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Team:UCL/Science/Experiment
From 2014.igem.org
Experiments
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About our project
Experiments
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[CHECK these steps with: TO / AD / LB / DT]- Genes, Plasmids, and BioBricks (Genes and Parts that we're working with)
- Expt 00: Identifying and Confirming Necessary BioBricks from iGEM Parts Registry / Distribution (ID, transform, miniprep (MP), digest, gel)
- Expt 01: Isolating and Purifying Genes from Lisbon Plasmids (Transform, MP)
- Expt 02: Confirming Identity of Genes from Lisbon Plasmids (Digest, gel)
- Expt 03: Converting Lisbon Genes into BioBrick Part (Format) (Primer design/order, (site-directed mutatgenesis) PCR)
- Expt 04: Confirming Successful Conversion to BioBirck Format (Subclone: digest, ligate, transform, MP, digest, gel)
- Expt 05: Assembling BioBrick Device(s) (Digest, ligate, transform, MP, digest, gel. Repeat ad infinitum...)
- Expt 06: Characterisation- Azoreductase Assays (See Standard Operating Procedure (SOP))
Genes, Plasmids, and BioBricks
[CHECK: column width adjustment!][Internal hyperlinks to different sections?]
| No. | ID | Name / Function | Source | State / Concentration / Date Made | Gene Size / Sequence | Initial Plasmid / Vector | Comments |
|---|---|---|---|---|---|---|---|
| 1 | pAzoR / BBa_K1336000 | FMN-dependent NADH-azoreductase 1 | Pseudomonas putida | Miniprep,
48 ng/uL, 15/07/17, TO. |
597 bp [Check! Not 612 bp?],
Genomic Sequence |
Expression vector pET-21a (+) (ampicillin resistant (ampR)), initially cloned between NdeI and BamHI. | Plasmid provided by Lisbon; with Paper. |
| 2 | p1B6 (AzoR 1B6) / BBa_K1336001 | Mutant: Heat-stable; FMN-dependent NADH-azoreductase 1 | Pseudomonas putida | Miniprep,
68 ng/uL, 15/07/14, TO. |
597 bp [Check! Not 612 bp?],
Genomic Sequence[Add sequence! Sent from Lisbon, see DT] |
Expression vector pET-21a (+) (ampR), initially cloned between NdeI and BamHI. | Plasmid provided by Lisbon; with Paper. |
| 3 | pCotA / BBa_K1336002 | Spore Coat Protein Laccase | Bacillus subtilis | Miniprep,
103 ng/uL, 15/07/14, TO. |
1733 bp [Check! Not 1539 bp?]
Genomic Sequence[Add sequence! Sent from Lisbon, see DT] |
Expression vector pET-21a (+) (ampR), initially cloned between NheI and BamHI. | Plasmid provided by Lisbon; with Paper. |
| 4 | LiP / BBa_K1336003 | Lignin Peroxidase | Phanerochaete chrysosporium (White-Rot Fungi) | [Being synthesised by Gene Oracle],
X ng/uL, dd/mm/yy, Gene Oracle. |
X bp,
Genomic Sequence |
[Cloned directly into expression vector, pSB1C3, between EcoRI and PstI.] | Synthesised (for free) by Gene Oracle. Sequence from Paper. |
| 5 | pBsDyP / BBa_K1336004 | Dye Decolourising Peroxidase BSU38260 | Bacillus subtilis | Miniprep,
51 ng/uL, 15/07/14, TO. |
1251 bp,
Genomic Sequence[Add sequence! Sent from Lisbon, see DT] |
Expression vector pET-21a (+) (ampR), initially cloned between NdeI and BamHI. | Plasmid provided by Lisbon; with Paper. |
| 6 | pPpDyP / BBa_K1336005 | Dye Decolourising Peroxidase PP_3248 | Pseudomonas putida | Miniprep,
55 ng/uL, 15/07/14, TO. |
861 bp [Check! Not 864 bp?],
Genomic Sequence[Add sequence! Sent from Lisbon, see DT] |
Expression vector pET-21a (+) (ampR), initially cloned between NdeI and BamHI. | Plasmid provided by Lisbon; with Paper. |
| 7 | BBa_J04450 | RFP Coding Device | Spring 2014 BioBrick Distribution.
Plate 4, Well 4B. [Check! DT?]. |
(1) Miniprep,
333 ng/uL, 01/07/14, TO. (2) Miniprep, 38 ng/uL (NanoDrop, dodgy!) 01/07/14, TO. |
1069 bp,
Genomic Sequence[Add sequence! Made from combined BioBricks?] |
Plasmid Backbone: pSB1C3, i.e. chloramphenicol resistant (camR). | LacI-, and CAP-, sensitive; can fail if system contains LacI or CAP protein!
RFP Coding Device contains: LacI (R0010), strong RBS (B0034), mRFP1 (E1010), and double terminator (B0015 = B0010+B0012). |
| 8 | BBa_R0010 | Promoter (LacI regulated) | Spring 2014 BioBrick Distribution.
Plate 3, Well 4G. [Check! DT?]. |
Miniprep,
329.1 ng/uL, 01/07/14, TO. |
200 bp,
Genomic Sequence[Add sequence!] |
Plasmid Backbone: pSB1C3, i.e. chloramphenicol resistant (camR).
