Team:UNIPV-Pavia/Calendar/July/settimana5

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JULY: WEEK 5

July, 26th

July, 27th

July, 28th

July, 29th

We used our new synthesized primers to modify through PCR <partinfo>BBa_K208001</partinfo> phasin in order to create two new parts without stop codon, with Standard prefix and Silver suffix and Silver prefix and suffix.

Gel run for PCR-modified phasins

Gel extraction for phasins showed the following quantifications:

Pha-10S-1: 15 ng/ul
Pha-10S-2: 18,5 ng/ul
Pha-SS-1: 22,8 ng/ul
Pha-SS-2: 22,4 ng/ul

Phasins were digested X-S for 3 hours and were quantified:

Pha-10S-1 (X-S): 14 ng/ul
Pha-10S-2 (X-S): 13,2 ng/ul
Pha-SS-1 (X-S): 15 ng/ul
Pha-SS-2 (X-S): 14,9 ng/ul

Competentization of MC1061 (again) because we suspect the presence of a contaminant (it grew without reason on Cm plates).

Transformation of new MC1061 competent cells with:

1 ul (4ng) of miniprepped ENTERO-pSB4C5 (positive control);
1 ul of RING ligation (RING shouldn't be propagated in MC1061);
1 ul of MilliQ (negative control).

Transformed cells have been plated on Cm 12,5 ug/ml agar plates and incubated overnight at 37°C.

Tecan Test

July, 30th

We checked the presence of colonies in plates.

MC1061 transformed with ENTERO-pSB4C5 (positive control)

MC1061 transformed with RING

MC1061 transformed with MilliQ (negative control)

We calculated (thanks Federica) efficiency as #colonies/ug DNA plated

Strain	Vector	#colonies	Efficiency
MC1061	ENTERO-pSB4C5	3700	~10^6
MC1061	RING	0	-
MC1061	NOTHING	0	-

As espected RING and NOTHING didn't grow. MC1061 competent cells don't replicate RING :) !!!

Miniprep of J04450 to take the vector pSB1A3

3-hour digestion (X-S) and gel run to extract the backbone (~2157 bp).

Culture	Kind	Final reaction volume (ul)	DNA (ul)	H20 (ul)	Enzyme 1 (ul)	Enzyme 2 (ul)	Buffer H
<partinfo>BBa_J04450</partinfo>	Vector	25	17,2	3,3	1 X	1 S	2,5

Gel run of J04450 to take pSB1A3 vector

Gel extraction was quantified 15,5 ng/ul.

Ligation of:

I20: Pha-10S-1 (X-S) + pSB1A3 (X-S)
I21: Pha-SS-1 (X-S) + pSB1A3 (X-S)

July, 31st

Transformation of I20 and I21 into E. coli DH5-alpha. Cells were plated on LB+Amp agar plates and grown overnight at 37°C.

August, 1st

All plates showed colonies (there were also red colonies that contained a wrong ligated plasmid). So we picked three colonies each plate (the right ones) and inoculated them into 5 ml LB+Amp. They were let grow ON at 37°C, 220 rpm.

I20 ligation plate

I21 ligation plate

week 5