Team:KIT-Kyoto/Notebook/LabNoteJ/DIAP2-MALT8

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Latest revision as of 16:45, 5 October 2011

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8th, August

Member

Matsunami, Yokoigawa

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

API2-MALT1

F primer:GCCGCTCGAGAACATAGTAGAAAACAGCAT

Tm value　57.8°C

R　primer:GCCGGCTAGCTCATTTTTCAGAAATTCTGA

Tm value　56.5°C

amplicon size　　3131 bp

DIAP2

F primer:GCTTCTCGAGACGGAGCTGGGCATGGAGCT

Tm value　69°C

R primer:GCCGTCTAGATCACGAAAGGAACGTGCGCA

Tm value　66.4°C

amplicon size　　1514 bp

1.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	51.5°C	30sec
Extension	72°C	3min20sec
+Extension	72°C	10min
End	4°C	keep

2.DIAP2

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	56.9°C	30sec
Extension	72°C	1min40sec
+Extension	72°C	10min
End	4°C	keep

9th, August

Member

Matsunami, Yokoigawa

1. We carried out agarose gel electrophoresis to detect the PCR products.

2. We transformed E. coli XL-1 blue with the plasmid pUAST-flag.

Results

1. Image of the agarose gel.

Lane 1；size marker(1 kbp ladder）

Lane 2；the amplified API2-MALT1 cDNA fragment

Lane 3；the amplified DIAP2 cDNA fragment

Sizes of the fragments were different from the expected sizes.

2. The transformed bacterial colonies were detected.

10th, August

Member

Matsunami

1. I have repeated the PCR reactions to amplify API2-MALT1 cDNA and DIAP2 cDNA under the same conditions as those carried out on 8th, August.

2. I picked up the colonies and grew them in liquid culture.

Results

2. I have successfully grown the transformed bacteria.

11th, August

Member

Matsunami

I have isolated the plasmid DNAs (pUAST flag ) by alkaline-lysis method and electrophoresed them in agarose gel.

Results

Image of the agarose gel.

Lane 1； size marker （1 Kbp ladder）

Lanes 2～9；pUAST-flag

Lane 10；The authentic pUAST-flag vector

Lane 11；the amplified API2-MALT1 cDNA fragment

Lane 12；the amplified DIAP2 cDNA fragment

12th, August

Member

Matsunami, Yokoigawa

1. Amounts of the isolated plasmid DNA samples were quantified by measuring the absorbance at OD260.

2. We grew the transformed bacteria (25 ml x 2) and the plasmid pUAST-flag DNA was isolated by Midi-prep (Invitrogen).

Results

1. The absorbance at OD260 of two independent plasmid DNA samples are shown in Table 1.

Table 1 (OD260)

sample 1

0.189

0.208

0.192

0.190

0.191

Average value was 0.194.

Concentration of DNA was 0.970 µg/µl.

sample 2

0.282

0.276

0.278

0.269

Average value was 0.275.

Concentration of DNA was 1.37 µg/µl.

2. Image of the agarose gel.

Lane 1: DNA size marker (1Kb ladder)

Lane 6: sample 1

Lane 7: sample 2

Lane 8: The authentic pUAST-flag vector

DNAs from samples 1 and 2 migrated to the same positions as the pUAST-flag.

15th, August

Member

Matsunami, Yokoigawa

We have tried different Annealing conditions to amplify API2-MALT1 cDNA and DIAP2 cDNA. The other conditions for the PCR reactions were same as those carried out on 8th, August.

API2-MALT1

Anneling

58.9°C

DIAP2

Anneling

53°C

PCR products were applied to the agarose gel electrophoresis.

Results

Image of the agarose gel.

Lane 1；DNA size marker（1 Kbp ladder）

Lane 2；API2-MALT1 cDNA

Lane 3；DIAP2 cDNA

Size of the amplified fragments for API2-MALT1was different from the expected size and multiple DNA fragments were detected for the DIAP2.

16th, August

Member

Matsunami

Again different annealing conditions were tested.

API2-MALT1

Anneling

53°C

DIAP2

Anneling

58.9°C

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

Lane 4；DIAP2 cDNA

In lane 3, the DNA fragment with the expected size (3 kb) with the additional 2kb fragment was detected for API2-MALT1. Multiple :DNA fragments were still detected for the DIAP2.