Plasmid / Vector Map. |
This part is an inverting regulator sensitive to LacI and CAP. In the absence of LacI and CAP proteins, this part promotes transcription; in their presence, the part inhibits transcription. LacI can be inhibited by IPTG. |
| 9 | BBa_R0011 | Promoter (LacI regulated, lambda pL hybrid) | Spring 2014 BioBrick Distribution.
Plate 2, Well 6D (Inconsistent sequencing!). [Check! DT? / Maybe use Spring 2013 Distribution, Plate 5, Well 6G.]. |
Miniprep,
38 ng/uL (NanoDrop, dodgy!), 01/07/14, TO. |
55 bp,
Genomic Sequence[Add sequence!] |
Plasmid Backbone: pSB1C3, i.e. chloramphenicol resistant (camR).
Plasmid / Vector Map. |
Inverting regulatory region controlled by LacI (BBa_C0010, BBa_C0012, etc.) The PLlac 0-1 promoter is a hybrid regulatory region consisting of the promoter P(L) of phage lambda with the cI binding sites replaced with lacO1. |
| 10 | BBa_K314103 | Lac induced expression cassette | Spring 2014 BioBrick Distribution.
Plate 1, Well 4D. [Check! DT?]. |
Miniprep,
334 ng/uL, 01/07/14, TO. |
1638 bp,
Genomic Sequence[Add sequence!] |
Plasmid Backbone: pSB1C3, i.e. chloramphenicol resistant (camR).
Plasmid / Vector Map. |
Lactose (IPTG) inducible protein expression insert includes f1 origin (K314110), a Lac I generator (K314111), a lactose inducible promoter (R0011), and the Elowitz standard RBS (B0034). |
| 11 | BBa_K206000 | pBAD Strong Promoter | Spring 2014 BioBrick Distribution.
Plate 3, Well 14A. [Check! DT?]. |
Miniprep,
144 ng/uL, 01/07/14, TO. |
130 bp,
Genomic Sequence[Add sequence!] |
Plasmid Backbone: pSB1C3, i.e. chloramphenicol resistant (camR).
Plasmid / Vector Map |
pBAD is an E. coli promoter that is induced by L-arabinose. In the absence of arabinose, the repressor protein AraC (BBa_I13458) binds to the AraI1 operator site of pBAD and the upstream operator site AraO2, blocking transcription; in its presence, transcription is permitted. |
| 12 | BBa_B0034 | RBS | Spring 2014 BioBrick Distribution.
Plate 4, Well 1N. [Check! DT?]. |
Miniprep,
156.5 ng/uL, 01/07/14, TO. |
12 bp,
Genomic Sequence[Add sequence!] |
Plasmid Backbone: pSB1A2, i.e. ampicillin resistant (ampR).
Plasmid / Vector Map |
RBS based on Elowitz (1999) repressilator. |
| 13 | BBa_K518012 | RBS + RFP + double Terminator | Spring 2014 BioBrick Distribution.
Plate 1, Well 18C. [Check! DT?]. |
(1) Miniprep,
49 ng/uL, 01/07/14, TO. (2) Miniprep, 219.2 ng/uL, 08/08/14, YKH. |
828 bp,
Genomic Sequence[Add sequence!] |
Plasmid Backbone: pSB1C3, i.e. chloramphenicol resistant (camR).
Plasmid / Vector Map |
This Coding Device contains: RBS.3 (medium) (B0032), mRFP1 (E1010), and double terminator (B0014 = B0012+B0011). |
| 14 | [CHECK: BAD PART !]
BBa_B0012 (2) |
Transcription Terminator for E. coli RNA polymerase | Spring 2014 BioBrick Distribution.
Plate 2, Well 2B. [Check! DT?]. |
Miniprep,
128 ng/uL, 01/07/14, TO. |
41 bp,
Genomic Sequence[Add sequence!] |
Plasmid Backbone: pSB1C3, i.e. chloramphenicol resistant (camR).
Plasmid / Vector Map |
TE from coliphage T7. This is a bad terminator (Experience: Fails). It is a promoter in the reverse direction. |
| # | ID | Name / Function | Source | State / Concentration / Date Made | Gene Size / Sequence | Initial Plasmid / Vector | Comments |
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Pellentesque habitant morbi tristique senectus et netus et malesuada fames ac turpis egestas. Vestibulum tortor quam, feugiat vitae, ultricies eget, tempor sit amet, ante. Donec eu libero sit amet quam egestas semper. Aenean ultricies mi vitae est. Mauris placerat eleifend leo. Quisque sit amet est et sapien ullamcorper pharetra. Vestibulum erat wisi, condimentum sed, commodo vitae, ornare sit amet, wisi. Aenean fermentum, elit eget tincidunt condimentum, eros ipsum rutrum orci, sagittis tempus lacus enim ac dui. Donec non enim in turpis pulvinar facilisis. Ut felis.
Pellentesque habitant morbi tristique senectus et netus et malesuada fames ac turpis egestas. Vestibulum tortor quam, feugiat vitae, ultricies eget, tempor sit amet, ante. Donec eu libero sit amet quam egestas semper. Aenean ultricies mi vitae est. Mauris placerat eleifend leo. Quisque sit amet est et sapien ullamcorper pharetra. Vestibulum erat wisi, condimentum sed, commodo vitae, ornare sit amet, wisi. Aenean fermentum, elit eget tincidunt condimentum, eros ipsum rutrum orci, sagittis tempus lacus enim ac dui. Donec non enim in turpis pulvinar facilisis. Ut felis.
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