemicals not covered by groups A23B4/02 or A23B4/12
    • A23B4/18Preserving with chemicals not covered by groups A23B4/02 or A23B4/12 in the form of liquids or solids
    • A23B4/24Inorganic compounds

Definitions

  • Mesotrophs typically the food-borne pathogens such as Salmonella, E. coli and gram positive anaerobes such as Clostridia, are now
  • chlorinated contact disinfectants A major problem with such use of chlorinated contact disinfectants is reaction of the agent with meat components to produce chloro-organic derivatives such as chloro-substituted lipids and chloro-aromatic compounds.
  • chloro-organic derivatives such as chloro-substituted lipids and chloro-aromatic compounds.
  • chlorinated derivates pose a potential health hazard, especially the class of halomethanes (known to be carcinogenic) formed by reaction of bactericidal levels of hypochlorous acid with humic or other or ⁇ ganic substances. Reaction of chlorine dioxide at bactericidal concentrations with meat components results in lower but detectable levels of organic chlorine.
  • a principal object of the present invention is to provide a process which prevents the attach ⁇ ment and growth of spoilage organisms at the surface of freshly slaughtered meat carcasses. ' A further object is to prevent establishment of spoilage bacteria on carcass surfaces without completely destroying the microflora thereof. A still further object is to pre ⁇ vent establishment of spoilage bacteria on carcass sur ⁇ faces without utilizing bactericidal concentrations of chlorine dioxide known to result in detectable levels of organic chlorine upon reaction with meat components.
  • Chlorine dioxide solutions at concentrations as low as 100 fold lower than heretofore used are ef ⁇ fective for inhibiting attachment provided that their application to carcass surfaces commences at a time substantially coincident with contaminating events, as during slaughter procedures and subsequent chilling. At such low concentrations, no detectable organic chlorine is produced by reaction of the chlorine dioxide with meat components.
  • FIG. I is a rectilinear plot of the data presented in parts A and B of Example I.
  • aqueous solutions of chlorine dioxide are first applied substantially coincident with (that is, as close as feasible in point of time with) a significant contaminating event, and thereafter con ⁇ tinued by intermittent spraying.
  • aqueous solutions of chlorine dioxide so weak as to be substantially sub- toxic, are first applied substantially coincident with (that is, as close as feasible in point of time with) a significant contaminating event, and thereafter con ⁇ tinued by intermittent spraying.
  • a solution is first applied as a low pressure (less than 45 psi) spray to meat carcass sur ⁇ face immediately post-slaughter and substantially co ⁇ incident in time with dehiding and dressing procedures on the kill floor.
  • shrouds for beef may be soaked in the chlorine dioxide solution prior to draping.
  • Carcasses customarily in halves or quarters) are then conveyed to a chill room and an aqueous chlorine dioxide solution is intermittently applied to such carcass portions over a conventional 14-24 hr. chill period.
  • This method is adapted to such processing of fresh meat of domestic animals including but not limited to pork, beef, veal, and lamb.
  • the chlorine dioxide is generated on site with conventional apparatus and formed into solution with potable water to a concentration of 0.04- 1.0 ppm (mg/1) , preferably less than about 0.1 ppm (mg/1) prior to application.
  • concentration 0.04- 1.0 ppm (mg/1) , preferably less than about 0.1 ppm (mg/1) prior to application.
  • the solution be applied to carcass surfaces on the kill floor at a time substantially coirtident with contaminating events such as dehiding, disembowelment, etc.
  • the chlorine dioxide solution is applied intermittently during chilling for such intervals and in such volume as prescribed by USDA regulations (generally a maximum total of 0.5 hr. spraying time in increments during the entire chill cycle) .
  • the term "cold storage'' includes chilling of freshly slaughtered carcasses; and the term "substantially coincident with a contaminating event” means either immediately before such event, or as it takes place, or so shortly there ⁇ after that attachment of meat spoilage organisms has not yet in fact occurred. While the preferred method of applying the solution to meat surfaces is by spraying, other methods may be used, such as washing or dipping at the time of kill, or on any contaminating event there ⁇ after, or in the storage room; while and during cold
  • O. PI storage application may be by such a procedure or by misting into the atmosphere at a constant low rate in ⁇ stead of intermittent spraying.
  • a solution should be effective to kill at least about 85%-90% of contaminating bacteria, as disclosed in U.S. Patent No. 4,021,585. That patent shows chlorine dioxide is so bactericidal at concentra ⁇ tions minimally 5.0 ppm.
  • bio ⁇ logical attachment mechanism refers to those macro- molecular components of the bacterial cell surface which effect specific adherence to some substrates but not others. Biological attachment is thus distinguished from the mere nonspecific entrapment of bacteria, in
