ABSTRACT
1. Small sections cut from commercial crates used to transport live poultry to the processing plant were artificially contaminated with effluent taken from a commercial crate-cleaning system. 2. Laboratory trials, involving the immersion of these sections in an ultrasonic water bath (4 kW energy) showed that aerobic plate counts (APC) and counts of Enterobacteriaceae were progressively reduced as the immersion time was increased from 0 to 120 s and the water temperature raised from 35 to 58 degrees C. 3. In subsequent trials at a processing plant, using commercially cleaned crates, there was relatively little effect of ultrasound (or pressure washing) on the biofilm present. However, ultrasonic treatment in combination with an immersion temperature of 60 degrees C reduced counts of Enterobacteriaceae to below the detection limit (log(10) 2.3 cfu) within 1 to 3 min, while APC were reduced by >2 log(10) units after 3 min. 4. It was concluded that ultrasonic treatment has a possible role in the crate-cleaning process, when used in conjunction with higher immersion temperatures. In this way, it could contribute significantly to hygiene control.
Subject(s)
Housing, Animal , Poultry/microbiology , Transportation/instrumentation , Ultrasonics , Animals , Biofilms , Disinfection , Equipment Design , Food Contamination/prevention & control , HygieneABSTRACT
1. The present systems for cleaning the plastic crates (drawers) used to transport live poultry to the processing plant are known to be inadequate for removing microbial contamination. 2. To investigate possible improvements, a mobile experimental rig was constructed and operated in the lairage of a poultry processing plant. The cleaning rig could simulate the conditions of commercial cleaning systems and utilise freshly emptied crates from the processing plant. 3. The aim of the study was to improve cleaning by enhancing the removal of adherent organic material on the crates and by reducing microbial contamination by at least 4 log(10) units. 4. Trials showed that the most effective treatments against Campylobacter were either (a) the combination of soaking at 55 degrees C, brushing for 90 s, washing for 15 s at 60 degrees C, followed by the application of disinfectant (Virkon S in this study) or (b) the use of ultrasound (4 kW) at 65 degrees C for 3 to 6 min, with or without mechanical brushing of crates. 5. Both of these treatments also achieved a 4 log(10) reduction or more in the counts of Enterobacteriaceae but were less effective in reducing aerobic plate counts. 6. It was noted that there was little correlation between the visual assessment of crate cleanliness and microbiological counts. 7. It was concluded that the demonstrated enhanced cleaning could contribute significantly to overall hygiene control in poultry meat production.
Subject(s)
Campylobacter/isolation & purification , Hygiene , Poultry/microbiology , Transportation/standards , Animals , Detergents , Disinfection , Equipment Design , Food MicrobiologyABSTRACT
This paper describes a novel method of measuring the contamination of raw foods with airborne bacteria during primary processing. To demonstrate the approach, this study aimed to quantify the role of airborne bacteria in the contamination of broiler chicken carcasses undergoing processing in an evisceration room. Settle plates and broiler carcasses were exposed to the evisceration room air or to ultra-clean air provided by a high efficiency particulate air (HEPA) unit located within the room. The use of ultra-clean air reduced the total aerobic counts on horizontal settle plates by 68-fold, and on vertical settle plates by 14-fold. The use of ultra-clean air had no significant effect on the total aerobic counts on carcasses as measured by sponging (3.5 log(10) CFU cm(-2)) or skin excision (4.0 log(10) CFU cm(-2)). The novel approach was able to show that the carcasses entering the room were so heavily contaminated that the airborne bacteria in the evisceration room contributed less than 1% of the total numbers of bacteria on the carcasses.
Subject(s)
Air Microbiology , Bacteria/isolation & purification , Chickens/microbiology , Food Contamination/analysis , Food Handling/methods , Food-Processing Industry/standards , Animals , Colony Count, Microbial , Filtration , Food Contamination/prevention & control , Food Microbiology , Food-Processing Industry/methods , HumansABSTRACT
1. A readily identifiable strain of Escherichia coli K12 was used as a 'marker' organism to determine the sources, routes and patterns of microbial cross-contamination during mechanical defeathering of broiler chicken carcases. 2. Inoculation of scald water with the marker organism led to a relatively even pattern of carcase contamination during subsequent defeathering. Microbial cross-contamination was greater by this route of inoculation than by either surface inoculation of a 'seeder' carcase or oral inoculation of a live bird one day before slaughter. 3. Dispersal of the marker organism was strongly influenced by the mechanical action of the defeathering machines. Forward transmission of the marker occurred by aerosol or large airborne droplets and particulates such as feathers. Moving carcases through the defeathering machines when these were non-operational clearly reduced backward transmission of the marker. 4. Although microbial dispersal was unaffected by increasing the spacing between individual carcases or installing a water curtain at the entry and exit of the defeathering machines, shielding of carcases with aluminium baffles reduced counts of the marker organism from contaminated carcases by > 90%. 5. The results imply that microbial cross-contamination of broiler chicken carcases during defeathering occurs mainly via the airborne route, which could be contained by physical means.
