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Team:Peking/Notebook/YWChen
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Yiwei Chen's Notes
Contents
July
7.26
PbrR MBP construction plan
August
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8.1
Ⅰ.Use Tag PCR "PbrR MBP(≈500bp)" for commercial plasmid(PET-21a) and standard plasmid (PSB1K3)
Ⅱ.Digestion:The products of PCR(PbrR MBP)[backbone 4100bp;digest site PstⅠ&NdeⅠ]
Ⅲ.Gel for identification & Retrieve the gel
Ⅳ.Miniprep pbrR-mbp-commercial for backups
8.2
Lpp-OmpA-MBP construction plan
Ⅰ.Use Pfu Mix PCR Nde1+Lpp-OmpA(437bp)+Sal1 & E(EcoR1)NX(Xba1)+Lpp-OmpA+Sal1
Ⅱ.Digest the PCR products by Ndel,Sall&EcoR,Sall ,respectively
Ⅲ.if the products above got right ,Retrieve the gel ,if not ,back to Ⅰuse gel retrieve kit then digestion for 2h,after that, go to purification.
8.3
MBP construction plan
Ⅰ.Pfu PCR Sall+N-MBP+Bspel
Bspel+C-MBP+SNP
Bspel+C-MBP+Xhol
Ⅱ.Identify them using agarose gel electrophoresis.if right ,go to retrieve the gel, if not ,back to Ⅰ
8.4
Lpp-OmpA,N-MBP,+C-MBP with backbone PET21a and PSBIK3
Ⅰ.Ligation,Nde1+Lpp-OmpA(437bp)+Sal1 with Sall+N-MBP+Bspel & Bspel+C-MBP+Xhol & PET21a
Ⅱ.Ligation, E(EcoR1)NX(Xba1)+Lpp-OmpA+Sal1 with Sall+N-MBP+Bspel & Bspel+C-MBP+SNP & PSBIK3
Ⅲ.Learn to do the western blotting. Write the protocols.
8.5
Transformation the products of 4 fragments above.
8.6
There is something wrong with the primer ,so it doesn't work, back to the work from 8.2
8.7
Ⅰ.Use Pfu Mix PCR Nde1+Lpp-OmpA(437bp)+Sal1 & E(EcoR1)NX(Xba1)+Lpp-OmpA+Sal1
Ⅱ.Digest the PCR products by Ndel,Sall&EcoR,Sall ,respectively
8.8
Ⅰ.Pfu PCR Sall+N-MBP+Bspel
Bspel+C-MBP+SNP
Bspel+C-MBP+Xhol
Ⅱ.Gel to identification
8.9
Ⅰ.Ligation,Nde1+Lpp-OmpA(437bp)+Sal1 with Sall+N-MBP+Bspel & Bspel+C-MBP+Xhol & PET21a
Ⅱ.Ligation, E(EcoR1)NX(Xba1)+Lpp-OmpA+Sal1 with Sall+N-MBP+Bspel & Bspel+C-MBP+SNP & PSBIK3
8.10
Transform the ligation product into Trans5α strain.
8.11
Help a teammate transform P(RBS+T3pol 1)&PmerR-PSB1C3 Plasmid to OmniMAX2-T1 Competent cell
Digestion:
Ⅰ.RBS+T3pol 1 with XbaI and pstI(insert)
Ⅱ.PmerR-PSB1C3 with SpeI and PstI (vector)
Retrieve the gel
Ligation the parts above.
