Difference between revisions of "Team:NEFU China/Experiments"
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− | <p | + | <p><span style="font-size:20px"><span style="font-family:arial,helvetica,sans-serif">National Food Safety Standard (GB 4789.3—2010)</span></span></p> |
− | <p> | + | <p><span style="font-family:arial,helvetica,sans-serif"><span style="font-size:20px">Food microbiological examination: Enumeration of coliforms</span></span></p> |
− | <span style="font-family:arial,helvetica,sans-serif"> | + | |
− | <p>< | + | <p><span style="font-size:18px"><span style="font-family:arial,helvetica,sans-serif">Operating Steps</span></span></p> |
− | <span style="font-family:arial,helvetica,sans-serif"> | + | |
− | <p> | + | <p> </p> |
− | + | ||
− | <p>< | + | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1 Diluting the samples</span></span></p> |
− | <span style="font-family:arial,helvetica,sans-serif"> | + | |
− | <p> | + | <p> </p> |
− | + | ||
− | <p>< | + | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1.1</span> <span style="font-family:arial,helvetica,sans-serif"><span style="color:rgb(0, 0, 0)">Solid and semi-solid samples:Weigh and take 25 g sample, put it in an aseptic homogenizing cup which contains 225 ml phosphate buffer solution or physiological saline, and homogenize it 8000 r/min to 10000 r/min for 1 to 2 minutes; or put it in an aseptic homogenizing bag which contains 225 ml phosphate buffer solution or physiological saline and homogenize it by flapping with a smack type homogenizer for 1 to 2 minutes to get 1:10 homogenous sample liquor.</span></span></span></p> |
− | <span style="font-family:arial,helvetica,sans-serif"> | + | |
+ | <p> </p> | ||
+ | |||
+ | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1.2 Liquid samples: Suck 25 ml sample with an aseptic suction tube, put it in an aseptic conical flask (with a certain number of aseptic glass beads placed inside beforehand) which contains 225 ml phosphate buffer solution or physiological saline, and blend the solution properly to get 1:10 homogenous sample liquor.</span></span></p> | ||
+ | |||
+ | <p> </p> | ||
+ | |||
+ | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1.3 pH value of the homogenous sample liquor should be between 6.5 and 7.5. Regulate its pH value with 1mol/L sodium hydroxide (NaOH) or 1 mol/L hydrochloric acid (HCL) respectively, when necessary.</span></span></p> | ||
+ | |||
+ | <p> </p> | ||
+ | |||
+ | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1.4 Suck 1 ml 1:10 homogenous sample liquor with a 1ml aseptic suction tube or micro pipettor, empty it in an aseptic test tube (attention: the pointed end of test tube or sucker should not touch the diluting liquid) which contains 9 ml phosphate buffer solution or physiological saline slowly along the tube wall, jolt the test tube or beat upon it with a 1 ml aseptic suction tube so that it will be homogenized properly to get 1:100 homogenous sample liquor.</span></span></p> | ||
+ | |||
+ | <p> </p> | ||
+ | |||
+ | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1.5 According to estimation of sample pollution, make homogenous sample liquor series diluted by 10 times and above as per the above-stated operating steps. For every increased diluting degree, replace one 1 ml aseptic suction tube or sucker. From preparation of homogenous sample liquor to completion of inoculation, the whole process should be within 15 minutes.</span></span></p> | ||
+ | |||
+ | <p> </p> | ||
+ | |||
+ | <p><span style="font-size:20px"><span style="font-family:arial,helvetica,sans-serif">2 Primary fermentation test</span></span></p> | ||
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">For every sample, select homogenous sample liquors with three suitable consecutive dilution degrees (stock solution may be chosen in case of liquid sample), and for every dilution degree, inoculate 3 tubes of lauryl sulfate tryptone (LST) broth, 1ml each tube (if more than 1ml is inoculated, double LST broth should be adopted). Make them cultured in 36°C ±1°C for 24h ± 2h and observe whether bubbles are generated in the tubes; if there is no any bubble, make them cultured for 48±2h in total. Tubes without bubbles are coliform negative and tubes with bubbles go through secondary fermentation test.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:20px"><span style="font-family:arial,helvetica,sans-serif">3 Secondary fermentation</span></span></p> |
<p> </p> | <p> </p> | ||