  • Example I indicates that the specific bio ⁇ logical attachment mechanism of spoilage bacteria is strongly inhibited by the use of substantially non- toxic levels of chlorine dioxide in aqueous solution.
  • flagellated :E. coli K-12 (see Example II) , known to exhibit specific biological attachment to an ⁇ imal skin, shows only a low-level nonspecific "attach ⁇ ment" to raw meat surfaces.
  • Aeromonas hydrophilis was isolated from con ⁇ taminated beef samples embedded in 0.5% McConkey agar and incubated at 37° for three days. Glistening mucoid colonies grew up at the surface of the meat, spreading outward into the soft agar.
  • This isolate A. hydrophilis was grown in modi ⁇ fied tryptone broth (5.0 g/1 Difco tryptone, 0.5 g/1 Difco yeast extract, 5.0 g/1 NaCl, o.l% glucose) sup ⁇ plemented with 5.0 uC/ml H-leucine (New England Nuclear) to a density of approximately 3 x 10 cells/ml.
  • the culture was centrifuged at 8,000 r.p. . in a Sorval centrifuge, washed two times in minimal buffer (0.01 M KPO. pH 7.0, 0.5% NaCl, 0.001 M MgSO.) , and resuspended in " minimal buffer, which serves as the attachment medium.
  • beef cubes (ap ⁇ proximately 1.0 gram), excised aseptically from the cen ⁇ ter of a freshly slaughtered beef round, were first treated by immersion in 25 ml of various concentrations of aqueous chlorine dioxide for 3 minutes. The cubes were removed, blotted dry aseptically, and immersed in 10 ml of the bacterial suspension. Bacteria were allowed to attach for 5 minutes at 23° C. They were rinsed by immersion in an excess of minimal buffer, blotted and
  • Viability was determined by plating aliqu ⁇ ts of serial dilutions of a homogenate prepared by blending the beef cubes in a conventional blender in 25 ml of mini ⁇ mal buffer.
  • beef cubes were first immersed in 10 ml of the bacteria suspension for 5 minutes at 23 C. to permit attachment, drained and blotted. The cubes were then rinsed by immersion in an excess of minimal buffer, blotted and immersed in 25 ml of various concentrations of chlorine dioxide for 3 minutes. The cubes were then rinsed again in an excess
  • A. hydrophilis was uniformly 3 labeled with H-leucine and tested for attachment to beef cubes after treatment with various concentrations of C10_.
  • the data show that pre-treatment of meat cubes with chlorine dioxide at levels at least as low as 0.04 ppm substantially prevents attachment or adherence of microorganisms to the meat substrate compared to the un ⁇ treated control.
  • bacteria already attached or adhering to the meat are not readily killed at concentrations of C10 2 less than about 0.1 to 0.5 ppm, as indicated by colony-forming ability at 0.04 ppm approaching that of the untreated control.
  • bacteria In order to form a colony, bacteria must be able to reproduce, synthesizing macromolecular cellular components such as protein, nucleic acids, etc. Low
  • Table II summarizes the results of an experi ⁇ ment identical in format to part A of Example I, except that a wild-type E. coli lacking K88 and pili-associated adhesion antigens was substituted for the A. hydrophilis,
  • 3 H-thymidine (5uC/ml) was substituted for 3H-leucine in cell-labelling. Also, the cell suspension contained greater than 2.5 x 10 cells/ml since binding levels, as determined in pilot experiments, were markedly lower than for A. hydrophilis.
  • the present data indicates that a wild-type E. coli (lacking a pathogenic biological attachment mechanism) , also appears to lack a biological mechanism for attachment to meat. This suggests that the present process is particularly effective against organisms having a biological attachment mechanism (spoilage bacteria and possibly pathogens) ; it does not affect the nonpathogenic "free riders" which do not grow ap ⁇ preciably under refrigeration to cause spoilage.
  • Meat cubes were prepared and treated, as described in Example I hereinabove, with aqueous chlorine dioxide in various concentrations (zero, trace, 0.1, 0.5, 5.0, 10.0, 50.0 and 100.0).
  • the cubes, seeded with A. hydrophilis, were placed spacedly in Petri plates.
  • Molten soft McConky agar (0.2%) supplemented with 2 x 10 ⁇ M glucose was poured into the plates so as to fully im ⁇ merse the cubes. The plates were covered tightly to avoid evaporative loss of water and incubated for four days at 37° C.
  • the slime formation was confined to a narrow perimeter (l-2mm) around the cubes; whereas the trace and control cubes showed a spreading slime front wider than 1 cm.
  • An advantage of the present invention is minimiza ⁇ tion of the production of chloro-organic derivatives such as chloro-substituted lipids and chloro-aromatic compounds, generally referred to herein as organic chlorine. These are suspect of being carcinogenic or toxic. The health risks from such organic chlorine de ⁇ creases at least in proportion to the concentration of the chlorine disinfectant applied to meat. Chlorine dioxide in solution at approximately the lowest prior art level, 7 ppm, when applied to hog skin, has been found to cause formation of a level or organic chlorine barely within the resolution capability of available instrumentation. No detectable levels will be found of chlorine dioxide concentrations as low as 0.04 to 1.0 ppm. Thus, in the present use of chlorine dioxide at levels as low as 100 fold lower than heretofore used, any formation of organic chlorine is minimal.

