Team:KIT-Kyoto/Notebook/LabNote/GFPMLF9
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!align="right"|Language:[[Team:KIT-Kyoto/Notebook/LabNote/GFPMLF9|English]]/[[Team:KIT-Kyoto/Notebook/LabNote/GFPMLF9J|Japanese]] | !align="right"|Language:[[Team:KIT-Kyoto/Notebook/LabNote/GFPMLF9|English]]/[[Team:KIT-Kyoto/Notebook/LabNote/GFPMLF9J|Japanese]] | ||
|} | |} | ||
+ | |||
+ | ==''1st, September''== | ||
+ | <b>Member</b> | ||
+ | <br> | ||
+ | :Nakagawa | ||
+ | <br> | ||
+ | :1.Using [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx|QIAquick Gel Extraction Kit] and extracted DNA of pSB1C3 from the gel. | ||
+ | :2.DNA bands in the agarose gel. | ||
+ | : After extracting DNA,I measured 5µl ,and diluted it for 20 times. | ||
+ | : And I measured its density. | ||
+ | :3.PCR reaction was carried out by using primers designed on August 30th. The reaction conditions are summarized below. | ||
+ | |||
+ | :<table border="0"><tr><td> | ||
+ | :<table border="0" width="150px"> | ||
+ | :<tr><td align=center>PCR reaction</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="250px"> | ||
+ | :<tr><td width="150px" align=center>10 µM Primer F</td><td width="100px" align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 µM Primer R</td><td align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>BBa_E0240</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x PCR Buffer for KOD Plus</td><td align=right>5 µl</td></tr> | ||
+ | :<tr><td align=center>dNTPs</td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>MgSO<sub>4</sub></td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>32 µl</td></tr> | ||
+ | :<tr><td align=center>KOD Plus</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 50 µl</td></tr> | ||
+ | :</table> | ||
+ | :</td><TD></TD><TD></TD><td> | ||
+ | :<table border="0" width="100px"> | ||
+ | :<tr><td align=center>Cycle</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="400px"> | ||
+ | :<tr><td width="100px" align=center>Pre-Denature</td><td width="100px" align=center>95°C</td><td width="100px" align=center>30sec</td><td width="100px"> </td></tr> | ||
+ | :<tr><td align=center>Denature</td><td align=center>95°C</td><td align=center>30sec</td><td align=center rowspan=3>30 Cycle</td></tr> | ||
+ | :<tr><td align=center>Anneling</td><td align=center>48.5°C</td><td align=center>1min</td></tr> | ||
+ | :<tr><td align=center>Extension</td><td align=center>68°C</td><td align=center>1kb/min</td></tr> | ||
+ | :<tr><td align=center>End</td><td align=center>4°C</td><td align=center>keep</td><td width="100px"> </td></tr> | ||
+ | :</table> | ||
+ | :</td></tr> | ||
+ | :</table> | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :2.Image of the agarose gel.<BR> | ||
+ | :<html><body> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/1/17/2011.09.01_%E3%83%99%E3%82%AF%E3%82%BF%E3%83%BC%E3%82%B2%E3%83%AB%E6%8A%BD.JPG" width="250px" height="250px" border="0"> | ||
+ | </body></html> | ||
+ | <br> | ||
+ | :You can see DNA band at around 2kbp. | ||
+ | <br> | ||
+ | :density(ng/µl) | ||
+ | :<table border=1 width="160px"> | ||
+ | :<tr><td width="70px" align=center>1</td><td width="90px" align=right>19.0</td></tr> | ||
+ | :<tr><td align=center>2</td><td align=right>13.0</td></tr> | ||
+ | :<tr><td align=center>3</td><td align=right>19.0</td></tr> | ||
+ | :<tr><td align=center>4</td><td align=right>22.0</td></tr> | ||
+ | :<tr><td align=center>5</td><td align=right>16.0</td></tr> | ||
+ | :<tr><td align=center>ave.</td><td align=right>17.8</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | ==''2nd, September''== | ||
+ | <b>Member</b> | ||
+ | <br> | ||
+ | :Nakagawa | ||
+ | <br> | ||
+ | :Isolate BBa_E0240 by phenol-chloroform treatment,Agarose gel electrophoresis and carried out to detect the PCR products. | ||
+ | :I digested PCR products with the following restriction enzymes (at 37°C for 16 hours). | ||
+ | |||
+ | <table border=1 width="220px"> | ||
+ | <tr><td width="130px" align=center>ddH<sub>2</sub>O</td><td width="90px" align=right>2 µl</td></tr> | ||
+ | <tr><td align=center>BBa_E0240</td><td align=right>50 µl</td></tr> | ||
+ | <tr><td align=center><em>Eco</em>RⅠ</td><td align=right>1 µl</td></tr> | ||
+ | <tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>1 µl</td></tr> | ||
+ | <tr><td align=center>10 x H Buffer</td><td align=right>6 µl</td></tr> | ||
+ | <tr><td align=center> </td><td align=right>total 60 µl</td></tr> | ||
+ | </table> | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :2.Image of the agarose gel.<BR> | ||
+ | :<html><body> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/8/86/2011.09.02_%E4%B8%AD%E5%B7%9D.JPG | ||
+ | " width="250px" height="250px" border="0"> | ||
+ | </body></html> | ||
+ | <br> | ||
+ | :I can see BBa_E0240 band at the correct place.And the density was enough to watch it. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''3rd,September''== | ||
+ | <b>Member</b> | ||
+ | <br> | ||
+ | :Nakagawa | ||
+ | <br> | ||
+ | :Using [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx|QIAquick Gel Extraction Kit] and extracted DNA of pSB1C3 from the gel. | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :<html><body> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/b/bb/2011.09.03_%E4%B8%AD%E5%B7%9D%E3%82%B2%E3%83%AB%E6%8A%BD%E5%87%BA.JPG | ||
+ | " width="250px" height="250px" border="0"> | ||
+ | </body></html> | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''5th,September''== | ||
+ | <b>Member</b> | ||
+ | <br> | ||
+ | :Nakagawa | ||
+ | <br> | ||
+ | :Ligate BBa_E0240.which doesn’t have ATG codons and pSB1C3 | ||
+ | ::I have transformed ''E. coli DH5 alpha'' with it. | ||
+ | ::Before I made BBa_E0240.which doesn’t have ATG codons and pSB1C3. | ||
+ | ::The densities are 19ng/µl and 25ng/µl. | ||
+ | ::DNA samples were digested by the following restriction enzymes at 37 ℃ for 30 min. | ||
+ | |||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>BBa_E0240</td><td width="70px" align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>pSB1C3</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 5 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :After ligate them, I have transformed E. coli DH5 alpha with it. | ||
+ | <BR> | ||
+ | <b>Results</b> | ||
+ | :There aren’t any colonies on the plate. | ||
+ | :However I heared the success probability is very low, so next time I want to be careful about the density. | ||
+ | |||
+ | ==''6th,September''== | ||
+ | <b>Member</b> | ||
+ | <br> | ||
+ | :Yoshimura,Nakagawa | ||
+ | <br> | ||
+ | :1.Ligate BBa_E0240.which doesn’t have ATG codons and pSB1C3 | ||
