Team:KIT-Kyoto/Notebook/LabNote/DIAP2-MALT9

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Revision as of 19:45, 5 October 2011

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1st, September

Member

Takeda

Again different annealing conditions were tested.

PCR reaction

10 µM Primer F	1.5 µl
10 µM Primer R	1.5 µl
Template DNA	1 µl
10 x PCR Buffer	5 µl
dNTPs	5 µl
MgSO₄	2 µl or 4 µl
ddH₂O	33 µl or 31 µl
KOD⁺ polymelase	1 µl
	total 50 µl

Cycle

Pre-Denature	94°C	2min
Denature	94°C	15sec	35 Cyle
Anneling	50.5°C	30sec
Extension	68°C	100sec
End	4°C	keep

PCR products were applied to the agarose gel electrophoresis.

Results

Image of the agarose gel.

5th, September

Member

Yokoigawa, Takeda

The PCR products for DIAP2 was treated wit phenol-chloroform and then digested with the XhoI for 20 hours at 37°C.

DIAP2

PCR reaction in ddH₂O	44 μl
10 x H Buffer	5 μl
XhoⅠ	1 μl
	total 50 μl

6th, September

Member

Yokoigawa, Takeda

The PCR products for DIAP2 was treated wit phenol-chloroform and then digested with the XbaI for 20 hours at 37°C.

DIAP2

PCR reaction in ddH₂O	44 μl
10 x M Buffer	5 μl
XbaⅠ	1 μl
	total 50 μl

7th, September

Member

Yokoigawa, Takeda

The restriction enzyme-digested PCR fragments and pUAST-flag DNA were extracted from the agarose gel byQIAquick Gel Extraction Kit.

Results

PCR products for DIAP2 Was not successfully recovered from the agarose gel.

12th, September

Member

Matsunami, Yokoigawa

To amplify DIAP2 cDNA, PCR reactions were carried out by using the following primers and under the following conditions.

F primer GCTTCTCGATTGACGGAGCTGGGCATGGAGCT

Tm value　　　　62 °C

R primer GCCGTCTAGATCACGAAAGGAACGTGCGCA

Tm value　　　　66.4°C

amplicon size　　1514 bp

PCR reaction

10 µM Primer F	1.5 µl
10 µM Primer R	1.5 µl
Template DNA	1 µl
10 x PCR Buffer	5 µl
dNTPs	5 µl
MgSO₄	2 µl
ddH₂O	33 µl
KOD⁺ polymelase	1 µl
	total 50 µl

Cycle

Pre-Denature	94°C	2min
Denature	94°C	15sec	35 Cycle
Anneling	50.5°C	30sec
Extension	68°C	1min40sec
End	4°C	keep

Again different annealing conditions were tested.

Annealing 50.5°C

13th, September

Member

Matsunami, Yokoigawa

PCR products on 12th September were applied to the agarose gel electrophoresis.

Results

Image of the agarose gel.

Lane 1；DNA size marker（1 Kbp ladder）

Lanes 2 and 3；DIAP2 cDNA

Amplified DNA fragments were barely detectable for the DIAP2.

14th, September

Members

Matsunami,Yokoigawa

To amplify API2-MALT1 cDNA and, PCR reactions were carried out by using the following primers and under the following conditions.

F primer GCCGCTCGAGACATAGTAGAAAACAGCAT

Tm value　　　　57.7 °C

R primer GCCGGCTAGCTCATTTTTCAGAAATTCTGA

Tm value　　　　56.5 °C

amplicon size　　約3131 bp

PCR reaction

10 µM Primer F	0.4 µl
10 µM Primer R	0.4 µl
Template DNA	1 µl
10 x Ex Taq Buffer	2 µl
Takara Ex Taq	0.1 µl
2.0 mM dNTPs	2 µl
ddH₂O	14.1 µl
	total 20 µl

Cycle

Pre-Denature	94°C	2min
Denature	94°C	30sec	37 Cycle
Anneling	51.5°C	30sec
Extension	72°C	3min20sec
+Extension	72°C	10min
End	4°C	keep

PCR products were applied to the agarose gel electrophoresis.

Results

Image of the agarose gel.

