IGEM:Peking/2007/Count-Conjugation-Notebook/2007-8-13: Difference between revisions

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=Tandem Ori-T by Qu Mingzhi=
=Tandem Ori-T by Mingzhi Qu, Ze Ren=
==Trimethoprim(TLC) antibiotic Efficiency Test ==
==Trimethoprim(TLC) antibiotic Efficiency Test ==
*new antibiotic,test efficiency, use Dh5α+pSB1A2(Amp+) as control.
*new antibiotic,test efficiency, use Dh5α+pSB1A2(Amp+) as control.
Line 12: Line 12:
*¢:can be seen by centrifugal.
*¢:can be seen by centrifugal.
*<+ means less than + by centrifugal.
*<+ means less than + by centrifugal.
==(8.15-8.16) Trimethoprim(TLC) antibiotic Efficiency Test(II) ==
*culture in solid LB.
<pre>
TLC(working solution):    4ug/mL    8ug/mL  12ug/mL  15ug/mL  20ug/mL  LB-  Amp+  Tc+
R751(TLC+):                ++§      ++      ++        ++      ++      ++    -    -
Dh5α+pSB1A2(Amp+):        +¢        <+      <<+      <<<<+      -      ++  ++    -
pSC101(Tc+)                +¢        <+      <<+      <<<<+      -      ++    -    ++
</pre>
*§:grown
*¢:can be seen by centrifugal.
*<+ means less than "+",still can be seen by centrifugal.


===colony PCR Test for pSC101 Conjugation Test===
*Conjugation Test
*Test Lb- R751 plate, Lb- pSC101 have the correct plasmid.
*Test plate:LB- R751, Lb- pSB101, R751-pSC101 X Dh5α-R0040,  R751 X Dh5α-R0040
*primer :R751 OriT primer, pSC101 primer.
*according to <Colony PCR STANDARD PROTOCOL>
*PCR system contains(each well):
<pre>
0.5  µl      Primer 1(100uM)
0.5  µl      Primer 2
2    µl      dNTP(2.5uM)
2.5  µl      10X Taq Buffer
0.25 µl      Taq
19  µl      dH20
1    µl      template
--------------------------
~25  µl      Total
</pre>
*PCR program condition 1: 94℃ 5min, 94℃ 30s, '''51℃ 30s''', 72℃ 45s, Go to step 2 for 29 times, 72℃ 10min, 4℃ end.
*PCR program condition 2: 94℃ 5min, 94℃ 30s, '''55℃ 30s''', 72℃ 45s, Go to step 2 for 29 times, 72℃ 10min, 4℃ end .
====electrophorsis result====
*top:from ''left'' to ''right''
**1-5  R751-pSC101 X Dh5α-R0040
**6-10  R751 X Dh5α-R0040
**11    R751
**13  Maker(DL2000 plus)
*botton:from ''left'' to ''right''
**1-4  R751
**5-10  psc101
**11    Maker(DL2000 plus)
[[Image:Peking_2007-8-12_colony_PCRII.jpg‎]]


=Lock & Key By Yu Tao=
=Lock & Key By Yu Tao=
Line 61: Line 104:
#marker (DL2000 Plus)  
#marker (DL2000 Plus)  
[[Image:Example.jpg]]
[[Image:Example.jpg]]
==Ligation and Transformation: J01010 and J01008 PCR product -> pEASY-T3 cloning vector==
*For sequencing.
*Use Transgen pEASY-T3 vector.
*Transform the ligation product, result to be seen tomorrow.

Latest revision as of 04:24, 2 September 2007

Tandem Ori-T by Mingzhi Qu, Ze Ren

Trimethoprim(TLC) antibiotic Efficiency Test

  • new antibiotic,test efficiency, use Dh5α+pSB1A2(Amp+) as control.
  • Preservative:1mg/mL in 2.5% acetic acid.
TLC(working solution):   0.5ug/mL  1ug/mL  2ug/mL  3ug/mL  4ug/mL  5ug/mL     LB-  amp+ 
R751(TLC+):                ++§       ++      ++      ++       ++     ++        +    /
Dh5α+pSB1A2(Amp+):         +¢        <+      <<+    <<<+     <<<<+  <<<<<+     +    +
empty:                     -         /        /       /        /     -         -    /
  • §:grown
  • ¢:can be seen by centrifugal.
  • <+ means less than + by centrifugal.