+ | : DNA samples were digested by the following restriction enzymes at 37 ℃ for 30 min | ||
+ | |||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 5 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :However, I ligated them with this density ratio (bector: insert=1:9) | ||
+ | :After ligate them, I have transformed E. coli DH5 alpha with it. | ||
+ | |||
+ | :2. We attached restriction enzyme site of EcoRⅠand XbaⅠto the Flag-tag dMLF from pUAST Flag-tag dMLF. | ||
+ | :We isolated Flag-tag dMLF from pUAST Flag-tag dMLF. | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :1.There are 4 colonies on the LB plate. | ||
+ | :2.F:AAA<font color="#ff0000">GAATTC</font>AAA<font color="#ff0000">TCTAGA</font>AAAATGGACTACAAGGACGA<br> | ||
+ | : <em>Eco</em>RⅠ <em>Xba</em>Ⅰ<br> | ||
+ | :Tm value:72.14℃ 38bases | ||
+ | |||
+ | :R:AAA<font color="#ff0000">CTGCAG</font>AAA<font color="#ff0000">ACTAGT</font>AAATACCCTACTTCTTCTTGCC<br> | ||
+ | : <em>Pst</em>Ⅰ <em>Spe</em>Ⅰ<br> | ||
+ | :Tm value:72.16℃ 40bases | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''7th.September''== | ||
+ | <b>Member</b> | ||
+ | <br> | ||
+ | :Nakagawa | ||
+ | <br> | ||
+ | :I did pre-culture of yesterday colonies and pSB1C3. | ||
+ | :PCR and restriction enzyme with MLF | ||
+ | |||
+ | :<table border="0"><tr><td> | ||
+ | :<table border="0" width="150px"> | ||
+ | :<tr><td align=center>PCR reaction</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="250px"> | ||
+ | :<tr><td width="150px" align=center>10 µM GFP Primer F</td><td width="100px" align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 µM GFP Primer R</td><td align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>BBa_E0240</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x PCR Buffer for KOD Plus</td><td align=right>5 µl</td></tr> | ||
+ | :<tr><td align=center>dNTPs</td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>MgSO<sub>4</sub></td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>32 µl</td></tr> | ||
+ | :<tr><td align=center>KOD Plus</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 50 µl</td></tr> | ||
+ | :</table> | ||
+ | :</td><TD></TD><TD></TD><td> | ||
+ | :<table border="0" width="100px"> | ||
+ | :<tr><td align=center>Cycle</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="400px"> | ||
+ | :<tr><td width="100px" align=center>Pre-Denature</td><td width="100px" align=center>95°C</td><td width="100px" align=center>30sec</td><td width="100px"> </td></tr> | ||
+ | :<tr><td align=center>Denature</td><td align=center>95°C</td><td align=center>30sec</td><td align=center rowspan=3>30 Cycle</td></tr> | ||
+ | :<tr><td align=center>Anneling</td><td align=center>50°C</td><td align=center>1min</td></tr> | ||
+ | :<tr><td align=center>Extension</td><td align=center>68°C</td><td align=center>1min</td></tr> | ||
+ | :<tr><td align=center>End</td><td align=center>4°C</td><td align=center>keep</td><td width="100px"> </td></tr> | ||
+ | :</table> | ||
+ | :</td></tr> | ||
+ | :</table> | ||
+ | <BR> | ||
+ | |||
+ | :After that, I isolated MLF with restriction enzyme. | ||
+ | :DNA samples were digested by the following restriction enzymes at 37 ℃ for 16 hours. | ||
+ | |||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>ddH<sub>2</sub>O</td><td width="90px" align=right>2 µl</td></tr> | ||
+ | :<tr><td align=center>Flag tag dMLF</td><td align=right>50 µl</td></tr> | ||
+ | :<tr><td align=center><em>Eco</em>RⅠ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x H Buffer</td><td align=right>6 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 60 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | ==''8th,September''== | ||
+ | <b>Member</b> | ||
+ | <br> | ||
+ | :Nakagawa | ||
+ | <br> | ||
+ | :Using [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx|QIAquick Gel Extraction Kit] and extracted DNA of Flag tag dMLF from the gel. | ||
+ | |||
+ | :Isolatioe pSB1C3 by the alkaline-lysis method by phenol-chloroform treatment, DNA was digested with the following restriction enzymes (30 min at 37℃). | ||
+ | |||
+ | :I digested the DNA of pSB1C3 with the following restriction enzymes (at 37°C for 16 hours). | ||
+ | |||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>ddH<sub>2</sub>O</td><td width="90px" align=right>2 µl</td></tr> | ||
+ | :<tr><td align=center>pSB1C3</td><td align=right>50 µl</td></tr> | ||
+ | :<tr><td align=center><em>Eco</em>RⅠ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x H Buffer</td><td align=right>6 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 60 µl</td></tr> | ||
+ | :</table> | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :We cannot see any bands of MLF from the gel. | ||
+ | :So, we are effort to ligate with pSB1C3 and BBa_E0240. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''9th,September''== | ||
+ | <b>Member</b> | ||
+ | <br> | ||
+ | :Nakagawa | ||
+ | <br> | ||
+ | :I planned to give efficiency of the ligation by giving rise to the density of GFP and vector by ethanol precipitating | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :I failed to rise the densities of vector and the DNA of insert. | ||
+ | :We lost DNA In the middle of ethanol precipitation. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''12th,September''== | ||
+ | <b>Members</b> | ||
+ | <br> | ||
+ | :Yoshimura, Nakagawa | ||
+ | <br> | ||
+ | :1.We amplified the Flag-MLF by using primer which was made on September 6th. | ||
+ | :We did PCR reaction with following conditions. | ||
+ | |||
+ | :<table border="0"><tr><td> | ||
+ | :<table border="0" width="150px"> | ||
+ | :<tr><td align=center>PCR reaction(1)</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="250px"> | ||
+ | :<tr><td width="150px" align=center>10 µM Primer F</td><td width="100px" align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 µM Primer R</td><td align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>Template DNA</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x PCR Buffer for KOD Plus</td><td align=right>5 µl</td></tr> | ||
+ | :<tr><td align=center>dNTPs</td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>MgSO<sub>4</sub></td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>32 µl</td></tr> | ||
+ | :<tr><td align=center>KOD Plus</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 50 µl</td></tr> | ||
+ | :</table> | ||
+ | :</td><TD></TD><TD></TD><td> | ||
+ | :<table border="0" width="100px"> | ||
+ | :<tr><td align=center>Cycle</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="400px"> | ||
+ | :<tr><td width="100px" align=center>Pre-Denature</td><td width="100px" align=center>94°C</td><td width="100px" align=center>2min</td><td width="100px"> </td></tr> | ||
