Minnesota/22 July 2008
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|''NOTE:'' Parts chosen that had good 'spec' results, meaning there is a high concentration of DNA. R2 = RFP, Y+2 = YFP with LVA tag, Y+4 = YFP with LVA tag, R+4 = RFP with LVA tag, Lac Pro. = LacI repressed promoter, p22 cII = gene for p22 cII, BV = base vector. DNA added into each one correlates with which part is being used, for example: R2 would have 2.0uL of RFP, and Y+2 would have 2.0uL of YFP with LVA tag, etc.. | |''NOTE:'' Parts chosen that had good 'spec' results, meaning there is a high concentration of DNA. R2 = RFP, Y+2 = YFP with LVA tag, Y+4 = YFP with LVA tag, R+4 = RFP with LVA tag, Lac Pro. = LacI repressed promoter, p22 cII = gene for p22 cII, BV = base vector. DNA added into each one correlates with which part is being used, for example: R2 would have 2.0uL of RFP, and Y+2 would have 2.0uL of YFP with LVA tag, etc.. | ||
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|'''5. Vector Dephosphorylation:''' Same dephos. procedure used on GFP:Terminator sample and BV sample. After dephosphorylation, incubate @37C for 30 mins. Heat inactivate dephosphorylation enzyme for 15 mins in 65C water bath. | |'''5. Vector Dephosphorylation:''' Same dephos. procedure used on GFP:Terminator sample and BV sample. After dephosphorylation, incubate @37C for 30 mins. Heat inactivate dephosphorylation enzyme for 15 mins in 65C water bath. |
Revision as of 21:38, 22 July 2008
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1. Pick Colonies from plates made 07-21-2008 Start cultures. | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
2. Plasmid prep: Prep RFP, YFP, GFP, TetR promoter, Terminator. Follow QIA miniprep procedure --> 1hr long. | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
3. Spec the prep products: Using spectrophotometry, the DNA concentration of the plasmid prep products were measured. | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
4. Double digest: Follow Kat's DNA work procedure to perform Double digest on: LacI Promoter, p22 cII gene, RFP, YFP, BV (dual promoters, GFP:Term already d.dig.). Incubate digested products for 2 hours @37C. Heat inactivate digestion enzyme for 15 mins @ 65C water bath. Follow the table below for double digest guidelines:
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NOTE: Parts chosen that had good 'spec' results, meaning there is a high concentration of DNA. R2 = RFP, Y+2 = YFP with LVA tag, Y+4 = YFP with LVA tag, R+4 = RFP with LVA tag, Lac Pro. = LacI repressed promoter, p22 cII = gene for p22 cII, BV = base vector. DNA added into each one correlates with which part is being used, for example: R2 would have 2.0uL of RFP, and Y+2 would have 2.0uL of YFP with LVA tag, etc.. | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
5. Vector Dephosphorylation: Same dephos. procedure used on GFP:Terminator sample and BV sample. After dephosphorylation, incubate @37C for 30 mins. Heat inactivate dephosphorylation enzyme for 15 mins in 65C water bath. | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
6. Ligation Reactions: Procedure performed in 20 minutes. Once all were ligated, were then incubated @ 16C for 1 hour. Heat inactivated enzyme @ 65C for 15 minutes. Ligated the following using L4 DNA Ligase: | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
a. BV + TetR:p22 promoter + RFP | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
b. BV + TetR:p22 promoter + YFP | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
c. LacI:LambdacI + GFP:Terminator | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
d. LacI Promoter + p22 cII + BV | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
7. Transformation: Procedure performed in 30 minutes. Transform all ligation products. Incubate in 2mL LB cultures for 2 hours @37C with shaking @ 220rpm's. | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
8. Plate transformations: Plate transformation cultures. | ||||||||||||||||||||||||||||||||||||||||||||||||||||||||
9. Prepare sequencing reactions: Prepare sequencing rxns IF POSSIBLE. |