Difference between revisions of "Team:MIT/InterlabStudy"
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| − | The iGEM Interlab Study's aim | + | The iGEM Interlab Study's aim is "to obtain fluorescence data for three specific genetic devices expressing GFP from iGEM teams around the world”. It is an opportunity for teams throughout the world to build and characterize parts. The purpose of the study as a whole is to be able to “test the consistency of the teams’ data of the measured devices”. |
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DNA Kit Plate Instructions (http://parts.igem.org/Help:2015_DNA_Distribution) | DNA Kit Plate Instructions (http://parts.igem.org/Help:2015_DNA_Distribution) | ||
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• if growing from another liquid culture, 100 uL should be plenty (replacing the 1 colony). Almost no amount is too small, just ensure that you get cells. | • if growing from another liquid culture, 100 uL should be plenty (replacing the 1 colony). Almost no amount is too small, just ensure that you get cells. | ||
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<a href = "http://www.hawaii.edu/microbiology/MO/docs/diversity/Qia-Miniprep.pdf">Miniprep – using Qiagen protocol</a> | <a href = "http://www.hawaii.edu/microbiology/MO/docs/diversity/Qia-Miniprep.pdf">Miniprep – using Qiagen protocol</a> | ||
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Making Liquid Culture (see above) | Making Liquid Culture (see above) | ||
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Generalized E coli Flow Cytometry Protocol( created by Nicholas Delateur Weiss Lab MIT) | Generalized E coli Flow Cytometry Protocol( created by Nicholas Delateur Weiss Lab MIT) | ||
Revision as of 15:15, 13 September 2015
Project
Interlab Study
Introduction
The iGEM Interlab Study's aim is "to obtain fluorescence data for three specific genetic devices expressing GFP from iGEM teams around the world”. It is an opportunity for teams throughout the world to build and characterize parts. The purpose of the study as a whole is to be able to “test the consistency of the teams’ data of the measured devices”.
Devices Built and Measured: (Chassis : E coli)
Device 1 : J23101 + I13504 (B0034-E0040-B0015) -> backbone:PSB1C3 (3 biological replicates)
Device 2 : J23106 + I13504 (B0034-E0040-B0015) -> backbone:PSB1C3 (3 biological replicates)
Device 3 : J23117 + I13504 (B0034-E0040-B0015) -> backbone: PSB1C3 (3 biological replicates)
Device 2 : J23106 + I13504 (B0034-E0040-B0015) -> backbone:PSB1C3 (3 biological replicates)
Device 3 : J23117 + I13504 (B0034-E0040-B0015) -> backbone: PSB1C3 (3 biological replicates)
Measurement Controls:
Positive Control: I20270 PSB1C3 -> J23151 + I20270(B0032-E0040-B0010-B0012)
Negative Control: BBa_R0040
Negative Control : NEB 10 B Competent Cells
Negative Control: BBa_R0040
Negative Control : NEB 10 B Competent Cells
Protocols:
DNA Kit Plate Instructions (http://parts.igem.org/Help:2015_DNA_Distribution)
Transformation (http://parts.igem.org/Help:Protocols/Transformation)
Making Liquid cultures:
Transformation (http://parts.igem.org/Help:Protocols/Transformation)
Making Liquid cultures:
- • Prepare culture in a 15 mL, round bottom tube.
- • Add 5mL LB using a seriological pipette • Add 5uL of 1000x antibiotic (Chloramphenicol.)
- • Pick colony using a 10 ul pipette tip on a p2. Eject tip into tube (tip should remain in tube). • if growing from another liquid culture, 100 uL should be plenty (replacing the 1 colony). Almost no amount is too small, just ensure that you get cells. Miniprep – using Qiagen protocol 3 Antibiotic Assembly protocol Transformation Colony PCR (selecting transformants from the transformation plates) Making Liquid Culture (see above)
Measuring in flow cytometer
1) measured beads
2) measured 3 types of devices
3) measured positive control : I20270 (GFP construct)
4) measure negative controls : Untransformed competent cell and R0040
Sequencing
