Team:Osaka/week8
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(Difference between revisions)
(New page: ==September 12 (Sun)== # Miniprep of Fcex, 006, 007, 010, 011 # Restriction digests of 006, 007, 010, 011 with EcoRI, SpeI; Fcex with XbaI, PstI # Gel electrophoresis of digests #* (RESULT...) |
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==September 12 (Sun)== | ==September 12 (Sun)== | ||
# Miniprep of Fcex, 006, 007, 010, 011 | # Miniprep of Fcex, 006, 007, 010, 011 | ||
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#* ''tried 2 times but couldn't get amplification product!'' | #* ''tried 2 times but couldn't get amplification product!'' | ||
# Transfer to solution culture: 004, 005, 008, 009, 018, 019 | # Transfer to solution culture: 004, 005, 008, 009, 018, 019 | ||
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+ | [[Team:Osaka/Notebook|Back to Notebook]] |
Latest revision as of 09:42, 13 October 2010
September 12 (Sun)
- Miniprep of Fcex, 006, 007, 010, 011
- Restriction digests of 006, 007, 010, 011 with EcoRI, SpeI; Fcex with XbaI, PstI
- Gel electrophoresis of digests
- (RESULTS)
- Ligation for 3A assembly
- 014: 011 as upstream, 1-13D as downstream, 1-3A as vector
- Transformation of 014 using 2μl ligation product with 50μl competent cells
- Moved yesterday's transformation plates (012, 013) to 4°C refrigerator no RFP expression from vector plasmids at all?
- Transfer of A01, A02, A03 (previously transformed) to solution culture
September 13 (Mon)
- Miniprep of A01, A03; restriction digest with EcoRI followed by electrophoresis
- (RESULTS?)
- PCR test
- re-cloning of beta-glucosidase from F1 (received from Edinburgh team) into Silver standard-compatible format
- cloning of pgsC from A01
- note: primers were misdesigned but PCR performed anyway to confirm whether sequences were complementary, and to identify PCR parameters
- Gel electrophoresis of PCR products
- (RESULTS?)
- Gel purification of PCR product from F1
- Restriction digest of PCR product (F1) and 1-5A, both with EcoRI, SpeI
- Gel electrophoresis of PCR product from A01
- band visible around 400~500bp, which was correct length -> PCR conditions identified!
- Transformation of A01, A02, A03
- Transfer of 012, 013, 014 to solution culture
- RFP expressed from vector plasmids on 012, 013 plates during refrigeration period, so selection of colonies with inserts now possible
September 14 (Tue)
- Miniprep of A02, 012, 013, 014
- Restriction digests
- 012, 013, 014 with EcoRI, PstI
- A02 with EcoRI
- Gel electrophoresis of digests
- A02 was discarded (bad size?)
- 012~014: digestions repeated with 1μl each of EcoRI, PstI (previous digestions were 0.5μl each)
- gel electrophoresis of repeat digestions again showed bad sizes for all parts
- 1-13D terminator part is bad? -> cut check of 1-13D
- failure to inactivate restriction enzymes before ligations? -> re-ligation
- 1-13D cut check with XbaI, PstI
- Re-ligation (3A assembly)
- previously digested 009, 008, 011 inactivated at 80°C for 20min before ligation
- 012: 009 as upstream, 1-13D as downstream, 1-3A as vector (same as on 9/11)
- 013: 008 as upstream, 1-13D as downstream, 1-3A as vector (same as on 9/11)
- 014: 011 as upstream, 1-13D as downstream, 1-3A as vector (same as on 9/12)
- Transformation of ligated products (012~014)
- Gel electrophoresis of yesterday's restriction digests of 1-5A and PCR product from F1 followed by their ligation (1-5A as vector, PCR product as insert)
- Transfer of A01, A02, A03 to LB liquid culture medium supplanted with 25μl of 2M glucose to prevent leaky expression from Lac promoter (may be affecting growth)
- Received additional cellulase parts from Karita-sensei: Cel5, Xyn10, Cel44, Man26, Cel8
- plasmid DNA resuspended in 10μl MiliQ water each
- transformation with 2μl DNA solution
September 15 (Wed)
- Miniprep A02, A03 (E. coli failed to grow in A01)
- Cut check of A02, A03 with EcoRI
- A02 is ok
- Transformation of 3-22G
- (INFO?)
