Protocol/13

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Protocol 13: Vector dephosphorylation protocol
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Protocol 13: Vector Dephosphorylation
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What you will need:
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Reagents:
* Antarctic phosphatase
* Antarctic phosphatase
* 10x Antarctic phosphatase buffer
* 10x Antarctic phosphatase buffer
 +
Procedure:
Procedure:
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* Add 1/10 volume of 10x antarctic phosphatase reaction buffer to 1-5 ug of DNA cut with any restriction endonuclease in any buffer
+
* Add 1/10 volume of 10x antarctic phosphatase reaction buffer to 1-5ug of DNA cut with any restriction endonuclease in any buffer.
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* Add 1 ul of Antarctic phosphatase and mix
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* Add 1ul of Antarctic phosphatase and mix.
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* Incubate 5 min at 37 C
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* Incubate 5 minutes at 37<sup>o</sup>C.
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* Heat inactivate for 5 minutes at 65 C
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* Heat inactivate for 5 minutes at 65<sup>o</sup>C.
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* Proceed with ligation
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* Proceed with ligation.
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Notes:
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* Vector dephosphorylation can be useful in cutting transformation background, but it is very harsh.
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* It chews off 5' phosphates, but it also keeps chewing on the DNA ends, reducing total transformation efficiency.
 +
* Try without dephosphorylation first, and minimize exposure to phosphatase if you must resort to using it.
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** See also Sambrook.
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==Notes==
 
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Vector dephosphorylation can be useful in cutting transformation background, but it is very harsh. It chews off 5' phosphates, but it also keeps chewing on the DNA ends, reducing total transformation efficiency. Try without dephosphorylation first, and minimize exposure to phosphatase if you must resort to using it. See also Sambrook.
 
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[[Team:Alberta/Notebook/protocols| Back]]
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Revision as of 01:37, 26 October 2010

TEAM ALBERTA

Protocol 13: Vector Dephosphorylation


Reagents:

  • Antarctic phosphatase
  • 10x Antarctic phosphatase buffer


Procedure:

  • Add 1/10 volume of 10x antarctic phosphatase reaction buffer to 1-5ug of DNA cut with any restriction endonuclease in any buffer.
  • Add 1ul of Antarctic phosphatase and mix.
  • Incubate 5 minutes at 37oC.
  • Heat inactivate for 5 minutes at 65oC.
  • Proceed with ligation.


Notes:

  • Vector dephosphorylation can be useful in cutting transformation background, but it is very harsh.
  • It chews off 5' phosphates, but it also keeps chewing on the DNA ends, reducing total transformation efficiency.
  • Try without dephosphorylation first, and minimize exposure to phosphatase if you must resort to using it.
    • See also Sambrook.


Back

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