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GB 4789.6-2016 PDF English

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GB 4789.6-2016: National food safety standard -- Microbiological examination of food -- Examination of diarrheagenic Escherichia coli
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GB 4789.6: Historical versions

Standard IDUSDBUY PDFDeliveryStandard Title (Description)Status
GB 4789.6-2016155 Add to Cart Auto, 9 seconds. National food safety standard -- Microbiological examination of food -- Examination of diarrheagenic Escherichia coli Valid
GB/T 4789.6-2003279 Add to Cart 3 days Microbiological examination of food hygiene -- Examination of diarrheagenic Escherichia coli Obsolete
GB 4789.6-1994RFQ ASK 3 days Microbiological examination of food hygiene. Examination of diarrheogenic Escherichia coli Obsolete
GB 4789.6-1984RFQ ASK 3 days Microbiological examination of food hygiene--Examination of enteropathogenic escherichia coli Obsolete

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GB 4789.6-2016: National food safety standard -- Microbiological examination of food -- Examination of diarrheagenic Escherichia coli


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GB NATIONAL STANDARD OF THE PEOPLE’S REPUBLIC OF CHINA National Food Safety Standard - Food Microbiological Examination - Diarrheagenic Escherichia Coli ISSUED ON: DECEMBER 23, 2016 IMPLEMENTED ON: JUNE 23, 2017 Issued by: National Health Commission of the People’s Republic of China; State Administration for Market Regulation.

Table of Contents

Foreword ... 3 1 Scope ... 4 2 Terms, Definitions and Abbreviations ... 4 3 Apparatus and Materials ... 6 4 Media and Reagents ... 7 5 Examination Procedures ... 8 6 Operation Steps ... 10 7 Result Report ... 17 Appendix A Media and Reagents ... 18 National Food Safety Standard - Food Microbiological Examination - Diarrheagenic Escherichia Coli

1 Scope

This standard specifies the examination method of diarrheagenic Escherichia coli in foods. This standard applies to the examination of diarrheagenic Escherichia coli in foods.

2 Terms, Definitions and Abbreviations

2.1 Terms and definitions For the purpose of this standard, the following terms and definitions apply. 2.1.1 Diarrheagenic Escherichia coli A kind of Escherichia coli can cause diarrhea-based symptom in human body via contaminated food. The common diarrheagenic Escherichia coli mainly includes enteropathogenic Escherichia coli, enteroinvasive Escherichia coli, enterotoxigenic Escherichia coli, Shiga toxin-producing Escherichia coli (including enterohemorrhagic Escherichia coli) and enteroaggregative Escherichia coli. 2.1.2 Enteropathogenic Escherichia coli The Escherichia coli that can cause adhesion and wiping damage of host intestinal mucosa epithelial cell and does not produce Shiga toxin. This bacterium is the main pathogenic bacteria causing infant diarrhea, with high infectivity, which can be fatal in severe cases. 2.1.3 Enteroinvasive Escherichia coli The Escherichia coli that can invade intestinal epithelial cell to cause dysentery-like diarrhea. This bacterium is free from power, lysine decarboxylic reaction and lactose fermentation, while with both biochemical reaction and antigenic structure approximate to that of Shigella dysenteriae. The key genes intruding epithelial cell are antigen encoding gene and controlling gene of invasive plasmid, such as ipaH-gene and ipaR-gene (also referred to as invE-gene). 2.1.4 Enterotoxigenic Escherichia coli The Escherichia coli that can secrete heat-stable enterotoxin or/and heat-labile enterotoxin. This bacterium may cause infant and tourist diarrhea, which shows mild water-like diarrhea generally, and may shows serious cholera-like symptom, with low fever or no fever. Diarrhea is often self-limiting and can be self-healing in 2d~3d generally. 2.1.5 Shiga toxin-producing Escherichia coli (Enterohemorrhagic Escherichia coli) The Escherichia coli that can secrete Shiga toxin and cause adhesion and wiping damage of host intestinal mucosa epithelial cell. Some Shiga toxin-producing Escherichia coli can cause clinically hemorrhagic colitis (HC) and bloody diarrhea in human, and may be further developed to become hemolytic uremic syndrome (HUS), this kind of Shiga toxin-producing Escherichia coli refers to enterohemorrhagic Escherichia coli. 2.1.6 Enteroaggregative Escherichia coli Enteroaggregative Escherichia coli does not invade intestinal epithelial cell, but can cause intestinal fluid accumulation. It neither produces heat-stable enterotoxin/heat-labile enterotoxin nor Shiga toxin. It is only characterized by enteroaggregative adhesion on Hep-2 cell, thus also referred to as Hep-2 cell adhesive Escherichia coli. 2.2 Abbreviations For the purposes of this standard, the following abbreviations apply. 2.2.1 DEC: Diarrheagenic Escherichia coli 2.2.2 EPEC: Enteropathogenic Escherichia coli 2.2.3 EIEC: Enteroinvasive Escherichia coli 2.2.4 ETEC: Enterotoxigenic Escherichia coli 2.2.5 STEC: Shiga toxin-producing Escherichia coli 2.2.6 EHEC: Enterohemorrhagic Escherichia coli 2.2.7 EAEC: Enteroaggregative Escherichia coli 2.2.8 escV: gene encoding LEE-encoded type Ⅲ secretion system factor 2.2.9 eae: gene encoding intimin for Escherichia coli attaching and effacing 2.2.10 bfpB: bundle-forming pilus B; 2.2.11 stx1: Shiga toxin one