+ | :<tr><td align=center>Denature</td><td align=center>94°C</td><td align=center>15sec</td><td align=center rowspan=3>35 Cycle</td></tr> | ||
+ | :<tr><td align=center>Anneling</td><td align=center>55°C</td><td align=center>30sec</td></tr> | ||
+ | :<tr><td align=center>Extension</td><td align=center>68°C</td><td align=center>1min 20sec</td></tr> | ||
+ | :<tr><td align=center>End</td><td align=center>4°C</td><td align=center>keep</td><td width="100px"> </td></tr> | ||
+ | :</table> | ||
+ | :</td></tr> | ||
+ | :</table> | ||
+ | <br> | ||
+ | :<table border="0"><tr><td> | ||
+ | :<table border="0" width="150px"> | ||
+ | :<tr><td align=center>PCR reaction(2)</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="250px"> | ||
+ | :<tr><td width="150px" align=center>10 µM Primer F</td><td width="100px" align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 µM Primer R</td><td align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>Template DNA</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x PCR Buffer for KOD Plus</td><td align=right>5 µl</td></tr> | ||
+ | :<tr><td align=center>dNTPs</td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>MgSO<sub>4</sub></td><td align=right>2 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>34 µl</td></tr> | ||
+ | :<tr><td align=center>KOD Plus</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 50 µl</td></tr> | ||
+ | :</table> | ||
+ | :</td><TD></TD><TD></TD><td> | ||
+ | :<table border="0" width="100px"> | ||
+ | :<tr><td align=center>Cycle</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="400px"> | ||
+ | :<tr><td width="100px" align=center>Pre-Denature</td><td width="100px" align=center>94°C</td><td width="100px" align=center>2min</td><td width="100px"> </td></tr> | ||
+ | :<tr><td align=center>Denature</td><td align=center>94°C</td><td align=center>15sec</td><td align=center rowspan=3>35 Cycle</td></tr> | ||
+ | :<tr><td align=center>Anneling</td><td align=center>55°C</td><td align=center>30sec</td></tr> | ||
+ | :<tr><td align=center>Extension</td><td align=center>68°C</td><td align=center>1min 20sec</td></tr> | ||
+ | :<tr><td align=center>End</td><td align=center>4°C</td><td align=center>keep</td><td width="100px"> </td></tr> | ||
+ | :</table> | ||
+ | :</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :We collected each sample and kept them in -20°C. | ||
+ | :2.Pre-culture of E.coli(DH5α)which contains pSB1C3. | ||
+ | : I tried doing PCR reaction with following conditions with BBa_E0240 again. | ||
+ | |||
+ | :<table border="0"><tr><td> | ||
+ | :<table border="0" width="150px"> | ||
+ | :<tr><td align=center>PCR reaction</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="250px"> | ||
+ | :<tr><td width="150px" align=center>10 µM Primer F</td><td width="100px" align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 µM Primer R</td><td align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>GFP</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x PCR Buffer for KOD Plus</td><td align=right>5 µl</td></tr> | ||
+ | :<tr><td align=center>dNTPs</td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>MgSO<sub>4</sub></td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>32 µl</td></tr> | ||
+ | :<tr><td align=center>KOD Plus</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 50 µl</td></tr> | ||
+ | :</table> | ||
+ | :</td><TD></TD><TD></TD><td> | ||
+ | :<table border="0" width="100px"> | ||
+ | :<tr><td align=center>Cycle</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="400px"> | ||
+ | :<tr><td width="100px" align=center>Pre-Denature</td><td width="100px" align=center>95°C</td><td width="100px" align=center>30sec</td><td width="100px"> </td></tr> | ||
+ | :<tr><td align=center>Denature</td><td align=center>95°C</td><td align=center>30sec</td><td align=center rowspan=3>30 Cycle</td></tr> | ||
+ | :<tr><td align=center>Anneling</td><td align=center>48.5°C</td><td align=center>1min</td></tr> | ||
+ | :<tr><td align=center>Extension</td><td align=center>68°C</td><td align=center>1kb/min</td></tr> | ||
+ | :<tr><td align=center>End</td><td align=center>4°C</td><td align=center>keep</td><td width="100px"> </td></tr> | ||
+ | :</table> | ||
+ | :</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | : I isolated pSB1C3 by phenol-chloroform treatment .I digested DNA with the following restriction enzymes (30 minutes at 37°C). | ||
+ | |||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>ddH<sub>2</sub>O</td><td width="90px" align=right>2 µl</td></tr> | ||
+ | :<tr><td align=center>BBa_E0240</td><td align=right>50 µl</td></tr> | ||
+ | :<tr><td align=center><em>Eco</em>RⅠ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x H Buffer</td><td align=right>6 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 60 µl</td></tr> | ||
+ | :</table> | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :The E.coli (DH5α) which contains pSB1C3 was increased, but there are some colonies which doesn’t correct color. | ||
+ | :Possibly deterioration may begin in plate in itself. | ||
+ | :The DNA of PCR reaction increased next day. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''13th,September''== | ||
+ | <b>Member</b> | ||
+ | <br> | ||
+ | :Yoshimura, Nakagawa | ||
+ | <br> | ||
+ | :1.We carried out agarose gel electrophoresis to detect the PCR products. | ||
+ | :2.We amplified Flag-tag dMLF by using the primer which I manufactured on 6th September. | ||
+ | : Restriction enzyme processing. | ||
+ | : This is because after examining a sequence of Flag-tag dMLF, a restriction enzyme site of PstI and XbaI was seen. | ||
+ | : So, I examined whether PCR product of Flag-tag dMLF is cut by PstI and XbaI. | ||
+ | |||
+ | (1)<br> | ||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>MilliQ</td><td width="90px" align=right>6.5 µl</td></tr> | ||
+ | :<tr><td align=center>Flag-tag dMLF</td><td align=right>20 µl</td></tr> | ||
+ | :<tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 x H Buffer</td><td align=right>3 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 30 µl</td></tr> | ||
+ | :</table> | ||
+ | <br> | ||
+ | |||
+ | (2)<br> | ||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>MilliQ</td><td width="90px" align=right>6.5 µl</td></tr> | ||
+ | :<tr><td align=center>Flag-tag dMLF</td><td align=right>20 µl</td></tr> | ||
+ | :<tr><td align=center><em>Xba</em>Ⅰ</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 x M Buffer</td><td align=right>3 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 30 µl</td></tr> | ||
+ | :</table> | ||
+ | <br> | ||
+ | |||
+ | (3)<br> | ||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>MilliQ</td><td width="90px" align=right>6 µl</td></tr> | ||