− | <p style=" | + | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">Take 1 circle of cultures from each of all LST broth tubes which ferment and generate gas within 48h±2h </span><span style="font-family:arial,helvetica,sans-serif">respectively with an inoculation ring, transfer-inoculate them to brilliant green lactose bile (BGLB) broth, culture them in </span><span style="font-family:arial,helvetica,sans-serif">36°C</span><span style="font-family:arial,helvetica,sans-serif">±1° for </span><span style="font-family:arial,helvetica,sans-serif">48±2h, observe bubblegeneration.</span><span style="font-family:arial,helvetica,sans-serif">Tubes which generate bubbles are recorded as coliform positive.</span></span></p> |
− | <p style=" | + | <p><span style="font-size:20px"><span style="font-family:arial,helvetica,sans-serif">4 Reporting most probable number (MPN) of coliforms</span></span></p> |
− | <p>< | + | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">According to the number of tubes which are coliform positive verified through 3, search the MPN Table (see Annex B) to report coliform MPN counts in every gram (or ml) of sample.</span></span></p> |
− | <p>< | + | <p><img alt="" src="https://static.igem.org/mediawiki/2015/2/24/NEFU_China_55C9E13C-5371-4399-86EE-5F4143C9B437.png" style="height:902px; width:700px" /></p> |
− | <span style="font-family:arial,helvetica,sans-serif"> | + | |
+ | <p><span style="font-size:20px"><span style="font-family:arial,helvetica,sans-serif"><strong>Media Component (g/L) , 25℃ </strong></span></span></p> | ||
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px">1. Modified Chalmers Agar (MC):</span></p> |
+ | |||
+ | <p><img alt="" src="https://static.igem.org/mediawiki/2015/7/76/NEFU_China_059E9F91-6698-447D-BD37-5DD46C5AF8FE.png" style="height:218px; width:500px" /></p> | ||
+ | |||
+ | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">2. Lauryl Sulfate Tryptose Broth (LST) :</span></span></p> | ||
+ | |||
+ | <p><img alt="" src="https://static.igem.org/mediawiki/2015/7/78/NEFU_China_995DDE3E-379D-483C-BFF3-C6F8028D3F15.png" style="height:182px; width:500px" /></p> | ||
+ | |||
+ | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">3. Brilliant Green Lactose Bile Broth (BGLB): </span></span></p> | ||
+ | |||
+ | <p><img alt="" src="https://static.igem.org/mediawiki/2015/d/d8/NEFU_China_3E7B651E-0142-45E3-A6A2-C1E567C68C9A.png" style="height:270px; width:500px" /></p> | ||
+ | |||
+ | <p> </p> | ||
+ | |||
+ | <p> </p> | ||
+ | |||
+ | <p><strong><span style="font-size:22px">The microbiological test of <em>Lactobacillus</em> in yogurt (GB/T16347-1996)</span></strong></p> | ||
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1. Put 25 ml full-shaked sample into sterilized wide mouth bottle containing 225 ml sterile saline aseptically to make uniform dilution of 1:10.Samples are selected for the same brand of yogurt which date 4, 10, 20 days,and expired one day.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">2. Suck up 1ml 1:10 dilution with 1ml sterile pipette and inject it slowly into a test tube containing 9 ml sterile saline along the tube wall (note not to touch the tip of the pipette tube dilution).</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">3. Increase by 10-fold dilution increments every time, that is replaced with a 1 ml sterile pipette according to the above steps. So it is total diluted 10<sup>-15</sup>.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">4. Choose dilutions from 10<sup>-6</sup> to 10<sup>-15</sup> and suck up 1 ml dilution into sterile plates respectively while doing the 10-fold dilution increments. Make two plates each dilution.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">5. Inject 15 ml <em>Lactobacillus</em> count medium (modified MC) which was cooled to 50℃ into the plate as soon as the dilutions was shifted into the plate. Rotate it to mix them. Meanwhile, to make a blank comparison, pour the count medium of<em> Lactobacillus</em> into a sterile plate containing sterile saline which is used to test 1 ml dilution. The whole process including adding the culture to the plate to finishing pouring should be done within 20 minutes.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">6. Invert the plate and put it into a 36 ± 1℃ incubator for 72±3 hours after the agar has set. Observe the lactobacillus in the plate, select colonies between 30 to 300 and count them. After the calculation, the colonies are randomly taken the Gram stain: (1) fix the smear.