Team:SouthBend-Mishawaka-HS-2/Notebook
From 2011.igem.org
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(1)Vortex E0840, J45119, and PSB1T3. | (1)Vortex E0840, J45119, and PSB1T3. | ||
- | (2)Add 1 uL of SpeI enzyme and 1 uL of PstI enzyme to 8 uL of E0840 in order to cut both ends of the wanted DNA. Also add .5 uL of BSA and 5 uL. | + | (2)Add 1 uL of SpeI enzyme and 1 uL of PstI enzyme to 8 uL of E0840 in order to cut both ends of the wanted DNA.<br> Also add .5 uL of BSA and 5 uL. |
- | (3)Add 1 uL of EcoRI enzyme and 1 uL of XbaI enzyme to J45119 in order to cut both ends of the wanted DNA. Also add .5 microliters of BSA and 5 microliters. | + | (3)Add 1 uL of EcoRI enzyme and 1 uL of XbaI enzyme to J45119 in order to cut both ends of the wanted DNA.<br> Also add .5 microliters of BSA and 5 microliters. |
(4)Add 1 uL of EcoRI enzyme and 1 uL of PstI enzyme to PSB1T3 in order to cut both ends of the wanted DNA. | (4)Add 1 uL of EcoRI enzyme and 1 uL of PstI enzyme to PSB1T3 in order to cut both ends of the wanted DNA. | ||
- | (5)Place E0840, J45119, and PSB1T3 in a water bath at 37 degrees C for 20 minutes so that all the parts are sufficiently cut. | + | (5)Place E0840, J45119, and PSB1T3 in a water bath at 37 degrees C for 20 minutes so that all the parts are<br> sufficiently cut. |
- | (6)Assemble the new plasmid by combining 2 uL of E0840, 2 uL J45119, and 2 uL PSB1T3 plasmids in one container. Also add 2 micro liters of buffer and 1 microliter of ligase. | + | (6)Assemble the new plasmid by combining 2 uL of E0840, 2 uL J45119, and 2 uL PSB1T3 plasmids in one container.<br> Also add 2 micro liters of buffer and 1 microliter of ligase. |
(7)Place the new assembly of E0840, J45119, and PSB1T3 in the water bath at 37 degrees C for 20 minutes. | (7)Place the new assembly of E0840, J45119, and PSB1T3 in the water bath at 37 degrees C for 20 minutes. |
Revision as of 14:50, 21 June 2011
Home | Team | Official Team Profile | Project | Parts Submitted to the Registry | Modeling | Notebook | Safety | Attributions |
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Notebook
May 2011
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19 Agenda:Transformation Test Run |
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24 Agenda: Establishment of the K346002 Hg Sensitive Promotor |
25 Agenda: Examining Results of Establishment of the K346002 Hg Sensitive Promotor |
26 Agenda: Examining Results of Establishment of the K346002 Hg Sensitive Promotor Round II
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June 2011
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2 Agenda: Transformation of promoter part K346002 in E.Coli Bacteria |
3 Agenda: No Growth of E.col with K346002 |
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15 |
16 Agenda: Added Enzymes to E0840, J45119, and PSB1T3 |
17Agenda: Change in Promoter from Hg detection to As Detection |
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19 |
20 Agenda: K190015 (ArsR regulated promoter) Transformed |
21 Agenda: K190015 (ArsR regulated promoter) No Growth |
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05/19/11 Agenda:Transformation Test Run
(1) Obtained a vial of 2mL of TOP-10 electro competent E. coli cells 3-16-11 (44-0003/793762)
(2) Added 50 microliters of BIO-RAD transformation solution (Control number 31000008916 recd 1-17-11 GT)
(3) Added 2 microliters of DNA from Registry plate 2 well 5b
(4) Incubate on ice 5 minutes.
(5) Heat shocked 40 degrees C for 50 seconds
(6) Incubated 4 degrees C for 50 seconds
(7) Added 1mL LB 5-17-11 D.G.
(8) Plate 100 microliters and 25 microliters of transformed cells on LB-AMP (5-19-11 "who")
05/24/11 Agenda: Establishment of the K346002 Hg Sensitive Promotor
(1)Electroporation of K346002 into Top 10 cells.
(2)40 microliters of Top 10 cells (JH 5-23-10)10E9 + 2 microliters K346002 DNA from Registry.
(3)Parameters of electroporation: not recorded.
(4)Added 1 microliter of SOB media (JH 2-11-11)immediately after electroporation.
