BS 4285-2 5-1989 Microbiological examination for dairy purposes - Methods of general application for enumeration of microorganisms - Enumeration of bacteria by direct microscopic c.pdf
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1、BRITISH STANDARD BS4285-2.5: 1989 Direct counts Microbiological examination for dairy purposes Part2: Methods of general application for enumeration of microorganisms Section2.5 Enumeration of bacteria by direct microscopic counts IMPORTANT NOTE.It is essential that Parts0 and1 of this standard, whi
2、ch are published separately, be read in conjunction with this Section. UDC637.1.055.07:579.67+637.1.055.075:579.672.083.16:579.8.087.23BS4285-2.5:1989 This British Standard, having been prepared under the directionof the Dairying Standards Policy Committee, waspublished under the authorityof the Boa
3、rd of BSI andcomes into effect on 29 September 1989 BSI04-1999 BS4285 first published March 1968 Supplement No.1 to BS4285:1968 first published April1970 First revision, Section2.5, December 1984 Second revision, The Committees responsible for this British Standard are shown inPart0. The following B
4、SI references relate to the work on this standard: Committee reference DAC/4 Draft for comment88/52307DC ISBN 0 580 17390 9 Foreword This Section of BS4285 has been prepared under the direction of the Dairying Standards Policy Committee. It supersedes BS4285-2.5:1984 which is withdrawn. This revisio
5、n of this Section of BS4285 incorporates a more detailed description of the direct epifluorescent filter technique (DEFT) (seeclause5), the direct microscopic count technique (seeclause4) being identical with that in the 1984 edition. A British Standard does not purport to include all the necessary
6、provisions of a contract. Users of British Standards are responsible for their correct application. Compliance with a British Standard does not of itself confer immunity from legal obligation. Summary of pages This document comprises a front cover, an inside front cover, pages i and ii, pages1 to4,
7、an inside back cover and a back cover. This standard has been updated (see copyright date) and may have had amendments incorporated. This will be indicated in the amendment table on the inside front cover. Amendments issued since publication Amd. No. Date of issue CommentsBS4285-2.5:1989 BSI 04-1999
8、 i Contents Page Foreword Inside front cover 1 Scope 1 2 Definition 1 3 Principle 1 4 Method A. Direct microscopic count technique 1 5 Method B. Direct epifluorescent filter technique (DEFT) 2 6 Test report 4 Table 1 Microscope factors 2 Table 2 Quantities of sample, trypsin and surfactant solutions
9、 for test 4 Publications referred to Inside back coverii blankBS4285-2.5:1989 BSI 04-1999 1 1 Scope This Section of BS4285 describes two methods of general application for the direct enumeration of bacteria: a) method A: direct microscopic count technique for total counts in milk; b) method B: direc
10、t epifluorescent filter technique (DEFT) for total counts or counts of bacteria in milk, certain milk products and samples such as rinses. NOTE 1In samples (including plant rinses) that have received some degree of heat treatment (equivalent to pasteurisation or greater), certain organisms, particul
11、arly Gram-positive cocci, will fluoresce orange (i.e.as active) but will be non-viable by plate count methods. Therefore great care is needed in interpreting results using such samples. NOTE 2The titles of the publications referred to in this standard are listed on inside back cover. 2 Definition Fo
12、r the purposes of this Section of BS4285, the following definition applies. bacteria. those organisms which can be recognized from experience, under the microscope, as having the characteristic size and appearance of organisms known as bacteria which, in method A, are stained the appropriate colour
13、or, in method B, fluoresce green, yellow or orangered after staining with acridine orange 3 Principle 3.1 Method A A small test portion is fixed on a microscope slide4.2.4, defatted, and stained with methylene blue or Newmans stain4.1. The prepared film is examined, the bacteria counted and the numb
14、er per millilitre of sample calculated. 3.2 Method B A known quantity of sample or primary dilution is treated with trypsin and surfactant and then filtered so that bacteria are concentrated on the filter where they are stained with acridine orange. The bacteria are counted and the number per millil
15、itre of sample calculated. 4 Method A. Direct microscopic count technique 4.1 Reagents 4.1.1 Methylene blue stain Dissolve the methylene blue in the ethanol and add the water. 4.1.2 Newmans stain Add the ethanol to the tetrachloroethane and heat on a water bath in a fume cupboard to a temperature no
16、t exceeding70 C. Add the methylene blue and shake until the dye dissolves. Cool, add acetic acid slowly, mix and filter. WARNING. The vapour of tetrachloroethane is toxic and all operations involving Newmans stain shall be carried out in a fume cupboard. 4.1.3 Xylene, or other suitable fat solvent 4
17、.1.4 Ethanol,95%V/V 4.2 Apparatus NOTEFor details of apparatus including its preparation and sterilization, see BS4285-1.2. 4.2.1 Ordinary microbiological laboratory apparatus. 4.2.2 Pipettes or syringes, calibrated to deliver0.01mL. 4.2.3 Microscope, with2.1mm oil immersion objective and 10 eyepiec
18、e. 4.2.4 Microscope slides, having a square with10mm sides either: a) outlined on the surface by etching or other suitable means; or b) using a template to outline this area on a plain slide. The slides shall be new and fat-free. 4.3 Determination of the microscope factor Measure the diameter of the
19、 microscope field with a stage micrometer with0.01mm divisions using the2.1mm objective, the10 eyepiece and a standard draw tube length. Take the mean of three measurements and calculate the radius in millimetres. Methylene blue(3,7-Bis(dimethylamino) phenothiazin-S-ylium chloride) 0.3g Ethanol,95%
20、V/V 30mL Water 100mL Methylene blue 1.0g Ethanol,95% V/V 54mL 1,1,2,2-tetrachloroethane 40mL Glacial acetic acid 6mLBS4285-2.5:1989 2 BSI 04-1999 If0.01mL of sample is spread over an area of100mm 2 , calculate the microscope factor from the formula: where r is the radius of the microscope field (inm
21、m). Table 1 gives the microscope factors corresponding to different field diameters. Table 1 Microscope factors 4.4 Sampling Take the laboratory sample in accordance with BS4285-1.1. 4.5 Preparation of test sample Prepare the test sample from the laboratory sample in accordance with BS4285-1.1. 4.6
22、Procedure 4.6.1 Preparation of film. Using the pipette(4.2.2) remove0.01mL of the well-mixed sample, wipe the exterior of the pipette except the tip with absorbent paper and spread the sample evenly over the area on a slide(4.2.4). Dry the preparation at a temperature of40C to45C on a level surface
23、protected from dust. The drying time shall not exceed5min, but shall not be too short or the film will not be fixed properly. 4.6.2 Staining. Carry out the procedure in eithera) orb). a) Procedure using methylene blue. Defat the fixed sample by flooding the slide with xylene or other suitable fat so
24、lvent for at least1min. Drain and allow to dry. Flood with ethanol for1min, drain and allow to dry. Flood the slide with methylene blue stain for10s to15s. Do not exceed this time or the slide will be overstained. Rinse carefully in water, drain and allow to dry slowly. When properly prepared, the b
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