(2) stain for 1 min with ammonium oxalate crystal violet. (3) wash with running water.(4) add iodine to cover approximately 1 minute. (5) wash with water and absorb the water with absorbent paper. (6) add a few drops of 95% alcohol and gently shake to decolorize it. Wash with water after 20 seconds and absorb the water. (7) stain with fan red for 1 minute,wash it with running water, dry it and then take microscopic examination. Gram-positive bacteria are blue-purple and gram-negative bacteria are red.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">7. Do the catalase test: pick up a colony from the solid media into a clean tube, drop 2 ml 3% hydrogen peroxide solution and observe. Those who has bubbles in 30 s are positive, the others are negative.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">8. Results identification: The <em>Lactobacillius</em> can be identified according to the following fades: gram-positive, catalase-negative, non-spore sphaerita or bacillus. Calculate the number of<em> Lactobacillus</em> in one plate and multiply the dilution and then we get the number of <em>Lactobacillus</em> of per milliliter of the sample.</span></span></p> |
<p> </p> | <p> </p> | ||
− | <p style="text-align:center"><span style="font-family:arial,helvetica,sans-serif"> | + | <p style="text-align:center"><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">Table1 The colony morphology of lactobacillus in the modified MC medium</span></span></p> |
− | <p><img alt="" src="https://static.igem.org/mediawiki/2015/ | + | <p style="text-align:center"><img alt="" src="https://static.igem.org/mediawiki/2015/0/07/NEFU_China_F733489D-8373-4A41-8CFF-891334DEE58D.png" style="height:250px; width:750px" /><br /> |
− | + | </p> | |
<p><br /> | <p><br /> | ||
− | + | </p> | |
− | + | ||
− | <p> | + | <p><strong><span style="font-size:22px">Genome Extraction</span></strong></p> |
− | <p><span style="font-family:arial,helvetica,sans-serif"> | + | <p><br /> |
− | < | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">For bacterial gDNA extraction we used the easy DNA Kit from Invitrogen according to the <a href="http://www.tiangen.com/en/?productShow/t1/4/id/9.html">manufacturer's instructions</a>.</span></span></p> |
− | + | ||
− | <p> | + | <p> </p> |
− | + | ||
− | <p><strong><span style="font-size:22px"> | + | <p><strong><span style="font-size:22px">Plasmids extraction</span></strong></p> |
− | + | ||
− | <p>< | + | <p><br /> |
− | <span style="font-family:arial,helvetica,sans-serif">For | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">For the plasmid extraction we used <a href="http://www.tiangen.com/en/?productShow/t1/4/id/33.html">TIANprep Midi Plasmid Kit</a> according to manufacturer's instructions. </span></span><br /> |
<br /> | <br /> | ||
− | <strong><span style="font-size:22px">Gel Extraction</span></strong> <br /> | + | <strong><span style="font-size:22px">Gel Extraction</span></strong> </p> |
− | <span style="font-family:arial,helvetica,sans-serif"> | + | |
+ | <p><br /> | ||
+ | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">For the Gel Extraction we used TIANgel Midi Purification Kit according to <a href="http://www.tiangen.com/en/?productShow/t1/4/id/41.html">manufacturer's instructions</a>.</span></span></p> | ||
<p><strong><span style="font-size:22px">AI-2 Quantification</span></strong></p> | <p><strong><span style="font-size:22px">AI-2 Quantification</span></strong></p> | ||
− | <p><span style="font-family:arial,helvetica,sans-serif">1. <em>E.coli</em> and<em> Bacillus</em> were inoculated into LB media (2%, v/v), respectively, and shaken overnight at 37°C.</span></p> | + | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1. <em>E.coli</em> and<em> Bacillus</em> were inoculated into LB media (2%, v/v), respectively, and shaken overnight at 37°C.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">2. The bacteria were centrifuged at 6000 g for 3 min. The supernatant was collected and filtered through a 0.22μm membrane</span></p> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">2. The bacteria were centrifuged at 6000 g for 3 min. The supernatant was collected and filtered through a 0.22μm membrane</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">3. Preparing the working solution: A working solution of 10 mM 1, 10-phenanthroline/3.32 mM Fe (III) was prepared by dissolving 0.198 g of 1,10-phenanthroline in 50 ml of deionized distilled water. The solution was adjusted to pH 2 using 1M HCl. Ferric ammonium sulphate (0.16g) was added and the solution was brought to 100 ml using deionized distilled water.