17th, August

Member

Matsunami, Yokoigawa

Again different annealing conditions were tested.

API2-MALT1

Anneling

53.5°C

DIAP2

Anneling

50.5°C

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

Lane 4；DIAP2 cDNA

Size of the amplified fragments for API2-MALT1was different from the expected size and amplified DNA fragments were barely detectable for the DIAP2.

23rd, August

Member

Matsunami

Again different annealing conditions were tested.

API2-MALT1

Anneling

53°C

DIAP2

Anneling

50.5°C

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

Lanes 4 and 5；DIAP2 cDNA

Again the DNA fragments with the expected sizes were not detected.

24th, August

Member

Matsunami

We have decreased the amount of the template API2-MALT1DNA by diluting 10 X and 100X, then used for the PCR reactions under the following conditions.

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 2；DNA size marker（1 Kbp ladder）

Lanes 3~6；API2-MALT1 cDNA (10 X diluted)

Lanes 8~11；API2-MALT1 cDNA(100 X diluted)

No amplified DNA was detected.

25th, August

Member

Matsunami

Again different annealing conditions were tested.

API2-MALT1

Anneling

51.5°C

DIAP2

Anneling

50.5°C

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

Lanes 4 and 5；DIAP2 cDNA

No PCR product was detected for API2-MALT1. The PCR products with the expected size (1.5 kb) were detected for DIAP2.

29th, August

Member

Takeda、Yokoigawa

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

pUAST-flag vector

pUAST-flag vector(500 ng/µl)	10 µl
ddH₂O	34 µl
10 x H Buffer	5 µl
XhoⅠ	1 µl
	total 50 µl

30th, August

Member

Takeda, Yokoigawa

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 M Buffer	5 µl
XbaⅠ	1 µl
	total 50 µl

pUAST-flag vector

pUAST-flag vector(500 ng/µl)	10 μl
ddH₂O	34 µl
10 x H Buffer	5 µl
XhoⅠ	1 µl
	total 50 µl

31st, August

Member

Takeda, Yokoigawa

The restriction enzyme-digested PCR fragments and pUAST-flag DNA were extracted from the agarose gel by [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx QIAquick Gel Extraction Kit].

Results

Image of agarose gel after DNA fragment isolation.

The amount of the purified pUAST-flag vector was 45.0375 ng/µl.

