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Put recently arrived primers in solution to 100uM using TE buffer (added and vortexed).
PCR
Product | Gene | Starting Plasmid | Forward Primer | Reverse Primer | Tm hi/lo (anneal) |
---|---|---|---|---|---|
CD79A | CD79A | pENTR CD79A (pDONR223) | iGEM KRB 003 F | iGEM KRB 004 R | 62/61 (61) |
CD79A-TCS | CD79A | pENTR CD79A (pDONR223) | iGEM KRB 003 F | iGEM KRB 005 R | 62/61 (61) |
mKate | mKate | pENTR_L1_mKate_L2 | iGEM KRB 006 F | iGEM KRB 007 R | 58/61 (58) |
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Used 20 uL reaction. For plasmids, diluted to concentration 1ng/uL in EB buffer and added 1uL of each dilution to a separate PCR mix. Also diluted Diluted primers from 100uM stocks to 10uM with TE buffer.
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STEP | TEMP | TIME |
Initial Denaturation | 98°C | 30 seconds |
25-35 Cycles | 98°C 60°C 72°C | 10 seconds 30 seconds 60 seconds |
Final Extension | 72°C | 5 minutes |
Hold | 4°C |
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Lane 3: CD79A + TCS
Lane 4: mKate linker + mKate
When loading wells with PCR products, used Parafilm to mix 1uL of 6X Orange dye with 5uL of sample and loaded 5uL of this mixture in a lane. Ran gel at 120V for 30 minutes.
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