</span></p> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">3. Preparing the working solution: A working solution of 10 mM 1, 10-phenanthroline/3.32 mM Fe (III) was prepared by dissolving 0.198 g of 1,10-phenanthroline in 50 ml of deionized distilled water. The solution was adjusted to pH 2 using 1M HCl. Ferric ammonium sulphate (0.16g) was added and the solution was brought to 100 ml using deionized distilled water.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">4. For the Fe (III) ion reduction test, 1ml of the cell free supernatant was mixed with 1 ml working solution to develop the full color. The solution was then diluted to 5ml and filtered through a 0.22 μm membrane,followed by scanning for the absorption spectrum against a blank solution within 3 min using a Lambda 25 UV/VIS spectrometer. </span></p> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">4. For the Fe (III) ion reduction test, 1ml of the cell free supernatant was mixed with 1 ml working solution to develop the full color. The solution was then diluted to 5ml and filtered through a 0.22 μm membrane,followed by scanning for the absorption spectrum against a blank solution within 3 min using a Lambda 25 UV/VIS spectrometer. </span></span></p> |
<p> </p> | <p> </p> | ||
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<p><span style="font-size:22px"><strong>Transformation by electroporation</strong></span></p> | <p><span style="font-size:22px"><strong>Transformation by electroporation</strong></span></p> | ||
− | <p><span style="font-family:arial,helvetica,sans-serif">1. Inoculate 100 μl bacterial culture into 50 ml of MRS and incubate the bacteria at 37°C overnight. </span></p> | + | <p><span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1. Inoculate 100 μl bacterial culture into 50 ml of MRS and incubate the bacteria at 37°C overnight. </span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">2. Harvest the cells by centrifugation.</span></p> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">2. Harvest the cells by centrifugation.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">3. Washed the bacteria three times with cold electroporation buffer (PB).</span></p> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">3. Washed the bacteria three times with cold electroporation buffer (PB).</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">4. Resuspend the cells in PB to | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">4. Resuspend the cells in PB to </span>reach the<span style="font-family:arial,helvetica,sans-serif"> OD<sub>600</sub> at about 0.5.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">5. Mix 100 μl electrocompetent cells with 10 μl plasmid DNA.</span></p> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">5. Mix 100 μl electrocompetent cells with 10 μl plasmid DNA.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">6. | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">6.Carefully transfer the cell/DNA mix into a chilled cuvette without introducing bubbles and make sure that the cells deposit across the bottom of the cuvette. </span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">7. | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">7.Electroporate using the following conditions for BTX ECM 630 and Bio-Rad GenePulser electroporators: 2.4kV, 200Ω, 25μF electric pulse in a 0.2 cm cuvette.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">8. | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">8. Immediately add 950 µl of 37 °C SMRS to the cuvette, gently mix up and down twice, then transfer to the 1.5 ml tube.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">9. Incubate | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">9.Incubate at 37 °C for 2 h.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">10. | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">10. Dilute the cells as appropriate then spread 100-200 μl cells onto a pre-warmed selective plate.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">11. Incubate the plates at 37°C for 2 to 3 days under anaerobic conditions.</span></p> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">11.Incubate the plates at 37 °C for 2 to 3 days under anaerobic conditions.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">12. Use isolated colonies to check the correct insertion.</span></p> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">12. Use isolated colonies to check the correct insertion.</span></span></p> |
