Team:KIT-Kyoto/Notebook/LabNote/DIAP2-MALT8
From 2011.igem.org
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<br> | <br> | ||
:1. We carried out agarose gel electrophoresis to detect the PCR products. | :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. | + | :2. We transformed ''E. coli'' ''XL-1 blue'' with the plasmid pUAST-flag. |
<br> | <br> | ||
<b>Results</b> | <b>Results</b> | ||
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:Lane 2;API2-MALT1 cDNA | :Lane 2;API2-MALT1 cDNA | ||
:Lane 3;DIAP2 cDNA | :Lane 3;DIAP2 cDNA | ||
- | :Size of the amplified fragments for API2- | + | :Size of the amplified fragments for API2-MALT1 was different from the expected size and multiple DNA fragments were detected for the DIAP2. |
<br> | <br> | ||
Line 322: | Line 322: | ||
:Matsunami | :Matsunami | ||
<br> | <br> | ||
- | :We have decreased the amount of the template API2- | + | :We have decreased the amount of the template API2-MALT1 cDNA by diluting 10 x and 100 x , then used for the PCR reactions under the following conditions. |
:<table border="0"><tr><td> | :<table border="0"><tr><td> | ||
Line 405: | Line 405: | ||
:Takeda、Yokoigawa | :Takeda、Yokoigawa | ||
<br> | <br> | ||
- | :The PCR products for DIAP2 was treated | + | :The PCR products for DIAP2 was treated with phenol-chloroform and then digested with the ''Xho''I for 20 hours at 37°C. |
:DIAP2<br> | :DIAP2<br> | ||
Line 439: | Line 439: | ||
:Takeda, Yokoigawa | :Takeda, Yokoigawa | ||
<br> | <br> | ||
- | :The PCR products for DIAP2 was treated | + | :The PCR products for DIAP2 was treated with phenol-chloroform and then digested with the ''Xba''I for 20 hours at 37°C. |
:<table border="0"><tr><td> | :<table border="0"><tr><td> | ||
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:<tr><td align="center">ddH<sub>2</sub>O</td><td align="right">34 µl</td></tr> | :<tr><td align="center">ddH<sub>2</sub>O</td><td align="right">34 µl</td></tr> | ||
:<tr><td align="center">10 x H Buffer</td><td align="right">5 µl</td></tr> | :<tr><td align="center">10 x H Buffer</td><td align="right">5 µl</td></tr> | ||
- | :<tr><td align="center"><i> | + | :<tr><td align="center"><i>''Xba''</i>Ⅰ</td><td align="right">1 µl</td></tr> |
:<tr><td> </td><td align="right">total 50 µl</td></tr> | :<tr><td> </td><td align="right">total 50 µl</td></tr> | ||
:</table></td></tr></table> | :</table></td></tr></table> | ||
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<br> | <br> | ||
:The amount of the purified pUAST-flag vector was 45.0375 ng/µl. | :The amount of the purified pUAST-flag vector was 45.0375 ng/µl. | ||
- | :PCR products for DIAP2 | + | :PCR products for DIAP2 was not successfully recovered from the agarose gel. |
<br> | <br> | ||
</div> | </div> |
Latest revision as of 03:26, 6 October 2011
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8th, August
Member
- Matsunami, Yokoigawa
- To amplify API2-MALT1 cDNA and DIAP2 cDNA, 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
- F primer:GCCGCTCGAGAACATAGTAGAAAACAGCAT
- DIAP2
- F primer:GCTTCTCGAGACGGAGCTGGGCATGGAGCT
- Tm value 69°C
- R primer:GCCGTCTAGATCACGAAAGGAACGTGCGCA
- Tm value 66.4°C
- amplicon size 1514 bp
- F primer:GCTTCTCGAGACGGAGCTGGGCATGGAGCT
- 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 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-MALT1 was 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-MALT1 was 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-MALT1 cDNA by diluting 10 x and 100 x , 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 with phenol-chloroform and then digested with the XhoI for 20 hours at 37°C.
- DIAP2
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 with 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 pUAST-flag vector pUAST-flag vector(500 ng/µl) 10 μl ddH2O 34 µl 10 x H Buffer 5 µl XbaⅠ 1 µl total 50 µl
31th, 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.