Griffitts:Restriction digest: Difference between revisions

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{{Griffitts}}
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<font size="5">Restriction Digest</font>
<font size="5">Restriction Digest</font>
==Materials==
==Materials==
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===15 μL reaction===
===15 μL reaction===
* 5 μL DNA
* 5 μL DNA
* 1.8 μL appropriate 10X buffer
* 1.5 μL appropriate 10X buffer
* 1.5 μL 10X BSA (if needed--see below)
* 1.5 μL 10X BSA (if needed&mdash;see below)
* Restriction enzyme(s) (see specific enzymes below for exact amounts)
* Restriction enzyme(s) (see specific enzymes below for exact amounts)
** Don't immerse the tip, draw from the surface to avoid excess enzyme
** Don't immerse the tip, draw from the surface to avoid excess enzyme
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===30 μL reaction===
===30 μL reaction===
* 12 μL DNA
* 12 μL DNA
* 4.3 μL appropriate 10X buffer
* 3.0 μL appropriate 10X buffer
* 4.0 μL 10X BSA (if needed--see below)
* 3.0 μL 10X BSA (if needed&mdash;see below)
* Restriction enzyme(s) (see specific enzymes below for exact amounts)
* Restriction enzyme(s) (see specific enzymes below for exact amounts)
** Don't immerse the tip, draw from the surface to avoid excess enzyme
** Don't immerse the tip, draw from the surface to avoid excess enzyme
* Add ddH<sub>2</sub>0 to bring the final volume to 30 μL
* Add ddH<sub>2</sub>0 to bring the final volume to 30 μL
Note: Use this recipe when your DNA concentrations are sufficient
Note: Use this recipe when your DNA concentrations are sufficient<br>
Note: For a ''Bam''HI&ndash;''Xba''I double-digest, use 3.3 μL of 10X buffer
 
===40 μL reaction===
===40 μL reaction===
* 20 μL DNA
* 20 μL DNA
* 4.3 μL appropriate 10X buffer
* 4.0 μL appropriate 10X buffer
* 4.0 μL 10X BSA (if needed--see below)
* 4.0 μL 10X BSA (if needed&mdash;see below)
* Restriction enzyme(s) (see specific enzymes below for exact amounts)
* Restriction enzyme(s) (see specific enzymes below for exact amounts)
** Don't immerse the tip, draw from the surface to avoid excess enzyme
** Don't immerse the tip, draw from the surface to avoid excess enzyme
* Add ddH<sub>2</sub>0 to bring the final volume to 40 μL
* Add ddH<sub>2</sub>0 to bring the final volume to 40 μL
Note: Use this recipe when your DNA concentrations are low
Note: Use this recipe when your DNA concentrations are low<br>
Note: For a ''Bam''HI&ndash;''Xba''I double-digest, use 4.3 μL of 10X buffer


==Procedure==
==Procedure==
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* Incubate at 37°C for 2.5 to 8 hours
* Incubate at 37°C for 2.5 to 8 hours
* If preparing a ligation, add 0.5 μL CIP to the vector 30 minutes prior to ending the reaction
* If preparing a ligation, add 0.5 μL CIP to the vector 30 minutes prior to ending the reaction
* When the reaction is complete you can store your samples in the -20°C freezer
* When the reaction is complete you can store your samples in the -20°C freezer or proceed to [[Griffitts:In-gel ligation|in-gel ligation]]
 
==Enzymes==
==Enzymes==
{| border="1" cellpadding="5" cellspacing="0" class="wikitable sortable"
{| border="1" cellpadding="5" cellspacing="0" class="wikitable sortable"
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|-
|-
| ''Bam'' HI
| ''Bam'' HI
| 1 μL
| 0.8 μL
| g/gatcc
| g/gatcc
| gatc
| gatc
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| '''100'''
| '''100'''
| 75
| 75
| 75
| '''100'''
| None
| None
| 37°C
| 37°C
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|-
|-
| '''''Bam'' HI'''
| '''''Bam'' HI'''
| seq<sup>1</sup>
| seq<sup><font color=red>1</font></sup>
| -
| -
| -
| -
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| '''''Xba'' I'''
| '''''Xba'' I'''
| 2
| 2
| seq
| seq<sup><font color=red>2</font></sup>
| 2
| 2
| 2
| 2
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|-
|-
|}
|}
<sup>1</sup> Sequential digest recommended.
<sup><font color=red>1</font></sup>Sequential digest recommended.<br>
<sup><font color=red>2</font></sup>We actually prefer to do the double-digest and use Buffer 2 for the ''Bam''HI&ndash;''Xba''I double-digest.<br>
Note that a double-digest of ''Bam'' HI and ''Xba'' I is not recommended. However, by following [[Griffitts:Restriction digest#30 μL reaction|the procedure above]] you won't have any problems.
<br><br>
<br><br>
''Adapted from New England BioLabs 2005-06 Catalog and Technical Reference.''
Adapted from ''New England BioLabs 2005-06 Catalog and Technical Reference.''