+ | :<tr><td align=center>Flag-tag dMLF</td><td align=right>20 µl</td></tr> | ||
+ | :<tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center><em>Xba</em>Ⅰ</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 x M Buffer</td><td align=right>3 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 30 µl</td></tr> | ||
+ | :</table> | ||
+ | :After incubate it in 37°C for 50 minutes, I performed electrophoresis with agarose gel. | ||
+ | :Photograph after the electrophoresis. | ||
+ | |||
+ | :3.To amplify Flag-tag dMLF cDNA, PCR reactions were carried out under the following conditions. | ||
+ | |||
+ | :<table border="0"><tr><td> | ||
+ | :<table border="0" width="150px"> | ||
+ | :<tr><td align=center>PCR reaction</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="250px"> | ||
+ | :<tr><td width="150px" align=center>10 µM Primer F</td><td width="100px" align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 µM Primer R</td><td align=right>1.5 µl</td></tr> | ||
+ | :<tr><td align=center>Template DNA</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x PCR Buffer for KOD Plus</td><td align=right>5 µl</td></tr> | ||
+ | :<tr><td align=center>dNTPs</td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>MgSO<sub>4</sub></td><td align=right>4 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>32 µl</td></tr> | ||
+ | :<tr><td align=center>KOD Plus</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 50 µl</td></tr> | ||
+ | :</table> | ||
+ | :</td><TD></TD><TD></TD><td> | ||
+ | :<table border="0" width="100px"> | ||
+ | :<tr><td align=center>Cycle</td></tr> | ||
+ | :</table> | ||
+ | :<table border=1 width="400px"> | ||
+ | :<tr><td width="100px" align=center>Pre-Denature</td><td width="100px" align=center>94°C</td><td width="100px" align=center>2min</td><td width="100px"> </td></tr> | ||
+ | :<tr><td align=center>Denature</td><td align=center>94°C</td><td align=center>15sec</td><td align=center rowspan=3>35 Cycle</td></tr> | ||
+ | :<tr><td align=center>Anneling</td><td align=center>55°C</td><td align=center>30sec</td></tr> | ||
+ | :<tr><td align=center>Extension</td><td align=center>68°C</td><td align=center>1min 20sec</td></tr> | ||
+ | :<tr><td align=center>End</td><td align=center>4°C</td><td align=center>keep</td><td width="100px"> </td></tr> | ||
+ | :</table> | ||
+ | :</td></tr> | ||
+ | :</table> | ||
+ | :We collected each sample and kept them in -20°C. | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :1.Image of the agarose gel. | ||
+ | :<html><body> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/9/99/2011.09.13_%E4%B8%AD%E5%B7%9D.JPG | ||
+ | " width="240px" height="280px" border="0"> | ||
+ | </body></html> | ||
+ | <br> | ||
+ | :2.Images of the agarose gel. | ||
+ | : | ||
+ | :<html><body> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/8/8a/2011.09.13MLF%E3%83%81%E3%82%A7%E3%83%83%E3%82%AFPst.Xba.JPG | ||
+ | " width="240px" height="280px" border="0"> | ||
+ | <BR> | ||
+ | :<IMG src="https://static.igem.org/mediawiki/2011/d/dc/2011.09.13MLF%E3%83%81%E3%82%A7%E3%83%83%E3%82%AFXba.JPG | ||
+ | " width="240px" height="280px" border="0"> | ||
+ | </body></html> | ||
+ | :Flag-tag dMLF aren’t cut by restriction enzyme of PstI and XbaI. | ||
+ | :A marker did not enough to drift. | ||
+ | <br> | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''14th,September''== | ||
+ | <b>Members</b> | ||
+ | <br> | ||
+ | :Yoshimura | ||
+ | <br> | ||
+ | :1.We carried out agarose gel electrophoresis to detect the PCR products. | ||
+ | :2.I extracted GFP, DNA of the vector from gel using [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx|QIAquick Gel Extraction Kit]. | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | 1.Image of the agarose gel. | ||
+ | <br> | ||
+ | :<html><body> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/5/53/2011.09.14MLF-PCR%E3%83%81%E3%82%A7%E3%83%83%E3%82%AF.JPG | ||
+ | " width="240px" height="280px" border="0"> | ||
+ | </body></html> | ||
+ | <br> | ||
+ | :After doubling the density of gel, a marker did not drift. | ||
+ | :I will decide to perform it with 2% of agarose gel about the electrophoresis of Flag-tag MLF in future. | ||
+ | 2.I measured the density with an absorbance meter afterwards. | ||
+ | |||
+ | :GFP | ||
+ | :<table border=1 width="160px"> | ||
+ | :<tr><td width="70px" align=center>1</td><td width="90px" align=right>0.158</td></tr> | ||
+ | :<tr><td align=center>2</td><td align=right>0.147</td></tr> | ||
+ | :<tr><td align=center>3</td><td align=right>0.160</td></tr> | ||
+ | :<tr><td align=center>4</td><td align=right>0.159</td></tr> | ||
+ | :<tr><td align=center>5</td><td align=right>0.158</td></tr> | ||
+ | :<tr><td align=center>ave.</td><td align=right>0.156</td></tr> | ||
+ | :</table> | ||
+ | :pSB1C3<BR> | ||
+ | :<table border=1 width="160px"> | ||
+ | :<tr><td width="70px" align=center>1</td><td width="90px" align=right>0.029</td></tr> | ||
+ | :<tr><td align=center>2</td><td align=right>0.021</td></tr> | ||
+ | :<tr><td align=center>3</td><td align=right>0.028</td></tr> | ||
+ | :<tr><td align=center>4</td><td align=right>0.022</td></tr> | ||
+ | :<tr><td align=center>5</td><td align=right>0.025</td></tr> | ||
+ | :<tr><td align=center>ave.</td><td align=right>0.025</td></tr> | ||
+ | :</table> | ||
+ | <br> | ||
+ | :GFP<BR> | ||
+ | :<HTML><BODY> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/3/3d/2011.09.14_%E4%B8%AD%E5%B7%9D.JPG | ||
+ | " width="240px" height="280px" border="0"> | ||
+ | </BODY></HTML> | ||
+ | :pSB1C3 | ||
+ | :<HTML><BODY> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/3/3a/2011.09.26_%E3%83%99%E3%82%AF%E3%82%BF%E3%83%BC%E3%82%B2%E3%83%AB%E6%8A%BD%E5%87%BA%282%29.JPG | ||
+ | " width="240px" height="280px" border="0"> | ||
+ | </BODY></HTML> | ||
+ | <br> | ||
+ | :The BBa_E0240 succeeded in the extraction from gel and recorded 156ng/µl by the measurement with the absorbance meter and the pSB1C3 became 25ng/µl. | ||
+ | :Therefore I decided to begin an experiment of the ligation again from the next day. | ||
+ | |||
+ | ==''17th,September''== | ||
+ | <b>Members</b> | ||
+ | <br> | ||
+ | :Nakagawa | ||
+ | <br> | ||
+ | :1.Ligate with BBa_E0240 and pSB1C3 | ||
+ | :2.Pre-culture and the alkaline-lysis method of pSB1C3 | ||
+ | <br> | ||
+ | :I adjusted reaction liquid according to the following composition. | ||
+ | |||
+ | pSB1C3:GFP=1:2<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>0.3 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>2.0µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.7 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 7 µl</td></tr> | ||
