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Team:Peking/Notebook/DHLiang
From 2010.igem.org
| Line 102: | Line 102: | ||
===7.1=== | ===7.1=== | ||
Dissolve primers | Dissolve primers | ||
| + | |||
Design PCR programme | Design PCR programme | ||
===7.4=== | ===7.4=== | ||
MerR PCR, MBP PCR | MerR PCR, MBP PCR | ||
| + | |||
Retrieve the PCR product | Retrieve the PCR product | ||
===7.5=== | ===7.5=== | ||
Digest the plasmid pET-39(B)+ with SacII and EcoRI | Digest the plasmid pET-39(B)+ with SacII and EcoRI | ||
| + | |||
Digest the PCR product with SacII and EcoRI | Digest the PCR product with SacII and EcoRI | ||
| + | |||
Retrieve the digested product | Retrieve the digested product | ||
| + | |||
Ligated the digested plasmid pET-39(b)+ and the PCR product | Ligated the digested plasmid pET-39(b)+ and the PCR product | ||
| + | |||
Transform the ligation product into Trans5αstrain. | Transform the ligation product into Trans5αstrain. | ||
===7.6=== | ===7.6=== | ||
Part I handle the job for YHu | Part I handle the job for YHu | ||
| + | |||
Digest pET-21a with NdeI and XhoI | Digest pET-21a with NdeI and XhoI | ||
| + | |||
Retrieve the digested product | Retrieve the digested product | ||
| + | |||
Ligated the digested pET-21a with MBP digested fragments | Ligated the digested pET-21a with MBP digested fragments | ||
| + | |||
Transform the ligation product | Transform the ligation product | ||
| + | |||
Part II Periplasmic Construction | Part II Periplasmic Construction | ||
| + | |||
Pick the six single clones for the plate transformed last night | Pick the six single clones for the plate transformed last night | ||
| + | |||
PCR the clones to identify the successfully ligated clone | PCR the clones to identify the successfully ligated clone | ||
| + | |||
Clones 1\3\5 shows positive result and go on shaking at 37℃ overnight | Clones 1\3\5 shows positive result and go on shaking at 37℃ overnight | ||
===7.7=== | ===7.7=== | ||
Part I handle the job for YHu | Part I handle the job for YHu | ||
| + | |||
Pick clones from the plate transformed yesterday and shake at 37℃ for ten hours | Pick clones from the plate transformed yesterday and shake at 37℃ for ten hours | ||
| + | |||
Miniprep the plasmid from the clones | Miniprep the plasmid from the clones | ||
| + | |||
Part II Periplasmic Construction | Part II Periplasmic Construction | ||
| + | |||
Miniprep clone 1\3\5 and send them for sequencing | Miniprep clone 1\3\5 and send them for sequencing | ||
===7.8=== | ===7.8=== | ||
Part I handle the job for YHu | Part I handle the job for YHu | ||
| + | |||
Digest the plasmid minipreped yesterday and identify by Electrophoresis | Digest the plasmid minipreped yesterday and identify by Electrophoresis | ||
| + | |||
No positive result showed | No positive result showed | ||
| + | |||
Redo the experiment starting with PCR the MBP | Redo the experiment starting with PCR the MBP | ||
| + | |||
Part II Periplasmic Construction | Part II Periplasmic Construction | ||
| + | |||
Positive Transformation of DsbA-MerR | Positive Transformation of DsbA-MerR | ||
| + | |||
Start the construction of DsbA-MBP | Start the construction of DsbA-MBP | ||
| + | |||
PCR MBP overnight | PCR MBP overnight | ||
===7.9=== | ===7.9=== | ||
Part I handle the job for YHu | Part I handle the job for YHu | ||
| + | |||
Redo the ligation of MBP into pET-21a | Redo the ligation of MBP into pET-21a | ||
| + | |||
Transformation | Transformation | ||
| + | |||
Part II Periplasmic Construction | Part II Periplasmic Construction | ||
| + | |||
The sequence of Clone 1 from DsbA-MerR is correct | The sequence of Clone 1 from DsbA-MerR is correct | ||
| + | |||
Retrieve the MBP PCR product | Retrieve the MBP PCR product | ||
===7.10=== | ===7.10=== | ||
