IGEM:Peking/2007/Count-Conjugation-Notebook/2007-7-25: Difference between revisions
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(New page: ==R0040<-crRNA== *Ligation transformants do not grow. *Re-ligation tonight, and overnight, plan to ligate under 16℃ tomorrow morning. *In case it is the XbaI/PstI digestion of the PCR pr...) |
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=OriT Knock Out= | |||
==oriT Knock Out== | |||
*By Xu Anting | |||
*Successfully ligated up- and downstream fragments of 600 bp to 1200 bp using overlapped PCR, but agarose gel also showed that there are unspecific bands (750 bp) in PCR products. Therefore I chose gel separation to get purified products. | |||
*Use BamHI and SalI to digest the fragment in 37 centigrade, overnight. | |||
*Ready to ligate fragments to pUC18 and have them transformed and sequenced. | |||
==Conjugation Test== | |||
*By Liu Ting | |||
*pSC101 competent cells are ready. I transformed pUC18 to test their efficiency and will get the result tomorrow. | |||
*failed to purify the pSC101 plasmid (~9 kb) from E. coli. Will try again tomorrow. | |||
=Key & Lock by Yu Tao and Zheng Qinsi= | |||
==R0040<-crRNA== | ==R0040<-crRNA== | ||
*Ligation transformants do not grow. | *Ligation transformants do not grow. | ||
| Line 4: | Line 17: | ||
*In case it is the XbaI/PstI digestion of the PCR product ends that failed. We will rePCR tonight, see below. | *In case it is the XbaI/PstI digestion of the PCR product ends that failed. We will rePCR tonight, see below. | ||
== | ===Transformation result of R0040<-J23078=== | ||
* | *There are no colonies in the experimental plate and the negative control plate but thousands of colonies in the positive control plate. | ||
* | *I think it is because of the inefficiency of the double digestion of J23078, though I can not rule other possibilities out. | ||
* | *I suggest do the double digestion, purification, ligation and transformation once more. | ||
==Double Digesting R0010 and J23066== | |||
*Digesting R0010 with SpeI/PstI and J23066 with PstI/XbaI. | |||
*Digestion system contains: | |||
<pre> | |||
0.5 µl EcoRI | |||
0.5 µl PstI | |||
10 µl Plasmid | |||
2 µl 10*H | |||
8 µl ddH20 | |||
-------------------------- | |||
20 µl Total | |||
</pre> | |||
*Treat each plasmid with two 20uL systems(So totally 40uL system per plasmid). | |||
*37℃ culutre for 8 hours. | |||
==R0010, J23066 Digestion Product purification== | |||
*use Transgen EasyPure PCR Purification Kit / Quick Gel Extraction Kit. | |||
*30uL after purflication, respectively | |||
===electrophorsis result=== | |||
*from ''left'' to ''right'': | |||
#Purified R0010 (vector) @ SpeI/PstI | |||
#Purified J23066 (fragment) @ PstI/XbaI | |||
#Precise Quantified Marker I | |||
[[Image:Peking_2007-7-25-r0010 and j23066 after purification.jpg]] | |||
==Ligation: R0010<-J23066== | |||
*Ligate the J23066 fragment and $$$$$ vector | |||
*Ligation system contains: | |||
<pre> | |||
7 µl J23066 fragment | |||
1 µl R0010 vector | |||
1 µl T4-Ligase | |||
1 µl 10 X ligation buffer | |||
0 µl ddH20 | |||
-------------------------- | |||
10 µl Total | |||
</pre> | |||
*The negative control group contains no fragment but 7uL ddH2O instead. | |||
*4℃ overnight. | |||
==PCR J23078== | |||
*J23078 forward and reverse primer: stored as 50uM. | |||
*PCR system contains: | |||
<pre> | |||
0.5 µL Primer pf1 | |||
0.5 µL Primer pr1 | |||
4 µL dNTP | |||
0.5 µL Taq | |||
5µL 10 X buffer | |||
39.5µL dH20 | |||
-------------------------- | |||
50 µl Total | |||
</pre> | |||
*Primer final concentration 0.5uM. | |||
*Add a drop of liquid paraffin to each system. | |||
*PCR program setting: | |||
<pre> | |||
Step1 94℃ 5min | |||
Step2 94℃ 30s | |||
Step3 60℃ 30s | |||
Step4 72℃ 30s | |||
Step5 Go to step 2 for 4 times | |||
Step6 72℃ 10min | |||
End | |||
</pre> | |||
== | ==J23078 PCR product purification== | ||
* | *Use Transgen EasyPure PCR Purification Kit. | ||
*50uL after purflication. | |||
* | |||
Latest revision as of 19:48, 15 August 2007
OriT Knock Out
oriT Knock Out
- By Xu Anting
- Successfully ligated up- and downstream fragments of 600 bp to 1200 bp using overlapped PCR, but agarose gel also showed that there are unspecific bands (750 bp) in PCR products. Therefore I chose gel separation to get purified products.