+ | :</table> | ||
+ | pSB1C3:GFP=1:5<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>2.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 7 µl</td></tr> | ||
+ | :</table> | ||
+ | pSB1C3:GFP=1:10<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.3 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.7 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 7 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :I incubated them in 16°C for 30 min. | ||
+ | :After that, I transformed them, and I poured them into 300 µl of SOC medium and add them on the plate after culture for 30 minutes. | ||
+ | |||
+ | :I thought that I tried to pick at only a red colony as a point to keep in mind of this time and lowered the possibility of contaminating it. | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :Here are many colonies on the LB medium. | ||
+ | :Possibly contaminating is thought for example an antibiotic does not work. | ||
+ | :The pSB1C3 was not able to be refined again. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''19th,September''== | ||
+ | <b>Members</b> | ||
+ | <br> | ||
+ | :Yoshimura Nakagawa | ||
+ | <br> | ||
+ | :1.We transformed and performed restriction enzyme processing | ||
+ | :2.Density check of BBa_E0240 and pSB1C3 | ||
+ | :3.Pre-culture with yesterday colony and pSB1C3 to the new LB plate | ||
+ | <br> | ||
+ | :I digested with the ''Xho''I according to the following composition. | ||
+ | |||
+ | :(1)<br> | ||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>MilliQ</td><td width="90px" align=right>6.5 µl</td></tr> | ||
+ | :<tr><td align=center>Flag-tag dMLF</td><td align=right>20 µl</td></tr> | ||
+ | :<tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 x H Buffer</td><td align=right>3 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 30 µl</td></tr> | ||
+ | :</table> | ||
+ | <br> | ||
+ | |||
+ | :(2)<br> | ||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>MilliQ</td><td width="90px" align=right>6.5 µl</td></tr> | ||
+ | :<tr><td align=center>Flag-tag dMLF</td><td align=right>20 µl</td></tr> | ||
+ | :<tr><td align=center><em>Xba</em>Ⅰ</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 x M Buffer</td><td align=right>3 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 30 µl</td></tr> | ||
+ | :</table> | ||
+ | <br> | ||
+ | |||
+ | :(3)<br> | ||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>MilliQ</td><td width="90px" align=right>6 µl</td></tr> | ||
+ | :<tr><td align=center>Flag-tag dMLF</td><td align=right>20 µl</td></tr> | ||
+ | :<tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center><em>Xba</em>Ⅰ</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>10 x M Buffer</td><td align=right>3 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 30 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :After incubate it in 37 ゜ C for 18 hours, I performed agarose gel electrophoresis. | ||
+ | <br> | ||
+ | :Checking the amount of the purified GFP, | ||
+ | :<table border=1 width="160px"> | ||
+ | :<tr><td width="70px" align=center>1 x </td><td width="90px" align=right>1µl</td></tr> | ||
+ | :<tr><td align=center>2 x </td><td align=right>1µl</td></tr> | ||
+ | :<tr><td align=center>4 x </td><td align=right>1µl</td></tr> | ||
+ | :<tr><td align=center>8 x </td><td align=right>1µl</td></tr> | ||
+ | :</table><BR> | ||
+ | :Image of agarose gel after DNA fragment isolation for Checking the amount of the purified GFP. | ||
+ | <br> | ||
+ | :<HTML><BODY> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/5/52/2011.09.19_GFP%E6%BF%83%E5%BA%A6%E3%83%81%E3%82%A7%E3%83%83%E3%82%AF.JPG" width="250px" height="250px" border="0"> | ||
+ | </BODY></HTML> | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :The increase of BBa_E0240 was good, and upbringing of the big colony was seen. | ||
+ | :pSB1C3 was not BBa_E0240 too, but was all right because some number grew. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''24th,September''== | ||
+ | <b>Members</b> | ||
+ | <br> | ||
+ | :Yoshimura Nakagawa | ||
+ | <br> | ||
+ | :1.alkaline-lysis method, phenol-chloroform treatment | ||
+ | :2.restriction enzymes, extraction with pSB1C3 | ||
+ | :3.restriction enzymes processing with BBa_E0240 | ||
+ | |||
+ | :Yield rose markedly when I exchanged isopropanol. | ||
+ | :After alkaline-lysis method, phenol-chloroform treatment with pSB1C3,restriction enzymes processing with BBa_E0240 and pSB1C3 | ||
+ | :According to a list shown below, I performed restriction enzyme processing at 37 overnight. | ||
+ | |||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>ddH<sub>2</sub>O</td><td width="90px" align=right>2 µl</td></tr> | ||
+ | :<tr><td align=center>BBa_E0240</td><td align=right>50 µl</td></tr> | ||
+ | :<tr><td align=center><em>Eco</em>RⅠ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x H Buffer</td><td align=right>6 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 60 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :The restriction enzyme-digested pSB1C3 were extracted from the agarose gel by QIAquick Gel Extraction Kit. | ||
+ | :Photograph after the extraction. | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | |||
+ | <br> | ||
+ | :Image of agarose gel after DNA fragment isolation. | ||
+ | :<html><body> | ||
+ | <IMG src="https://static.igem.org/mediawiki/2011/1/1b/2011.09.24_%E3%82%B2%E3%83%AB%E6%8A%BD%E5%87%BA.JPG" width="250px" height="250px" border="0"> | ||
+ | </body></html> | ||
+ | <br> | ||
+ | :A band was seen to about 2kb. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''26th,September''== | ||
+ | <b>Members</b> | ||
+ | <br> | ||
+ | :Yoshimura Nakagawa | ||
+ | <br> | ||
+ | :1.Ligation | ||
+ | :2.restriction enzyme handling of liquid pSB1C3 | ||
+ | |||
+ | :restriction enzymes processing with pSB1C3 | ||
+ | :According to a list shown below, I performed restriction enzyme processing at 37 for 30 minutes. | ||
+ | |||
+ | :<table border=1 width="220px"> | ||
+ | :<tr><td width="130px" align=center>ddH<sub>2</sub>O</td><td width="90px" align=right>2 µl</td></tr> | ||
+ | :<tr><td align=center>BBa_E0240</td><td align=right>50 µl</td></tr> | ||
+ | :<tr><td align=center><em>Eco</em>RⅠ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center><em>Pst</em>Ⅰ</td><td align=right>1 µl</td></tr> | ||
+ | :<tr><td align=center>10 x H Buffer</td><td align=right>6 µl</td></tr> | ||
+ | :<tr><td align=center> </td><td align=right>total 60 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :Next ligate with following list. | ||
+ | |||
+ | :At first I dilute the density of vector to become 10 pg/µl. | ||
