Team:Cornell/Week 10

From 2011.igem.org

Revision as of 22:37, 7 August 2011

August 7th - August 13th

Sunday, August 7

Morning lab work done by: Youjin Cho and Claire Paduano

Objective

Prepare VioE in Avi-Tagged pZE12 vector backbone for VioA and VioB gene inserts

Digestion Setup

23.65μL H2O

18.6μL VioE in Avi-Tagged pZE12 vector backbone (1μg)

5μL 10x NEBuffer 2

0.5μL 100x BSA

1.25μL KpnI

1μL HindIII

50μL Total

KpnI has only 75% efficiency in Buffer 2, so added 0.25uL more KpnI to digestion mixture

Incubate in 37°C water bath for 2 hours

Afternoon lab work done by: Jim Mathew, Charlie Chung

Objective

Ligate vioA and vioB genes onto their own pZE12 vector backbone, in place of the vioE that is now digested out

Ligation Reaction Setup

• vioA + Avi-Tagged pZE12 vector backbone

11.4μL pZE12 backbone (cut with KpnI & HindIII; former vioE gene digested out)

3.3μL vioA gene insert (cut with KpnI & HindIII)

2.3μL H2O

2μL 10x T4 DNA ligase buffer

1μL T4 DNA ligase

20μL Total

• vioB + Avi-Tagged pZE12 vector backbone

9μL vioB gene insert (cut with KpnI & HindIII)

8μL pZE12 backbone (cut with KpnI & HindIII; former vioE gene digested out)

2μL 10x T4 DNA ligase buffer

1μL T4 DNA ligase

20μL Total

• Control Ligation for vioA and vioB Gene Inserts

11.4μL pZE12 backbone (cut with KpnI & HindIII; former vioE gene digested out)

5.6μL H2O (gene insert volumes go toward water volume)

2μL 10x T4 DNA ligase buffer

1μL T4 DNA ligase

20μL Total

Incubate all ligation reaction constructs overnight in 16°C waterbath.

Monday

Tuesday

Wednesday

Thursday

Friday

Saturday