<p> </p> | <p> </p> | ||
<p><strong><span style="font-size:22px">Functional identification of the engineered bacteria</span></strong><br /> | <p><strong><span style="font-size:22px">Functional identification of the engineered bacteria</span></strong><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">1. Inoculate | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1.Inoculate E. Coli CD-2 and E. Coli DH5alpha into 100 ml liquid LB medium, cultured at 37 °C 180 rpm for 8 hours.<br /> |
+ | 2.Centrifuge at 12,000 rpm for 2 min, then harvest the culture supernatant.</span></span></p> | ||
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">3.The liquid culture supernatant was filtrated through the 0.22 μm filters.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">4. Then the supernantant was added into the culture medium of Lactobcillus.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">5. Nisin was added at a final concentration of 50 ng/ml.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">6.Incubate the engineered Lactobcillus overnight.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif"> | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">7.Centrifuge at 6000 rpm for 5min, discard the supernatant then take photo. </span></span></p> |
+ | |||
+ | <p> </p> | ||
<p><br /> | <p><br /> | ||
− | |||
<br /> | <br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">1. Incubate | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">1.Incubate E. Coli CD-2 and E. Coli DH5alpha on LB agar plate overnight at 37 °C.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">2. Wash the colonies with fresh MRS | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">2. Wash the colonies with fresh MRS.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">3. | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">3. The liquid culture supernatant was filtrated through the 0.22 μm filters.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">4. | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">4. Then the supernantant was added into the culture medium of Lactobcillus.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">5. | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">5. Nisin was added at a final concentration of 50 ng/ml.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">6. Incubate the engineered | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">6.Incubate the engineered Lactobcillus overnight.</span></span></p> |
<p><br /> | <p><br /> | ||
− | <span style="font-family:arial,helvetica,sans-serif">7. Centrifuge at 6000 rpm for | + | <span style="font-size:16px"><span style="font-family:arial,helvetica,sans-serif">7.Centrifuge at 6000 rpm for 5min, discard the supernatant then take photo.</span></span></p> |
− | < | + | <div> </div> |
<p class="footer" style="color:white;margin-top:20px;text-align:center;"><span>Generated by </span><a href="https://2015.igem.org/Team:NEFU_China/Software">Flight iGEM</a>.</p> | <p class="footer" style="color:white;margin-top:20px;text-align:center;"><span>Generated by </span><a href="https://2015.igem.org/Team:NEFU_China/Software">Flight iGEM</a>.</p> | ||
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Revision as of 21:28, 18 September 2015
Protocols
National Food Safety Standard (GB 4789.3—2010)
Food microbiological examination: Enumeration of coliforms
Operating Steps
1 Diluting the samples
1.1 Solid and semi-solid samples:Weigh and take 25 g sample, put it in an aseptic homogenizing cup which contains 225 ml phosphate buffer solution or physiological saline, and homogenize it 8000 r/min to 10000 r/min for 1 to 2 minutes; or put it in an aseptic homogenizing bag which contains 225 ml phosphate buffer solution or physiological saline and homogenize it by flapping with a smack type homogenizer for 1 to 2 minutes to get 1:10 homogenous sample liquor.
1.2 Liquid samples: Suck 25 ml sample with an aseptic suction tube, put it in an aseptic conical flask (with a certain number of aseptic glass beads placed inside beforehand) which contains 225 ml phosphate buffer solution or physiological saline, and blend the solution properly to get 1:10 homogenous sample liquor.
1.3 pH value of the homogenous sample liquor should be between 6.5 and 7.5. Regulate its pH value with 1mol/L sodium hydroxide (NaOH) or 1 mol/L hydrochloric acid (HCL) respectively, when necessary.
