Team:TUDelft/3 August 2009

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3 August 2009

Calin

Tim pointed out that the plasmids should be linearized before doing the gel. Here are possible digestions on some of the parts:

Backbone Part Unique Sites Present
pSB1A2 oriT-R AatII AccI AflIII BglI BspLU11I BstAPI
DrdI Eam1105I EcoRI FspI NspI PstI
PvuI RsaI ScaI
SgrAI SpeI SspI
StyI TatI VspI XbaI XmnI ZraI
BBa_J61002 strong promoter AatII AlwNI AvrII BglI BsiWI BspLU11I
BstXI DrdI EcoRI FspI HaeII HpaI
NcoI NspI PflMI PshAI PstI PvuI
PvuII RsrII ScaI SgrAI SpeI SspI
TatI VspI XbaI XmnI ZraI
pSB1AK3 ccdB AatII AccB1I AccI BamHI BanII BglI
BspLU11I
BsrGI BssHII BstXI BstZ17I BtrI
ClaI DraIII DrdI Eam1105I EcoNI EcoRI
FspI HaeII
HincII HindIII MscI
NruI NspI PflMI PstI ScaI SgfI
SpeI
SrfI XbaI XmnI ZraI
pSB4C5 ccdB AatII AccI AclI AflII ApaLI BamHI
BbeI BseRI
BsrGI BssHII BstAPI BstXI
BstZ17I BtrI Cfr10I EcoRI EcoRV HaeII
HincII KasI NarI NdeI PstI
PvuII SacI ScaI SfoI
SmaI SpeI
SphI
SrfI StyI XbaI XmaI ZraI

Growth on all plates. The pSB4C5 and R751 plates were parafilmed and placed in fridge.


Did linearization of oriT-R, promoter, pSB1AK3, and pSB4C5 using EcoRI.

Did digests of oriT-R (9uL) and pSB4C5 (4.5uL).

Did ligation CA and CB:

Assembly name position Components volume in µl
CA Upstream pTet-GFP 2
Downstream oriT-R 2
Backbone pSB4C5 2
H20 11
CB Upstream rbs-GFP-term 2
Downstream oriT-R 2
Backbone pSB1C3 2
H20 11


Ran a 2% gel to check various parts and digests.

Gel03082009-conj.png

Well Part Expected Plasmid Size Status
1 oriT-R linear 2079
2 oriT-R old digest 2079 + ~278
3 oriT-R control 2079
4 oriT-R new digest 2079 + ~278
5 promo linear
6 promo control
7 DNA Ladder
8 pSB1AK3 linear 3864
9 pSB1AK3 control 3864
10 pSB4C5 linear 3896
11 pSB4C5 control 3896
12 pTet digest
13 GFP-gen digest
14 pSB1C3 digest
15 DNA Ladder
16  !B assembly ligation circular
17  !C assembly ligation circular
18

Orr

Made some LB Agar medium and some agarose gel with pre-made TBE at concentration 1x.