+ | :And I dilute it as I calculate one and MLF 60 ng/µl of GFP 70 ng/µl to be able to go by combination below and am composed follows at 1 µl. | ||
+ | :I combined it in the ratio of follows afterwards. | ||
+ | |||
+ | pSB1C3:GFP=1:10<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 6.0 µl</td></tr> | ||
+ | :</table> | ||
+ | pSB1C3:GFP=1:20<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total6.0µl</td></tr> | ||
+ | :</table> | ||
+ | pSB1C3:GFP=1:40<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 6 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :I incubated them in 16°C for 30 min. | ||
+ | :After that, I transformed them, and I poured them into 300 µl of SOC medium and add them on the plate after culture for 30 minutes. | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :There are no colonies. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''29th,September''== | ||
+ | <b>Members</b> | ||
+ | <br> | ||
+ | :Yoshimura, Nakagawa | ||
+ | <br> | ||
+ | :At first I dilute the density of vector to become 10 pg/µl. | ||
+ | :And I dilute it as I calculate one and MLF 60 ng/µl of GFP 70 ng/µl to be able to go by combination below and am composed follows at 1 µl. | ||
+ | :I combined it in the ratio of follows afterwards. | ||
+ | |||
+ | pSB1C3:GFP=1:10<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 6.0 µl</td></tr> | ||
+ | :</table> | ||
+ | pSB1C3:GFP=1:20<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total6.0µl</td></tr> | ||
+ | :</table> | ||
+ | pSB1C3:GFP=1:40<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 6 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :I incubated them in 16°C for 30 min. | ||
+ | :After that, I transformed them, and I poured them into 300 µl of SOC medium and add them on the plate after culture for 30 minutes. | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :There are some colonies on the plate. | ||
+ | :However there aren’t any MLF colonies. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | |||
+ | ==''30th,September''== | ||
+ | <b>Members</b> | ||
+ | <br> | ||
+ | :Yoshimura, Nakagawa | ||
+ | <br> | ||
+ | :At first I dilute the density of vector to become 10 pg/µl | ||
+ | :And I dilute it as I calculate one and MLF 60 ng/µl of GFP 70 ng/µl to be able to go by combination below and am composed follows at 1 µl | ||
+ | :I combined it in the ratio of follows afterwards | ||
+ | |||
+ | pSB1C3:GFP=1:10<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 6.0 µl</td></tr> | ||
+ | :</table> | ||
+ | pSB1C3:GFP=1:20<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total6.0µl</td></tr> | ||
+ | :</table> | ||
+ | pSB1C3:GFP=1:40<BR> | ||
+ | :<table border=1 width="200px"> | ||
+ | :<tr><td width="130px" align=center>insert</td><td width="70px" align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>vector</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td align=center>10 x Buffer</td><td align=right>2.5 µl</td></tr> | ||
+ | :<tr><td align=center>F4 ligase</td><td align=right>0.5 µl</td></tr> | ||
+ | :<tr><td align=center>ddH<sub>2</sub>O</td><td align=right>1.0 µl</td></tr> | ||
+ | :<tr><td> </td><td align=right>total 6 µl</td></tr> | ||
+ | :</table> | ||
+ | |||
+ | :I incubated them in 16°C for 30 min. | ||
+ | :After that, I transformed them, and I poured them into 300 µl of SOC medium and add them on the plate after culture for 30 minutes. | ||
+ | :After that We did alkaline-lysis method restriction and enzymes processing with ligation products. | ||
+ | <br> | ||
+ | <b>Results</b> | ||
+ | :After all MLF did not exist even if there was the BBa_E0240 in ligation products. | ||
+ | :And the first turn of parts was completed today. | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | <br> | ||
+ | |||
+ | |||
+ | |||
+ | |||
+ | |||
</div> | </div> |
Latest revision as of 03:45, 6 October 2011
Home | Team | Project | Parts | Notebook | Safety | Human Practice | Attributions |
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Home > Notebook > Lab Note > September | Language:English/Japanese |
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1st, September
Member
- Nakagawa
- 1.Using [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx|QIAquick Gel Extraction Kit] and extracted DNA of pSB1C3 from the gel.
- 2.DNA bands in the agarose gel.
- After extracting DNA,I measured 5µl ,and diluted it for 20 times.
- And I measured its density.
- 3.PCR reaction was carried out by using primers designed on August 30th. The reaction conditions are summarized below.
PCR reaction 10 µM Primer F 1.5 µl 10 µM Primer R 1.5 µl BBa_E0240 1 µl 10 x PCR Buffer for KOD Plus 5 µl dNTPs 4 µl MgSO4 4 µl ddH2O 32 µl KOD Plus 1 µl total 50 µl Cycle Pre-Denature 95°C 30sec Denature 95°C 30sec 30 Cycle Anneling 48.5°C 1min Extension 68°C 1kb/min End 4°C keep
Results
- 2.Image of the agarose gel.
- You can see DNA band at around 2kbp.
- density(ng/µl)
1 19.0 2 13.0 3 19.0 4 22.0 5 16.0 ave. 17.8
2nd, September
Member
- Nakagawa
- Isolate BBa_E0240 by phenol-chloroform treatment,Agarose gel electrophoresis and carried out to detect the PCR products.
- I digested PCR products with the following restriction enzymes (at 37°C for 16 hours).
ddH2O | 2 µl |
BBa_E0240 | 50 µl |
EcoRⅠ | 1 µl |
PstⅠ | 1 µl |
10 x H Buffer | 6 µl |
total 60 µl |
Results
- 2.Image of the agarose gel.
- I can see BBa_E0240 band at the correct place.And the density was enough to watch it.
3rd,September
Member
- Nakagawa
- Using [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx|QIAquick Gel Extraction Kit] and extracted DNA of pSB1C3 from the gel.
Results
5th,September
Member
- Nakagawa
- Ligate BBa_E0240.which doesn’t have ATG codons and pSB1C3
- I have transformed E. coli DH5 alpha with it.
- Before I made BBa_E0240.which doesn’t have ATG codons and pSB1C3.
- The densities are 19ng/µl and 25ng/µl.
- DNA samples were digested by the following restriction enzymes at 37 ℃ for 30 min.
BBa_E0240 0.5 µl pSB1C3 0.5 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total 5 µl
- After ligate them, I have transformed E. coli DH5 alpha with it.
Results
- There aren’t any colonies on the plate.
- However I heared the success probability is very low, so next time I want to be careful about the density.
6th,September
Member
- Yoshimura,Nakagawa
- 1.Ligate BBa_E0240.which doesn’t have ATG codons and pSB1C3
- DNA samples were digested by the following restriction enzymes at 37 ℃ for 30 min
insert 0.5 µl vector 0.5 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total 5 µl
- However, I ligated them with this density ratio (bector: insert=1:9)
- After ligate them, I have transformed E. coli DH5 alpha with it.