Lane 1；DNA size marker（1 Kbp ladder）

Lanes 2 and 3；API2-MALT1 cDNA

No PCR product was detected for API2-MALT1.

15th, September

Members

Matsunami,Yokoigawa

To amplify API2-MALT1 cDNA and DIAP2cDNA, PCR reactions were carried out by using under the following conditions.

API2-MALT1

PCR reaction

10 µM Primer F	0.4 µl
10 µM Primer R	0.4 µl
Template DNA	1 µl
10 x Ex Taq Buffer	2 µl
Takara Ex Taq	0.1 µl
2.0 mM dNTPs	2 µl
ddH₂O	14.1 µl
	total 20 µl

Cycle

Pre-Denature	94°C	2min
Denature	94°C	30sec	37 Cycle
Anneling	53°C	30sec
Extension	72°C	3min20sec
+Extension	72°C	10min
End	4°C	keep

DIAP2

PCR reaction

10 µM Primer F	1.5 µl
10 µM Primer R	1.5 µl
Template DNA	1 µl
10 x PCR Buffer for KOD Plus	5 µl
dNTPs	5 µl
MgSO₄	2 µl
ddH₂O	33 µl
KOD Plus	1 µl
	total 50 µl

Cycle

Pre-Denature	94°C	2min
Denature	94°C	15sec	35 Cycle
Anneling	50.5°C	30sec
Extension	68°C	1min 40sec
End	4°C	keep

PCR products were applied to the agarose gel electrophoresis.

The PCR products for DIAP2 was treated wit phenol-chloroform and then digested with the XhoI for 20 hours at 37°C.

DIAP2

PCR products in ddH₂O	44 µl
10 x H Buffer	5 µl
XhoⅠ	1 µl
	total 50 µl

Results

Image of the agarose gel.

Lane 1；DNA size marker（1 Kbp ladder）

Lanes 2~5；DIAP2 cDNA

Lane 6~8；API2-MALT1 cDNA

16th, September

Members

Matsunami,Yokoigawa

The PCR products for DIAP2 was treated with phenol-chloroform and then digested with the XbaI for 20 hours at 37°C.

DIAP2

PCR products in ddH₂O	44 µl
10 x M Buffer	5 µl
XbaⅠ	1 µl
	total 50 µl

17th, September

Members

Matsunami,Yokoigawa

The restriction enzyme-digested PCR fragments were extracted from the agarose gel by Gel Extraction Kit.

Results

Image of agarose gel.

PCR products for DIAP2 Was not successfully recovered from the agarose gel.

18th, September

Member

Matsunami

I have streaked E.coli DH5 alpha on LB plate and incubated for 16h.

19th, September

Member

Matsunami

I have picked a single colony up, transferred it into 250 ml of SOB medium in a flask.

I have incubated it at 18°C with shaking.

21th, September

Member

Matsunami

1.SOB medium in a flask was quantified by measuring the absorbance at OD600.

2. I have repeated the PCR reactions to amplify DIAP2 cDNA under the same conditions as those carried out on 12th September.

PCR reaction

10 µM Primer F	1.5 µl
10 µM Primer R	1.5 µl
Template DNA	1 µl
10 x PCR Buffer	5 µl
dNTPs	5 µl
MgSO₄	2 µl
ddH₂O	33 µl
KOD⁺ polymelase	1 µl
	total 50 µl

Cycle

Pre-Denature	94°C	2min
Denature	94°C	15sec	35 Cycle
Anneling	50.5°C	30sec
Extension	68°C	1kb/min
End	4°C	keep

Amplified DNA fragments were detectable for the DIAP2.

The PCR products for DIAP2 was treated with phenol-chloroform and then digested with the XhoI for 20 hours at 37°C.

DIAP2

PCR products in ddH₂O	44 µl
10 x H Buffer	5 µl
XhoⅠ	1 µl
	total 50 µl

Results

1. The absorbance OD600 was over at 0.9.

2.Image of agarose gel.

