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From 2012.igem.org

Revision as of 07:38, 6 June 2012 (view source) MarkvanVeen (Talk | contribs) (→week 5: 4 june - 8 june) ← Older edit		Revision as of 09:25, 7 June 2012 (view source) MarkvanVeen (Talk | contribs) (→Office work) Newer edit →
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	*Design the master-plan for the wiki further		*Design the master-plan for the wiki further
	*Creating the wiki homepage		*Creating the wiki homepage
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	Wednesday:		Wednesday:
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	*Changing every Wensday into Wednesday		*Changing every Wensday into Wednesday
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		+	Thursday:
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		+	*Update notebook and protocols
	'''Munich'''		'''Munich'''
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	Monday:		Monday:

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Revision as of 09:25, 7 June 2012

week 6: 4 june - 8 june

Office work

Wiki page

Monday:

• Update notebook and protocols
• Start to disign the master-plan for wiki page
• Creating the wiki template further

This monday we've worked further on updating the wiki, we are now on schedule with the notebook and protocols. We also made a master plan on how the wiki should look like. The first steps are being made to create a prize winning wiki page.

Tuesday:

• Update notebook and protocols
• Design the master-plan for the wiki further
• Creating the wiki homepage

Wednesday:

• Update notebook and protocols
• Changing every Wensday into Wednesday

Thursday:

• Update notebook and protocols

Munich

Monday:

• Review the two abstracts

Tuesday:

• Review further the two abstacts
• Submit the abstracts

Other

Tuesday:

• Start designing the WageningenUR clothing

[Meeting]

written by: Mark

Lab work

CCMV Bricking:

Monday:

• Check agar plates for colonies
• Grow colonies in LB medium + kanamycin, checked optical density
• Colonies:

1. CCMV-1
2. CCMV-2
3. d26-CCMV-1
4. d26-CCMV-2
5. d26-CCMV-3

• overnight in shaker 37 degree Celcius

The monday morning of this week started with a bit of a shock: our plates with our transformed E.coli we're almost completely empty. Luckely there was at least one colony on both of the plates with transformed E.coli containing bricks. We put them in Greiner tubes with LB-medium and a antibiotic and after a few hours checked their optical density. In the afternoon we prepared the samples for a PCR to validate the bricks.

Tuesday:

• Checked Greiner tubes
• Colonies:

1. CCMV-1: growth
2. CCMV-2: no growth
3. d26-CCMV-1: growth
4. d26-CCMV-2: growth
5. d26-CCMV-3: growth

• Mini prep the 4 remaining samples
• Prepare the mini prep samples for PCR
• Run the PCR
• Check PCR, not succesful digestion repeat process tomorrow.

Wednesday:

• Prepare the mini prep samples for PCR

CCMV test protocol:

Monday:

• Prepared two samples for dialysis according to the dialysis protocol
• Change: instead of sonicator for cell lysis, French press was used for one of the samples

We've also made two samples of wt CCMV VLP ready for dialysis. There is only one modification applied in the protocol, instead of using the horrible sonicator, we used the French press, which is a great apparatus and easy to use. In the late afternoon we started with the dialysis.

Tuesday:

• Changed the buffer 3 times according to the dialysis protocol
• Made an appointment for DLS

Wednesday:

• Changed the buffer 3 times according to the dialysis protocol

written by: Mark