| - | YHu's job is officially handled by XTeng.I begin to conduct the experiment of the periplasmic module of the bioabsorbent display alone | + | YHu's job is officially handled by XTeng.I begin to conduct the experiment of the periplasmic module of the |
| + | bioabsorbent display alone | ||
| + | |||
Digest pET-39(b)+ and the retrieved MBP PCR product | Digest pET-39(b)+ and the retrieved MBP PCR product | ||
| + | |||
Ligate the product overnight | Ligate the product overnight | ||
| + | |||
Start the standardization of DsbA-MerR | Start the standardization of DsbA-MerR | ||
| + | |||
PCR DsbA-MerR with standadized primers | PCR DsbA-MerR with standadized primers | ||
===7.11=== | ===7.11=== | ||
Transformation of the ligated DsbA-MBP | Transformation of the ligated DsbA-MBP | ||
| + | |||
Transformation of standardization of DsbA-MerR | Transformation of standardization of DsbA-MerR | ||
===7.12=== | ===7.12=== | ||
| Line 157: | Line 193: | ||
===7.13=== | ===7.13=== | ||
Digest the product of DsbA-MerR with EcoRI and SacII and do the identificate by Electrophoresis | Digest the product of DsbA-MerR with EcoRI and SacII and do the identificate by Electrophoresis | ||
| + | |||
Digest the product of standardization of DsbA-MerR with EcoRI and PstI and do the identificate by Electrophoresis | Digest the product of standardization of DsbA-MerR with EcoRI and PstI and do the identificate by Electrophoresis | ||
| + | |||
No postive result showed | No postive result showed | ||
===7.14=== | ===7.14=== | ||
re-Conduct the experiment | re-Conduct the experiment | ||
| + | |||
PCR MBP and retrieve the product | PCR MBP and retrieve the product | ||
| + | |||
PCR DsbA-MerR and retrieve the product | PCR DsbA-MerR and retrieve the product | ||
| + | |||
Digest the product with EcoRI and SacII | Digest the product with EcoRI and SacII | ||
| + | |||
Digest the the standardization product with EcoRI and PstI | Digest the the standardization product with EcoRI and PstI | ||
| + | |||
Retrieve the product and ligate with digested pET-39(b)+ | Retrieve the product and ligate with digested pET-39(b)+ | ||
| + | |||
Transform the ligated product | Transform the ligated product | ||
===7.15=== | ===7.15=== | ||
Pick 24 clones from the plates and shake at 37℃ for ten hours | Pick 24 clones from the plates and shake at 37℃ for ten hours | ||
| + | |||
Start the construction of MerR into pET-21a | Start the construction of MerR into pET-21a | ||
| + | |||
PCR MerR and retrieve | PCR MerR and retrieve | ||
| + | |||
Digest it with XhoI and NdeI | Digest it with XhoI and NdeI | ||
| + | |||
Retrieve the digested product and ligate with digested pET-21a | Retrieve the digested product and ligate with digested pET-21a | ||
===7.16=== | ===7.16=== | ||
Plasmid Miniprep from the 24 clones | Plasmid Miniprep from the 24 clones | ||
| + | |||
Pick 21 clones from the plates of the standardization of DsbA-MerR and shake at 37℃ for ten hours | Pick 21 clones from the plates of the standardization of DsbA-MerR and shake at 37℃ for ten hours | ||
| + | |||
Digest the Plasmid Miniprep product and identificate by Electrophoresis | Digest the Plasmid Miniprep product and identificate by Electrophoresis | ||
===7.17=== | ===7.17=== | ||
Positive result showed among the clones,they are A21 A22 A23 A27 C15 C21 C22 | Positive result showed among the clones,they are A21 A22 A23 A27 C15 C21 C22 | ||
| + | |||
Positive transform of A22 A27 C15 C22 | Positive transform of A22 A27 C15 C22 | ||
===7.18-7.24=== | ===7.18-7.24=== | ||
Go to ShangHai EXPO on a vocation. | Go to ShangHai EXPO on a vocation. | ||
| + | |||
The sequence result( done by Xteng) showed the construction of DsbA-MBP failed again. | The sequence result( done by Xteng) showed the construction of DsbA-MBP failed again. | ||
| - | Meanwhile since we later discovered there is a PstI restriction site right in the middle of DsbA ,unfortuanately we uesd to digest the Standardized PCR product of DsbA-MerR with PstI,so this part failed, too. | + | |
