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From 2013.igem.org

Contents 1 208 1.1 Main purpose 1.2 Who was in the lab 1.3 Procedure 1.3.1 USER reaction and transformation 1.3.2 Restriction analysis 1.3.3 Primer diluting 1.3.4 PCR to extract Nir from Pseudosomonas with new USER primers 1.3.5 PCR with USER-primers on HAO and AMO 1.4 Results 1.5 first gel 1.6 purification gel 1.7 gel for restriction analysis 1.8 Conclusion

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Main purpose

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Who was in the lab

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Henrike, Julia, Gosia, Kristian

Procedure

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USER reaction and transformation

We perform USER reaction, samples are as follows:

• plasmid pZA21 and AMO
• plasmid pZA21 and HAO
• negative control with water instead of insert

Reaction is performed in the same way as on 18-07-2013 with increased amount of insert (up to 14 uL due to low DNA concentration).

With the same procedure we also preformed a USER reaction with pZA21::RFP PCR-amplified with no promoter and araBAD from BBa_K808000.

Restriction analysis

From last week transformants with AMO and HAO in pZA21 we performed plasmid isolation.

We perform restriction analysis with EcoRI. Expected fragments are as follows:

• For pZA21 with AMO:

3309 pz, 2283 pz

• For pZA21 with HAO:

2233 pz, 2124 pz, 930 pz

Primer diluting

PCR to extract Nir from Pseudosomonas with new USER primers

Tubes have 4 labels (pZA21 only has 3), in vertical order:

• 'Nir' or 'pZ', tells which product is being made
• '1' - part 1 of Nir OR '2' - part 2 of Nir OR 'w' - whole Nir (on the pZ tubes 1 and 2 are just duplicates)
• '5' - used 5uL of N.europeae culture as template OR '10' - used 10uL of N.europeae culture as template
• 'ex' - extraction PCR, using the new non-USER primers that Jakob made OR 'U' - using the new USER primers that Jakob made

two programs:

all extraction PCRs and part 2 of Nir with USER primers - 54C, 5:00

part 1 of Nir with USER primers and pZA21 for ligation with Nir - 50C, 5:00

PCR with USER-primers on HAO and AMO

Standard USER-PCR was made with the HAO and AMO templates purified earlier today. The reactions where done in duplicates and with 2 different concentrations:

• HAO 5 is with 5uL template
• HAO 10 is with 10uL template
• AMO 5 is with 5uL template
• AMO 10 is with 10uL template

All tubes where run with 52C annealing temperature and 3 min extension time.

Results

first gel

decided to purify RFP in pZA21 without promoter as well as HAO, AMO and cycAX

purification gel

loaded the complete PCR reaction (~45 uL), cut out the bands of our products and used QIAgen gel extraction kit

• 1: 1 kb ladder
• 2: HAO
• 3: AMO
• 4: cycAX
• 5: RPF in pZA21 without promoter
• 6: RPF in pZA21 without promoter
• 7: RPF in pZA21 without promoter

gel for restriction analysis

Conclusion: We only get one band for each plasmid, so the inserts are not present.

Conclusion

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