User:DrJones1935/21 July 2012

From 2012.igem.org

I. PCR

  • Mix Reagents:
  • Mix according to the following table, where 2 = LacZ, 3 = CAT*, 4 = tetr, 0.1-0.3 = +template, and 0.4 = -template
  • For example, 2.1 = lacZ sample, 2.4 = lacZ control
2.1 2.2 2.3 2.4 3.1 3.2 3.3 3.4 4.1 4.2 4.3 4.4
Reagent (uL) (uL) (uL) (uL) (uL) (uL) (uL) (uL) (uL) (uL) (uL) (uL)
water 33.5 33.5 33.5 33.5 33.5 33.5 33.5 33.5 32.5 32.5 32.5 33.5
5x Phusion HiFi buffer 10 10 10 10 10 10 10 10 10 10 10 10
10 mM dNTP mix 1 1 1 1 1 1 1 1 1 1 1 1
10 uM primer (F) 2.5 (p2f_2) 2.5 (p2f_2 2.5 (p2f_2) 2.5 (p2f_2) 2.5 (p3f_2) 2.5 (p3f_2) 2.5 (p3f_2) 2.5 (p3f_2) 2.5 (p4f) 2.5 (p4f) 2.5 (p4f) 2.5 (p4f)
10 uM primer (R) 2.5 (p2r_2) 2.5 (p2r_2) 2.5 (p2r_2) 2.5 (p2r_2) 2.5 (p3r) 2.5 (p3r) 2.5 (p3r) 2.5 (p3r) 2.5 (p4r_2) 2.5 (p4r_2) 2.5 (p4r_2) 2.5 (p4r_2)
Template ECNR2 colony* ECNR2 colony* ECNR2 colony* 0 ECFI5 colony* ECFI5 colony* ECFI5 colony* 0 1 (pBR322) 1 (pBR322) 1 (pBR322) 0
Phusion HiFi polymerase 0.5 0.5 0.5 0.5 0.5 0.5 0.5 0.5 0.5 0.5 0.5 0.5

*For these templates, I touched a colony with a sterile pipette tip and spread it on the bottom of the PCR tube before adding reagents

  • Run PCR
Step Temp (oC) Time
1 94 4 m
2 94 30 s
3 53 30 s
4 72 1.5 m
5 GOTO 2 7x
6 94 30 s
7 66 30 s
8 72 1.5 m
9 GOTO 6 30x
10 72 5 m
11 4 ∞*
  • Store tubes on ice after PCR is finished