| + | Meanwhile since we later discovered there is a PstI restriction site right in the middle of DsbA ,unfortuanately we | ||
| + | uesd to digest the Standardized PCR product of DsbA-MerR with PstI,so this part failed, too. | ||
===7.25=== | ===7.25=== | ||
Digest pET-39(b)+ with XbaI and XhoI | Digest pET-39(b)+ with XbaI and XhoI | ||
| + | |||
PCR MBP and retrieve the product | PCR MBP and retrieve the product | ||
| + | |||
Digest it with XbaI and XhoI | Digest it with XbaI and XhoI | ||
| + | |||
Ligate the digested vector and the PCR product | Ligate the digested vector and the PCR product | ||
===7.26=== | ===7.26=== | ||
Transform the ligated product | Transform the ligated product | ||
| + | |||
Pick clones from the plate and shake at 37℃ ovenight | Pick clones from the plate and shake at 37℃ ovenight | ||
===7.27=== | ===7.27=== | ||
| Line 196: | Line 254: | ||
===7.28=== | ===7.28=== | ||
PCR DsbA-MerR | PCR DsbA-MerR | ||
| + | |||
Positive transform DsbA-MerR into Omni Strain | Positive transform DsbA-MerR into Omni Strain | ||
===7.29=== | ===7.29=== | ||
| - | The Sequence of DsbA-MBP result failed again, but reveal that the original plasmid containing MBP from Summers is incorrect. | + | The Sequence of DsbA-MBP result failed again, but reveal that the original plasmid containing MBP from Summers is |
| + | incorrect. | ||
| + | |||
We design to do the three fragment Ligation strategy to construct the MBP | We design to do the three fragment Ligation strategy to construct the MBP | ||
| + | |||
PCR Strain NRI/PASK-MBD with two pairs of primers | PCR Strain NRI/PASK-MBD with two pairs of primers | ||
| + | |||
Retrieve the product | Retrieve the product | ||
| + | |||
Start the nested PCR of DsbA-MerR to finish its Standradization. | Start the nested PCR of DsbA-MerR to finish its Standradization. | ||
===7.30=== | ===7.30=== | ||
Digest the pEt-39(b)+ with XbaI and XhoI | Digest the pEt-39(b)+ with XbaI and XhoI | ||
| + | |||
Digest the MBD-Part I with XbaI and BamHi | Digest the MBD-Part I with XbaI and BamHi | ||
| + | |||
Digest the MBD-Part II with XhoI and BamHi | Digest the MBD-Part II with XhoI and BamHi | ||
| + | |||
Rerieve the three products and ligate them together for three hours | Rerieve the three products and ligate them together for three hours | ||
| + | |||
Transform the ligated product | Transform the ligated product | ||
| + | |||
Identificate the Standradization of DsbA-MerR but failed | Identificate the Standradization of DsbA-MerR but failed | ||
===7.31=== | ===7.31=== | ||
Yesterday's transformation failed | Yesterday's transformation failed | ||
| + | |||
Re-ligate the three fragments for three hours | Re-ligate the three fragments for three hours | ||
| + | |||
Transform the product | Transform the product | ||
| - | + | ||
| + | Redo the first round nested PCR of DsbA-MerR | ||
| + | |||
Retrieve the product | Retrieve the product | ||
| - | + | ||
| + | The Transformation seems to be successful and pick 12 clones from the plate | ||
| + | |||
Do the second round nested PCR of DsbA-MerR==August== | Do the second round nested PCR of DsbA-MerR==August== | ||
Revision as of 15:35, 25 October 2010
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Donghai Liang's Notes
Contents
July
| Mon | Tue | Wed | Thu | Fri | Sat | Sun |
| - | - | - | - | 1 | 2 | 3 |
| 4 | 5 | 6 | 7 | 8 | 9 | 10 |
| 11 | 12 | 13 | 14 | 15 | 16 | 17 |
| 18 | 19 | 20 | 21 | 22 | 23 | 24 |
| 25 | 26 | 27 | 28 | 29 | 30 | 31 |
| - | - | - | - | - | - | - |
[TOP]
7.1
Dissolve primers
Design PCR programme
7.4
MerR PCR, MBP PCR
Retrieve the PCR product
7.5
Digest the plasmid pET-39(B)+ with SacII and EcoRI
Digest the PCR product with SacII and EcoRI
Retrieve the digested product
Ligated the digested plasmid pET-39(b)+ and the PCR product
Transform the ligation product into Trans5αstrain.