Lane 1；DNA size marker（1 Kbp ladder）

Lanes 2~7；DIAP2 cDNA

９月２２日

Member

不明★

DIAP2のPCR産物を、下表に従って制限酵素処理を行った。(37°C、overnight)

DIAP2

PCR産物 in ddH₂O	44 µl
10 x M Buffer	5 µl
XbaⅠ	1 µl
	total 50 µl

９月２３日

Member

松浪

制限酵素処理を行ったDIAP2のプラスミドを確認するため、電気泳動を行った。

Results

泳動後の写真

マーカー（1 Kbp）のみバンドが見られ、制限酵素処理を行ったDIAP2のサンプルはすべてバンドが見られなった。

９月２５日

Member

松浪

コンピテントセル(DH5α)を作成した。

９月２７日

Member

松浪

コンピテントセル(DH5α)を作成した。

@@ Line 186: / Line 186: @@
 :<table border="0"><tr><td>
 :<table border="0" width="150px">
-:<tr><td align=center>PCR条件</td></tr>
+:<tr><td align=center>PCR reaction</td></tr>
 :</table>
 :<table border=1 width="250px">
@@ Line 200: / Line 200: @@
 :</td><TD></TD><TD></TD><td>
 :<table border="0" width="100px">
-:<tr><td align=center>Cycle条件</td></tr>
+:<tr><td align=center>Cycle</td></tr>
 :</table>
 :<table border=1 width="400px">
@@ Line 236: / Line 236: @@
 :<table border="0"><tr><td>
 :<table border="0" width="150px">
-:<tr><td align=center>PCR条件</td></tr>
+:<tr><td align=center>PCR reaction</td></tr>
 :</table>
 :<table border=1 width="250px">
@@ Line 250: / Line 250: @@
 :</td><TD></TD><TD></TD><td>
 :<table border="0" width="100px">
-:<tr><td align=center>Cycle条件</td></tr>
+:<tr><td align=center>Cycle</td></tr>
 :</table>
 :<table border=1 width="400px">
@@ Line 266: / Line 266: @@
 :<table border="0"><tr><td>
 :<table border="0" width="150px">
-:<tr><td align=center>PCR条件</td></tr>
+:<tr><td align=center>PCR reaction</td></tr>
 :</table>
 :<table border=1 width="250px">
@@ Line 281: / Line 281: @@
 :</td><TD></TD><TD></TD><td>
 :<table border="0" width="100px">
-:<tr><td align=center>Cycle条件</td></tr>
+:<tr><td align=center>Cycle</td></tr>
 :</table>
 :<table border=1 width="400px">
@@ Line 301: / Line 301: @@
 :</table>
 :<table border=1 width="250px">
-:<tr><td width="150px" align=center>PCR産物 in ddH<sub>2</sub>O</td><td width="100px" align=right>44 µl</td></tr>
+:<tr><td width="150px" align=center>PCR products in ddH<sub>2</sub>O</td><td width="100px" align=right>44 µl</td></tr>
 :<tr><td align=center>10 x H Buffer</td><td align=right>5 µl</td></tr>
 :<tr><td align=center><I>Xho</I>Ⅰ</td><td align=right>1 µl</td></tr>
@@ Line 319: / Line 319: @@
 <br>
-==''９月１６日''==
+==''16th, September''==
-<b>Member</b>
+<b>Members</b>
 <br>
-:松浪、横井川
+:Matsunami,Yokoigawa
 <br>
-:DIAP2のPCR産物を、下表に従って制限酵素処理を行った。(37°C、overnight)
+:The PCR products for DIAP2 was treated with phenol-chloroform and then digested with the XbaI for 20 hours at 37°C.
 :<table border="0">
@@ Line 330: / Line 330: @@
 :</table>
 :<table border=1 width="250px">
-:<tr><td width="150px" align=center>PCR産物 in ddH<sub>2</sub>O</td><td width="100px" align=right>44 µl</td></tr>
+:<tr><td width="150px" align=center>PCR products in ddH<sub>2</sub>O</td><td width="100px" align=right>44 µl</td></tr>
 :<tr><td align=center>10 x M Buffer</td><td align=right>5 µl</td></tr>
 :<tr><td align=center><I>Xba</I>Ⅰ</td><td align=right>1 µl</td></tr>
@@ Line 337: / Line 337: @@
 <br>
-==''９月１７日''==
+==''17th, September''==