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

@@ Line 1: / Line 1: @@
 {{Template:KIT-Kyoto/Notebook}}
-{{Template:KIT-Kyoto/menu}}
+{{Template:KIT-Kyoto/menu1}}
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 {| style="color:#000080;background-color:transparent;" cellpadding="3" cellspacing="1" border="0" bordercolor="#0000FF" width="900px" align="center"
-!align="left"|[[Team:KIT-Kyoto/home|Home]] > [[Team:KIT-Kyoto/Notebook|Notebook]] > [[Team:KIT-Kyoto/Notebook/LabNote|Lab Note]] > [[Team:KIT-Kyoto/Notebook/LabNote/DIAP2-MALT8|August]]
+!align="left"|[[Team:KIT-Kyoto|Home]] > [[Team:KIT-Kyoto/Notebook|Notebook]] > [[Team:KIT-Kyoto/Notebook/LabNote|Lab Note]] > [[Team:KIT-Kyoto/Notebook/LabNoteJ/DIAP2-MALT8|August]]
 !align="right"|Language：[[Team:KIT-Kyoto/Notebook/LabNote/DIAP2-MALT8|English]]/[[Team:KIT-Kyoto/Notebook/LabNoteJ/DIAP2-MALTJ8|Japanese]]
 |}
-==''８月８日''==
+==''8th, August''==
 <b>Member</b>
 <br>
-:松浪、横井川
+:Matsunami, Yokoigawa
 <br>
-:API2-MALT1、DIAP2について以下のプライマーを用いて、以下の条件でPCRを行った。
+:To amplify API2-MALT1 cDNA and DIAP2cDNA, PCR reactions were carried out by using the following primers and under the following conditions.
 <br>
 :API2-MALT1
 ::F primer:GCCGCTCGAGAACATAGTAGAAAACAGCAT<br>
-::Tm値　57.8°C<br>
+::Tm value　57.8°C<br>
 ::R　primer:GCCGGCTAGCTCATTTTTCAGAAATTCTGA<br>
-::Tm値　56.5°C<br>
+::Tm value　56.5°C<br>
-::増幅サイズ　　約3131 bp<br>
+::amplicon size　　3131 bp<br>
 :DIAP2
 ::F primer:GCTTCTCGAGACGGAGCTGGGCATGGAGCT<br>
-::Tm値　69°C<br>
+::Tm value　69°C<br>
 ::R primer:GCCGTCTAGATCACGAAAGGAACGTGCGCA<br>
-::Tm値　66.4°C<br>
+::Tm value　66.4°C<br>
-::増幅サイズ　　約1514 bp
+::amplicon size　　1514 bp
 <br>
@@ Line 35: / Line 35: @@
 :<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 49: / Line 49: @@
 :</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 65: / Line 65: @@
 :<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 79: / Line 79: @@
 :</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 93: / Line 93: @@
 <br>
-==''８月９日''==
+==''9th, August''==
 <b>Member</b>
 <br>
-:松浪、横井川
+:Matsunami, Yokoigawa
 <br>
-:1.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。
+:1. We carried out agarose gel electrophoresis to detect the PCR products.
-:2.pUAST溶液のトランスフォーメーションを行った。
+:2. We transformed E. coli XL-1 blue with the plasmid pUAST-flag.
 <br>
 <b>Results</b>
-:1.泳動後の写真<BR>
+:1. Image of the agarose gel. <BR>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/b/bc/2011.08.09_API2-MALT1.DIAP2.JPG" width="250px" height="250px" border="0">
 </body></html>
 <br>
-:1レーン；マーカー（1 Kbp）、2レーン；API2-MALT1、3レーン；DIAP2
+:Lane 1；size marker(1 kbp ladder）
-:2つとも予想される位置にバンドが確認されなかった。
+:Lane 2；the amplified API2-MALT1 cDNA fragment
+:Lane 3；the amplified DIAP2 cDNA fragment
+:Sizes of the fragments were different from the expected sizes.
 <br>
-:2.コロニーの生育がみられた。
+:2. The transformed bacterial colonies were detected.
 <br>
-==''８月１０日''==
+==''10th, August''==
 <b>Member</b>
 <br>
-:松浪
+:Matsunami
 <br>
-:1.API2-MALT1、DIAP2について、８月８日と同じ条件でPCRを行った。
+:1.  I have repeated the PCR reactions to amplify API2-MALT1 cDNA and DIAP2 cDNA under the same conditions as those carried out on 8th, August.
-:2.pUASTのプレカルチャー
+:2. I picked up the colonies and grew them in liquid culture.
 <br>
 <b>Results</b>
-:2.全てのサンプルに大腸菌の増殖がみられた。
+:2. I have successfully grown the transformed bacteria.
 <br>
-==''８月１１日''==
+==''11th, August''==
 <b>Member</b>
 <br>
-:松浪
+:Matsunami
 <br>