Landscapes

  • Life Sciences & Earth Sciences (AREA)
  • Engineering & Computer Science (AREA)
  • Chemical & Material Sciences (AREA)
  • Wood Science & Technology (AREA)
  • Zoology (AREA)
  • Food Science & Technology (AREA)
  • Polymers & Plastics (AREA)
  • Chemical Kinetics & Catalysis (AREA)
  • General Chemical & Material Sciences (AREA)
  • Inorganic Chemistry (AREA)
  • Meat, Egg Or Seafood Products (AREA)

Abstract

Procede permettant d'empecher la viande de s'avarier, specialement pour de la viande fraiche de betes venant d'etre abattues. Une solution aqueuse de bioxyde de chlore est formee avec une concentration de 0,04-1,0 ppm, pour empecher les organismes de deterioration de la viande de se fixer sur celle-ci, mais non toxique pour les organismes. Des corps d'animaux recemment abattus sont laves avec la solution avant la fixation de ces organismes de deterioration de la viande sur ceux-ci. Ensuite, la solution est appliquee par intermittence sur ces pieces de viande pendant la refrigeration.Method for preventing meat from spoiling, especially for fresh meat from animals that have just been slaughtered. An aqueous solution of chlorine dioxide is formed with a concentration of 0.04-1.0 ppm, to prevent organisms from spoiling the meat from settling on it, but not toxic to the organisms. Bodies of recently slaughtered animals are washed with the solution before these meat spoilage organisms are attached to them. Then the solution is applied intermittently to these pieces of meat during refrigeration.

