Team:Caltech/Protocols/Folate assay
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===Purpose=== | ===Purpose=== | ||
To quantify and measure levels of folate production in the cell lysate and supernatant of 'E.coli' transformed with high copy folate biosynthesis genes 'folB,' 'folKE,' 'folBKE'. | To quantify and measure levels of folate production in the cell lysate and supernatant of 'E.coli' transformed with high copy folate biosynthesis genes 'folB,' 'folKE,' 'folBKE'. | ||
+ | |||
+ | The assay uses growth of the folate-dependent strain ''L. rhamnosus'' as an indicator of folate concentrations in the sample. Growth is measured by taking the OD at 546nm. | ||
+ | |||
+ | ===Important Notes=== | ||
+ | *Almost every ingredient in this assay is light sensitive- take extreme caution to limit exposure of buffers, folic acid mixtures, and sample tubes to light. I usually wrapped the buffers, assay media, and standard curve folic acid dilutions in aluminum foil. I also started covering the entire rack of samples with foil during incubation, but decided it would be ridiculous to covered each sample tube with foil. | ||
+ | |||
+ | * Previously, we had been using this protocol with the other folate-dependent strain ''Entercoccus hirae'' ATCC 8043, and were able to generate a linear standard curve from 0.1-1ng. However, this strain did not grow in our samples, and so we switched to ''L. rhamnosus.'' | ||
+ | |||
+ | * This is why we used Lactobacilli Broth AOAC instead of the recommended Lactobacilli MRS broth. | ||
===Materials=== | ===Materials=== | ||
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* Human plasma (Sigma, P9523-1ML)(for deconjugation mix) | * Human plasma (Sigma, P9523-1ML)(for deconjugation mix) | ||
* Lactobacillus rhamnosus (ATCC 7469) | * Lactobacillus rhamnosus (ATCC 7469) | ||
+ | * Saline (0.9% NaCl in H20) | ||
===Deconjugation Mixture <cite>Sybesma</cite>=== | ===Deconjugation Mixture <cite>Sybesma</cite>=== | ||
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3. Add 2.5% (vol/vol) concentration of the clarified human plasma solution to the folate samples. | 3. Add 2.5% (vol/vol) concentration of the clarified human plasma solution to the folate samples. | ||
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+ | ===''L. rhamnosus'' inoculum preparation=== | ||
+ | 1. Inoculate 5 mL of Lactobacilli Broth AOAC with ''L.rhamnosus.'' | ||
+ | |||
+ | 2. Incubate for 12-24 hours. | ||
+ | |||
+ | 3. Centrifuge the culture, (13,000x g, 10 min, 20C), remove the supernatant. | ||
+ | |||
+ | 4. Wash twice with saline (0.9% NaCl in H20) | ||
+ | |||
+ | 5. Resuspend in folate assay media, adjust OD (546nm) to approximately 1.0. | ||
===Sample Preparation=== | ===Sample Preparation=== | ||
- | 1. Centrifuge the full-grown cell culture (5ml) after centrifugation ( | + | 1. Centrifuge the full-grown cell culture (5ml) after centrifugation (13,000x g, 10 min, 20 C). |
- | 2. Recover both cells and supernatant. | + | 2. Recover both cells and supernatant. |
- | 3. Dilute the supernatant 1:1 with 0.1M sodium acetate buffer (pH4.8) -1% ascorbic acid. | + | 3. Dilute the supernatant 1:1 with 0.1M sodium acetate buffer (pH4.8) -1% ascorbic acid. |
- | 4. Wash with the 0.1M sodium acetate-1% ascorbic acid and resuspend in 5 mL of the same buffer. | + | 4. Wash with the 0.1M sodium acetate-1% ascorbic acid and resuspend in 5 mL of the same buffer. |
- | 5. Release folate from the cells by incubating the samples at 100C for 5 min (determined to be optimal for folate release + the heat inactivates the bacteria) | + | 5. Release folate from the cells by incubating the samples at 100C for 5 min (determined to be optimal for folate release + the heat inactivates the bacteria) |