1.4 Suck 1 ml 1:10 homogenous sample liquor with a 1ml aseptic suction tube or micro pipettor, empty it in an aseptic test tube (attention: the pointed end of test tube or sucker should not touch the diluting liquid) which contains 9 ml phosphate buffer solution or physiological saline slowly along the tube wall, jolt the test tube or beat upon it with a 1 ml aseptic suction tube so that it will be homogenized properly to get 1:100 homogenous sample liquor.
1.5 According to estimation of sample pollution, make homogenous sample liquor series diluted by 10 times and above as per the above-stated operating steps. For every increased diluting degree, replace one 1 ml aseptic suction tube or sucker. From preparation of homogenous sample liquor to completion of inoculation, the whole process should be within 15 minutes.
2 Primary fermentation test
For every sample, select homogenous sample liquors with three suitable consecutive dilution degrees (stock solution may be chosen in case of liquid sample), and for every dilution degree, inoculate 3 tubes of lauryl sulfate tryptone (LST) broth, 1ml each tube (if more than 1ml is inoculated, double LST broth should be adopted). Make them cultured in 36°C ±1°C for 24h ± 2h and observe whether bubbles are generated in the tubes; if there is no any bubble, make them cultured for 48±2h in total. Tubes without bubbles are coliform negative and tubes with bubbles go through secondary fermentation test.
3 Secondary fermentation
Take 1 circle of cultures from each of all LST broth tubes which ferment and generate gas within 48h±2h respectively with an inoculation ring, transfer-inoculate them to brilliant green lactose bile (BGLB) broth, culture them in 36°C±1° for 48±2h, observe bubblegeneration.Tubes which generate bubbles are recorded as coliform positive.
4 Reporting most probable number (MPN) of coliforms
According to the number of tubes which are coliform positive verified through 3, search the MPN Table (see Annex B) to report coliform MPN counts in every gram (or ml) of sample.
Media Component (g/L) , 25℃
1. Modified Chalmers Agar (MC):
2. Lauryl Sulfate Tryptose Broth (LST) :
3. Brilliant Green Lactose Bile Broth (BGLB):
The microbiological test of Lactobacillus in yogurt (GB/T16347-1996)
1. Put 25 ml full-shaked sample into sterilized wide mouth bottle containing 225 ml sterile saline aseptically to make uniform dilution of 1:10.Samples are selected for the same brand of yogurt which date 4, 10, 20 days,and expired one day.
2. Suck up 1ml 1:10 dilution with 1ml sterile pipette and inject it slowly into a test tube containing 9 ml sterile saline along the tube wall (note not to touch the tip of the pipette tube dilution).
3. Increase by 10-fold dilution increments every time, that is replaced with a 1 ml sterile pipette according to the above steps. So it is total diluted 10-15.
4. Choose dilutions from 10-6 to 10-15 and suck up 1 ml dilution into sterile plates respectively while doing the 10-fold dilution increments. Make two plates each dilution.
5. Inject 15 ml Lactobacillus count medium (modified MC) which was cooled to 50℃ into the plate as soon as the dilutions was shifted into the plate. Rotate it to mix them. Meanwhile, to make a blank comparison, pour the count medium of Lactobacillus into a sterile plate containing sterile saline which is used to test 1 ml dilution. The whole process including adding the culture to the plate to finishing pouring should be done within 20 minutes.
6. Invert the plate and put it into a 36 ± 1℃ incubator for 72±3 hours after the agar has set. Observe the lactobacillus in the plate, select colonies between 30 to 300 and count them. After the calculation, the colonies are randomly taken the Gram stain: (1) fix the smear.(2) stain for 1 min with ammonium oxalate crystal violet. (3) wash with running water.(4) add iodine to cover approximately 1 minute. (5) wash with water and absorb the water with absorbent paper. (6) add a few drops of 95% alcohol and gently shake to decolorize it. Wash with water after 20 seconds and absorb the water. (7) stain with fan red for 1 minute,wash it with running water, dry it and then take microscopic examination. Gram-positive bacteria are blue-purple and gram-negative bacteria are red.
7. Do the catalase test: pick up a colony from the solid media into a clean tube, drop 2 ml 3% hydrogen peroxide solution and observe. Those who has bubbles in 30 s are positive, the others are negative.