(5)Incubated tube at 37 degrees Celsius for 30 minutes.
(6)Plated 200 microliters of transformation mixture on LB Agar AMP 5 micrograms/microliter (4-21-10).Stored mixture at 4 degrees Celsius.
Expected: 10 to 50 colonies projected to grow.
05/25/11 Agenda: Examining Results of Establishment of the K346002 Hg Sensitive Promotor
(1) Examined results from yesterday: Lawn of bacteria!
(2) Conclusion: No selection either due to inconclusive AMP or fabulous transformation.
(3) Replated 100 microliters K346002 on LB AMP Agar (AM 5-19-11)
Expected: 10 to 50 colonies projected to grow.
05/26/11 Agenda: Examining Results of Establishment of the K346002 Hg Sensitive Promotor Round II
(1) Results: NO GROWTH!
(2) Conclusion: Perhaps no transformation and bad AMP on 4-21-10 plate. However, could still be some transformants present.
(3) Q-tip swabbed up lawn and resuspended in AMP LB broth. Resuspension fluid placed in photospectrometer.
(4) Photospectrometer results for K346002:
Time A600 nm 0 hr. .315 1 hr. .148 2.5 hr. .133
(5) Results: absorbance is declining meaning cells are dying, thus no transformation has resulted. Will leave in incubator overnight to see if transformants grow out.
05/26/11 Agenda: Transforming Top 10 cells to Establish Hg sensitive promoter part K346002
(1) 5 microliters of transformation media (BIO RAD Catalogue 166-0409 received 1-17-11 GT) added to 40 microliters of competent cells in LB broth.
(2) 2 microliters of K346002 DNA added to broth.
(3) Solution was placed in ice bath for 5 minutes.
(4) Placed in 44.7 degree Celsius water for 50 seconds.
(5) Placed in ice bath for 5 minutes.
(6) 1 microliter of SOB buffer at rrom temperature added to broth (in order to close plasmid channels).
(7) PLated 100 microliters of cells on LB AMP plates (5-26-11 AM).
Expected: 10 to 50 colonies projected to grow.
06/02/11 Agenda: Transformation of promoter part K346002 in E.Coli Bacteria
Decided to Transform E.col: three transformations with the E080 part, the J45004 part, and the K346002 part. We follow this procedure.
(1)105 E.col: calls were added to 100ul BioRad Transformation Solution.
(2)1ul of each part of DNA from the Registery was added to the cells which were incubated 30min on ice.
(3)Cells were heat shocked by swirling in water at 42 degree water bath for 2min. Then return to ice for 30min.
(4)1ml 50B buffer was added to the cells and they were incubated for 2 hrs. at room temp.
(5)100ul of the transformed cells were plated on a fresh LB/AMP plate.
06/03/11 Agenda: No Growth of E.col with K346002
The E.col that was transformed on 6/02/11 did not have any growth.
06/16/11 Agenda: Added Enzymes to E0840, J45119, and PSB1T3
(1)Vortex E0840, J45119, and PSB1T3.
(2)Add 1 uL of SpeI enzyme and 1 uL of PstI enzyme to 8 uL of E0840 in order to cut both ends of the wanted DNA.
Also add .5 uL of BSA and 5 uL.
(3)Add 1 uL of EcoRI enzyme and 1 uL of XbaI enzyme to J45119 in order to cut both ends of the wanted DNA.
Also add .5 microliters of BSA and 5 microliters.
(4)Add 1 uL of EcoRI enzyme and 1 uL of PstI enzyme to PSB1T3 in order to cut both ends of the wanted DNA.
(5)Place E0840, J45119, and PSB1T3 in a water bath at 37 degrees C for 20 minutes so that all the parts are
sufficiently cut.
(6)Assemble the new plasmid by combining 2 uL of E0840, 2 uL J45119, and 2 uL PSB1T3 plasmids in one container.
Also add 2 micro liters of buffer and 1 microliter of ligase.
(7)Place the new assembly of E0840, J45119, and PSB1T3 in the water bath at 37 degrees C for 20 minutes.
Ligation
(1)Incubate at room temperature for 10 minutes and then heat inactive at 80 degrees C for 20 min.
(2)Transform 2 uL of the ligation product into 50 uL of competent E. coli cells.
06/17/11 Agenda: Change in Promoter from Hg detection to As Detection
Because of many failed attempts with the Hg promoter, we will be changing our project to a device that detects Arsenic with a promoter that is activated with the presents of arsenic.