- | 6. Add the deconjugation reaction mixture (2.5% vol/vol) | + | 6. Add the deconjugation reaction mixture (2.5% vol/vol) |
- | 7. Incubate for 4h at 37C, you should see obvious cell debris at the bottom of the cell lysate tubes. | + | 7. Incubate for 4h at 37C, you should see obvious cell debris at the bottom of the cell lysate tubes. |
- | 8. Add 50uL of prepared ''L.rhamnosus'' inoculum to each assay tube. | + | 8. Filter sterilize 2.5 mL of each sample into a clean glass tube. |
+ | |||
+ | 9. Add 2.5 mL of folate assay media to each tube, bringing the volume up to 5mL. | ||
+ | |||
+ | 10. Add 50uL of prepared ''L.rhamnosus'' inoculum to each assay tube. | ||
+ | |||
+ | 11. Incubate for 16-20 hours at 37C. | ||
+ | |||
+ | 12. Read the absorbances of the samples at 546 nm on a plate reader (200uL per well). The protocol recommends refrigerating the samples at 4C for 15-30 minutes prior to reading, but I don't think it makes a difference, particularly if you intend on returning the samples to the incubator to take later timepoints. | ||
===Standard Curve=== | ===Standard Curve=== | ||
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===Sources=== | ===Sources=== |
Revision as of 09:57, 23 August 2008
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Folate Microbiological Assay ProtocolPurposeTo quantify and measure levels of folate production in the cell lysate and supernatant of 'E.coli' transformed with high copy folate biosynthesis genes 'folB,' 'folKE,' 'folBKE'. The assay uses growth of the folate-dependent strain L. rhamnosus as an indicator of folate concentrations in the sample. Growth is measured by taking the OD at 546nm. Important Notes
Materials
Deconjugation Mixture Sybesma1. Dilute 1 g of human plasma in 5ml of 0.1M 2-mercaptoethanol-0.5% sodium ascorbate 2. Clear from precipitates by centrifugation (10,000xg,2 min) 3. Add 2.5% (vol/vol) concentration of the clarified human plasma solution to the folate samples. L. rhamnosus inoculum preparation1. Inoculate 5 mL of Lactobacilli Broth AOAC with L.rhamnosus. 2. Incubate for 12-24 hours. 3. Centrifuge the culture, (13,000x g, 10 min, 20C), remove the supernatant. 4. Wash twice with saline (0.9% NaCl in H20) 5. Resuspend in folate assay media, adjust OD (546nm) to approximately 1.0. Sample Preparation1. Centrifuge the full-grown cell culture (5ml) after centrifugation (13,000x g, 10 min, 20 C). 2. Recover both cells and supernatant. 3. Dilute the supernatant 1:1 with 0.1M sodium acetate buffer (pH4.8) -1% ascorbic acid. 4. Wash with the 0.1M sodium acetate-1% ascorbic acid and resuspend in 5 mL of the same buffer. 5. Release folate from the cells by incubating the samples at 100C for 5 min (determined to be optimal for folate release + the heat inactivates the bacteria) 6. Add the deconjugation reaction mixture (2.5% vol/vol) 7. Incubate for 4h at 37C, you should see obvious cell debris at the bottom of the cell lysate tubes. 8. Filter sterilize 2.5 mL of each sample into a clean glass tube. 9. Add 2.5 mL of folate assay media to each tube, bringing the volume up to 5mL. 10. Add 50uL of prepared L.rhamnosus inoculum to each assay tube. 11. Incubate for 16-20 hours at 37C. 12. Read the absorbances of the samples at 546 nm on a plate reader (200uL per well). The protocol recommends refrigerating the samples at 4C for 15-30 minutes prior to reading, but I don't think it makes a difference, particularly if you intend on returning the samples to the incubator to take later timepoints. Standard Curve===Sources=== |