6 Operation Steps

6.1 Sample preparation 6.1.1 Solid or semi-solid sample Foe solid or semi-solid sample, weigh 25g of examined sample by aseptic operation, add it into a homogenizing cup with 225mL of nutrient broth to homogenize by a spinning blade-type homogenizer at 8000r/min~10000r/min for 1min~2min; or add the examined sample into a homogenizing bag with 225mL of nutrient broth to homogenize by a slap-type homogenizer for 1min~2min. 6.1.2 Liquid sample Weight 25mL of examined sample by aseptic technique, add it into an aseptic conical flask with 225mL of nutrient broth (proper amount of aseptic glass beads may be preset in the flask), and then oscillate the flask to mix them well. 6.2 Enrichment Culture the homogeneous sample solution prepared in 6.1 at 36℃±1℃ for 6h. Take 10μL of the solution, inoculate it into 30mL enterobacteria enrichment broth tube, and then culture at 42℃±1℃ for 18h. 6.3 Isolation Carry out streak inoculation for the enrichment broth into MAC and EMB agar plates, culture them at 36℃±1℃ for 18h~24h, and then observe colony characteristics. On the MAC agar plate, the typical colony decomposing lactose is brick red to peach while the colony not decomposing lactose is colorless or light pink. On the EMB agar plate, the typical colony decomposing lactose is purple black with or without metallic luster in center while the colony not decomposing lactose is colorless or light pink. 6.4 Biochemical test 6.4.1 Select 10~20 suspicious colonies from the plates (select all colonies in case of 10 below), therein lactose-fermented, lactose non-fermented and delayed fermented colonies shall be picked up to inoculate TSI slants respectively. Simultaneously, inoculate these cultures to peptone water, urea agar (pH 7.2) and KCN broth respectively. Culture them at 36℃±1℃ for 18h~24h. 6.4.2 In the case that TSI slant produces acid or fails to produce acid, bottom layer produces acid, indole is positive, as well as both H2S and urase are negative, the culture is Escherichia coli. In the case that TSI slant and bottom layer fails to produce acid, or any one of H2S, KCN and urea is positive, the culture is non-Escherichia coli. If necessary, gram stain and oxidase test shall be carried out. The Escherichia coli is gram negative bacillus and oxidase is negative. 6.4.3 If biochemical identification kit or microbial identification system is adopted, the depurated colonies shall be picked from nutrient agar plate to prepare bacterial suspension with appropriate turbidity by aseptic diluent, and then identified by biochemical identification kit or microbial identification system. 6.5 PCR confirmatory test 6.5.1 Adopt the colonies with biochemical reaction in conformity to Escherichia coli characteristic to carry out PCR confirmatory test. Note: PCR laboratory location planning, basic working principles and attentions shall refer to the "Construction Standard of Center for Disease Control and Prevention" (JIANBIAO 127-2009) and the Appendix (Working Guideline of Clinical Gene Amplification Examination Laboratory in Medical Institution) of "Management Method for Clinical Gene Amplification in Medical Institution" issued by the National Health and Family Planning Commission of the People's Republic of China (the original Ministry of Health of the People's Republic of China) (2010). 6.5.2 Apply 1μL inoculating loop to scrape the colonies cultured for 18h~24h from nutrient agar plate or slant, suspend them in 200μL of 0.85% aseptic normal saline, sufficiently scatter and prepare bacterial suspension, centrifuge at 13000r/min for 3min, and then discard the supernatant. Add 1mL of aseptic deionized water to sufficiently mix the thallus well, and maintain in 100℃ water bath or metal bath for 10min. After cooling by ice bath, centrifuge at 13000r/min for 3min, collect supernatant and dilute it by aseptic deionized water in the proportion of 1: 10, and then adopt 2μL of which to serve as the template for PCR detection. All the treated DNA templates are directly used for PCR reaction or stored temporarily at 4℃ and subjected to PCR reaction; otherwise, they shall be preserved at -20℃ below for standby (within one week). Bacterial genomic extraction kit may also be adopted for extracting bacterial DNA, which shall be operated according to the instruction of bacterial genomic extraction kit. 6.5.3 For each PCR reaction, EPEC, EIEC, ETEC, STEC/EHEC and EAEC standard strains shall be adopted as positive control. Meanwhile, Escherichia coli ATCC 25922 or equivalent standard bacterial strain shall