7.6
Part I handle the job for YHu
Digest pET-21a with NdeI and XhoI
Retrieve the digested product
Ligated the digested pET-21a with MBP digested fragments
Transform the ligation product
Part II Periplasmic Construction
Pick the six single clones for the plate transformed last night
PCR the clones to identify the successfully ligated clone
Clones 1\3\5 shows positive result and go on shaking at 37℃ overnight
7.7
Part I handle the job for YHu
Pick clones from the plate transformed yesterday and shake at 37℃ for ten hours
Miniprep the plasmid from the clones
Part II Periplasmic Construction
Miniprep clone 1\3\5 and send them for sequencing
7.8
Part I handle the job for YHu
Digest the plasmid minipreped yesterday and identify by Electrophoresis
No positive result showed
Redo the experiment starting with PCR the MBP
Part II Periplasmic Construction
Positive Transformation of DsbA-MerR
Start the construction of DsbA-MBP
PCR MBP overnight
7.9
Part I handle the job for YHu
Redo the ligation of MBP into pET-21a
Transformation
Part II Periplasmic Construction
The sequence of Clone 1 from DsbA-MerR is correct
Retrieve the MBP PCR product
7.10
YHu's job is officially handled by XTeng.I begin to conduct the experiment of the periplasmic module of the bioabsorbent display alone
Digest pET-39(b)+ and the retrieved MBP PCR product
Ligate the product overnight
Start the standardization of DsbA-MerR
PCR DsbA-MerR with standadized primers
7.11
Transformation of the ligated DsbA-MBP
Transformation of standardization of DsbA-MerR
7.12
Plasmid Miniprep from the transformation product
7.13
Digest the product of DsbA-MerR with EcoRI and SacII and do the identificate by Electrophoresis
Digest the product of standardization of DsbA-MerR with EcoRI and PstI and do the identificate by Electrophoresis
No postive result showed
7.14
re-Conduct the experiment
PCR MBP and retrieve the product
PCR DsbA-MerR and retrieve the product
Digest the product with EcoRI and SacII
Digest the the standardization product with EcoRI and PstI
Retrieve the product and ligate with digested pET-39(b)+
Transform the ligated product
7.15
Pick 24 clones from the plates and shake at 37℃ for ten hours
Start the construction of MerR into pET-21a
PCR MerR and retrieve
Digest it with XhoI and NdeI
Retrieve the digested product and ligate with digested pET-21a
7.16
Plasmid Miniprep from the 24 clones
Pick 21 clones from the plates of the standardization of DsbA-MerR and shake at 37℃ for ten hours
Digest the Plasmid Miniprep product and identificate by Electrophoresis
7.17
Positive result showed among the clones,they are A21 A22 A23 A27 C15 C21 C22
Positive transform of A22 A27 C15 C22
7.18-7.24
Go to ShangHai EXPO on a vocation.
The sequence result( done by Xteng) showed the construction of DsbA-MBP failed again.
Meanwhile since we later discovered there is a PstI restriction site right in the middle of DsbA ,unfortuanately we uesd to digest the Standardized PCR product of DsbA-MerR with PstI,so this part failed, too.
7.25
Digest pET-39(b)+ with XbaI and XhoI
PCR MBP and retrieve the product
Digest it with XbaI and XhoI
Ligate the digested vector and the PCR product
7.26
Transform the ligated product
Pick clones from the plate and shake at 37℃ ovenight
7.27
Plasmid Miniprep and send for sequencing
7.28
PCR DsbA-MerR
Positive transform DsbA-MerR into Omni Strain
7.29
The Sequence of DsbA-MBP result failed again, but reveal that the original plasmid containing MBP from Summers is incorrect.
We design to do the three fragment Ligation strategy to construct the MBP
PCR Strain NRI/PASK-MBD with two pairs of primers
Retrieve the product
Start the nested PCR of DsbA-MerR to finish its Standradization.
7.30
Digest the pEt-39(b)+ with XbaI and XhoI
Digest the MBD-Part I with XbaI and BamHi
Digest the MBD-Part II with XhoI and BamHi
Rerieve the three products and ligate them together for three hours
Transform the ligated product
Identificate the Standradization of DsbA-MerR but failed
7.31
Yesterday's transformation failed
Re-ligate the three fragments for three hours
Transform the product
Redo the first round nested PCR of DsbA-MerR
Retrieve the product
The Transformation seems to be successful and pick 12 clones from the plate
Do the second round nested PCR of DsbA-MerR==August==