Description

- MEAT SPOILAGE INHIBITING PROCESS
Modern rapid distribution systems for fresh meats rely upon refrigeration and plant sanitation to provide a wholesome product to the consumer. Although fresh meats in the United States are generally safe and free of hazardous levels of pathogens, the microbial quality may be poor; high levels of non-pathogenic spoilage bacteria, frequently present, dramatically shorten shelf-life and affect the taste and appearance of the meat. In response to this problem, several states and the Federal Government have adopted or proposed standards regulating the bacterial content of fresh meat.
It is recognized that refrigeration is not a complete solution to spoilage problems because the principal spoilage bacteria are psychrotrophs which grow well at.5° -15° C, or mesotrophs which are adapted to grow at lower temperatures. Ayres, J. C. (Food Re¬ search, _25_:1, 1960) found that the dominant microorganisms growing on refrigerated beef comprised the Micrococci and Pseudomonads; even at temperatures as high as 15 C. the growing bacterial population was dominated by motile gram negative rods of the Pseudomonas generae. Other bacteria commonly present on fresh meat include the gram negative, flagellated generae: Serratia, Aeromonas, Proteus, etc. Together with the Pseudomonads these are responsible for off-color and slime produc¬ tion in decaying meat. Mesotrophs, typically the food-borne pathogens such as Salmonella, E. coli and gram positive anaerobes such as Clostridia, are now
O.MPI believed to be "free riders" and, particularly at re¬ frigerated temperatures, do not grow appreciably on meat surfaces; despite their dangerous nature they have no substantial role in food spoilage. (For example, see Goepfert, J.M., J. Milk- Food Technol., 38_:449, 1975).
Bacterial contamination of retail meat has been the subject of extensive studies whose conclusions are here set forth. The microorganisms present in re¬ tail portions are derived directly from the initial bacterial load on the carcass surface immediately post- slaughter; thus, meat portions, such as hamburger, having high bacterial counts are traceable to carcasses having high surface contamination. (For example, see Elliot, et al., Applied Microbiology, 9_:452, 1961). The primary source of such contamination is the gut and hide of the animal itself, although the packing house en¬ vironment (floors, chill room, cutting room, etc.), and handling by packing house workers are all substantial sources of contamination. (Frazier, Food Microbiology, Chapt. 16, 2d ed., 1967). Prolonged storage, as in aging, also increases contamination from the air, etc. Subsequent handling, as in transit, cutting, boning and packing, may offer serious contaminating events.
Several available processes eliminate bacteria from meat by killing them with a contact disinfectant(s) applied in the form of a spray to the carcass surface during chilling. U.S. Patent No. 3,745,026 (Hansen) discloses such a process utilizing 50-200 ppm of aqueous chlorine (hypochlorous acid). U.S. Patent No. 4,021,585 (Svoboda, et al.) describes an alternative process utilizing 5-50 ppm of aqueous chlorine dioxide. Both processes achieve reduced bacterial counts during the chill cycle (1S-24 hrs. post-slaughter) by killing - bacteria introduced onto the carcass during slaughter procedures. This is shown by the reduction in viable colony-forming bacteria present at the end of the chill cycle as compared with counts at the beginning of such period after carcasses are conveyed to the chill room from the kill floor.
A major problem with such use of chlorinated contact disinfectants is reaction of the agent with meat components to produce chloro-organic derivatives such as chloro-substituted lipids and chloro-aromatic compounds. These chlorinated derivates pose a potential health hazard, especially the class of halomethanes (known to be carcinogenic) formed by reaction of bactericidal levels of hypochlorous acid with humic or other or¬ ganic substances. Reaction of chlorine dioxide at bactericidal concentrations with meat components results in lower but detectable levels of organic chlorine.
Other agents such as inorganic and organic acids have also been applied to carcass surfaces in the form of aqueous sprays, as described in Carpenter, J.A., Proc. Meat Indust. Res. Conf. , Chicago, 1972. Use of these agents has not received widespread ac¬ ceptance because of substantial surface damage to the carcass, and the off-odors and flavors imparted to the meat at bacteriosta ic concentrations.
Summary of the Invention
A principal object of the present invention is to provide a process which prevents the attach¬ ment and growth of spoilage organisms at the surface of freshly slaughtered meat carcasses. ' A further object is to prevent establishment of spoilage bacteria on carcass surfaces without completely destroying the microflora thereof. A still further object is to pre¬ vent establishment of spoilage bacteria on carcass sur¬ faces without utilizing bactericidal concentrations of chlorine dioxide known to result in detectable levels of organic chlorine upon reaction with meat components.
Briefly summarizing, and without limiting the scope hereof, I have discovered that application to car¬ cass surfaces of aqueous chlorine dioxide at concentra¬ tions too low to be effective as a bactericide never¬ theless substantially inhibits attachment of spoilage organisms and prevents their growth upon the meat sub¬ strate. Chlorine dioxide solutions at concentrations as low as 100 fold lower than heretofore used are ef¬ fective for inhibiting attachment provided that their application to carcass surfaces commences at a time substantially coincident with contaminating events, as during slaughter procedures and subsequent chilling. At such low concentrations, no detectable organic chlorine is produced by reaction of the chlorine dioxide with meat components.
Brief Description of the Drawing
FIG. I is a rectilinear plot of the data presented in parts A and B of Example I.
Description of the Preferred Embodiment
In the present method, aqueous solutions of chlorine dioxide, so weak as to be substantially sub- toxic, are first applied substantially coincident with (that is, as close as feasible in point of time with) a significant contaminating event, and thereafter con¬ tinued by intermittent spraying. Thus, in slaughtering operations, such a solution is first applied as a low pressure (less than 45 psi) spray to meat carcass sur¬ face immediately post-slaughter and substantially co¬ incident in time with dehiding and dressing procedures on the kill floor. In addition, shrouds for beef may be soaked in the chlorine dioxide solution prior to draping. Carcasses customarily in halves or quarters) are then conveyed to a chill room and an aqueous chlorine dioxide solution is intermittently applied to such carcass portions over a conventional 14-24 hr. chill period. This method is adapted to such processing of fresh meat of domestic animals including but not limited to pork, beef, veal, and lamb.