Subject(s)
Air Microbiology , Escherichia coli Infections/veterinary , Escherichia coli/isolation & purification , Feathers , Poultry Diseases/transmission , Abattoirs/standards , Animal Husbandry , Animals , Escherichia coli Infections/prevention & control , Escherichia coli Infections/transmission , Poultry Diseases/microbiology , Poultry Diseases/prevention & control , WaterABSTRACT
1. The extent of cross contamination between carcases and the dispersal of micro-organisms to the environs during defeathering was measured in a commercial processing plant. 2. Defeathering reduced the numbers of a marker organism, a nalidixic acid-resistant strain of Escherichia coli K12, on inoculated carcases but dispersed the organism on to preceding and following carcases. 3. The pattern of microbial dispersal during defeathering was similar for naturally occurring bacteria on the carcase, for example, total aerobic counts and counts of presumptive coliforms, suggesting that the marker organism mimics the natural situation realistically. 4. The majority of feathers, together with micro-organisms, were removed during the first 10 s of the defeathering process, which was completed in 45 s, indicating that control measures to minimise cross contamination would be most effective if applied in the early stages of the process. 5. The method of defeathering used by the machine influenced the pattern of microbial dispersal and the extent of cross contamination to other carcases on the same processing line.
Subject(s)
Abattoirs , Bacteria, Aerobic/isolation & purification , Escherichia coli/isolation & purification , Feathers/microbiology , Feathers/physiology , Animals , ChickensSubject(s)
Abattoirs/instrumentation , Animal Welfare , Electroshock/veterinary , Poultry , Animals , Time FactorsABSTRACT
Two series of experiments were carried out to investigate methods of reducing contamination of lamb carcasses in low-throughput abattoirs, where cradle dressing is normally employed. In the first series, cradle design and pelt removal procedure were investigated, and a method was developed for assessing gross visible contamination. Significant improvements in microbiological and gross visible contamination (P < 0.01) were achieved by procedural changes only; modifications to the cradle design had no effect. In the second series of experiments, two improved methods of pelt removal and the effect of hand washing prior to carcass contact during the pelt removal procedure were investigated. The improved methods comprised a Frame system, in which the pelt was removed in a manner similar to that in a high-throughput inverted line, and a Hybrid system, in which the pelt was removed from the forequarters on a conventional cradle before the carcass was suspended in an "inverted" vertical position for removal of the pelt from the abdomen and hindquarters. The results of microbiological and gross visible contamination from these methods, with and without hand washing, were compared with the conventional Cradle method of pelt removal. Both the Hybrid and Frame systems had significantly less microbiological and gross visible contamination (P < 0.01). However, hand washing had no significant effect on the level of carcass contamination for all three methods of pelt removal. Greatest reductions in microbiological and gross visible contamination were achieved using techniques that minimized hand contact with the carcass during pelt removal by adoption of inverted dressing procedures. Equipment redesign did not reduce carcass contamination.
Subject(s)
Abattoirs/standards , Food Contamination/prevention & control , Food Handling/methods , Sheep/microbiology , Animals , Colony Count, Microbial , Disinfection , Equipment Contamination , Hand Disinfection , Humans , HygieneABSTRACT
1. An experimental rig, designed and built to simulate conditions found in commercial poultry chilling systems, was used to investigate the effects of varying air temperature and chilling duration, and the effect of chlorinated water sprays, on the microbial load present on the skin and in the body cavity of freshly eviscerated poultry carcases; deep muscle and skin temperatures were monitored during chilling at three different temperatures. 2. During dry chilling for 2 h, total viable microbe counts (TVC) and counts of coliforms and pseudomonads from the body cavity fell by between half and one log unit; smaller reductions were observed in samples from the breast skin. 3. The situation changed when chlorinated water sprays (50, 100 or 250 ppm available chlorine) were applied for the first hour of chilling; spraying carcases enhanced the reduction in numbers on the skin; the effect was most pronounced with 250 ppm chlorine; conversely in the body cavity, the general effects of sprays was to increase contamination by up to one log unit. 4. There was no evidence that sprays increased the rate of chilling. 5. When carcases were held overnight in the rig at 11 degrees C after chilling, microbe counts on dry-chilled carcases remained stable, but increased on carcases that had been sprayed with chlorinated water.
Subject(s)
Chickens/microbiology , Cold Temperature , Food Preservation/methods , Food-Processing Industry/methods , Meat/microbiology , Animals , Chlorine , Colony Count, Microbial/veterinary , Disinfectants , Enterobacteriaceae/isolation & purification , Food Preservation/instrumentation , Food-Processing Industry/instrumentation , Foodborne Diseases/prevention & control , Pseudomonas/isolation & purification , Refrigeration , Skin/microbiologyABSTRACT
Studies of the metabolic and physiological changes that bears undergo during hibernation have, for the most part, supported the paradigm that bears use only fatty tissues as a metabolic substrate during hibernation. This study was performed to document the extent of protein loss and alteration of muscle-fiber characteristics of selected muscles in black bears during winter dormancy. Muscle biopsies were removed from the gastrocnemius and biceps femoris from seven free-ranging female black bears on the Uncompahgre Plateau in west-central Colorado. Six of the seven bears produced cubs during the hibernating season. Muscle samples were collected from the left hind limb shortly after bears entered their dens (fall), and additional samples were collected from the right hind limb just prior to bears leaving their dens (spring). Protein concentration, fast- and slow-twitch muscle-fiber ratios and muscle-fiber cross-sectional areas, and citrate synthase activity were measured in the laboratory. While protein concentration decreased in both muscles during the hibernation period, it was lower than predicted for lactating females. In addition, muscle-fiber number and cross-sectional area were unchanged in these muscles, suggesting only limited muscle atrophy. In support of these observations, there was a moderate but significant increase in the proportion of fast-twitch fibers only in the biceps femoris, with a concomitant decrease in citrate synthase activity, but no alteration of the fiber ratio in the gastrocnemius during hibernation. These findings suggest that hibernating bears, particularly lactating females, do use some protein, in concert with fat catabolism, as a metabolic substrate and as a source of water. However, the extent of this protein use is moderate and is associated with limited alteration of muscle structure, characteristic of disuse atrophy.