- PCR cloning of pgsC from A02
- Colony check & transfer of cellulase parts from Karita-sensei to solution culture
- Preparation of lysis buffer for yeast genome DNA extraction according to [insert reference]
Component | Volume Added | Final Concentration |
---|---|---|
Triton X-100 | 100μl | 2% |
10%SDS | 500μl | 1% |
5M NaCl | 100μl | 100mM |
20mM Tris-HCl(ph8.0) | 2.5ml | 10mM |
0.5M EDTA(ph8.0) | 10μl | 1mM |
dH2O | 1790μl | |
TOTAL | 5ml |
- PCR to clone pgsA, pgsB by 'Megaprimer' method using NEB Phusion polymerase
September 16 (Thu)
- Gel electrophoresis to verify yesterday's PCR results
- pgsA megaprimer: 750bp -> OK
- pgsB megaprimer: 170bp -> OK
- pgsC: 450bp -> very faint band?
- Gel extraction of pgsA, pgsB megaprimers
- 2nd step of megaprimer PCR for pgsA, pgsB
- failure; possible causes:
- short annealing step?
- low denaturation temperature?
- mistakes in procedure?
- failure; possible causes:
- PCR
- pgsC using correct (redesigned) primers
- pgsA, B megaprimer 2nd step repeat using reaction mix composition modified from OpenWetWare
- gel purification of PCR products
- Miniprep of BglX (temporary designation for part cloned from F1 with faulty primer), Cel5, Cel8, Cel44, Man26, Xyn10
- Cut check of miniprepped parts with XbaI, PstI
- Yeast genome DNA extraction (detailed protocol will be provided elsewhere) according to [reference article]
- Gel electrophoresis
- yeast genome DNA
- PCR products
- pgsC -> OK
- Restriction digest
- pgsC (PCR product) with EcoRI, PstI
- 1-1C, 1-3A, 1-5A (vectors) with EcoRI, SpeI
September 17 (Fri)
- PCR cloning of ADH1 terminator from yeast genome DNA
- 4 simultaneous attempts with varying template concentration, thermocycle settings & timing of polymerase addition (before or after initial denaturation)
- gel electrophoresis showed no PCR product obtained for any of the reactions -> annealing temperatures were too stringent?
- PCR of ADH1 terminator (repeat)
- annealing temperature was lowered from 70°C to 60°C
- PCR failed again -> possible RNA contamination?
- PCR of ADH1 terminator (2nd repeat)
- genomic DNA treated with RNase (0.1μl added to 1μl genome DNA; incubation at 37°C for 15min) before using as template
- Gel electrophoresis of yesterday's digests: pgsC, 1-1C, 1-3A, 1-5A
- Miniprep of 013 and 3-22G
- 012, 014 culture solutions have turned red -> picked-up colonies had RFP-carrying vectors, not ligated plasmids; discarded!
- Cut check of 3-22G with XbaI, PstI; 013 with EcoRI, PstI
- (RESULTS?)
- Ligations
- 018: 3A assembly with 004 as upstream, Fcex as downstream, 1-1C as vector
- 019: pgsC as insert, 1-1C as vector (cut at?)
- PCR cloning of XynA CBM, pgsA
- Colony pick-up & transfer to solution culture: 006, 007 (9/10 ligation/transformation) more plasmids needed?
- Transformation of 004, 005, 008, 009, 018, 019
September 18 (Sat)
- PCR cloning of pgsA by overlap extension megaprimer method doesn't seem to work so well
- Gel electrophoresis of PCR product (after overlap step) of pgsA
- correct band seems to be obtained
- Gel extraction followed by restriction digest of PCR product with EcoRI, PstI
- Miniprep of 006, 007
- Restriction digest with EcoRI, PstI followed by gel electrophoresis
- PCR of pgsB (1st fragment for overlap extension)
- tried 2 times but couldn't get amplification product!
- Transfer to solution culture: 004, 005, 008, 009, 018, 019