(8.15-8.16) Trimethoprim(TLC) antibiotic Efficiency Test(II)

  • culture in solid LB.
TLC(working solution):    4ug/mL    8ug/mL  12ug/mL  15ug/mL  20ug/mL   LB-  Amp+  Tc+
R751(TLC+):                ++§       ++      ++        ++       ++      ++    -     -
Dh5α+pSB1A2(Amp+):         +¢        <+      <<+      <<<<+      -      ++   ++     -
pSC101(Tc+)                +¢        <+      <<+      <<<<+      -      ++    -     ++
  • §:grown
  • ¢:can be seen by centrifugal.
  • <+ means less than "+",still can be seen by centrifugal.

colony PCR Test for pSC101 Conjugation Test

  • Conjugation Test
  • Test Lb- R751 plate, Lb- pSC101 have the correct plasmid.
  • Test plate:LB- R751, Lb- pSB101, R751-pSC101 X Dh5α-R0040, R751 X Dh5α-R0040
  • primer :R751 OriT primer, pSC101 primer.
  • according to <Colony PCR STANDARD PROTOCOL>
  • PCR system contains(each well):
0.5  µl      Primer 1(100uM)
0.5  µl      Primer 2
2    µl      dNTP(2.5uM)
2.5  µl      10X Taq Buffer
0.25 µl      Taq
19   µl      dH20
1    µl      template
--------------------------
~25  µl      Total
  • PCR program condition 1: 94℃ 5min, 94℃ 30s, 51℃ 30s, 72℃ 45s, Go to step 2 for 29 times, 72℃ 10min, 4℃ end.
  • PCR program condition 2: 94℃ 5min, 94℃ 30s, 55℃ 30s, 72℃ 45s, Go to step 2 for 29 times, 72℃ 10min, 4℃ end .

electrophorsis result

  • top:from left to right
    • 1-5 R751-pSC101 X Dh5α-R0040
    • 6-10 R751 X Dh5α-R0040
    • 11 R751
    • 13 Maker(DL2000 plus)
  • botton:from left to right
    • 1-4 R751
    • 5-10 psc101
    • 11 Maker(DL2000 plus)

Lock & Key By Yu Tao

Efficiency Test

Transformation Result: Competent Cells II

  • To our superise, there are colonies both in the experimental plate and the negative control plate.
  • Select some colonies from the negative plate, culture them in liquid LB overnight for mini-prep.
  • I decided to redo the efficiency test, with all possible controls. I use the good competent cells and DH5a as control groups, and culture each group on Amp+, Kan+ and Empty LB plate.

Recheck Test Result

     | Competent Cells II | Good Competent Cells |      DH5a
--------------------------------------------------------------------
Amp+ |         +          |          -           |        -
--------------------------------------------------------------------
Kan+ |         -          |          -           |        -
--------------------------------------------------------------------
LB-  |         +          |          +           |        +
  • Conclusion: I need to reprepare the competent cells again. ... -_-:

Mini-prep: R0010<-J01008 and R0040<-J01010

  • Using Transgen mini plasmid purification kit.
  • 50 uL per tube after purification, 2 tubes per type of plasmids.

Mini-prep Double Digesting Test Result

  • Digesting all the newly minipreped plasmids with EcoRI/PstI.
  • Each digestion system contains:
1 µl       10*H buffer
0.25 µl    EcoRI
0.25 µl    PstI
5 µl       Plasmid
3.5 µl     ddH20
--------------------------
10 µl      Total
  • 37℃ culutre for 3 hours.
  • from left to right:
  1. R0040<-J01010-1 @ EcoRI/PstI
  2. R0040<-J01010-2 @ EcoRI/PstI
  3. R0010<-J01008-1 @ EcoRI/PstI
  4. R0010<-J01008-2 @ EcoRI/PstI
  5. R0040 negative ligation control @ EcoRI/PstI
  6. R0010 negative ligation control @ EcoRI/PstI
  7. J01008 PCR product
  8. J01010 PCR product
  9. marker (DL2000 Plus)

Ligation and Transformation: J01010 and J01008 PCR product -> pEASY-T3 cloning vector

  • For sequencing.
  • Use Transgen pEASY-T3 vector.
  • Transform the ligation product, result to be seen tomorrow.
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