-:pUAST flag vectorのアルカリミニプレップをした後、プラスミドの確認をするため、電気泳動を行った。
+:I have isolated the plasmid DNAs (pUAST flag ) by alkaline-lysis method and electrophoresed them in agarose gel.
 <br>
 <b>Results</b>
-:泳動後の写真<BR>
+:Image of the agarose gel.<BR>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/2/21/2011.08.11_API2-MALT1.DIAP2.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）、2～9レーン；pUAST、10レーン；flag、11レーン；API2-MALT1、12レーン；DIAP2<br>
+:Lane 1； size marker （1 Kbp ladder）
-:pUASTは予想される位置にバンドが確認されたが、API2-MALT1、DIAP2は確認されなかった。
+:Lanes 2～9；pUAST-flag
+:Lane 10；The authentic pUAST-flag vector
+:Lane 11；the amplified API2-MALT1 cDNA fragment
+:Lane 12；the amplified DIAP2 cDNA fragment
 <br>
-==''８月１２日''==
+==''12th, August''==
 <b>Member</b>
 <br>
-:松浪、横井川
+:Matsunami, Yokoigawa
 <br>
-:1.pUAST flag vectorのアルカリミディプレップをした後、DNA濃度測定を行った。
+:1. Amounts of the isolated plasmid DNA samples were quantified by measuring the absorbance at OD260.
-:2.プラスミドの確認をするため、電気泳動を行った。
+:2. We grew the transformed bacteria (25 ml x 2) and the plasmid pUAST-flag DNA was isolated by Midi-prep (Invitrogen).
 <br>
 <b>Results</b>
-:1.サンプル1、2の吸光度を測定した結果を以下に示す（表1）。
+:1. The absorbance at OD260 of two independent plasmid DNA samples are shown in Table 1.
 <br>
-:表1、サンプル1、2の吸光度の値
+:Table 1 (OD260)
-:サンプル1
+:sample 1
 :<table border=1 width="500px">
 :<tr><td width="100px" align=rjght>0.189</td><td width="100px" align=rjght>0.208</td><td width="100px" align=rjght>0.192</td><td width="100px" align=rjght>0.190</td><td width="100px" align=rjght>0.191</td></tr>
 :</table>
-:平均は0.194であった。
+:Average value was 0.194.
-:これより、サンプル1のDNA濃度は0.970 µg/µlであった。<br>
+:Concentration of DNA was 0.970 µg/µl.<br>
 <br>
-:サンプル2
+:sample 2
 :<table border=1 width="500px">
 :<tr><td width="100px" align=rjght>0.282</td><td width="100px" align=rjght>0.276</td><td width="100px" align=rjght>0.278</td><td width="100px" align=rjght>0.269</td><td width="100px" align=rjght>0.269</td></tr>
 :</table>
-:平均は0.275でった。
+:Average value was 0.275.
-:これより、サンプル2のDNA濃度は1.37 µg/µlであった。
+:Concentration of DNA was 1.37 µg/µl.
 <br>
-.:泳動後の写真<BR>
+. Image of the agarose gel.<BR>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/3/30/2011.08.14_%E6%9D%BE%E6%B5%AA.JPG" width="250px" height="250px" border="0">
 </body></html>
 <br>
-:左がマーカー(1kb)、右から順にサンプル1、サンプル2、flagである。
+:Lane 1: DNA size marker (1Kb ladder)
-:予想される位置にバンドが見られた。
+:Lane 6: sample 1
+:Lane 7: sample 2
+:Lane 8: The authentic pUAST-flag vector
+:DNAs from samples 1 and 2 migrated to the same positions as the pUAST-flag.
 <br>
-==''８月１５日''==
+==''15th, August''==
 <b>Member</b>
 <br>
-:松浪、横井川
+:Matsunami, Yokoigawa
 <br>
-:API2-MALT1、DIAP2について、８月８日と同じ条件でAnnelingを以下のように変更してPCRを行った。
+:We have tried different Annealing conditions to amplify API2-MALT1 cDNA and DIAP2 cDNA. The other conditions for the PCR reactions were same as those carried out on 8th, August.
 :API2-MALT1<br>
@@ Line 194: / Line 205: @@
 :</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。
+:PCR products were applied to the agarose gel electrophoresis.
 <br>
 <b>Results</b>
-:泳動後の写真<BR>
+:Image of the agarose gel.<BR>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/0/0c/2011.08.15_API2-MALT1.DIAP2.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レーン；API2-MALT1、3レーン；DIAP2<br>
+:Lane 1；DNA size marker（1 Kbp ladder）
-:API2-MALT1は予想される位置にバンドが確認されず、DIAP2は複数本のバンドが見られた。
+:Lane 2；API2-MALT1 cDNA
+:Lane 3；DIAP2 cDNA