Typically, the chlorine dioxide is generated on site with conventional apparatus and formed into solution with potable water to a concentration of 0.04- 1.0 ppm (mg/1) , preferably less than about 0.1 ppm (mg/1) prior to application. For reasons hereinafter more fully explained, it is critical that the solution be applied to carcass surfaces on the kill floor at a time substantially coirtident with contaminating events such as dehiding, disembowelment, etc. Thereafter, the chlorine dioxide solution is applied intermittently during chilling for such intervals and in such volume as prescribed by USDA regulations (generally a maximum total of 0.5 hr. spraying time in increments during the entire chill cycle) .
Significant contaminating events may occur thereafter, for example where carcasses are trans¬ shipped such as by rail or on ocean-going vessels. Handling as during such transshipment may expose the meat to substantial numbers of spoilage organisms. Hence, promptly on any significant contaminating event, the chlorine dioxide solution is applied to their surfaces and is thereafter applied, - preferably by intermittent spraying, during subsequent cold storage.
For purpose of this application, the term "cold storage'' includes chilling of freshly slaughtered carcasses; and the term "substantially coincident with a contaminating event" means either immediately before such event, or as it takes place, or so shortly there¬ after that attachment of meat spoilage organisms has not yet in fact occurred. While the preferred method of applying the solution to meat surfaces is by spraying, other methods may be used, such as washing or dipping at the time of kill, or on any contaminating event there¬ after, or in the storage room; while and during cold
O. PI storage application may be by such a procedure or by misting into the atmosphere at a constant low rate in¬ stead of intermittent spraying.
To be considered bactericidal in the meat slaughtering field, a solution should be effective to kill at least about 85%-90% of contaminating bacteria, as disclosed in U.S. Patent No. 4,021,585. That patent shows chlorine dioxide is so bactericidal at concentra¬ tions minimally 5.0 ppm.
In the present process, application of chlorine dioxide solutions at substantially subtoxic concentra¬ tions, that is, less than considered bactericidal, and preferably about 0.04-1.0 ppm, has been found to pre¬ vent attachment of spoilage microorganisms to meat sur¬ faces. Further, application of such substantially non- toxic concentrations will prevent growth of spoilage organisms on the meat surface, so as to avoid subsequent spoilage. Therefore, in the present process, the solu¬ tion is applied before the spoilage organisms have any opportunity to attach. Thus, in contrast to previous methods, application of such solutions is begun on the kill floor where the bacterial load derived from the hide and gut first comes into contact with the meat surface. Thereafter, subsequent contamination is pre¬ vented by further applications of the solution, as by intermittent spraying of carcasses during the chill cycle.
The examples herein demonstrate that typical spoilage organisms, i.e., Aeromonas, Pseudomonas, etc. possess a biological attachment mechanism when contacted with a raw meat surface. As used herein, the term bio¬ logical attachment mechanism refers to those macro- molecular components of the bacterial cell surface which effect specific adherence to some substrates but not others. Biological attachment is thus distinguished from the mere nonspecific entrapment of bacteria, in
'ϋ ' t'i z-A which dead cells adhere, as well as live ones, in a fibrous matrix such as meat, or from simple electro¬ static interaction.
Example I indicates that the specific bio¬ logical attachment mechanism of spoilage bacteria is strongly inhibited by the use of substantially non- toxic levels of chlorine dioxide in aqueous solution. Surprisingly, flagellated :E. coli K-12 (see Example II) , known to exhibit specific biological attachment to an¬ imal skin, shows only a low-level nonspecific "attach¬ ment" to raw meat surfaces. These results suggest that the present process is particularly suitable for elim¬ inating contamination of raw meat by spoilage organisms without further disturbing the microecology of the meat. Thus, rapid spoilage of fresh meat is avoided and for¬ mation of slime produced by the gram negative psychro- troph is retarded without providing a selective ad¬ vantage to pathogens.
Other advantages in the present process will become apparent from the following examples.
EXAMPLE I
The following tests demonstrated that coneen-.. trations of chlorine dioxide insufficient to be toxic to meat spoilage organisms nevertheless prevented their attachment to beef cubes.
Aeromonas hydrophilis was isolated from con¬ taminated beef samples embedded in 0.5% McConkey agar and incubated at 37° for three days. Glistening mucoid colonies grew up at the surface of the meat, spreading outward into the soft agar.
This isolate A. hydrophilis was grown in modi¬ fied tryptone broth (5.0 g/1 Difco tryptone, 0.5 g/1 Difco yeast extract, 5.0 g/1 NaCl, o.l% glucose) sup¬ plemented with 5.0 uC/ml H-leucine (New England Nuclear) to a density of approximately 3 x 10 cells/ml. The culture was centrifuged at 8,000 r.p. . in a Sorval centrifuge, washed two times in minimal buffer (0.01 M KPO. pH 7.0, 0.5% NaCl, 0.001 M MgSO.) , and resuspended in"minimal buffer, which serves as the attachment medium.
As part A of these tests, beef cubes (ap¬ proximately 1.0 gram), excised aseptically from the cen¬ ter of a freshly slaughtered beef round, were first treated by immersion in 25 ml of various concentrations of aqueous chlorine dioxide for 3 minutes. The cubes were removed, blotted dry aseptically, and immersed in 10 ml of the bacterial suspension. Bacteria were allowed to attach for 5 minutes at 23° C. They were rinsed by immersion in an excess of minimal buffer, blotted and
3 assayed for H in a Beckmann scintillation counter.
Viability was determined by plating aliquόts of serial dilutions of a homogenate prepared by blending the beef cubes in a conventional blender in 25 ml of mini¬ mal buffer.
As part B of the tests, beef cubes were first immersed in 10 ml of the bacteria suspension for 5 minutes at 23 C. to permit attachment, drained and blotted. The cubes were then rinsed by immersion in an excess of minimal buffer, blotted and immersed in 25 ml of various concentrations of chlorine dioxide for 3 minutes. The cubes were then rinsed again in an excess
3 ooff mmiinniimmaall bbuuiffer and assayed conventionally for H counts and viability.
Bo κ t.4 /
C.Y.PI Table I
A. hydrophilus ppm cιo2
0 0.04 0.08 5.0
A. *CPM-3H-labelled cells attaching after C10-, treatment... 743 150 91 50
% of control 100 20 13 7
% inhibition 0 80 87 93
B , Viability per gram of pre-attached cells treated subsequently with C102 5.0492** 4.8291 4.6749 4.1467