- 2. We attached restriction enzyme site of EcoRⅠand XbaⅠto the Flag-tag dMLF from pUAST Flag-tag dMLF.
- We isolated Flag-tag dMLF from pUAST Flag-tag dMLF.
Results
- 1.There are 4 colonies on the LB plate.
- 2.F:AAAGAATTCAAATCTAGAAAAATGGACTACAAGGACGA
- EcoRⅠ XbaⅠ
- Tm value:72.14℃ 38bases
- R:AAACTGCAGAAAACTAGTAAATACCCTACTTCTTCTTGCC
- PstⅠ SpeⅠ
- Tm value:72.16℃ 40bases
7th.September
Member
- Nakagawa
- I did pre-culture of yesterday colonies and pSB1C3.
- PCR and restriction enzyme with MLF
PCR reaction 10 µM GFP Primer F 1.5 µl 10 µM GFP Primer R 1.5 µl BBa_E0240 1 µl 10 x PCR Buffer for KOD Plus 5 µl dNTPs 4 µl MgSO4 4 µl ddH2O 32 µl KOD Plus 1 µl total 50 µl Cycle Pre-Denature 95°C 30sec Denature 95°C 30sec 30 Cycle Anneling 50°C 1min Extension 68°C 1min End 4°C keep
- After that, I isolated MLF with restriction enzyme.
- DNA samples were digested by the following restriction enzymes at 37 ℃ for 16 hours.
ddH2O 2 µl Flag tag dMLF 50 µl EcoRⅠ 1 µl PstⅠ 1 µl 10 x H Buffer 6 µl total 60 µl
8th,September
Member
- Nakagawa
- Using [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx|QIAquick Gel Extraction Kit] and extracted DNA of Flag tag dMLF from the gel.
- Isolatioe pSB1C3 by the alkaline-lysis method by phenol-chloroform treatment, DNA was digested with the following restriction enzymes (30 min at 37℃).
- I digested the DNA of pSB1C3 with the following restriction enzymes (at 37°C for 16 hours).
ddH2O 2 µl pSB1C3 50 µl EcoRⅠ 1 µl PstⅠ 1 µl 10 x H Buffer 6 µl total 60 µl
Results
- We cannot see any bands of MLF from the gel.
- So, we are effort to ligate with pSB1C3 and BBa_E0240.
9th,September
Member
- Nakagawa
- I planned to give efficiency of the ligation by giving rise to the density of GFP and vector by ethanol precipitating
Results
- I failed to rise the densities of vector and the DNA of insert.
- We lost DNA In the middle of ethanol precipitation.
12th,September
Members
- Yoshimura, Nakagawa
- 1.We amplified the Flag-MLF by using primer which was made on September 6th.
- We did PCR reaction with following conditions.
PCR reaction(1) 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 4 µl MgSO4 4 µl ddH2O 32 µl KOD Plus 1 µl total 50 µl Cycle Pre-Denature 94°C 2min Denature 94°C 15sec 35 Cycle Anneling 55°C 30sec Extension 68°C 1min 20sec End 4°C keep
PCR reaction(2) 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 4 µl MgSO4 2 µl ddH2O 34 µl KOD Plus 1 µl total 50 µl Cycle Pre-Denature 94°C 2min Denature 94°C 15sec 35 Cycle Anneling 55°C 30sec Extension 68°C 1min 20sec End 4°C keep
- We collected each sample and kept them in -20°C.
- 2.Pre-culture of E.coli(DH5α)which contains pSB1C3.
- I tried doing PCR reaction with following conditions with BBa_E0240 again.
PCR reaction 10 µM Primer F 1.5 µl 10 µM Primer R 1.5 µl GFP 1 µl 10 x PCR Buffer for KOD Plus 5 µl dNTPs 4 µl MgSO4 4 µl ddH2O 32 µl KOD Plus 1 µl total 50 µl Cycle Pre-Denature 95°C 30sec Denature 95°C 30sec 30 Cycle Anneling 48.5°C 1min Extension 68°C 1kb/min End 4°C keep
- I isolated pSB1C3 by phenol-chloroform treatment .I digested DNA with the following restriction enzymes (30 minutes at 37°C).
ddH2O 2 µl BBa_E0240 50 µl EcoRⅠ 1 µl PstⅠ 1 µl 10 x H Buffer 6 µl total 60 µl
Results
- The E.coli (DH5α) which contains pSB1C3 was increased, but there are some colonies which doesn’t correct color.
- Possibly deterioration may begin in plate in itself.
- The DNA of PCR reaction increased next day.
13th,September
Member
- Yoshimura, Nakagawa
- 1.We carried out agarose gel electrophoresis to detect the PCR products.
- 2.We amplified Flag-tag dMLF by using the primer which I manufactured on 6th September.
- Restriction enzyme processing.
- This is because after examining a sequence of Flag-tag dMLF, a restriction enzyme site of PstI and XbaI was seen.
- So, I examined whether PCR product of Flag-tag dMLF is cut by PstI and XbaI.
(1)
MilliQ 6.5 µl Flag-tag dMLF 20 µl PstⅠ 0.5 µl 10 x H Buffer 3 µl total 30 µl
(2)
MilliQ 6.5 µl Flag-tag dMLF 20 µl XbaⅠ 0.5 µl 10 x M Buffer 3 µl total 30 µl
(3)
MilliQ 6 µl Flag-tag dMLF 20 µl PstⅠ 0.5 µl XbaⅠ 0.5 µl 10 x M Buffer 3 µl total 30 µl - After incubate it in 37°C for 50 minutes, I performed electrophoresis with agarose gel.
- Photograph after the electrophoresis.
- 3.To amplify Flag-tag dMLF cDNA, PCR reactions were carried out under the following conditions.
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 4 µl MgSO4 4 µl ddH2O 32 µl KOD Plus 1 µl total 50 µl Cycle Pre-Denature 94°C 2min Denature 94°C 15sec 35 Cycle Anneling 55°C 30sec Extension 68°C 1min 20sec End 4°C keep - We collected each sample and kept them in -20°C.
Results
- 1.Image of the agarose gel.
- 2.Images of the agarose gel.
-
: - Flag-tag dMLF aren’t cut by restriction enzyme of PstI and XbaI.
- A marker did not enough to drift.
14th,September
Members
- Yoshimura
- 1.We carried out agarose gel electrophoresis to detect the PCR products.
- 2.I extracted GFP, DNA of the vector from gel using [http://www.qiagen.com/products/dnacleanup/gelpcrsicleanupsystems/qiaquickgelextractionkit.aspx|QIAquick Gel Extraction Kit].
Results
1.Image of the agarose gel.
- After doubling the density of gel, a marker did not drift.
- I will decide to perform it with 2% of agarose gel about the electrophoresis of Flag-tag MLF in future.
