Team:Harvard/Dailybook/Week7/Chemical and Light

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Contents

PCR

8/4: Cph/EnvZ, P1, P3, mtrB not BB

8-04 gel 1 MXHTA.jpg 1% agarose gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
11 kb plus ladder
2-5cph-EnvZ 50 °C annealing temperature (2.3kb)
6-7P1 (3kb)
8-9P3 (3kb)
10-11mtrB (2.1kb)
12-13HO-pcyA (1.4kb)
14-15ompR (750bp)

HO-pcyA and ompR bands excised, purified, and digested (ApaLI & Kpn overnight).

8/4 Colony PCR of putative mtrB samples

We picked 24 colonies each of old putative P98 and newly transformed putative P98+63 for colony PCR using the BioBrick primers and 55°C annealing for 30 cycles. If the colonies contained mtrB, a band at ~2.1 kb should appear. No colonies appeared to contain mtrB.

All gels with 1kb plus ladder

P98 P98 P98+63
8-04 gel 2 MXHTA.jpg8-04 gel 3 MXHTA.jpg8-04 gel 4 MXHTA.jpg
P98+63 Mix
8-04 gel 5 MXHTA.jpg8-04 gel 6 MXHTA.jpg

Lane 1: 1 kb plus ladder
Lane 2: P98+63 (~2100)
Lane 3: P98+63 (~2100)
Lane 4: P98 (~2100)
Lane 5: P98 (~2100)

8/4 CphEnvZ, P1, P3, mtrB

Pl05 (CphEnvZ w/ PstI site mutated out) conditions: 5min @ 94°C → 40x [30s @ 94°C → 30s @ (50.8, 51.5, 52.6, 53.9, 55.4, 56.7, 57.7, 58.3)°C → 2:30 @ 72°C] → 7min @ 72°C → ∞ @ 4°C

8/5: gels

08-05 cph p1,3 mtrb mxh.jpg 1.2% agarose E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
1-8P105 (50.8-58.3 annealing temp, increases LTR) - 2.2kb
91kb plus ladder
10P1 not BB - 3kb
11P3 not BB - 3kb
12mtrB not BB - 2.1kb
8-5 cph p1,3 hodgepodge.jpg Gel for excision (includes old PCR samples)
Lane Contents (approx. expected band size)
1, 151kb plus ladder
2-3P105 PCR product
4-6P3 PCR product
7-9mtrB not BB PCR product
10P1 PCR product
11-12ompR PCR product (720bp)
13HO-pcyA (1.4kb)
14CDF PCR product (900bp)


Bands excised and digested: Cph/P105 (AK), P3 (AK), mtrB (XP, ES)

Bands excised and saved: ompR, HO-pcyA, CDF

Ligations and transformations 08/06

We ligated P105 and P1/P3 not BB, and mtrB not BB and P1/P3 not BB. We tried letting the ligation reactions run for 5 and 10 minutes. We used P1/P3 not BB from 08/05 and from another date (older). We transformed using TOP10 and DH5α. We also retransformed P108, the Lac QPI with a high constitutive promoter in a p15A vector.

Results below

TOPO cloning

08/04

P1, mtrB

These had a few white colonies. Colony PCR, however, indicated that the correct PCR product was not incorporated.

ompR

All colonies were blue.

HO-pcyA

No colonies.

Transforming in XL10-Gold cells

Plate Marker # Colonies Description
XL10-Gold P75a + P63b (1:1)Kan2No fluor
XL10-Gold P75b + P63b (1:1)Kan61 fluor
XL10-Gold P75a + P63b (6:2)Kan0
XL10-Gold P75b + P63b (6:2)Kan1fluor
XL10-Gold P75a + P63b (7:1)Kan1no fluor
XL10-Gold P75b + P63b (7:1)Kan2both fluor
XL10-Gold Dephos P75a Kan1
XL10-Gold Dephos p75b Kan0
XL10-Gold P3 + (P39+p51) 2/6Kan
XL10-Gold P3 Topo w/ XGALAmp
XL10-Gold P1 Topo w/ XGALAmp
XL10-Gold mtrB Topo w/ XGALAmp
XL10-Gold pUC18Amp100sWhite, very small
XL10-Gold negative control Ampmanyextremely small
XL10-Gold negative controlKan0

Ligations

HO-pcyA, ompR, CDF

All three ligations yielded >50 colonies on the TOP10 cell plate with a 5 minute ligation in all combinations (HO-pcyA and ompR with P1 and old P3; CDF with P3). The P90 (CDF+P3) did not fluoresce. The DH5α cells did not have nearly as many (<5) and ligation times (10min, 30 min) did not appear to be significant.