8.12
Digestion MBP construct parts
Ligation 4 fragments
Nde1+Lpp-OmpA(437bp)+Sal1 with Sall+N-MBP+Bspel & Bspel+C-MBP+Xhol & PET21a//E(EcoR1)NX(Xba1)+Lpp-OmpA+Sal1 with Sall+N-MBP+Bspel & Bspel+C-MBP+SNP & PSBIK3 overnight
8.13
Digestion: PET21a 20 µl with NdeI and XhoI
Ligation again
Ⅰ.RBS+T3pol 1 with XbaI and pstI(insert)
Ⅱ.PmerR-PSB1C3 with SpeI and PstI (vector)
Insert:vector=1:7&2:6
Transform the ligation product
Finally got clone ,2:6 better than 1:7
Ⅲ.transformation 4 pieces fragments
8.14
Ⅰ.Plate PCR for identification 4 pieces fragments ligation products
Ⅱ.Miniprep
21a-(1~3) 1K3(1~3) 26-(1~2) 17-(3~4)
Ⅲ.Sent the plasmids for sequencing
8.15
Ⅰ.Got the right sequence 1K3(1~3) 26-(1~2) 17-(3~4) while 21a-(1~3) without MBP but have Lpp-OmpA inside
Ⅱ.transformation
1K3(1~3) 26-(1~2) 17-(3~4)
Ⅲ.Pick 20 single clones on 21a plate
Ⅳ.PCR for identification
Got the right size from agarose gel electrophoresis ( Lpp-OmpA+MBP=735bp)
Ⅴ.Digestion with NdeI and XhoI,then use PCR purification kit to retrieve products.
Ⅵ.Ligation 1(PET-21a):7
Ⅶ.Transformation
September
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9.5
Assembly:
T7p+RBS(B0034)+DsbA+MBP+TER(B0015)+T7p+RBS(B0034)+MBP+TER(B0015)+
T7p+RBS(B0034)+Lpp_OmpA+MBP+TER(B0015)
Ⅰ.Digestion:RBS with SpeI and PstI
1-23L terminator with EcoRI and XbaI
Ⅱ.Identify them using agarose gel electrophoresis.if right ,go to retrieve the gel
9.9
Ligation: RBS+MBP
DsbA+MBP
FORGET DIGESTION!!!!
9.10
Digestion:MBD with XbaI and PstI
DsbA-MBP with EcoRI and SpeI
Identify them using agarose gel electrophoresis.if right ,go to retrieve the gel
9.11
Transformation to BL21 for western blotting
Omni for preserve
9.13
Digestion :with XbaI and PstI (for ligation)
Miniprep T7p+RBS(B0034)+DsbA+MBP+Ter(1~3)&RBS+MBP(1~3)
9.15
Ⅰ.Sent the plasmids for sequencing【T7p+RBS(B0034)+DsbA+MBP+Ter(1~3)&RBS+MBP(1~3)】
T7p+RBS(B0034)+DsbA+MBP+Ter 1 got right sequence
Ⅱ.Digestion:
T7p+RBS(B0034)+DsbA+MBP+Ter with EcoRI and SpeI
Identify them using agarose gel electrophoresis.Then retrieve the gel(got the right size)
Ⅲ.Digestion:
RBS+MBP with XbaI and PstI
After Identify them by using agarose gel electrophoresis,the results turns wrong.
Digestion AGAIN!:
RBS+MBP with XbaI and PstI
Meanwhile: Pick 10 single clone for plate PCR by using tagmix
Digest the PCR products with XbaI and PstI ,10 clones all got the right size,so minipret them.
9.16
Ligation :RBS-MBP(XP)+Ter(SP)
Transformation it.
Culture the plates.