% of control 100 70.0 42.3 12.3
% reduction 0 30.0 57.7 87.7
*counts per minute/gram meat **log1Q cells/gram meat
In part A, above, A. hydrophilis was uniformly 3 labeled with H-leucine and tested for attachment to beef cubes after treatment with various concentrations of C10_. The data show that pre-treatment of meat cubes with chlorine dioxide at levels at least as low as 0.04 ppm substantially prevents attachment or adherence of microorganisms to the meat substrate compared to the un¬ treated control. In Part B, however, bacteria already attached or adhering to the meat are not readily killed at concentrations of C102 less than about 0.1 to 0.5 ppm, as indicated by colony-forming ability at 0.04 ppm approaching that of the untreated control.
In order to form a colony, bacteria must be able to reproduce, synthesizing macromolecular cellular components such as protein, nucleic acids, etc. Low
ffa -0MipPI levels °f CIO- thus do not substantially disrupt vital cell processes such as protein synthesis, but do in¬ terfere with the biological attachment mechanism of typical food-spoilage organisms. This experiment il¬ lustrates the efficacy of utilizing C102 at levels too low to produce detectable levels of chlorinated organic compounds upon contact with the meat, but which prevent attachment (and subsequent reproduction) of spoilage microorganisms.
The data of part A and part B of these ex¬ periments are plotted in FIG. 1 at 5.0 ppm, substantial¬ ly 90% of adherent bacteria are killed, in agreement with data disclosed in U.S. Patent No. 4,021,585, and at this high concentration inhibition of attachment of new contaminants (part A) is indistinguishable from cell killing. At lower concentrations, bactericidal ef- fectiveness decreases rapidly; however, new contaminants are powerfully inhibited from attaching at these low concentrations.
Example II
Table II summarizes the results of an experi¬ ment identical in format to part A of Example I, except that a wild-type E. coli lacking K88 and pili-associated adhesion antigens was substituted for the A. hydrophilis,
3 H-thymidine (5uC/ml) was substituted for 3H-leucine in cell-labelling. Also, the cell suspension contained greater than 2.5 x 10 cells/ml since binding levels, as determined in pilot experiments, were markedly lower than for A. hydrophilis.
CΛΪPI Table II
E . coli K-12* ppm cιo2
0.0 0.5 1.0 5.0
CPM**- H-labelled cells attaching after CIO- treatment 544 623 536 328
% of control 100 114 98.1 60.3
% inhibition 0 0 1.9 39.7
*Courtesy of B. Peoples, Department of Microbiology, St.
Louis University School of Medicine.
3 **Counts H per minute/gram meat
The data indicates that concentrations with
C102 up to known bactericidal levels were ineffective to prevent low level attachment of E_. coli to meat surfaces. Even cells actually killed at 5 ppm C102 treatment were only partially prevented from attaching; subtoxic levels of CIO- did not interfere with this nonspecific at¬ tachment.
The present data indicates that a wild-type E. coli (lacking a pathogenic biological attachment mechanism) , also appears to lack a biological mechanism for attachment to meat. This suggests that the present process is particularly effective against organisms having a biological attachment mechanism (spoilage bacteria and possibly pathogens) ; it does not affect the nonpathogenic "free riders" which do not grow ap¬ preciably under refrigeration to cause spoilage.
Example III
Pseudomonas aeruginosa (American Type Culture
Collection, courtesy of Midwest Medical Laboratory,' St.
Louis, Missouri) , another common meat spoilage organism,
3 was grown in modified tryptone broth containing H-leucine as described in Example I. Spot tests on thinly sliced
2 meat strips (1 cm ) were carried out as follows:
0.015 ml aliquot of the bacteria were spotted on the surface of meat strips previously treated by immersion in aqueous solutions of 0, 0.05, and 5.0 ppm C102. The spots so applied tended to spread out over the surface of the meat strips more or less uniformly. The strips were placed in Petri dishes and incubated for 2 hours at 37 C. The strips were then removed and rinsed in 3.0 is minimal buffer and the radioactivity in the rinse and on the meat was determined.
After the 2-hour incubation, 25.7% of total counts were bound to the meat surface treated with 5.0 ppm C10-, 21% of total counts were bound to the 0.05 ppm C102-treated strip, and 52% of total counts were bound to the untreated strip. The results indicate that at 0.05 ppm, bacterial attachment was inhibited, and the cells did not substantially recover their at¬ tachment function after 2 hours' incubation. The present process may therefore be carried out utilizing the in¬ termittent spray cycle mandated by the U.S. Department of Agriculture; it is not necessary to apply the C102 solution continuously.
Example IV
Meat cubes were prepared and treated, as described in Example I hereinabove, with aqueous chlorine dioxide in various concentrations (zero, trace, 0.1, 0.5, 5.0, 10.0, 50.0 and 100.0). The cubes, seeded with A. hydrophilis, were placed spacedly in Petri plates. Molten soft McConky agar (0.2%) supplemented with 2 x 10~ M glucose was poured into the plates so as to fully im¬ merse the cubes. The plates were covered tightly to avoid evaporative loss of water and incubated for four days at 37° C.
Results then observed were as follows: Those cubes treated with chlorine dioxide at concentrations of 5.0 ppm or greater (i.e., bactericidal concentrations) showed no slime development. At all lesser concentrations a spreading slime front, evidenc¬ ing bacterial growth, developed outwardly into the soft agar at the edges of the cubes.
At the concentrations of (0.1 ppm and 0.5 ppm), the slime formation was confined to a narrow perimeter (l-2mm) around the cubes; whereas the trace and control cubes showed a spreading slime front wider than 1 cm.
These results indicate that levels of chlorine dioxide insufficient to kill the cells nevertheless significantly retarded production of the slime char¬ acteristically secreted by the test organism.
An advantage of the present invention is minimiza¬ tion of the production of chloro-organic derivatives such as chloro-substituted lipids and chloro-aromatic compounds, generally referred to herein as organic chlorine. These are suspect of being carcinogenic or toxic. The health risks from such organic chlorine de¬ creases at least in proportion to the concentration of the chlorine disinfectant applied to meat. Chlorine dioxide in solution at approximately the lowest prior art level, 7 ppm, when applied to hog skin, has been found to cause formation of a level or organic chlorine barely within the resolution capability of available instrumentation. No detectable levels will be found of chlorine dioxide concentrations as low as 0.04 to 1.0 ppm. Thus, in the present use of chlorine dioxide at levels as low as 100 fold lower than heretofore used, any formation of organic chlorine is minimal.
SUBSTITUTE SKΞΞT