8. Results identification: The Lactobacillius can be identified according to the following fades: gram-positive, catalase-negative, non-spore sphaerita or bacillus. Calculate the number of Lactobacillus in one plate and multiply the dilution and then we get the number of Lactobacillus of per milliliter of the sample.
Table1 The colony morphology of lactobacillus in the modified MC medium
Genome Extraction
For bacterial gDNA extraction we used the easy DNA Kit from Invitrogen according to the manufacturer's instructions.
Plasmids extraction
For the plasmid extraction we used TIANprep Midi Plasmid Kit according to manufacturer's instructions.
Gel Extraction
For the Gel Extraction we used TIANgel Midi Purification Kit according to manufacturer's instructions.
AI-2 Quantification
1. E.coli and Bacillus were inoculated into LB media (2%, v/v), respectively, and shaken overnight at 37°C.
2. The bacteria were centrifuged at 6000 g for 3 min. The supernatant was collected and filtered through a 0.22μm membrane
3. Preparing the working solution: A working solution of 10 mM 1, 10-phenanthroline/3.32 mM Fe (III) was prepared by dissolving 0.198 g of 1,10-phenanthroline in 50 ml of deionized distilled water. The solution was adjusted to pH 2 using 1M HCl. Ferric ammonium sulphate (0.16g) was added and the solution was brought to 100 ml using deionized distilled water.
4. For the Fe (III) ion reduction test, 1ml of the cell free supernatant was mixed with 1 ml working solution to develop the full color. The solution was then diluted to 5ml and filtered through a 0.22 μm membrane,followed by scanning for the absorption spectrum against a blank solution within 3 min using a Lambda 25 UV/VIS spectrometer.
Transformation by electroporation
1. Inoculate 100 μl bacterial culture into 50 ml of MRS and incubate the bacteria at 37°C overnight.
2. Harvest the cells by centrifugation.
3. Washed the bacteria three times with cold electroporation buffer (PB).
4. Resuspend the cells in PB to reach the OD600 at about 0.5.
5. Mix 100 μl electrocompetent cells with 10 μl plasmid DNA.
6.Carefully transfer the cell/DNA mix into a chilled cuvette without introducing bubbles and make sure that the cells deposit across the bottom of the cuvette.
7.Electroporate using the following conditions for BTX ECM 630 and Bio-Rad GenePulser electroporators: 2.4kV, 200Ω, 25μF electric pulse in a 0.2 cm cuvette.
8. Immediately add 950 µl of 37 °C SMRS to the cuvette, gently mix up and down twice, then transfer to the 1.5 ml tube.
9.Incubate at 37 °C for 2 h.
10. Dilute the cells as appropriate then spread 100-200 μl cells onto a pre-warmed selective plate.
11.Incubate the plates at 37 °C for 2 to 3 days under anaerobic conditions.
12. Use isolated colonies to check the correct insertion.
Functional identification of the engineered bacteria
1.Inoculate E. Coli CD-2 and E. Coli DH5alpha into 100 ml liquid LB medium, cultured at 37 °C 180 rpm for 8 hours.
2.Centrifuge at 12,000 rpm for 2 min, then harvest the culture supernatant.
3.The liquid culture supernatant was filtrated through the 0.22 μm filters.
4. Then the supernantant was added into the culture medium of Lactobcillus.
5. Nisin was added at a final concentration of 50 ng/ml.
6.Incubate the engineered Lactobcillus overnight.
7.Centrifuge at 6000 rpm for 5min, discard the supernatant then take photo.
1.Incubate E. Coli CD-2 and E. Coli DH5alpha on LB agar plate overnight at 37 °C.
2. Wash the colonies with fresh MRS.
3. The liquid culture supernatant was filtrated through the 0.22 μm filters.
4. Then the supernantant was added into the culture medium of Lactobcillus.
5. Nisin was added at a final concentration of 50 ng/ml.
6.Incubate the engineered Lactobcillus overnight.
7.Centrifuge at 6000 rpm for 5min, discard the supernatant then take photo.