Difference: ProtocolsGibsonCloning (4 vs. 5)

Revision 52013-02-13 - NeilGottel

 
META TOPICPARENT name="ProtocolList"
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Gibson Assembly-Work In Progress (Neil)

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Gibson Assembly-Work In Progress, do not use yet

 

Background and Design

Gibson Cloning is a technique of DNA construct assembly that allows one to join multiple linear segments into either one large linear segment or, if the segments contain the appropriate components and overlaps, an intact plasmid. This protocol follows the one-step ISO assembly of overlapping dsDNA protocol. In order to assemble segments of DNA via Gibson Cloning, they must contain at least 40bp of homology to the segment they are being joined to. For example, if one was to make a construct that was Seg1-Seg2-Seg3 from individual PCRs of Seg1, Seg2, and Seg3, the 3' end of Seg1 would need 40bp of homology to the 5' end of Seg2 and Seg3 would require it 5' end to have 40bp of homology to Seg2. For constructing a plasmid, use a linearized vector backbone as one of your segments.

Supplies

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<		If mastermix aliquots are available, and less than 2 years old:
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>		If mastermix aliquots are available, and less than 1 year old:
 
  • 15uL aliquots of Gibson master mix, located on the top shelf of the -20°C in Welch. Tubes are in both a 96 well holder, and a 50mL tube.
  • Pure water
  • Positive control: 2 overlapping halves of pUC19 (one has AmpR, the other ori). ATH pUC19 1841-1865 "R", ATH pUC19 306-289 "F"

If no mastermix aliquots remain, but there is still <1 year old isothermal (ISO) reaction buffer available:

If no mastermix aliquots remain, and there is no ISO buffer, or the current ISO buffer is more than a year old:

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Primer Design Using Gibthon

 

Protocol

  1. Mix 10ng-100ng of each of your DNA segments together (such that their ratios are equimolar) into a 5uL total volume.
  2. Add that 5uL of DNA to the Gibson Master Mix, mix well by pipetting.
  3. Incubate the reaction at 50C for 1 hour.
  4. Dilute the reaction 1:5 in sterile, nuclease free water. Use this diluted sample for PCR (if linear) or transformation (if a plasmid).
  5. Run an aliquot of your final reaction on a gel to verify the presence of your construct. It may be used to do make a 'no incubation' control to determine if the chemistry of the reaction happened.

Expected Results

The positive control should yield ampicillin resistant colonies when transformed into E. coli. If ran a 1% agarose gel, expected size is

Common Problems/Troubleshooting

Positive control details

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<		AmpR half of pUC19, bp
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>		AmpR half of pUC19, ~1150bp
 
  • ATH pUC19 1841-1865 "R", 5’-CATGACCAAAATCCCTTAACGTGAG-3’
  • ATH pUC19 306-289 "F" 5’-GTAAAACGACGGCCAGTG-3’
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<		Ori half of pUC19, bp
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>		Ori half of pUC19, ~1600bp
 
  • ATH pUC19 1883-1861 "F" 5’-CGCTCAGTGGAACGAAAACTCAC-3’
  • ATH pUC19 266-283 "R" 5’-TCCCCGGGTACCGAGCTC-3’

Initial denaturation: 98°C for 30s

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<		25 Cycles of: 98°C for 10s, 60°C for 20s, 72°C for 60s
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>		25 Cycles of: 98°C for 10s, (60°C for 20s, 72°C for 60s
  final extension: 72°C for 5 minutes

Changed:
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<		-- BrianRenda - 26 Sep 2011 -- NeilGottel - 08 Feb 2013
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>		 -- NeilGottel - 13 Feb 2013
 
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