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Revision as of 11:35, 28 September 2007 (view source) Craig (Talk | contribs) (→Method including controls) ← Older edit		Latest revision as of 11:37, 28 September 2007 (view source) Craig (Talk | contribs) (→Equipement Required)
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	=====Equipement Required=====		=====Equipement Required=====
-	*1.5mL Microfuge tubes	+	*[[Melbourne/1.7ml microcentrifuge|microcentrifuge: 1.7ml]]
	*Pipettes		*Pipettes
	*Fridge		*Fridge
		+
	=====References=====		=====References=====
	*		*

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Latest revision as of 11:37, 28 September 2007

<Return to list of protocols> <Team home page>

• Applications: Ligate DNA fragments together

• Time to complete protocol: Overnight, 2 hours, or 10 minutes
  • Lab time: 5 minutes
  • Waiting time: Overnight, 2h, 10min
• Approximate cost of materials: $

Contents 1 Method from primary and secondary reagents 1.1 Primary & secondary Reagents Required including controls 1.2 Method including controls 1.3 Equipement Required 1.4 References

Method from primary and secondary reagents

Primary & secondary Reagents Required including controls

• T4 Ligase buffer 10X or T4 Ligase buffer 2X
• DNA for ligation
• T4 Ligase
• milliQ water

Method including controls

Add to a sterile 1.7ml Eppendorf

• Roughly an equal quantity of DNA fragments to be ligated together (usually 5ul of both vector and insert if gel-purified)
• 2ul of T4 Ligase buffer 10X or 10ul of T4 Ligase buffer 2X
• 1ul of T4 Ligase
• milliQ water to make up to 20ul

Incubate Overnight (if using 10X buffer) at 4 degrees, 2h or 5min (if using 2X buffer) at room temprature.

Equipement Required

• microcentrifuge: 1.7ml
• Pipettes
• Fridge

References