2.I measured the density with an absorbance meter afterwards.
- GFP
1 0.158 2 0.147 3 0.160 4 0.159 5 0.158 ave. 0.156 - pSB1C3
1 0.029 2 0.021 3 0.028 4 0.022 5 0.025 ave. 0.025
- GFP
- pSB1C3
- The BBa_E0240 succeeded in the extraction from gel and recorded 156ng/µl by the measurement with the absorbance meter and the pSB1C3 became 25ng/µl.
- Therefore I decided to begin an experiment of the ligation again from the next day.
17th,September
Members
- Nakagawa
- 1.Ligate with BBa_E0240 and pSB1C3
- 2.Pre-culture and the alkaline-lysis method of pSB1C3
- I adjusted reaction liquid according to the following composition.
pSB1C3:GFP=1:2
insert 0.3 µl vector 2.0µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.7 µl total 7 µl
pSB1C3:GFP=1:5
insert 1.0 µl vector 1.0 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 2.0 µl total 7 µl
pSB1C3:GFP=1:10
insert 1.3 µl vector 1.0 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.7 µl total 7 µl
- I incubated them in 16°C for 30 min.
- After that, I transformed them, and I poured them into 300 µl of SOC medium and add them on the plate after culture for 30 minutes.
- I thought that I tried to pick at only a red colony as a point to keep in mind of this time and lowered the possibility of contaminating it.
Results
- Here are many colonies on the LB medium.
- Possibly contaminating is thought for example an antibiotic does not work.
- The pSB1C3 was not able to be refined again.
19th,September
Members
- Yoshimura Nakagawa
- 1.We transformed and performed restriction enzyme processing
- 2.Density check of BBa_E0240 and pSB1C3
- 3.Pre-culture with yesterday colony and pSB1C3 to the new LB plate
- I digested with the XhoI according to the following composition.
- (1)
MilliQ 6.5 µl Flag-tag dMLF 20 µl PstⅠ 0.5 µl 10 x H Buffer 3 µl total 30 µl
- (2)
MilliQ 6.5 µl Flag-tag dMLF 20 µl XbaⅠ 0.5 µl 10 x M Buffer 3 µl total 30 µl
- (3)
MilliQ 6 µl Flag-tag dMLF 20 µl PstⅠ 0.5 µl XbaⅠ 0.5 µl 10 x M Buffer 3 µl total 30 µl
- After incubate it in 37 ゜ C for 18 hours, I performed agarose gel electrophoresis.
- Checking the amount of the purified GFP,
1 x 1µl 2 x 1µl 4 x 1µl 8 x 1µl
- Image of agarose gel after DNA fragment isolation for Checking the amount of the purified GFP.
Results
- The increase of BBa_E0240 was good, and upbringing of the big colony was seen.
- pSB1C3 was not BBa_E0240 too, but was all right because some number grew.
24th,September
Members
- Yoshimura Nakagawa
- 1.alkaline-lysis method, phenol-chloroform treatment
- 2.restriction enzymes, extraction with pSB1C3
- 3.restriction enzymes processing with BBa_E0240
- Yield rose markedly when I exchanged isopropanol.
- After alkaline-lysis method, phenol-chloroform treatment with pSB1C3,restriction enzymes processing with BBa_E0240 and pSB1C3
- According to a list shown below, I performed restriction enzyme processing at 37 overnight.
ddH2O 2 µl BBa_E0240 50 µl EcoRⅠ 1 µl PstⅠ 1 µl 10 x H Buffer 6 µl total 60 µl
- The restriction enzyme-digested pSB1C3 were extracted from the agarose gel by QIAquick Gel Extraction Kit.
- Photograph after the extraction.
Results
- Image of agarose gel after DNA fragment isolation.
- A band was seen to about 2kb.
26th,September
Members
- Yoshimura Nakagawa
- 1.Ligation
- 2.restriction enzyme handling of liquid pSB1C3
- restriction enzymes processing with pSB1C3
- According to a list shown below, I performed restriction enzyme processing at 37 for 30 minutes.
ddH2O 2 µl BBa_E0240 50 µl EcoRⅠ 1 µl PstⅠ 1 µl 10 x H Buffer 6 µl total 60 µl
- Next ligate with following list.
- At first I dilute the density of vector to become 10 pg/µl.
- And I dilute it as I calculate one and MLF 60 ng/µl of GFP 70 ng/µl to be able to go by combination below and am composed follows at 1 µl.
- I combined it in the ratio of follows afterwards.
pSB1C3:GFP=1:10
insert 1.0 µl vector 1.0µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total 6.0 µl
pSB1C3:GFP=1:20
insert 1.0 µl vector 1.0 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total6.0µl
pSB1C3:GFP=1:40
insert 1.0 µl vector 1.0 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total 6 µl
- I incubated them in 16°C for 30 min.
- After that, I transformed them, and I poured them into 300 µl of SOC medium and add them on the plate after culture for 30 minutes.
Results
- There are no colonies.
29th,September
Members
- Yoshimura, Nakagawa
- At first I dilute the density of vector to become 10 pg/µl.
- And I dilute it as I calculate one and MLF 60 ng/µl of GFP 70 ng/µl to be able to go by combination below and am composed follows at 1 µl.
- I combined it in the ratio of follows afterwards.
pSB1C3:GFP=1:10
insert 1.0 µl vector 1.0µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total 6.0 µl
pSB1C3:GFP=1:20
insert 1.0 µl vector 1.0 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total6.0µl
pSB1C3:GFP=1:40
insert 1.0 µl vector 1.0 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total 6 µl
- I incubated them in 16°C for 30 min.
- After that, I transformed them, and I poured them into 300 µl of SOC medium and add them on the plate after culture for 30 minutes.
Results
- There are some colonies on the plate.
- However there aren’t any MLF colonies.
30th,September
Members
- Yoshimura, Nakagawa
- At first I dilute the density of vector to become 10 pg/µl
- And I dilute it as I calculate one and MLF 60 ng/µl of GFP 70 ng/µl to be able to go by combination below and am composed follows at 1 µl
- I combined it in the ratio of follows afterwards
pSB1C3:GFP=1:10
insert 1.0 µl vector 1.0µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total 6.0 µl
pSB1C3:GFP=1:20
insert 1.0 µl vector 1.0 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total6.0µl
pSB1C3:GFP=1:40
insert 1.0 µl vector 1.0 µl 10 x Buffer 2.5 µl F4 ligase 0.5 µl ddH2O 1.0 µl total 6 µl
- I incubated them in 16°C for 30 min.
- After that, I transformed them, and I poured them into 300 µl of SOC medium and add them on the plate after culture for 30 minutes.
- After that We did alkaline-lysis method restriction and enzymes processing with ligation products.
Results
- After all MLF did not exist even if there was the BBa_E0240 in ligation products.
- And the first turn of parts was completed today.