"
Page
Discussion
View source
History
teams
Log in
Team:Jilin China/Outline
From 2014.igem.org
Revision as of 03:21, 18 October 2014 by
SimonSong
(
Talk
|
contribs
)
(
diff
)
← Older revision
|
Latest revision
(
diff
) |
Newer revision →
(
diff
)
HOME
TEAM
OUR TEAM
ATTRIBUTION
PROJECT
OUTLINE
CONTRUST
TEST
BLUEPRINT
IDEA
BACKGROUND
DESIGN
PRACTICE
COORPERATION
OBSERVATION
PROPAGATE
SURVEY
ACKNOWLEDGEMENT
Welcome!
Team Jilin_China
May, 2014
Data query and project theme select
Experiment scheme design
Codon optimization of MlrA gene by lactic acid bacteria codons)
MlrA gene sequence design and split
RFP-Mlr-GFP sequence design and split
June, 2014
MlrA gene synthesis and sequence
RFP-Mlr-GFP gene synthesis and sequence
July, 2014
MlrA gene expression and detection
RFP-Mlr-GFP gene expression and detection
Screening of microcystin LR sensitive promoter
August, 2014
construction of the recombinant vector pMG-mlr
construction of the recombinant vector pMG-mlr
Synthetic primer by company (33 pieces in total)
Repeat PCR for many times, recovery them and then get the complete gene product
Sub cloning vector and sequenced
Try to express by E.coli and analyze the effect of this protein
Express by lactic acid bacteria
July to Sept, 2014
Discussion about many possible paths include MC-LR
Try cloning Pseudomonas natural promoter.(non-coding sequences in Mlr enzyme series )
Synthesis by pieces then got complete product.
The gene transformed into E.coli and verify its functions.
Transform this gene by many ways into lactic acid bacteria and verify the function of promoter.
Top