Latest revision as of 11:38, 20 March 2012

Restriction Digest

Materials

  • ddH20
  • DNA sample on ice
  • Appropriate 10X buffer (see below) on ice
  • 10X BSA on ice (if necessary; see below)
  • Restriction enzyme(s) (see below) on ice
  • CIP (keep in freezer until needed)

Recipes

15 μL reaction

  • 5 μL DNA
  • 1.5 μL appropriate 10X buffer
  • 1.5 μL 10X BSA (if needed—see below)
  • Restriction enzyme(s) (see specific enzymes below for exact amounts)
    • Don't immerse the tip, draw from the surface to avoid excess enzyme
  • Add ddH20 to bring the final volume to 15 μL

Note: Use this recipe when verifying plasmid inserts
Note: You can check this reaction after 1 hour

30 μL reaction

  • 12 μL DNA
  • 3.0 μL appropriate 10X buffer
  • 3.0 μL 10X BSA (if needed—see below)
  • Restriction enzyme(s) (see specific enzymes below for exact amounts)
    • Don't immerse the tip, draw from the surface to avoid excess enzyme
  • Add ddH20 to bring the final volume to 30 μL

Note: Use this recipe when your DNA concentrations are sufficient
Note: For a BamHI–XbaI double-digest, use 3.3 μL of 10X buffer

40 μL reaction

  • 20 μL DNA
  • 4.0 μL appropriate 10X buffer
  • 4.0 μL 10X BSA (if needed—see below)
  • Restriction enzyme(s) (see specific enzymes below for exact amounts)
    • Don't immerse the tip, draw from the surface to avoid excess enzyme
  • Add ddH20 to bring the final volume to 40 μL

Note: Use this recipe when your DNA concentrations are low
Note: For a BamHI–XbaI double-digest, use 4.3 μL of 10X buffer

Procedure

  • Combine ingredients for recipe
  • Incubate at 37°C for 2.5 to 8 hours
  • If preparing a ligation, add 0.5 μL CIP to the vector 30 minutes prior to ending the reaction
  • When the reaction is complete you can store your samples in the -20°C freezer or proceed to in-gel ligation

Enzymes

Restriction Enzymes
Enzyme Amount Target Overhang NEBuffer1 NEBuffer2 NEBuffer3 NEBuffer4 Other Buffer BSA
Avr II c/ctagg ctag 100 1001 50 100 None 37°C No
Bam HI 0.8 μL g/gatcc gatc 75 100 50 75 Bam HI 37°C Yes
Bgl II a/gatct gatc 10 75 100 10 None 37°C No
Bst XI ccannnnn/ntgg nnnn 25 100 100 50 None 55°C No
Eco RI g/aattc aatt 100 100 100 100 Eco RI 37°C No
Eco RV gat/atc none 50 75 100 50 None 37°C Yes
Hind III a/agctt agct 50 100 10 50 None 37°C No
Kpn I ggtac/c gtac 100 75 0 75 None 37°C Yes
Nde I ca/tatg ta 75 100 75 100 None 37°C No
Pst I ctgca/g tgca 75 75 100 50 None 37°C Yes
Sac I gagct/c agct 100 50 10 100 None 37°C Yes
Sal I g/tcgac tcga 0 0 100 0 None 37°C Yes
Sma I ccc/ggg none 0 0 0 100 None 25°C No
Spe I a/ctagt ctag 75 100 25 75 None 37°C Yes
Sph I gcatg/c catg 100 100 50 100 None 37°C No
Xba I 1.5 μL t/ctaga ctag 0 100 75 100 None 37°C Yes
Xho I c/tcgag tcga 75 100 100 100 None 37°C Yes

1Boldface indicates the preferred buffer for the enzyme.

Adapted from New England BioLabs 2005-06 Catalog and Technical Reference.

Double Digests

Suggested Buffers
Enzyme Avr II Bam HI Bgl II Eco RI Eco RV Hind III Kpn I Nde I Pst I Sac I Sal I Sma I Spe I Sph I Xba I
Bam HI seq1 - - - - - - - - - - - - - -
Bgl II 3 Bam HI - - - - - - - - - - - - -
Eco RI Eco RI Eco RI Eco RI - - - - - - - - - - - -
Eco RV 2 Bam HI 3 Eco RI - - - - - - - - - - -
Hind III 2 seq 2 Eco RI 2 - - - - - - - - - -
Kpn I 1 seq 2 2 2 2 - - - - - - - - -
Nde I 4 Bam HI 3 Eco RI 2 2 1 - - - - - - - -
Pst I 3 Bam HI 3 Eco RI 3 2 1 3 - - - - - - -
Sac I 1 seq 2 seq 2 2 1 4 1 - - - - - -
Sal I seq Bam HI 3 Eco RI 3 seq seq 3 3 seq - - - - -
Sma I 4 seq seq seq 4 4 seq 4 4 4 seq - - - -
Spe I 2 Bam HI 2 Eco RI 2 2 1 2 2 1 seq 4 - - -
Sph I 2 Bam HI 2 Eco RI 2 2 1 2 2 1 seq 4 2 - -
Xba I 2 seq2 2 2 2 2 2 2 3 4 3 4 2 2 -
Xho I 2 Bam HI 3 Eco RI 3 2 1 4 3 1 3 4 2 2 2

1Sequential digest recommended.
2We actually prefer to do the double-digest and use Buffer 2 for the BamHI–XbaI double-digest.
Note that a double-digest of Bam HI and Xba I is not recommended. However, by following the procedure above you won't have any problems.

Adapted from New England BioLabs 2005-06 Catalog and Technical Reference.