Indiana/1 July 2009

From 2009.igem.org

(Difference between revisions)
 
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Remove Xba1 and Spe1 sites from pCB302
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'''Remove Xba1 and Spe1 sites from pCB302'''
1 uL pCB302 @ ~10ng/ul
1 uL pCB302 @ ~10ng/ul
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incubate 1 hour @ 37 C
incubate 1 hour @ 37 C
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'''Ligate plasmid back together'''
following incubation add the following the reaction:
following incubation add the following the reaction:
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Transform newly modified plasmid into E. coli  
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'''Transform newly modified plasmid into E. coli'''
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5 uL of reaction mixture into chemically competent E. coli
5 uL of reaction mixture into chemically competent E. coli
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Pull Parts from Kit:
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'''Pull Parts from Kit'''
J45119 - wintergreen
J45119 - wintergreen

Latest revision as of 19:05, 19 July 2009

Construction of plant plasmid pCB302 to fit iGEM standards.


Remove Xba1 and Spe1 sites from pCB302

1 uL pCB302 @ ~10ng/ul

2 uL NEB buffer 4

.3 uL Xba1

.3 uL Spe1

16.4 uL ddH2O


incubate 1 hour @ 37 C


Ligate plasmid back together

following incubation add the following the reaction:

4 uL ligase buffer

1 uL ligage

15 uL ddH2O

incubate at 16 C for ~3 hours



Transform newly modified plasmid into E. coli


5 uL of reaction mixture into chemically competent E. coli

keep on ice for 15 min

heat shock @ 37 C for 2 minutes

add to 500 uL LB, shake at 37 C for 30-60 minutes

spin down and resuspend in a smaller volume (50-100uL)

plated on kanmyacin plates




Pull Parts from Kit

J45119 - wintergreen

J45199 - banana

psB1AT3 - plasmid backbone

1) add 15 uL ddH2O to proper well on plate

2) let sit for ~5 minutes

3) transfer to tube for storage

4) transform using 1uL of part