Team:Caltech/Week 6
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==Monday 7/19== | ==Monday 7/19== | ||
+ | [[Image:DigestsGel7-19.jpg|200px|thumb|right|Digest test gel with US and DS digested bricks. (7/19)]] | ||
+ | * Group meeting! | ||
+ | ** Discussed issues with cloning and next week's focus. | ||
+ | * Performed a digest (now for 2hr) and ligations (L18-23). Transformed into DH5α. | ||
+ | * Turns out that the sequencing primers we ordered (G00100 & G00101) are incorrect - they appear to bind on the wrong sides of the insert. We ordered new primers designed to bind to the BioBrick prefix and suffix. | ||
+ | * Ran gel of digest product to verify correct bands. | ||
==Tuesday 7/20== | ==Tuesday 7/20== | ||
+ | * All ligation transformations failed. Will try 16hr ligations and purifying digest products with a PCR purification kit. | ||
+ | * Made new growth curves testing AIBN effect on cells in LB | ||
+ | * Performed another live/dead assay | ||
+ | ** Had solutions of cells in glycerol and AIBN | ||
+ | ** Plated cells every hour for three hours | ||
+ | ** Combined glycerol solutions with LB and plated the solution | ||
+ | * New 16hr ligation procedure: | ||
+ | ** 30μL total: 2μL T4 ligase, 3μL 10x ligase buffer, 5μL vector, 10μL of each brick. Incubate for 16hr at 16°C. | ||
+ | * Started more cultures to miniprep tomorrow: I13504, J04450, K274002, M30109. | ||
==Wednesday 7/21== | ==Wednesday 7/21== | ||
+ | * Transformed 3μL of each ligation product from yesterday (time constants all w/in 3.8-4.0). Plated 50μL of each on plates. | ||
==Thursday 7/22== | ==Thursday 7/22== | ||
+ | [[Image:Digest22-07.jpg|200px|thumb|right|Digest test gel with upstream, downstream, and backbone digested bricks. (7/22)]] | ||
+ | [[Image:CIT-cpcr-gel-7-22.jpg|200px|thumb|CPCR gel featuring L17, L18, L25, & L27. (7/22)]] | ||
+ | * Prepared new sequencing primers in preparation for CPCR. | ||
+ | * Transformation plates are almost completely empty - will centrifuge and plate remaining transformation cells. | ||
+ | * Colony PCR mixture: | ||
+ | ** 10μL 10x PCR buffer, 2μL dNTP mix, 1μL forward primer, 1μL reverse primer, 0.5μL Taq polymerase, fill to 100μL total. (Optional: add 20μL Qiagen Q buffer. Doesn't appear to help any of our reactions.) | ||
+ | ** Pick colony and add to water (85.5μL). Incubate at 100°C for 10min. Add remaining ingredients and begin PCR program: | ||
+ | *** Initial denaturation: 94°C, 4min | ||
+ | *** 30 cycles: | ||
+ | **** 94°C, 30s | ||
+ | **** 54°C, 30s | ||
+ | **** 72°C, 2min (1min/kb) | ||
+ | *** Final extension: 72°C, 10min | ||
+ | *** Finish: 5°C forever | ||
+ | * Ran colony PCR on 4 ligations, 2 had the correct insert length: L17, L27. | ||
+ | * Ran gel of digest products from yesterday to verify correctness of the digestion. | ||
==Friday 7/23== | ==Friday 7/23== | ||
+ | [[Image:CIT-cpcr-gel1-7-23.jpg|200px|thumb|CPCR gel featuring L16, L17, L18, & L21. (7/23)]] | ||
+ | [[Image:CIT-cpcr-gel2-7-23.jpg|200px|thumb|CPCR gel featuring L25, L26, L27, & L29. (7/23)]] | ||
+ | * Plates containing the centrifuged transformation cells contained many colonies! | ||
+ | * Began 21 more CPCR reactions on ligations: L17, L18, L21, L27, L29, L16, L26, L25 | ||
+ | ** Note that because L18 is a coding sequence, it required the coding prefix primer; all others used the noncoding prefix primer. | ||
+ | * Received our heat shock promoter from the Registry today! Made a plate and culture of this brick (K112400). | ||
+ | * Purified yesterday's 4 CPCR reactions using a PCR purification kit. | ||
+ | ** Concentrations of each are all quite low (<20ng/μL) - we may want to increase the number of PCR cycles. | ||
+ | * Ran 2 gels of all the CPCR results. | ||
==Weekend 7/24-25== | ==Weekend 7/24-25== | ||
+ | === Saturday 7/24=== | ||
+ | [[Image:CIT-cpcr-gel-7-24.jpg|200px|thumb|CPCR gel featuring L26 & L21. (7/24)]] | ||
+ | * Started 4 new CPCR reactions on L21 and L26 to verify them more accurately. | ||
+ | ** Disposed of all failed cultures... | ||
+ | ** Prepped successful clones: 17-6, 18-3, 21-3, 26-1, 27-4, 29-2, and the heat shock promoter (K112400). | ||
+ | * Prepared digest: | ||
+ | ** K215000 (u/d) | ||
+ | ** K112400 (u/d) | ||
+ | ** B0034 (u) | ||
+ | ** R0082 (u) | ||
+ | ** L17 (u) | ||
+ | ** L18 (u/d) | ||
+ | ** L26 (u) | ||
+ | ** I13504 (d) | ||
+ | ** L21 (d) | ||
+ | * Began ligations: L16, L19, L42, L43, L44, L23, L24, L31, L40, L34, L35 | ||
+ | * Ran another gel of the CPCR products. | ||
+ | |||
+ | === Sunday 7/25 === | ||
+ | * Transformed all ligations from yesterday (time constants all within 3.6-4.0). Used 4μL for all, except for L34 & L35, which sparked, so used 3μL instead. | ||
+ | * Made 2YT for making more electrocompetent cells. | ||
+ | * Plated all transformation cells (centrifuged at 1000g for 15min). | ||
+ | |||
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Latest revision as of 19:01, 28 July 2010
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Week 1 | Week 2 | Week 3 | Week 4 | Week 5 | Week 6 | Week 7 | Week 8 | Week 9 | Week 10 | Week 11 | Week 12 | Week 13 | Week 14 | Week 15
Monday 7/19
Tuesday 7/20
Wednesday 7/21
Thursday 7/22
Friday 7/23
Weekend 7/24-25Saturday 7/24
Sunday 7/25
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