Team:KIT-Kyoto/Notebook/ATF1/september

From 2013.igem.org

(Difference between revisions)

Revision as of 10:48, 26 September 2013

ATF1

September 1^st

Picked 32 colonies of ATF1 transformants.

September 3^rd

Checked the colonies by colony cracking.

No appropriate plasmid DNA was detected.

Digested ATF1 and pET-15b with at 37℃ overnight.

ATF1	24ul
Xho1	1ul
Bpu11021	1ul
BSA	1ul
2NEB Buffer	3ul

pET-15b	33ul
Xho1	1ul
Bpu11021	1ul
BSA	1ul
2NEB Buffer	4ul

September 4^th

Applied pET-15b and ATF1 to the blue gel electrophoresis.

No pET-15b was detected.

Extracted from Blue gel and purified ATF1.

September 11^th

PCR reaction was carried out using the primer.

Buffer	50ul
dNTP	20ul
Primer mix	1ul
Genome DNA	0.5ul
KOD-FX	2ul
H2O	26.5ul

Electrophoresed in 1% agarose gel. Verified as ATF1.

Purified PCR products of ATF1.

Digested ATF1 and pET-15b with Xho1 and Bpu11021 at 37℃ for 2 hours.

ATF1	15.5ul
Xho1	1ul
Bpu11021	1ul
BSA	0.5ul
2NEB Buffer	2ul

Added 1ul of BAP to the solution of pET-15b and incubated it at 37℃ for 30 minutes.

Ligated of pET-15b with ATF1 and transformed.

Applied pET-15b and ATF1 to the blue gel electrophoresis.

Isolated and purified them.

September 12th

Picked 32 colonies of ATF1 transformants.

September 13th

Checked the colonies by colony cracking.

Picked up the appropriate colonies and cultured in the LB in 3ml ampicillin(+) medium at 37℃ for 5 hours.

Miniprepped plasmid DNA.

Digested plasmid DNA with Xho1 and Bpu11021 at 37℃ for 2 hours.

ATF1 into pET-15b	15.5ul
Xho1	1ul
Bpu11021	1ul
BSA	0.5ul
2NEB Buffer	2ul

Applied pET-15b to the agarose gel electrophoresis.

No band was detected.

Plasmid DNA was digested with Xho1 and Bpu11021 at 37℃ (overnight).

ATF1 into pET-15b	15.5ul
Xho1	1ul
Bpu11021	1ul
BSA	0.5ul
2NEB Buffer	2ul

September 14^th

ATF1 and pET-15b were Applied to electrophoresis to the agarose gel.

No band was detected.

Digested ATF1 and pET-15b with Bpu11021 at 37℃ overnight.

ATF1	26ul
Bpu11021	1ul
Bpu Buffer	3ul

pET-15b	26ul
Bpu11021	1ul
Bpu Buffer	3ul

September 15^th

Purified ATF1 and pET-15b.

Digested ATF1 and pET-15b with Xho1.

ATF1	26ul
Xho1	1ul
Bpu Buffer	3ul

pET-15b	26ul
Xho11021	1ul
Bpu Buffer	3ul

pET-15b and ATF1 were applied to electrophoresis to the Blue gel and purified.

Ligated ATF1 with pET-15b and transformed them into E. coli cells.

September 16th

Picked 32 colonies of ATF1 transformants.

September 18th

Checked the colonies by colony cracking.

Picked up the colonies and cultured in 3ml LB medium with ampicillin at 37℃ (overnight).

September 19^th

plasmid DNA was purified and digested with Xho1 and Bpu11021 at 37℃ for 2 hours.

ATF1 into pET-15b	15.5ul
Xho1	1ul
Bpu11021	1ul
BSA	0.5ul
2NEB Buffer	2ul

ATF1 and pET-15b were applied to electrophoresis to the agarose gel.

No band was detected.

Digested ATF1 and pET-15b with Xho1 and Blp1.

ATF1	15.5ul
Xho1	1ul
Blp1	1ul
BSA	0.5ul
Buffer	2ul

pET-15b	15.5ul
Xho1	1ul
Blp1	1ul
BSA	0.5ul
Buffer	2ul

Added 1ul of BAP to the solution of pET-15b and incubated it at 37℃ for 30 minutes.

Applied pET-15b and ATF1 to the blue gel electrophoresis.

Isolated and purified them.

The ATF1 was ligated with pET-15b, and transformed into E. coli cells.

September 20^th

Picked 64 colonies of ATF1 transformants.

September 21st

Checked the colonies by colony cracking.

Picked up colonies and cultured in the LB in 3ml LB medium with ampicillin at 37℃ (overnight).

September 22nd

Miniprepped plasmid DNA and digested it with Xho1 and Blp1 at 37℃ for 2 hours.

Applied ATF1 into pET-15b to the agarose gel electrophoresis.

No band was detected.

@@ Line 13: / Line 13: @@
 <div id="doc-right" class="metro">
+<h2>ATF1</h2>
 <P STYLE="margin-bottom: 0cm"><FONT FACE=""><SPAN LANG="en-US"><FONT SIZE=4><B>September