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Revision as of 19:20, 27 April 2010 (view source) IGEM HQ (Talk | contribs) (Prototype team page) ← Older edit		Revision as of 15:14, 12 July 2010 (view source) Zacstewart (Talk | contribs) (Copied lab notebook) Newer edit →
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-	{|align="justify"
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-	|[[Image:Georgia_State_logo.png|200px|right|frame]]
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	==Notebook==		==Notebook==
		+	===July 8, 2010===
		+	''Angie, Kendra, Melissa, Nishedh, Alykhan''
		+	*Diluted pichia cells in a volume of 50mL to a OD<sub>600</sub> = .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&deg;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
-	You should make use of the calendar feature on the wiki and start a lab notebook.  This may be looked at by the judges to see how your work progressed throughout the summer.  It is a very useful organizational tool as well.	+	===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&deg;C at 7:35.

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Revision as of 15:14, 12 July 2010

Home	Team	Official Team Profile	Project	Parts Submitted to the Registry	Modeling	Notebook	Safety

Contents 1 Notebook 1.1 July 8, 2010 1.2 July 7, 2010 1.3 July 6, 2010 1.4 July 2, 2010 1.5 July 1, 2010

Notebook

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.