Claims

1. The process of avoiding spoilage of freshly slaughtered meat comprising the steps of forming an aqueous solution of chlorine dioxide in a concentration of 0.04-1.0 ppm, said concentration being great enough to substantially inhibit the attachment of meat spoilage organisms to said meat and, insufficient to form with the meat detectable levels of organic chlorine, washing, with said solution, freshly killed meat carcasses within a time prior to substantial attachment of such meat spoilage organisms to said meat carcasses and thereafter intermittently applying said solution to said car¬ casses during chilling.
2. The process of avoiding spoilage of freshly slaughtered meat comprising the steps of forming an aqueous solution of chlorine dioxide in a concentration of 0.04-1.0 ppm, said concentration being great enough to substantially inhibit the attachment of meat spoilage organisms to said meat and less than that which is toxic to such meat spoilage organisms; washing, with said solution, freshly killed meat carcasses within a time prior to substantial attachment of such meat spoilage organisms to said meat carcasses, and thereafter intermittently applying said solution to said carcasses during chilling.
3. The process of avoiding spoilage of raw meat comprising the steps of applying an aqueous solution of chlorine dioxide, in a concentration of 0.04-1.0 ppm, to the meat surfaces at a time substantially coincident with a contamina- ting event by meat spoilage microorganisms, said con¬ centration being less than that which is toxic to such meat spoilage microorganisms and great enough to substantially inhibit their at¬ tachment to the meat surfaces whereby to prevent establishment of such meat spoilage microorganisms on said meat surfaces and sub¬ stantially retard thereafter their secretion of slime, and thereafter applying such solution to said meat surfaces dur¬ ing cold storage.
O. PΓ
PCT/US1981/000033 1981-01-12 1981-01-12 Meat spoilage inhibiting process Ceased WO1982002322A1 (en)

Priority Applications (3)

Application Number Priority Date Filing Date Title
AU72226/81A AU7222681A (en) 1981-01-12 1981-01-12 Meat spoilage inhibiting process
EP81901410A EP0069120A1 (en) 1981-01-12 1981-01-12 Meat spoilage inhibiting process
PCT/US1981/000033 WO1982002322A1 (en) 1981-01-12 1981-01-12 Meat spoilage inhibiting process

Applications Claiming Priority (2)

Application Number Priority Date Filing Date Title
WOUS81/00033810112 1981-01-12
PCT/US1981/000033 WO1982002322A1 (en) 1981-01-12 1981-01-12 Meat spoilage inhibiting process

Publications (1)

Publication Number Publication Date
WO1982002322A1 true WO1982002322A1 (en) 1982-07-22

