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Protocol

1) We cultured bacterial strain with the LB medium which I added ampicillin to so that density becomes 100ug/ml overnight.(We made a nutrient medium of around 5 ml in 50 ml falcons)(Against 5 ml of nutrient mediums, Amp used 5ul)

2) Aliquot 1ml culture into a 1.5 ml microcentrifuge tube,and Made it spin at 10000rpm (4℃) for 1 min to harvest the bacteria.

3) Removed supernatant and performed 2)operation again, Removed supernatant .

4) Resuspended bacterial pellet by complete vortexing in 100ul SolutionⅠ(50 mM glucose:9g, 25 mM Tris-HCl(pH 8.0):25ml, 10mM EDTA:).

5) Inverted bacterial pellet by complete fall mixtureing in 200ul Solution Ⅱ resuspension buffer,and confirmed that it became transparent.

6) Cooled for three minutes in ice.

7) Inverted bacterial pellet by complete fall mixtureing in 150ul Solution Ⅲ resuspension buffer,and confirmed that it became Cloudiness.

8) Cooled for 3 minutes in ice.

9) Harvested the DNA by spinning at 10000rpm (4℃) for 10 min.

10) Gathered only supernatant and moved it in a new microcentrifuge tube.

11) Added 0.8ul Rnase(10mg/ml) and incubate the solution(37℃,1min)

12) Added 200ul phenol:chloroform(1:1) and inverted

13) Harvested by spinning at 10000rpm (4℃) for 5 min.

14) Removed only supernatant and moved it in a new microcentrifuge tube, after that tapped in 200ul chloroform.

15) Harvested by spinning at 10000rpm (4℃) for 1 min.

16) Moved its supernatant to a new microcentrifuge tube and add 15ul 3M sodium acetate.(Don't gather underlayer)(The ratio of the 3M sodium acetate and supernatant is made to be 10:1)

17)

@@ Line 55: / Line 55: @@
 <H1>Protocol</H1>
 <br>
+<font size="3">
+<p>
+:1) We cultured bacterial strain with the LB medium which I added ampicillin to so that density becomes 100ug/ml overnight.(We made a nutrient medium of around 5 ml in 50 ml falcons)(Against 5 ml of nutrient mediums, Amp used 5ul)
+</p>
+<p>
+:2) Aliquot 1ml culture into a 1.5 ml microcentrifuge tube,and Made it spin  at 10000rpm (4℃) for 1 min to harvest the bacteria.
+</p>
+<p>
+:3) Removed supernatant and  performed 2)operation again, Removed supernatant .
+</p>
+<p>
+:4) Resuspended bacterial pellet by complete vortexing in 100ul SolutionⅠ(50 mM glucose:9g, 25 mM Tris-HCl(pH 8.0):25ml, 10mM EDTA:).
+</p>
+<p>
+:5) Inverted bacterial pellet by complete fall mixtureing in 200ul Solution Ⅱ resuspension buffer,and confirmed that it became transparent.
+</p>
+<p>
+:6) Cooled  for three minutes in ice.
+</p>
+<p>
+:7) Inverted bacterial pellet by complete fall mixtureing in 150ul Solution Ⅲ resuspension buffer,and confirmed that it became Cloudiness.
+</p>
+<p>
+:8) Cooled  for 3 minutes in ice.
+</p>
+<p>
+:9) Harvested the DNA by spinning at 10000rpm (4℃) for 10 min.
+</p>
+<p>
+:10) Gathered only supernatant and moved it in a new microcentrifuge tube.
+</p>
+<p>
+:11) Added 0.8ul Rnase(10mg/ml) and incubate the solution(37℃,1min)
+</p>
+<p>
+:12) Added 200ul phenol:chloroform(1:1) and inverted
+</p>
+<p>
+:13) Harvested  by spinning at 10000rpm (4℃) for 5 min.
+</P>
+<p>
+:14)  Removed only supernatant and moved it in a new microcentrifuge tube, after that tapped in 200ul chloroform.
+</p>
+<p>
+:15)  Harvested  by spinning at 10000rpm (4℃) for 1 min.
+</p>
+<p>
+:16) Moved its supernatant to a new microcentrifuge tube and add 15ul 3M sodium acetate.(Don't gather underlayer)(The ratio of the 3M sodium acetate and supernatant is made to be 10:1)
+</p>
+<p>
+:17)
+</p>
+</font>

Team:KAIT Japan/Protocol

From 2014.igem.org

Revision as of 03:31, 21 August 2014

Protocol