Revision as of 11:55, 19 August 2011

iGEM 2011

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Objectives

PCR of B0015.
PCR of pSB1T3.
See the in Gel.
Restriction of B0015 and pSB1T3 backbone

Working

PCR of B0015

The point of this PCR is get double terminator and insert it into pSB1T3 backbone.

Amplified with preffix and suffix primers.

Reactives	μL
Buffer Taq Standard 10X	5
dNTPs 8mM	1.25
Oligo F/R	2.5/2.5
DNA B0015	1
H₂O	36.75
Taq DNA	1
Total	50μL

Gel B0015

Lane 1. Ladder
Lane 2 & 3. B0015

It's dirty but usefull

PCR of pSB1T3

PCR of pSB1T3/RFP, to amplify just backboney

Reactives	μL
Buffer Taq Platinum 10X	5
dNTPs 8mM	5
MgCl	1.5
Oligo SuffixF/PrefixR	2/2
DNA pSB1T3	1
H₂O	33
Taq Platinum DNA Pol	.5
Total	50μL

All 2X. Two PCRs.

Gel PCR of pSB1T3 backbone

Lane 1 Ladder
Lane 2 & 3 Backbone pSB1T3

As expected :) Both amplified.

Purification of PCR product

Both were purified with Roche´s Kit for PCR purification

Restriction

I performed restriction with EcoRI and PstI.

Poner esto RECUERDA!!!

@@ Line 93: / Line 93: @@
 ==Purification of PCR product==
 Both were purified with Roche´s Kit for PCR purification
+==Restriction==
+I performed restriction with EcoRI and PstI.
+{|
+Poner esto RECUERDA!!!
+|}
 <!-- ##### DO NOT edit below this line unless you know what you are doing. ##### -->
 __NOTOC__

User:Jose Fabricio Lopez/Notebook/Logbook/2011/08/18: Difference between revisions

Revision as of 11:55, 19 August 2011

Objectives

Working

PCR of B0015

Gel B0015

PCR of pSB1T3

Gel PCR of pSB1T3 backbone

Purification of PCR product

Restriction

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