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Revision as of 18:35, 9 August 2010 (view source) Zacstewart (Talk | contribs) (→Notebook) ← Older edit		Revision as of 18:36, 9 August 2010 (view source) Zacstewart (Talk | contribs) (→August 8, 2010) Newer edit →
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	===August 8, 2010===		===August 8, 2010===
	''Joe''		''Joe''
-	Prepared YPD+sorbitol	+	*Prepared YPD+sorbitol
	**10g yeast extract		**10g yeast extract
	**20g peptone		**20g peptone

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Revision as of 18:36, 9 August 2010

• Home
• Project
  • About The Toolkit
  • Oursystem
  • Producing The Antigen
  • Future Applications
  • Safety
• Toolkit
• Why Pichia
  • Pichia Vs Saccharomyces
  • Easy and Inexpensive to Culture
  • High production of foreign Protein while low levels of endogenous protein
  • Pichia pastoris versus Esherichia coli
• Protocols
  • Preparation Of Electrocompetent Cells
  • Preparation of Heat Shock Competent Cells
  • Transformation Using Electroporation
  • Transformation Using Heat Shock
• The Team
• Notebook

Contents 1 Notebook 1.1 August 8, 2010 1.2 August 5, 2010 1.3 August 4, 2010 1.4 August 3, 2010 1.5 July 22, 2010 1.6 July 20, 2010 1.7 July 15, 2010 1.8 July 14, 2010 1.9 July 13, 2010 1.10 July 8, 2010 1.11 July 7, 2010 1.12 July 6, 2010 1.13 July 2, 2010 1.14 July 1, 2010

Notebook

August 8, 2010

Joe

• Prepared YPD+sorbitol
  • 10g yeast extract
  • 20g peptone
  • 182.2g sorbitol
  • 900ml H₂0
• Inoculated 250ml flash of YPD with P. pastoris from 6-29-10 culture in SAB
  • added 500ml of SAB culture into ≈100-125ml YPD, stored in shaker in 30°C incubator

August 5, 2010

• 12E SpeI protocol, PstI protocol
• 9A PstI proocol
• 9A was purified as the Xba I previously used on it was not fast digest
• Gel extraction of 9A and 12E

August 4, 2010

Virginia 12E plasmid extraction from 5-min kit. Lysis solution and wash buffer taken from eppendorf kit needs to be confirmed on Nano Drop.

August 3, 2010

Joe, Virginia

• Tried to extract 12E plasmid with Jetgene kit starting with cells stored in resuspension buffer. (Started with step 2). Cell solution was very viscous. Difficult to pipette. Did not form a pellet in step 4.
• Inoculated LB+Ampicillin with 12E and stored at 37°C from glycerol stock in -80°C.
  • Will try again with fresh cells
  • Ran out of buffer in Jetgene kit.

July 22, 2010

Virginia

• Prep LB, YPD plate solution
• Prep NEB 2+3 buffer solutions

July 20, 2010

Melissa, Alykhan

• Prepared tris HCl for buffer solutions

July 15, 2010

Virginia, Angie, Alykhan, Joe

• Cut plasmid and ligated
• P. pastoris cells ready in -80°C

July 14, 2010

Virginia, Joe, Angie, Alykhan

• 10 glycerol stocks of 12E
• P. pasoris competent cells
• Started, ready at 2pm
• Plamid resuspension buffer made
• LB agar aliquots
  • warm in water bath
  • one 10mL tube for 1L agar
• extraction of 12E+9A plasmid parts: white tubes in freezer

July 13, 2010

Virginia

• 10 glycerol stocks of each
  • P. pastoris
  • 9A E. coli
• Inoculated 12E broth for plasmid extract and glycerol stocks
• Plate of P. pastoris for quality control

July 8, 2010

Angie, Kendra, Melissa, Nishedh, Alykhan

• Diluted pichia cells in a volume of 50mL to a OD₆₀₀ = .186+.201
• Transform pars 12E and 12M into E. coli

July 7, 2010

Joe, Kendra, Angie

• Replated colonies from 9A RFP plate (3 plates).
• Colonies on broth 100 µL for 9A but no fluorescence observed
• 9A survivor colonies replated onto 10 µg/mL ampicillin plates and incubated at 30°C
• Mother plate in fridge
• Made 1000mL YPD
• Growing P. anomala in YPD broth for competent cells protocol

July 6, 2010

Dan

• Replated E. coli culture

Alykhan

• Transformation 9A, 8I (digested) & GFP.

July 2, 2010

Alykhan and Virginia

• DNA purification and ligation
• Replated E. coli culture

July 1, 2010

Joe

• Plated transformed cells containing either GFP (control) or iGEM part onto LB plates with 10µg/mL ampicillin (2 plates each, 10mL or 100mL)
• Also plated ≈100mL (remaining amount) of cells onto LB plates not containing ampicillin.
• Spread plates with hockey stick and placed in 37°C at 7:35.