From 2010.igem.org

Tube	Part to be amplified	Template DNA	Forward primer	Reverse Primer	Melting Temperature (Tm in °C)	Size of the fragment (in bp)	*Extension time (in seconds)**
1	Plasmid Vector	pSB1C3	P1V1 forward	P2V1 reverse	58	2072 approx.	60
2	Pspacoid Promoter	pMutin4	P1P1 forward	P2P1 reverse	49	106 approx.	15
3	1st fragment of rocF CDS	B. subtilis 168 chromosome	P1S1 forward	P2S1 reverse	58	246 approx.	15
4	2nd fragment of rocF CDS	B. subtilis 168 chromosome	P3S2 forward	P4S2 reverse	65	597 approx.	20
5	3rd fragment of rocF CDS	B. subtilis 168 chromosome	P5S3 forward	P6S3 reverse	66	125 approx.	15
6	Double Terminator	pSB1AK3 consisting BBa_B0014 biobrick	P1T1 forward	P2T1 reverse	56	116 approx.	15

Table 1: Table represents 6 different Phusion PCR reactions and the parts which are amplified so that they can be ligated together with the help of Gibson Cloning method.

The extension rate of the Phusion polymerase is at 1Kb/ 30 seconds. Therefore the extension time of each PCR reaction is different.
To learn more about the rocF fragments, please refer to the Cloning strategy for rocF.

Discussion

The 6 Phusion PCR reactions were carried out and gel electrophoresis will be carried out tommorrow to check for the fragments.

Conclusion

Gel electrophoresis will be done tomorrow, 5th August, 2010 to confirm that the RocF fragments have been amplified.

@@ Line 81: / Line 81: @@
 ==Discussion==
-The 6 Phusion PCR reactions were done. However gel electrophoresis was not done to check for the fragments.
+The 6 Phusion PCR reactions were carried out and gel electrophoresis will be carried out tommorrow to check for the fragments.
 ==Conclusion==

Team:Newcastle/4 August 2010

From 2010.igem.org

Revision as of 22:47, 27 October 2010

Contents

Cloning the rocF BioBrick

Aim

Materials and Protocol

Phusion PCR

Discussion

Conclusion