Difference between revisions of "Part:BBa K649200:Experience"

Revision as of 08:48, 4 October 2011

Applications of BBa_K649200

In in vitro assay, the part was made linear using restriction enzymes. Cre recombinase was added to the linear DNA and incubated for 0.5, 2, and 4 hours. Images of the experiments have been added below.

[Sample]

sample	volume
PlacIQ-lox2272-GFP-lox2272(pSB1C3)	50 ng/μl × 4 μl
10× Cre recombination Buffer	1 μl
ddH2O	4 μl
Cre recombinase	1,000 units/ml × 1 μl
total	10 μl

[Method]
1. The part on pSB1C3 was made linear by EcoRV restriction site which is far from lox sites.

2. Three identical samples and one negative control supplied with ddH2O instead of Cre-recombinase had been prepared and those were incubated in 37°C for 0.5hr, 2hr and 4hr respectively. Negative control was incubated for 4hr.

3. After a period of time, the samples were kept in -20°C until the whole samples are arranged. The result was checked by electrophoresis
(0.8% EtBr(+) agarose gell, 100V, 400mA, 30min).

User Reviews

UNIQ91fa887f3a37fffe-partinfo-00000000-QINU UNIQ91fa887f3a37fffe-partinfo-00000001-QINU

@@ Line 37: / Line 37: @@
 <br />
 .	The part on pSB1C3 was made linear by EcoRV restriction site which is far from lox sites. <br /><br />
-.	Three identical samples and one negative control without Cre-recombinase had been prepared and those were incubated in 37°C for 0.5hr, 2hr and 4hr respectively. Negative control was incubated for 4hr.<br /><br />
+.	Three identical samples and one negative control supplied with ddH2O instead of Cre-recombinase had been prepared and those were incubated in 37°C for 0.5hr, 2hr and 4hr respectively. Negative control was incubated for 4hr.<br /><br />
 .	After a period of time, the samples were kept in -20°C until the whole samples are arranged. The result was checked by electrophoresis<br />(0.8% EtBr(+) agarose gell, 100V, 400mA, 30min).