be adopted as negative control, and aseptic deionized water as blank control, controlling PCR system pollution. See Table 1 for characteristic genes of diarrheagenic Escherichia coli. sufficiently mix them well, slightly pour the mould with comb, the length of gelation shall be greater than 10cm and the thickness should be 3mm~5mm. Inspect whether bubble exists below or among comb, if any, exhaust the bubble from agarose gel with disposable tip. After the agarose gel entirely coagulates and hardens, slightly pull out the comb, carefully put glue block and glue bed inside the electrophoresis tank, and place the sample hole at positive electrode. Add 1×TAE electrophoretic buffer into the electrophoresis tank, with liquid level 1mm~2mm above the glue surface. Well- mix the 5μL of PCR product with 1μL of 6×loading buffer solution, suck the mixed solution with micro pipettor and vertically stretch into the glue hole below liquid level and carefully add the sample into the hole; Add the PCR reaction product of positive control into the last swimming lane; add 2μL of molecular weight Marker into the first swimming lane. Switch on the electrophoresis apparatus, calculate and set the voltage value according to the Formula: voltage = the distance between the positive and negative electrodes of electrophoresis tank (cm)×5V/cm; turn on the switch of voltage, and the electrophoresis starts when bubbles appear in platinum at positive and negative electrodes. After electrophoresis for 30min~45min, cut off the power. Take out the gel and put it into gel-imaging apparatus to observe the result and photograph and record the date. 6.5.7 Result judgment. The blank control in electrophoresis result shall be free from band, negative control only appears uidA band amplification, and positive control appears all target bands, in this case, the PCR test result shall be true. According to the size of target bands in electrophoretogram, judge the kind of target band, record the kind of target band in each swimming lane, and search the category of diarrheagenic Escherichia coli corresponding to different target band kind and combination in Table 5. 6.5.8 If commercialized PCR kit or multiple PCR(MPCR) kit is adopted, the operation and result judgment shall be conducted according to its instruction. 6.6 Serological test(optional) 6.6.1 Adopt the strain confirmed as diarrheagenic Escherichia coli via PCR test for serological test. Note: the O antigen and H antigen shall be identified according to the operating instructions provided by the manufacturer. Where the operating instructions provided by the manufacturer may be deviated from the descriptions below, the former one shall prevail. 6.6.2 O antigen identification 6.6.2.1 Presumptive test: pick the colony confirmed as diarrheagenic Escherichia coli via biochemical test and PCR test on nutrient agar plate; according to the category of diarrheagenic Escherichia coli, adopt the univalent or multivalent OK serum of Escherichia coli to carry out slide agglutination test. Where agglutinated with a certain kind of multivalent OK serum, conduct agglutination test for the univalent OK serum involved in the multivalent serum. See Table 6 for the O antigen group included in Diarrheagenic Escherichia coli. If agglutination reaction presents for certain univalent OK serum, the presumptive test is positive. 6.6.2.2 Confirmatory test: prepare O antigen suspension with 0.85% aseptic normal saline, and dilute it to the concentration equivalent to MacFarland No. 3 turbidimetric tube. Dilute the O-serum with original valence of 1: 160~1: 320 by 0.5% of saline water to 1: 40. Mix the diluted serum with antigen suspension in 10mm×75mm test tube equivalently and carry out single-tube agglutination test. After mixing well, place it in a water bath at 50℃±1℃ for 16h to observe the result. If agglutination appears, it may be confirmed as O antigen. 6.6.3 Identification of H antigen 6.6.3.1 Adopt strain and inoculate into semi-solid agar tube by stabbing, culture it at 36℃±1℃ for 18h~24h, adopt one loop of top culture to inoculate into BHI liquid medium, and culture it at 36℃±1℃ for 18h~24h. Add formalin into it until the concentration reaches 0.5% to carry out slide agglutination or tube agglutination test. 6.6.3.2 If there is no obvious agglutination in both to-be-tested antigen and serum, ......
Source: Above contents are excerpted from the full-copy PDF -- translated/reviewed by: www.ChineseStandard.net / Wayne Zheng et al.
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