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From 2008.igem.org

Revision as of 02:44, 29 July 2008 (view source) Gracek (Talk | contribs) (→Transformation of GFP(f)+tt constructs into DH5α) ← Older edit		Revision as of 06:08, 29 July 2008 (view source) Ksalazar (Talk | contribs) (→Reconstruction of assemblies) Newer edit →
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	:<strong>Grace & Krystle</strong>		:<strong>Grace & Krystle</strong>
-	:* PCR reaction to retrieve ccdB gene and BioBrick MCS from pSB3K3.	+	:* PCR reaction to retrieve ccdB gene and BioBrick MCS from pSB1A3.
	:* Ran on gel to verify PCR product.		:* Ran on gel to verify PCR product.
	:* Gel purified PCR product.		:* Gel purified PCR product.

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Revision as of 06:08, 29 July 2008

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Things we did today

Wetlab work

Transformation

Margaret

• Transformation of I14032 into Db3.1

Colony PCR

Margaret

• Verifying the inserts of two I51020 (the base vector) and one colony of pSB1A7 (an insulated vector with high copy #)

PCR amplification of pRL1383a

Margaret

• The omega region from pSMC121 and the rep/mob region are giving primer dimers and misamplification respectively. I am trying a gradient PCR from 49°C to 55°C to see if this will fix the problem.

PCR for BB-pRL1383a construction/verification

Grace

• PCR of BB-pRL1383a (from plasmid prep) using VF2 & VR_B0034 primers to verify B0034 insert and MCS replacement
• PCR of B0034 with HindIII and BamHI primers in case we need to redo BB-pRL1383a construction

• Maintained everything on ice this time
• Used 0.5μl plasmid in PCR reaction
• Annealing at 55C
• Extension for 30 sec. at 72C

• Gel returned 3 bands + huge smear for B0034. Smear = lots of correct product. What are the three other bands (~120bp, ~170bp, ~200bp)?
• Gel gave two bands for BB-pRL1383a (~170bp, ~300bp)
• Will redo BB-pRL1383a construction using ccdB gene as insert/MCS

Plasmid preps

Grace

• Resuspended plasmid preps in 30 μl TE and checked concentrations on nanodrop spectrometer

• nir+B0034 = 13.6 ng/μl
• GFP+B0024 = 9 ng/μl
• GFPf+B0024= 7.1 ng/μl
• BB-pRL1383a = 166.3 ng/μl

• Restriction digested nir+B0034 plasmid prep to verify insert (GFP and GFPf constructs were verified last week)

• Digested w/ EcoRI and SpeI so we can extract from gel if insert is correct
• Incubated at 37C for 2 hours
• Band way too big 1000+bp
• Need to redo

GFP(f) + tt constructs

Grace

• Restriction digested GFP and GFPf w/ EcoRI and SpeI in 50 μl reactions for 3 hours
• Restriction digested B0024 (tt) with XbaI then EcoRI for 3 hours total
• Ran on an EtBr stained 3.8% agarose gel alongside GFP+B0024 ligation from 7/22 to see if ligation was successful (and the problem was with the colony we picked)

• GFPf+tt did not show a band ~800bp
• GFP ligation was okay the first time around (we picked a bad colony to plasmid prep?)

Reconstruction of assemblies

Grace & Krystle

• PCR reaction to retrieve ccdB gene and BioBrick MCS from pSB1A3.
• Ran on gel to verify PCR product.
• Gel purified PCR product.
• RE digested overnight in 20 μl reactions (10μl DNA):

• pRL1383a with HindIII in NEBuffer 2
• ccdB+MCS with HindIII in NEBuffer 2
• GFP with EcoRI and SpeI in NEBuffer EcoRI + BSA
• GFP fusion with EcoRI and SpeI in NEBuffer EcoRI + BSA
• nir with EcoRI and SpeI in NEBuffer EcoRI + BSA
• rbs (B0030) with XbaI in NEBuffer 2 + BSA
• tt (B0024) with XbaI in NEBuffer 2 + BSA

Drylab Work

Primer Design

Margaret

• I want to design primers for some replication proteins + origin from pSB2K3

Discussion

Quote of the Day

History is the only laboratory we have in which to test the consequences of thought. - Étienne Gilson

[http://manoa.hawaii.edu/ ][http://manoa.hawaii.edu/ovcrge/ ][http://www.ctahr.hawaii.edu ]

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