+:Size of the amplified fragments for API2-MALT1was different from the expected size and multiple DNA fragments were detected for the DIAP2.
 <br>
-==''８月１６日''==
+==''16th, August''==
 <b>Member</b>
 <br>
-:松浪
+:Matsunami
 <br>
-:API2-MALT1、DIAP2について、８月８日と同じ条件でAnnelingを以下のように変更してPCRを行った。
+:Again different annealing conditions were tested.
 :API2-MALT1<br>
@@ Line 223: / Line 237: @@
 :</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。
+:PCR products were applied to the agarose gel electrophoresis.
 <br>
 <b>Results</b>
-:泳動後の写真<BR>
+:Image of the agarose gel.<BR>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/c/c3/2011.08.16_API2-MALT1.DIAP2.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・3レーン；API2-MALT1、4レーン；DIAP2<br>
+:Lane 1；DNA size marker（1 Kbp ladder）
-レーン目のAPI2-MALT1は2 Kbpと3 Kbpにバンドが見られた。DIAP2はプライマーの特異性を高めたが、期待される位置にバンドはでなかった。
+:Lanes 2 and 3；API2-MALT1 cDNA
+:Lane 4；DIAP2 cDNA
+:In lane 3, the DNA fragment with the expected size (3 kb) with the additional 2kb fragment was detected for API2-MALT1. Multiple :DNA fragments were still detected for the DIAP2.
 <br>
-==''８月１７日''==
+==''17th, August''==
 <b>Member</b>
 <br>
-:松浪、横井川
+:Matsunami, Yokoigawa
 <br>
-:API2-MALT1、DIAP2について、８月８日と同じ条件でAnnelingを以下のように変更してPCRを行った。
+:Again different annealing conditions were tested.
 :API2-MALT1<br>
@@ Line 252: / Line 269: @@
 :</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。
+:PCR products were applied to the agarose gel electrophoresis.
 <br>
 <b>Results</b>
-:泳動後の写真<BR>
+:Image of the agarose gel.<BR>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/9/98/2011.08.17_API2-MALT1.DIAP2.JPG" width="250px" height="250px" border="0">
 </body></html>
 <br>
-右から順に1レーン；マーカー、2・3レーン；API2-MALT1、4レーン；DIAP2<br>
+:Lane 1；DNA size marker（1 Kbp ladder）
-API2-MALT1は前回の条件でPCRしたが、前回より3 Kbpのバンドが薄くなった。DIAP2は予想された位置にバンドが見えなかった。
+:Lanes 2 and 3；API2-MALT1 cDNA
+:Lane 4；DIAP2 cDNA
+:Size of the amplified fragments for API2-MALT1was different from the expected size and amplified DNA fragments were barely detectable for the DIAP2.
 <br>
-==''８月２３日''==
+==''23rd, August''==
 <b>Member</b>
 <br>
-:松浪
+:Matsunami
 <br>
-:API2-MALT1、DIAP2について、８月８日と同じ条件でAnnelingを以下のように変更してPCRを行った。
+:Again different annealing conditions were tested.
 :API2-MALT1<br>
@@ Line 281: / Line 301: @@
 :</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。
+:PCR products were applied to the agarose gel electrophoresis.
 <br>
 <b>Results</b>
-:泳動後の写真<BR>
+:Image of the agarose gel.<BR>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/6/68/2011.08.23_API2-MALT1.DIAP2.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レーン；API2-MALT1、3レーン；API2-MALT1、4レーン；DIAP2、5レーン；DIAP2<br>
+:Lane 1；DNA size marker（1 Kbp ladder）
-API2-MALT1についてDNAポリメラーゼを変更したが、期待されるバンドは見られなかった。
+:Lanes 2 and 3；API2-MALT1 cDNA
+:Lanes 4 and 5；DIAP2 cDNA
+:Again the DNA fragments with the expected sizes were not detected.
 <br>
-==''８月２４日''==
+==''24th, August''==
 <b>Member</b>
 <br>
-:松浪
+:Matsunami
 <br>
-:API2-MALT1について10、100倍希釈後、以下の条件でPCRを行った。
+:We have decreased the amount of the template API2-MALT1DNA by diluting 10 X and 100X, then used for the PCR reactions under the following conditions.
 :<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 316: / Line 340: @@
 :</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 329: / Line 353: @@
 :</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。
+:PCR products were applied to the agarose gel electrophoresis.
 <br>
 <b>Results</b>
