Latest revision as of 15:35, 16 October 2011

Introduction
Our Project
Tools
- Gibson Assembly
- MITOMI
Notebook
- Protocols
- May
- June
- July
- August
- September
- October
Considerations
- Human Practices
- Safety
Acknowledgements
- Sponsors
- Partners

Protocols

Molecular Biology

Products and stock preparation

Primer preparation: initial dilution of ordered primers.
Competent Cells: prepare cells for plasmid uptake.
Competent Cells. Protocol II (Inoue method).
Glycerol stock: stock transformed cells at -80°C.
Agar plate preparation: preparing agar plates for cell cultures.
Autoclave: to sterilize solutions and glassware.

Cloning, assembly, and mutations

Transformation: introduce foreign plasmid into competent cells.
Plating: plate transformed cells
Liquid cultures: when cells have grown on plates, put them in liquid cultures
Gibson assembly.
Linear template- TetR.
tetR Overlap Extension PCR: induce specific mutations on tetR linear template.
tetR Site-specific mutagenesis: induce site-specific mutations on a plasmid containing tetR.
Agarose gel electrophoresis: DNA samples analysis (can be followed by band purification).
Colony PCR: Analyze the plated transformed cells, to see if Gibson assembly worked
T7 extension PCR: Put T7 promoter upstream of a gene
Blunt-End Cloning: Making Blunt Ends

DNA recovery

Plasmid preparation - Miniprep: recover plasmids from a bacterial culture.
Gel purification: recover DNA separated by electrophoresis

Biochemistry

IPTG test: test expression of a gene downstream from Plac

Microfluidics

Worm culture

Agar plate preparation: preparing MG Agar plates for worm cultures.

@@ Line 1: / Line 1: @@
-==PDMS 2 layer device fabrication   ==16.05.2011
+{{:Team:EPF-Lausanne/Templates/Header|title=Protocols}}
-"Materials":
+== Molecular Biology ==
-•	flow and control layer molds
+=== Products and stock preparation ===
-•	Sylgard 184 silicone elastomer kit: Base part and a Curing agent
+* [[Team:EPF-Lausanne/Protocols/Primers preparation|Primer preparation]]: initial dilution of ordered primers.
-•	TMCS
+* [[Team:EPF-Lausanne/Protocols/Competent cells|Competent Cells]]: prepare cells for plasmid uptake.
+* [[Team:EPF-Lausanne/Protocols/Competent cells. Protocol II|Competent Cells. Protocol II (Inoue method)]].
+* [[Team:EPF-Lausanne/Protocols/Glycerol stock|Glycerol stock]]: stock transformed cells at -80°C.
+* [[Team:EPF-Lausanne/Protocols/Agar Plates|Agar plate preparation]]: preparing agar plates for cell cultures.
+* [[Team:EPF-Lausanne/Protocols/Autoclave|Autoclave]]: to sterilize solutions and glassware.
-"Method":
+=== Cloning, assembly, and mutations ===
-•	Place molds into a TMCS vapor chamber
+* [[Team:EPF-Lausanne/Protocols/Transformation|Transformation]]: introduce foreign plasmid into competent cells.
-•	Control layer mixture: 20g Base + 4g Curing agent
+* [[Team:EPF-Lausanne/Protocols/Plating|Plating]]: plate transformed cells
-•	Mix for 1 minute, degas for 2 minutes (standard protocol)
+* [[Team:EPF-Lausanne/Protocols/Liquid cultures|Liquid cultures]]: when cells have grown on plates, put them in liquid cultures
-•	pour onto control layer mold and place mold in vacuum chamber
+* [[Team:EPF-Lausanne/Protocols/Gibson assembly|Gibson assembly]].
-•	Flow layer mixture: 20g Base + 1g Curing agent
+* [[Team:EPF-Lausanne/Protocols/TetR|Linear template- TetR]].
-•	Mix for 1 minute and degas for 2 minutes (standard protocol)
+* [[Team:EPF-Lausanne/Protocols/TetR Extension PCR|tetR Overlap Extension PCR]]: induce specific mutations on tetR linear template.
-•	Spin coat onto flow layer at 2200-2400rpm for 35secs (so far you can use my protocol on a spin coater)
+* [[Team:EPF-Lausanne/Protocols/Site-specific mutagenesis|tetR Site-specific mutagenesis]]: induce site-specific mutations on a plasmid containing tetR.
-•	Remove control layer mold from vacuum chamber, making sure no bubbles are left on the surface (remove with a toothpick if you see some )
+* [[Team:EPF-Lausanne/Protocols/Gel_Electrophoresis|Agarose gel electrophoresis]]: DNA samples analysis (can be followed by band purification).
-•	Place the control and flow layer in a 80C convection oven and incubate for 30 minutes (timing is critical here!)
+* [[Team:EPF-Lausanne/Protocols/Colony PCR|Colony PCR]]: Analyze the plated transformed cells, to see if Gibson assembly worked
-•	Remove casts from oven, cut out control layer, punch holes, and align to flow layer
+* [[Team:EPF-Lausanne/Protocols/T7-ext|T7 extension PCR]]: Put T7 promoter upstream of a gene
-•	Put aligned device back into 80C oven and incubate for at least 90 minutes (and here you can increase the backing)
+* [[Team:EPF-Lausanne/Protocols/bluntends|Blunt-End Cloning]]: Making Blunt Ends
-•	Remove devices from oven and punch flow layer holes
+=== DNA recovery ===
+* [[Team:EPF-Lausanne/Protocols/Miniprep|Plasmid preparation - Miniprep]]: recover plasmids from a bacterial culture.
+* [[Team:EPF-Lausanne/Protocols/Gel purification|Gel purification]]: recover DNA separated by electrophoresis
+== Biochemistry ==
+* [[Team:EPF-Lausanne/Protocols/IPTG test|IPTG test]]: test expression of a gene downstream from Plac
+== Microfluidics ==
+* [[Team:EPF-Lausanne/Protocols/PDMS_two_layer_device_fabrication|PDMS two layer device fabrication]]
+* [[Team:EPF-Lausanne/Protocols/Master microfabrication for PDMS replica molding |Master microfabrication for PDMS replica molding]]
+* [[Team:EPF-Lausanne/Protocols/MITOMI_protein_DNA|MITOMI: Protein – DNA interactions]]
+* [[Team:EPF-Lausanne/Protocols/Klenow dsDNA synthesis|Klenow dsDNA synthesis]]
+== Worm culture ==
+* [[Team:EPF-Lausanne/Protocols/MG_Agar_Plates|Agar plate preparation]]: preparing MG Agar plates for worm cultures.
+{{:Team:EPF-Lausanne/Templates/Footer}}

Team:EPF-Lausanne/Protocols

From 2011.igem.org

Latest revision as of 15:35, 16 October 2011

Protocols

Contents

Molecular Biology

Products and stock preparation

Cloning, assembly, and mutations

DNA recovery

Biochemistry

Microfluidics

Worm culture