-<b>Member</b>
+<b>Members</b>
 <br>
-:松浪、横井川
+:Matsunami,Yokoigawa
 <br>
-:制限酵素処理を行ったDIAP2のプラスミドを確認するため、電気泳動を行った。
+:The restriction enzyme-digested PCR fragments were extracted from the agarose gel by [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx|QIAquick Gel Extraction Kit].
 <br>
 <b>Results</b>
-:泳動後の写真<br>
+:Image of agarose gel.<br>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/e/e9/%E6%9D%BE%E6%B5%AA%EF%BC%91.JPG" width="250px" height="250px" border="0">
 </body></html>
 <br>
-:マーカー（1 Kbp）のバンドのみが見られた。制限酵素処理を行ったDIAP2のサンプルはすべてバンドが見られなかった。
+:PCR products for DIAP2 Was not successfully recovered from the agarose gel.
 <br>
-==''９月１８日''==
+==''18th, September''==
 <b>Member</b>
 <br>
-:松浪
+:Matsunami
 <br>
-:コンピテントセル（DH5α）を作成した。
+:I have streaked E.coli DH5 alpha on LB plate and incubated for 16h.
 <br>
-==''９月１９日''==
+==''19th, September''==
 <b>Member</b>
 <br>
-:松浪
+:Matsunami
 <br>
-:コンピテントセル（DH5α）を作成した。
+:I have picked a single colony up, transferred it into 250 ml of SOB medium in a flask.
+:I have incubated it at 18°C with shaking.
 <br>
-==''９月２１日''==
+==''21th, September''==
 <b>Member</b>
 <br>
-:松浪
+:Matsunami
 <br>
-:1.コンピテントセル（DH5α）を作成した。
+:1.SOB medium in a flask was quantified by measuring the absorbance at OD600.
-:2.DIAP2について、以下の条件でPCRを行った。
+:2. I have repeated the PCR reactions to amplify DIAP2 cDNA under the same conditions as those carried out on 12th September.
 :<table border="0"><tr><td>
 :<table border="0" width="150px">
-:<tr><td align=center>PCR条件</td></tr>
+:<tr><td align=center>PCR reaction</td></tr>
 :</table>
 :<table border=1 width="250px">
@@ Line 395: / Line 395: @@
 :</td><TD></TD><TD></TD><td>
 :<table border="0" width="100px">
-:<tr><td align=center>Cycle条件</td></tr>
+:<tr><td align=center>Cycle</td></tr>
 :</table>
 :<table border=1 width="400px">
@@ Line 407: / Line 407: @@
 :</table>
-:PCR産物が増幅していることを確認するため、電気泳動を行った。
+:Amplified DNA fragments were detectable for the DIAP2.
 <br>
-:DIAP2のPCR産物を、下表に従って制限酵素処理を行った。(37°C、overnight)
+:The PCR products for DIAP2 was treated with phenol-chloroform and then digested with the XhoI for 20 hours at 37°C.
 <table border="0">
@@ Line 415: / Line 415: @@
 </table>
 <table border=1 width="250px">
-<tr><td width="150px" align=center>PCR産物 in ddH<sub>2</sub>O</td><td width="100px" align=right>44 µl</td></tr>
+<tr><td width="150px" align=center>PCR products in ddH<sub>2</sub>O</td><td width="100px" align=right>44 µl</td></tr>
 <tr><td align=center>10 x H Buffer</td><td align=right>5 µl</td></tr>
 <tr><td align=center><I>Xho</I>Ⅰ</td><td align=right>1 µl</td></tr>
@@ Line 422: / Line 422: @@
 <br>
 <b>Results</b>
-:1.ODを測定したが、OD＝0.9を超えてしまった。
+:1. The absorbance OD600 was over at 0.9.
-:泳動後の写真<br>
+:2.Image of agarose gel.<br>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/4/44/2011.09.21_DIAP2.2-7.JPG" width="250px" height="250px" border="0">
 </body></html>
 <br>
-:左から順に1レーン；マーカー（1 Kbp）、2～7レーン；DIAP2<br>
+:Lane 1；DNA size marker（1 Kbp ladder）
-:全てのサンプルでPCRが成功した。
+:Lanes 2~7；DIAP2 cDNA
 <br>