- Use BamHI and SalI to digest the fragment in 37 centigrade, overnight.
- Ready to ligate fragments to pUC18 and have them transformed and sequenced.
Conjugation Test
- By Liu Ting
- pSC101 competent cells are ready. I transformed pUC18 to test their efficiency and will get the result tomorrow.
- failed to purify the pSC101 plasmid (~9 kb) from E. coli. Will try again tomorrow.
Key & Lock by Yu Tao and Zheng Qinsi
R0040<-crRNA
- Ligation transformants do not grow.
- Re-ligation tonight, and overnight, plan to ligate under 16℃ tomorrow morning.
- In case it is the XbaI/PstI digestion of the PCR product ends that failed. We will rePCR tonight, see below.
Transformation result of R0040<-J23078
- There are no colonies in the experimental plate and the negative control plate but thousands of colonies in the positive control plate.
- I think it is because of the inefficiency of the double digestion of J23078, though I can not rule other possibilities out.
- I suggest do the double digestion, purification, ligation and transformation once more.
Double Digesting R0010 and J23066
- Digesting R0010 with SpeI/PstI and J23066 with PstI/XbaI.
- Digestion system contains:
0.5 µl EcoRI 0.5 µl PstI 10 µl Plasmid 2 µl 10*H 8 µl ddH20 -------------------------- 20 µl Total
- Treat each plasmid with two 20uL systems(So totally 40uL system per plasmid).
- 37℃ culutre for 8 hours.
R0010, J23066 Digestion Product purification
- use Transgen EasyPure PCR Purification Kit / Quick Gel Extraction Kit.
- 30uL after purflication, respectively
electrophorsis result
- from left to right:
- Purified R0010 (vector) @ SpeI/PstI
- Purified J23066 (fragment) @ PstI/XbaI
- Precise Quantified Marker I
File:Peking 2007-7-25-r0010 and j23066 after purification.jpg
Ligation: R0010<-J23066
- Ligate the J23066 fragment and $$$$$ vector
- Ligation system contains:
7 µl J23066 fragment 1 µl R0010 vector 1 µl T4-Ligase 1 µl 10 X ligation buffer 0 µl ddH20 -------------------------- 10 µl Total
- The negative control group contains no fragment but 7uL ddH2O instead.
- 4℃ overnight.
PCR J23078
- J23078 forward and reverse primer: stored as 50uM.
- PCR system contains:
0.5 µL Primer pf1 0.5 µL Primer pr1 4 µL dNTP 0.5 µL Taq 5µL 10 X buffer 39.5µL dH20 -------------------------- 50 µl Total
- Primer final concentration 0.5uM.
- Add a drop of liquid paraffin to each system.
- PCR program setting:
Step1 94℃ 5min Step2 94℃ 30s Step3 60℃ 30s Step4 72℃ 30s Step5 Go to step 2 for 4 times Step6 72℃ 10min End
J23078 PCR product purification
- Use Transgen EasyPure PCR Purification Kit.
- 50uL after purflication.
