"

From 2012.igem.org

Revision as of 08:24, 20 July 2012 (view source) Jeroenbosman (Talk | contribs) ← Older edit		Revision as of 08:45, 20 July 2012 (view source) Jeroenbosman (Talk | contribs) (→week 3: 14 may - 18 may) Newer edit →
Line 57:		Line 57:
	*Preparing samples for dialysis following dialysis protocol		*Preparing samples for dialysis following dialysis protocol
	*Start with dialysis		*Start with dialysis
		+
		+	----
		+	[[https://2012.igem.org/Team:Wageningen_UR/Journal/week2 previous week]]          [[https://2012.igem.org/Team:Wageningen_UR/Journal/week4 next week]]

---

Revision as of 08:45, 20 July 2012

week 3: 14 may - 18 may

Office work

[Life science symposium]

After the great symposium in Delft, we worked further with the protein prediction program phyre2. We've tried different types of modification to the monomers to see if the monomers will drastically change. Further more Thijs and Jasper worked on the webversion of the deconstructor, a program to optimize the PCR cloning strategy. Mark searched for alternative methods to determain if VLPs are formed.

[meeting]

written by: Mark

Lab work

Making competent cells

Tuesday:

• Culture picked for cryo-stock. Grown in 10 ml LB+kan. 10000x diluted plate was used.

Wednesday:

• Transformation results

1. Quality: all non-diluted plates overgrown: good quality
2. Quantity:
1. MACH1 333 3
2. DH5X 105 0

Testing CCMV protocol

Wednesday:

• Making CCMV-strain -80 degree Celcius storage

1. 500 ul overnight culture
2. 500 ul 30% glycerol stock

Thursday:

• CCMV-strain plated
• 1000x from overnight culture for - 80 in 30 degree Celcius
• Plated cryo 1 --> for use to check wheter the storage is good enough

Friday:

• Preparing samples for dialysis following dialysis protocol
• Start with dialysis

---

[previous week] [next week]