Team:Biwako Nagahama/Material & Method

From 2013.igem.org

(Difference between revisions)
(Genaral protocol)
(Genaral protocol)
Line 31: Line 31:
<p>↓Centrifuge 4℃ 13,000rpm 5min</p>
<p>↓Centrifuge 4℃ 13,000rpm 5min</p>
<p>Only supernatant was taken</p>
<p>Only supernatant was taken</p>
-
<p>↓</p>
 
----
----
<h3>EtOH crystalization</h3>
<h3>EtOH crystalization</h3>
----
----
-
<p>Add 1μL 20mg/mL Glycogen</p>
+
<p>↓Add 1μL 20mg/mL Glycogen</p>
<p>↓Mix</p>
<p>↓Mix</p>
-
<p>Add 1/10 volume 3M CH3COONa(pH5.2)</p>
+
<p>↓Add 1/10 volume 3M CH3COONa(pH5.2)</p>
-
<p>↓</p>
+
<p>↓Add 2.5 times volume 99.5% EtOH</p>
-
<p>Add 2.5 times volume 99.5% EtOH</p>
+
<p>↓Vortex</p>
<p>↓Vortex</p>
<p>↓Centrifuge 4℃ 13,000rpm 20min</p>
<p>↓Centrifuge 4℃ 13,000rpm 20min</p>
-
<p>Waste supernatant</p>
+
<p>↓Waste supernatant</p>
-
<p>↓</p>
+
<p>↓Add 500μL 70% EtOH</p>
-
<p>Add 500μL 70% EtOH</p>
+
<p>↓Mix</p>
<p>↓Mix</p>
<p>↓Centrifuge for 10s in a table-top microcentrifuge</p>
<p>↓Centrifuge for 10s in a table-top microcentrifuge</p>
-
<p>Waste supernatant</p>
+
<p>↓Waste supernatant</p>
-
<p>↓</p>
+
<p>↓65℃ Dry up</p>
-
<p>65℃ Dry up</p>
+
<p>↓Add 11μL TE buffer</p>
-
<p>↓</p>
+
-
<p>Add 11μL TE buffer</p>
+
== <h2>CelC</h2> ==
== <h2>CelC</h2> ==

Revision as of 17:36, 27 September 2013

Contents

Material & Method

Genaral protocol

Distribution kit

↓With a pipette tip, punch a hole in the foil

↓Add 10μL of dH2O,and pipetting

↓Put 5min

↓Pipette 1uL of the resuspended DNA Transformation into your desired 100μL of competent cells

↓Hold on ice for 20min

↓Heat shock at 42℃ for 30sec

↓quickly

↓On ice for 2min

↓Add 900μL of SOCborth

↓Hold at 37℃ for 30min

↓Plating 100μL of DNA Transformation

↓Centrifuge for 1 min(13,000rpm)

↓Waste supernatant for 800μL, and pipetting

↓Plating all

↓Incubate at 37℃ (over night)

Phenol-chloroform extraction

Add Phenol-chloroform where is equivalent to Exo Star process sample

↓Centrifuge 4℃ 13,000rpm 5min

Only supernatant was taken

EtOH crystalization

↓Add 1μL 20mg/mL Glycogen

↓Mix

↓Add 1/10 volume 3M CH3COONa(pH5.2)

↓Add 2.5 times volume 99.5% EtOH

↓Vortex

↓Centrifuge 4℃ 13,000rpm 20min

↓Waste supernatant

↓Add 500μL 70% EtOH

↓Mix

↓Centrifuge for 10s in a table-top microcentrifuge

↓Waste supernatant

↓65℃ Dry up

↓Add 11μL TE buffer

CelC

Crds

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