Team:UT-Tokyo/Restriction Enzyme digestion(Xba1/Pst1)—Once for all

From 2010.igem.org

(Difference between revisions)
(New page: __NOTOC__{{UT-Tokyo_CSS3}}{{UT-Tokyo_Head}} <h1>Restriction Enzyme digestion(Xba1/Pst1)—Once for all</h1> <h2>Preparation</h2> *plasmid *10× buffer (H and M in the freezer) *enz...)
 
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<h3>for extracting gel</h3>
<h3>for extracting gel</h3>
begin with 0.5μl enzyme and add to it if you worry (0.5μl is enough)
begin with 0.5μl enzyme and add to it if you worry (0.5μl is enough)
-
*1. add ?μl plasmid(30μl for 1000ng)
+
*1. add ?μl plasmid(30μl for 1000ng)<br />
-
     3μl 10× buffer
+
     3μl 10× buffer<br />
-
     0.5μl enzymeI
+
     0.5μl enzymeI<br />
-
     0.5μl enzymeII
+
     0.5μl enzymeII<br />
-
     MilliQ up to 30μl
+
     MilliQ up to 30μl<br />
-
*2. incubate at 37 degrees for over 1hour
+
*2. incubate at 37 degrees for over 1hour<br />
(for 3 or 4 hour makes it sure)
(for 3 or 4 hour makes it sure)
<h3>for cut check</h3>
<h3>for cut check</h3>
-
*1. add 1μl plasmid (regardless of the concentration)
+
*1. add 1μl plasmid (regardless of the concentration)<br />
-
     2μl 10× buffer
+
     2μl 10× buffer<br />
-
     0.5μl enzymeI
+
     0.5μl enzymeI<br />
-
     0.5μl enzymeII
+
     0.5μl enzymeII<br />
-
     MilliQ up to 20μl
+
     MilliQ up to 20μl<br />
-
*2. incubate at 37 degrees for over 1hour
+
*2. incubate at 37 degrees for over 1hour<br />
(for 3 or 4 hour makes it sure)
(for 3 or 4 hour makes it sure)
{{UT-Tokyo_Foot}}
{{UT-Tokyo_Foot}}

Latest revision as of 07:37, 23 September 2010

UT-Tokyo

Restriction Enzyme digestion(Xba1/Pst1)—Once for all

Preparation

  • plasmid
  • 10× buffer (H and M in the freezer)
  • enzymeI,enzymeII(in the freezer in the next room)
  • MilliQ
  • 1.5ml tube

■the correspondence of buffers

EX・・・M ES・・・H XP・・・M SP・・・H

Procedure

■attention

  • use 1.5ml tube
  • enzyme must always be on ice! / Don’t leave at room temperature and heat!

put back in the freezer immediately!

  • thaw frozen buffer fully! / you should spin down and vortex
  • change MilliQ into new one everyday

※add MilliQ first and enzyme last / mix before add enzyme


for extracting gel

begin with 0.5μl enzyme and add to it if you worry (0.5μl is enough)

  • 1. add ?μl plasmid(30μl for 1000ng)

     3μl 10× buffer
     0.5μl enzymeI
     0.5μl enzymeII
     MilliQ up to 30μl

  • 2. incubate at 37 degrees for over 1hour

(for 3 or 4 hour makes it sure)

for cut check

  • 1. add 1μl plasmid (regardless of the concentration)

     2μl 10× buffer
     0.5μl enzymeI
     0.5μl enzymeII
     MilliQ up to 20μl

  • 2. incubate at 37 degrees for over 1hour

(for 3 or 4 hour makes it sure)

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