Family

ID=22161031

Family Applications (1)

Application Number Title Priority Date Filing Date
PCT/US1981/000033 Ceased WO1982002322A1 (en) 1981-01-12 1981-01-12 Meat spoilage inhibiting process

Country Status (3)

Country Link
EP (1) EP0069120A1 (en)
AU (1) AU7222681A (en)
WO (1) WO1982002322A1 (en)

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2008073819A1 (en) * 2006-12-08 2008-06-19 Johnsondiversey, Inc. Cleaning apparatus and method

Citations (6)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US1681009A (en) * 1923-06-23 1928-08-14 Paul W Petersen Process of refrigerating and preserving comestibles
US3745026A (en) * 1971-03-31 1973-07-10 Swift & Co Carcass chilling process
US3819329A (en) * 1971-05-11 1974-06-25 Morton Norwich Products Inc Spray sanitizing system with electrolytic generator
US3958020A (en) * 1975-01-16 1976-05-18 Quad Corporation Bactericidal wash for meat
US3996386A (en) * 1971-12-15 1976-12-07 Yrjo Malkki Method for preventing microbial surface deterioration of foods and feeds
US4021585A (en) * 1976-01-16 1977-05-03 Krey Packing Company Chlorine dioxide spray process for chilling meat carcasses

Patent Citations (6)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US1681009A (en) * 1923-06-23 1928-08-14 Paul W Petersen Process of refrigerating and preserving comestibles
US3745026A (en) * 1971-03-31 1973-07-10 Swift & Co Carcass chilling process
US3819329A (en) * 1971-05-11 1974-06-25 Morton Norwich Products Inc Spray sanitizing system with electrolytic generator
US3996386A (en) * 1971-12-15 1976-12-07 Yrjo Malkki Method for preventing microbial surface deterioration of foods and feeds
US3958020A (en) * 1975-01-16 1976-05-18 Quad Corporation Bactericidal wash for meat
US4021585A (en) * 1976-01-16 1977-05-03 Krey Packing Company Chlorine dioxide spray process for chilling meat carcasses

Cited By (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2008073819A1 (en) * 2006-12-08 2008-06-19 Johnsondiversey, Inc. Cleaning apparatus and method
US8684799B2 (en) 2006-12-08 2014-04-01 Diversey, Inc. Cleaning apparatus and method

Also Published As

Publication number Publication date
AU7222681A (en) 1982-08-02
EP0069120A1 (en) 1983-01-12

Similar Documents

Publication Publication Date Title
US4244978A (en) Attachment inhibition of meat spoilage organisms to meat
US6039992A (en) Method for the broad spectrum prevention and removal of microbial contamination of food products by quaternary ammonium compounds
AU646797B2 (en) Antimicrobial compositions, film and method surface treatment of foodstuffs
Scannell et al. Determination of the influence of organic acids and nisin on shelf‐life and microbiologicalsafety aspects of fresh pork sausage
US8323673B2 (en) Concentrated, non-foaming solution of quaternary ammonium compounds and methods of use
Cutter et al. Reduction of Brochothrix thermosphacta on beef surfaces following immobilization of nisin in calcium alginate gels
US4362753A (en) Meat carcass sanitizing process
RS57302B1 (en) Pyrrolo[2,3-b]pyridin-4-yl-amines and pyrrolo[2m3-b]pyrimidin-4-yl-amines as janus kinase inhibitors
US5085873A (en) Process for the treatment of a non-liquid food product for assuring its microbial decontamination
Goncalves et al. Quantitative investigation on the effects of chemical treatments in reducing Listeria monocytogenes populations on chicken breast meat
WO1982002322A1 (en) Meat spoilage inhibiting process
CA1165618A (en) Attachment inhibition of meat spoilage organisms
US20050224097A1 (en) Methods of detaching microorganisms from, or of inhibiting microbial attachment to, animal or poultry carcasses or seafood or parts thereof
WO1981003110A1 (en) Meat sanitizing process
EP0868122A1 (en) Bacterial decontamination method
Paulsen Combining natural antimicrobial systems with other preservation techniques: the case of meat P. Paulsen and FJM Smulders, University of Veterinary Medicine Vienna, Austria
Paulsen et al. Reduction of the microbial contamination of carcasses and meat cuts with particular reference to the application of organic acids
Egan Ionising energy treatment of carcasses, packaged fresh meat and processed meats
Carlile Effectiveness of organic acids, bacteriocin-based biopreservatives and trisodium phosphate as beef sanitizers
Roberts et al. Control in Meat and Meat Products
Hippe Effect of spray-chilling on microbiological quality and weight loss in beef
AU7179481A (en) Meat sanitizing process

Legal Events

Date Code Title Description
AK Designated states

Designated state(s): AU RO

AL Designated countries for regional patents

Designated state(s): DE FR GB