본 연구는 계란가공전문업체에서 생산하는 즉석섭취 알가공품의 미생물학적 안전성을 분석한 연구로 제품의 종류에 따라 일반세균 및 coliforms의 오염수준의 차이가 매우 크며 식중독균의 증식/생존 양상에도 영향을 미치는 것으로 나타났다. 즉석섭취 알 가공품 중 계란구이의 가공 공정단계에서 미생물 오염도를 조사한 결과에 따르면 공정 초기단계에서 aerobic plate counts 오염 수준은 높았으나 가열 성형 공정 이후 급격하게 감소하여 공정 과정 이후 낮은 수준으로 유지하는 것으로 보아 HACCP 공정에서의 CCP 관리는 적절하게 수행되고 있는 것으로 나타났다. 완제품의 경우 치즈, 참치, 피자오믈렛과 계란구이, 계란 찜은 미생물 규격 기준에 부합하였으나 떡갈비오믈렛과 지단채는 허용 불가능한 수준으로 확인되었다. 특히 지단채의 경우 레토르트 공정을 거치지 않는 제조 공정에 따른 특성 때문인 것으로 판단되어 이를 보완할 수 있는 관리 방안이 필요할 것으로 보이며, 오믈렛의 경우 계란 이외의 내용물이 추가 주입되므로 부 재료의 관리도 중요한 것으로 나타났다. 또한 병원성 식중독균을 인위적으로 오염시킨 즉석섭취 알 가공품을 4, 10, 15℃에 저장하면서 미생물의 증식 및 생존을 관찰한 결과, L. monocytogenes는 저장 기간 내 모든 온도에서 증식하였다. 특히 계란구이에서 S. Typhimurium과 E. coli는 4℃와 10℃ 저장조건에서 사멸하였으나, 15℃ 저장조건에서는 동일한 저장기간 동안에 급격하게 성장하는 것으로 나타나, 유통/판매 조건에서 온도 관리 또한 철저하게 수행되어야 할 것으로 판단된다. 또한 계란구이에서 S. Typhimurium에 비해 S. Enteritidis의 증식 속도가 더 빠른 것으로 나타났으며 계란 찜에서도 S. Typhimurium는 사멸하는 반면 S. Enteritidis 증식은 잘 이루어 져 알 가공품에서의 S. Enteritidis의 증식 위험성이 더 큰 것으로 나타나 식용란이 생산되는 과 정에서도 S. Enteritidis 오염예방이 매우 중요한 것으로 판단된다. 또한 알 가공품의 경우 제조 시설에서의 위생적인 제품 생산뿐만 아니라 조리 시 적절한 가열, 가열 후 교차오염 방지, 조기섭취 등 유통/보관 후 소비자 섭취시점까지의 안전관리 방안이 필요하다.

The current standard solutions for somatic cells used for calibration of electronic somatic cell counts as reference material in raw milk are preserved with bronopol, boric acid, sodium azide, or potassium dichromate, and have a shelf-life of only up to 6 days at 4 ± 2℃. In the present study, a set of somatic cell standard solutions (SCSS) with a stability of 5 months for calibration of electronic instruments was developed. Somatic cells collected from cow’s milk and stored in a bulk tank at a dairy plant were treated with 10% formaldehyde in order to improve stability, and then separated by centrifugation. The resulting somatic cell suspension was preserved with glycerin, thimerosal, and dimethyl sulfoxide, and diluted in 3% processed skim milk solution ranging from 200,000～250,000 (low level), 350,000～ 450,000 (medium level), and 550,000～650,000 (high level) cells/㎖. Each SCSS was verified by direct microscope somatic cell counting (DMSCC), C-reader, and commercial standard samples. The average somatic cell count determined by DMSCC was 248, 214, 226 × 103 cells/㎖, 436, 382, 420 × 103 cells/㎖, and 612, 595, 609 × 103 cells/㎖. The coefficient of variation representing the repeatability of DMSCC decreased as the number of cells increased, and was <10.0% in almost all SCSS samples (range 4.6～7.1%). No statistically significant difference in somatic cell concentration was observed after storage at refrigeration temperature (2～6℃) over a period of 22 weeks (5 months). The stabilized SCSS may be useful as a reference material for determination of somatic cell count and quality control in testing of bovine raw milk.

We compared between an automated most-probable-number technique TEMPO®TVC and traditional plating methods PetrifilmTM for estimating populations of total aerobic bacteria in various livestock products. 257 samples randomly selected in local retail stores and 87 samples inoculated with E. coli ATCC 25922, Staphylococcus aureus ATCC 12868 were tested in this study. The degree of agreement was estimated according to the CCFRA (Campden and Chorleywood Food Research Association Group) Guideline 29 and the agreement indicates the difference of two kinds methods is lower than 1 log base 10(log10). The samples of hams, jerky products, ground meat products, milks, ice creams, infant formulas, and egg heat formed products were showed above 95% in the agreement of methods. In contrast, proportion of agreement on meat extract products, cheeses and sausages were 93.1%, 92.1%, 89.1%, respectively. One press ham and five sausages containing spice and seasoning, two pork cutlets containing spice and bread crumbs, two meat extract product and two natural cheeses and one processing cheese with a high fat content, and one ice cream containing chocolate of all samples showed the discrepancy. Our result suggest that TEMPO®TVC system is efficient to analyses total aerobic bacteria to compare manual method in time-consuming and laborious process except livestock products having limit of detection.