-:泳動後の写真<BR>
+:Image of the agarose gel.<BR>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/e/e6/2011.08.24_API2-MALT1_10.100%E5%80%8D%E5%B8%8C%E9%87%88.JPG" width="250px" height="250px" border="0">
 </body></html>
 <br>
-左から順に2レーン；マーカー、3～6レーン；API2-MALT1（10倍希釈）、8～11レーン；API2-MALT1（100倍希釈）<br>
+:Lane 2；DNA size marker（1 Kbp ladder）
-バンドは何も見られなかった。
+:Lanes 3~6；API2-MALT1 cDNA (10 X diluted)
+:Lanes 8~11；API2-MALT1 cDNA(100 X diluted)
+:No amplified DNA was detected.
 <br>
-==''８月２５日''==
+==''25th, August''==
 <b>Member</b>
 <br>
-:松浪
+:Matsunami
 <br>
-:API2-MALT1、DIAP2について、８月８日と同じ条件でAnnelingを以下のように変更してPCRを行った。
+:Again different annealing conditions were tested.
 :API2-MALT1<br>
@@ Line 358: / Line 385: @@
 :</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。
+:PCR products were applied to the agarose gel electrophoresis.
 <br>
 <b>Results</b>
-:泳動後の写真<BR>
+:Image of the agarose gel<BR>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/7/72/2011.08.25_API2-MALT1.DIAP2.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・3レーン；API2-MALT1、4・5レーン；DIAP2<br>
+:Lane 1；DNA size marker（1 Kbp ladder）
-API2-MALT1に関してバンドは見られなかった。DIAP2については予想される位置にバンドが見られた。
+:Lanes 2 and 3；API2-MALT1 cDNA
+:Lanes 4 and 5；DIAP2 cDNA
+:No PCR product was detected for API2-MALT1. The PCR products with the expected size (1.5 kb) were detected for DIAP2.
 <br>
-==''８月２９日''==
+==''29th, August''==
 <b>Member</b>
 <br>
-:武田、横井川
+:Takeda、Yokoigawa
 <br>
-:25日に確認したDIAP2をフェノールクロロホルム処理し、
+:The PCR products for DIAP2 was treated wit phenol-chloroform and then digested with the XhoI for 20 hours at 37°C.
-:pUAST-flag vectorとともに、下表に従って制限酵素処理を行った。(37°C、overnight)
 :DIAP2<br>
@@ Line 384: / Line 413: @@
 :</table>
 :<table border="1" width="250">
-:<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　reaction 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 403: / Line 432: @@
 :</table>
-°Cで20時間静置した。
 <br>
-==''８月３０日''==
+==''30th, August''==
 <b>Member</b>
 <br>
-:武田、横井川
+:Takeda, Yokoigawa
 <br>
-:25日に確認したDIAP2をフェノールクロロホルム処理し、
+:The PCR products for DIAP2 was treated wit phenol-chloroform and then digested with the XhoI for 20 hours at 37°C.
-:pUAST-flag vectorとともに、下表に従って制限酵素処理を行った。(37°C、overnight)
 :<table border="0"><tr><td>
@@ Line 419: / Line 446: @@
 :</table>
 :<table border="1" width="250">
-:<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 reaction 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 436: / Line 463: @@
 :</table></td></tr></table>
-°Cで20時間静置した 。
 <br>
-==''８月３０日''==
+==''31st, August''==
 <b>Member</b>
 <br>
-:武田、横井川
+:Takeda, Yokoigawa
 <br>
-:[http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx QIAquick Gel Extraction Kit]を使用してゲルからDIAP2のDNAとpUAST-flag vectorを抽出した。
+:The restriction enzyme-digested PCR fragments and pUAST-flag DNA were extracted from the agarose gel by [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx QIAquick Gel Extraction Kit].
 <br>
 <b>Results</b>
-:ゲル切り出し後の写真<br>
+:Image of agarose gel after DNA fragment isolation. <br>
 :<html><body>
 <IMG src="https://static.igem.org/mediawiki/2011/2/27/2011.08.31_%E6%A8%AA%E4%BA%95%E5%B7%9DpUAST-flag-vector.JPG" width="240px" height="280px" border="0">
 </body></html>
 <br>
-:pUAST-flag vectorは精製でき、濃度は45.0375 ng/µlであった。
+:The amount of the purified pUAST-flag vector was 45.0375 ng/µl.
-:DIAP2はゲル抽出でバンドが見られなかった。
+:PCR products for DIAP2 Was not successfully recovered from the agarose gel.
 <br>
 </div>