9.17
Pick the single clone to PCR, but failed
Meanwhile: Digest the RBS-MBP1 for backup
9.18
Digest the RBS-MBP(2&3)
Ligation: RBS-MBP(2&3) +T7p
Transformation the Ligation products
9.19
Use RBS-MBP(2&3) as templete,PCR(Fast pfu),got a mass of RBS-MBP
Identify them using agarose gel electrophoresis.Then go to retrieve the gel
9.20
Transformation:RBS-MBP-T7p
Culture the plates
9.21
Pick 3 single clone T7p-RBS-MBP(1~3)
Some for PCR some for Miniprep
9.22
Miniprep T7p-RBS-MBP(1~3)
Digestion:T7p-RBS-MBP(1~3) with EcoRI and SpeI
9.23
Wiki writing
Retrieve the digestion products T7p-RBS-MBP(1~3)ES
Ligation:
T7p-RBS-MBP(1~3)+Ter
Transformation:T7p-RBS-MBP-Ter(1~3)
Culture the plates
9.24
Pick 3 single clone from each plate(except1)
Miniprep T7p-RBS-MBP-Ter(2-1~3&3-1~3)
10µI for sequencing
10µI for digestion
Left 20µI
9.25
Digestion:T7p-RBS-MBP-Ter with SpeI and PstI
Gel for identification ,the size of T7p-RBS-MBP-Ter(2-1~3) are right
9.26
Digestion:PSB1C3 with EcoRI and PstI
Ligation:PSB1C3 + T7p-RBS-MBP-Ter+T7p+RBS+Lpp-OmpA+MBP+Ter
Gel retrieving
9.27
Transformation:Positive cloning
T7p+RBS+Lpp-OmpA+MBP+Ter&T7p+RBS(B0034)+DsbA+MBP+Ter
Culture the plates
9.28
The sequence of T7p-RBS-MBP-Ter(2-1~3&3-1~3) came out ,but without T7p inside.
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10.3
There is something wrong with PSBIC3(RFP inside )
Ligation Again!:
PSB1C3 + T7p-RBS-MBP-Ter+T7p+RBS+Lpp-OmpA+MBP+Ter
10.4
Pick 3 single clone from the plate
Miniprep them.
10.5
Transformation:Positive cloning:T7p+RBS(B0034)+DsbA+MBP+Ter
Digestion:RBS-MBP-Ter+T7p with XbaI and PstI
Identify them using agarose gel electrophoresis.Then go to retrieve the gel
10.6
Pick 3 single clone from the plate(T7p+RBS(B0034)+DsbA+MBP+Ter)
Digestion:PSB1C3 with XbaI and PstI (Change backbone)
Identify them using agarose gel electrophoresis.Then go to retrieve the gel
10.7
Miniprep T7p+RBS(B0034)+DsbA+MBP+Ter(1~3)
Digestion:RBS-MBP-Ter with XbaI and PstI
Ligation:RBS-MBP-Ter+T7p(sp) then transformation
10.8
Ligation again
T7p+RBS-MBP-Ter-+T7p+RBS+Lpp-OmpA+MBP+Ter
Transformation it
10.9
Transformation T7p+RBS+Lpp-OmpA+MBP+Ter(xp)-PSB1C3(xp)
PCR(tag mix) for identification T7p+RBS(B0034)+DsbA+MBP+Ter
Culture the plates, but it did not grow up
10.10
Ligation:T7p+RBS+Lpp-OmpA+MBP+Ter(EP)+PSB1C3
T7p+RBS+DsbA+MBP+Ter(EP)+PSB1C3
Transformation
Easy Mix PCR.
Culture the plates
10.11
ⅠDigestion:T7p+RBS+Lpp-OmpA+MBP+Ter(EP)
T7p+RBS+DsbA+MBP+Ter(EP)
Identify them using agarose gel electrophoresis.Then go to retrieve the gel
10.16
Ⅰ.Ligation: T7p-RBS-MBP-Ter
Ⅱ.Transformation :T7p-RBS-MBP-Ter
Ⅲ.Culture the plates
Pick 3 single clones
10.17
T7p-RBS-MBP-Ter for sequencing
10.20
Ⅰ.Liagation:T7p+RBS+DsbA+MBP+TER+T7p+RBS+MBP+TER+T7p+RBS+Lpp-OmpA+MBP+TER+PSBIC3
Ⅱ.Transformation
Ⅲ.Culture the plates
Pick 6 Single clones
Ⅳ.T7p+RBS+DsbA+MBP+TER+T7p+RBS+MBP+TER+T7p+RBS+Lpp-OmpA+MBP+TER+PSBIC3 for sequencing
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