Team:UST-Beijing/Notebook

From 2011.igem.org

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Combine the insert and vector with T4  ligase</p>
Combine the insert and vector with T4  ligase</p>
<p><h2>2.2 Gel electrophoresis</h2></p>
<p><h2>2.2 Gel electrophoresis</h2></p>
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<p><img src="https://static.igem.org/mediawiki/2011/8/8b/%E5%A4%A7%E7%B4%AB_%E5%8F%8C%E5%88%87.jpg" width="147" height="221" />
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<table width="333" height="84" border="1">
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1: wide range marker
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  <tr>
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</br>2: the constructed plasmid pSG5/PR cut with EcoR1 and BamH1</td>
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    <td width="316"><p><img src="https://static.igem.org/mediawiki/2011/8/8b/%E5%A4%A7%E7%B4%AB_%E5%8F%8C%E5%88%87.jpg" alt="" width="147" height="221" />1: wide range marker</p>
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</tr>
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    <p>2: the constructed plasmid pSG5/PR cut with EcoR1 and BamH1</p></td>
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    <td width="8">&nbsp;</td>
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  </tr>
</table>
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<br />
 
<p><h2>2.3  DNA sequencing</h2></p>
<p><h2>2.3  DNA sequencing</h2></p>
<p><img src="https://static.igem.org/mediawiki/2011/1/15/2.3.PNG" width="650" height="412" /></p>
<p><img src="https://static.igem.org/mediawiki/2011/1/15/2.3.PNG" width="650" height="412" /></p>

Revision as of 12:23, 12 September 2011



Project 2.

1.1:The construction of pSB1AC3/PR




 

 

 

 

 

 

 

 

PR + pSB1AC3 = pSB1AC3/PR (new part)

Cut PR w/EcoRI & SpeI

Cut pSB1AC3 w/EcoRI & SpeI

Combine the insert and vector with T4 ligase

1.2: Gel electrophoresis


1: wide range maker
2、3、4、5:the constructed plasmid cutted with SpeI and EcoRI restriction enzymes



 

 

 

 

 

 

 

 

 

 

1.3: DNA sequencing


The result of DNA sequencing demonstrates that there is no mutation in the new part by comparing to the original sequence.

 

2.1 The construction of pSG5/PR which is used for eukaryotic expression

PR + pSG5 = pSG5/PR
Cut PR w/EcoRI & BamH I
Cut pSG5 w/EcoRI & BamH I
Combine the insert and vector with T4 ligase

2.2 Gel electrophoresis

1: wide range marker

2: the constructed plasmid pSG5/PR cut with EcoR1 and BamH1

 

2.3 DNA sequencing

The result of DNA sequencing demonstrates that there is no mutation in PR by comparing to the original sequence.

3.1  The construction of pBABE/PR

1) PCR for amplifying more insert
Primer 1:         5'-ggg gaa ttc taa acc acc atg ctt gcc-3'
Primer 2:         5'-aaa gaa ttc tca cta tta ggc gtt gct-3'
Reaction system:
10XPCR buffer      5ul
dNTP               4ul
primer 1           1ul
primer 2           2ul
pfu                1ul
template           1ul
DMSO               5ul
ddH2O              31ul
Total              50ul
Reaction condition:
95℃       5min

****************
95℃       15s
52℃       15s
72℃       2min

25cycles

****************
72℃       10min
4℃        ∞

2) Ligation

PR + pBABE = pBABE/PR
Cut PR w/EcoRI
Cut pBABE w/EcoRI
Combine the insert and vector with T4 ligase

3.2 Gel electrophoresis

1:Middle range maker     1:DL2,000 DNA Marker

2:cut with EcoR I      2:cut with Sal I

Figure 1 indicates that the insert is combined with the vector successfully.
Figure 2 indicates that the insert is in the right direction.

3.3 DNA sequencing

As before, the result of DNA sequencing demonstrates that there is no mutation in PR by comparing to the original sequence.

 

 

Notebook

You should make use of the calendar feature on the wiki and start a lab notebook. This may be looked at by the judges to see how your work progressed throughout the summer. It is a very useful organizational tool as well.