We investigated the prevalence of the Listeria monocytogenes from livestock processed products in processing plants and retail markets of Korea from 2010 to 2011. A total of 1,380 samples were collected; Meat processed products such as cooked ham and sausage, jerked meat, and meat extract products. Milk processed products such as milk, butter, cheese, and ice cream. Egg processed products such as whole egg liquid and pidan. L. monocytogenes were isolated from samples using listeria enrichment broth, fraser broth and Oxford agar, and counted in Oxford agar. The three of L. monocytogenes strains (1.16%) were isolated from sausages, two (0.73%) from mixed pressed ham and one (0.51%) from jerked meat, respectively. The colony forming unit (CFU) of L. monocytogenes from all samples were below 10 CFU/g. The four isolates (66.6%) were 1/2b except two isolates (1/2a) in the serotypes. Further studies are needed to understand the transmission route of L. monocytogenes, including a survey of food handlers, environments of retail markets, and all potential risk factors in cooked sausages, mixed pressed hams, and jerked meat processing.

Horse population has been gradually increasing with the growth of the racing industry in Republic of Korea (ROK). Approximately 22,941 horses including native ponies were raised on 1,142 farms in 2006. Great care has been taken to prevent viral, bacterial and parasitic infections in horses. However, there has been few reports on equine infectious anemia (EIA) in ROK until recently since 1987. Therefore, we conducted a serological survey of EIA in ROK from 2007 through 2009. Using the agar gel immunodiffusion test, a total of 2,601 horses were tested in Foreign Animal Disease Division of Animal, Plant, and Fisheries Quarantine and Inspection Agency. This survey found no serological evidence of EIA presence in ROK. Although our surveillance found no evidence of EIA in ROK during the surveillance period, it is possible that EIA could be introduced into ROK in the near future. Increased cooperation between the government and other agencies, such as horse-racing authorities, is important for both the early detection of the disease and the development of effective veterinary and public health strategies.

To evaluate the performance of a new automated coliform enumeration system (TEMPO® CC) for the quantitative test of coliform bacteria contaminated in domestic livestock processed foods, a total of 507 samples of livestock foods were tested by the TEMPO® CC method, the most probable number (MPN) method, and Petrifilm method, respectively. The results of those three methods were compared to each other. Of 507 samples of livestock processed foods used in this study, 217 samples were contaminated artificially with coliform bacteria and the rest (n=290) were contaminated naturally. The results of the TEMPO® CC method for all samples were equivalent to those obtained from the MPN method, except 8 samples. In addition, 496 (97.8%) out of 507 samples made agreement between the TEMPO® CC method and the Petrifilm method. The correlation coefficients between TEMPO® CC and MPN methods as well as between TEMPO® CC method and Petrifilm method were above 0.9, and the slope and intercept of the linear regression model was different in less than 1 value. In conclusion, there were statistically equivalent levels of performance between the TEMPO® CC and the reference and alternative methods for the enumeration of coliform bacteria in livestock processed foods in this study.

We constructed a standard curve to quantify Listeria monocytogenes in ready-to-eat product, especially sausage samples, using real-time PCR. A standard curve was generated using serially diluted L. monocytogenes cells in distilled water. When cells were artificially inoculated in 10 g of sausage samples in 90㎖ buffered peptone water, the cell concentration of range was approximately 1.0×108 to 100 CFU/㎖. The standard curve of the serially diluted cells was linear for at least seven orders of magnitude from 103 to 109 CFU/㎖ of L. monocytogenes. When cells were diluted in sausages, the linearity range was from 104 to 108 CFU/㎖. The correlation coefficient (R2) of diluted cells was 0.9888 and the slope of the curve was —2.6621. The coefficient and slope of inoculated samples were 0.9916 and —2.747, respectively. The R2 value for serially diluted L. monocytogenes and artificially contaminated sausage samples were acceptable. The approach described in this study represents the potency of the quantification of L. monocytogenes in sausage samples by quantitative real-time PCR. It can be used in monitoring the presence and persistence of this pathogen in sausages.

To determine the prevalence of Campylobacter jejuni and Campylobacter coli in meats, a total of 4,161 samples (1,953 domestic and 2,208 imported) were collected from 304 slaughterhouses nationwide and registered cold storages for imported meats in Korea during 2005～2009. The isolation rates of C. jejuni and C. coli in domestic beef, pork, chicken and duck meats were 0.1% (1/630), 0% (0/630), and 0.1% (1/644), 0% (0/644) and 20.5% (125/609), 10.2% (62/609) and 25.7% (18/70), 20.0% (14/70), respectively. In the case of imported meats, C. jejuni were isolated from 0.1% (1/943) and 15.2% (83/546) of pork and chicken meats, respectively, and C. coli were detected only from 4.8% (26/546) of chicken meats. Neither C. jejuni nor C. coli were detected from imported beef, and C. coli were also not detected from imported pork. In conclusion, chicken meats had much higher rate of contamination with Campylobacter compared to beef and pork. Therefore, HACCP system that is now mandatory for slaughterhouses should be actively practiced for safe and sanitary processing, handling, and marketing of chicken meats. In addition, all critical control points should be determined by processing procedures at processing plants as well as farms and slaughterhouses, and monitoring should be carried out at regular intervals.