Colony PCR 8-6

We picked at least 18 colonies from each ligation set, patched a master plate, inoculated liquid cultures, and performed 12.5 μL colony PCR reactions. The BBp/sfx primer pair was used, annealing temperature was 50°C for first 10 cycles and 54°C for rest of the cycles. 2 controls were performed: one using a picked P20 colony, and another with miniprepped P20 plasmid.

Digests, 1-8

We ran the digests to see if PCR mutations could have introduced an internal cut site. However, even with the small amount of purified digest we had left, we could see a properly sized band for each of P1, ompR, and HO-pcyA PCR products.

8-6 pcr seveneth 11fromback.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
11 kb plus ladder
2Old P1 PCR product AK digested (3kb)
3ompR PCR product AK digested (720bp)
4HO-pcyA PCR product AK digested (1.4kb)
5-12HO-pcyA + P1 ligation colony PCR (1.6kb)

9-19

8-6 pcr eighteth 11fromback.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
11 kb plus ladder
2-11HO-pcyA + P1 ligation colony PCR (1.6kb)
12HO-pcyA + P3 ligation colony PCR (1.6kb)

20-30

8-6 pcr nineth 11 from back.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
11 kb plus ladder
2-12HO-pcyA + P3 ligation colony PCR (1.6kb)

31-41

8-6 pcr sixth 11 from back.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
11 kb plus ladder
2-7HO-pcyA + P3 ligation colony PCR (1.6kb)
8-12CDF + P3 ligation colony PCR (900bp)

42-52

8-6 pcr fifth 11 from back.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
11 kb plus ladder
2-12CDF + P3 ligation colony PCR (900bp)

53-63

8-6 pcr fourth 11 from back.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
11 kb plus ladder
2-7CDF + P3 ligation colony PCR (900bp)
8-12ompR + P1 ligation colony PCR (1kb)

64-74

8-6 pcr third 11 from back.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
1-11ompR + P1 ligation colony PCR (1kb) (#64 and 73 contain ompR, as verified by sequencing)
121 kb plus ladder

75-85

8-6 pcr second 11 from back.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
1-2ompR + P1 ligation colony PCR (1kb)
3-11ompR + P3 ligation colony PCR (1kb)
121 kb plus ladder

86-94, P20 controls

8-6 colony pcr mxh last 11.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
1-9ompR + P3 ligation colony PCR (1kb)
10P20 colony PCR (1122)
11P20 plasmid PCR
121 kb plus ladder

Making Thermoinducible cI System

Ligation from 8/1

Plate Results (also listed in Week 6):

Plate Marker # Colonies Description
E1 P75a + P63b (1:1)Kan0
E1 P75b + P63b (1:1)Kan0
E1 P75a + P63b (6:2)Kan1No Fluor, 3mm
E1 P75b + P63b (6:2)Kan1Fluorescent, 1mm.
E1 P75a + P63b (7:1)Kan0
E1 P75b + P63b (7:1)Kan0
Dephos P75b Kan0

Fluorescent colony was picked for liq culture and restreaked. Miniprep sent for sequencing-- ligation confirmed by sequencing (8/5).

Analytical Digest Gels from TOPO Cloning 8/5

8-5-08 analydig1 al.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
11 kB Ladder
2E1 RBS 4R, 2D 1
3E1 RBS 4R, 2D 2
4E1 RBS 4R, 2D 3
5E1 RBS 4R, 2D 4
6E1 BIG 4R, 2D 1
7E1 BIG 4R, 2D 2
8E1 BIG 4R, 2D 3
9E1 BIG 4R, 2D 4
10E1 RBS 2R, 2D Xg 1
11E1 RBS 2R, 2D Xg 2
12E1 RBS 2R, 2D Xg 3


8-5-08 analydig2 al.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
1BIG 4R, 4D Xg 1
2BIG 4R, 4D Xg 2
3BIG 4R, 4D Xg 3
4mtrB 0.5 A
5mtrB 0.5 B
6mtrB 2 A
7mtrB 2 B
8RBS gel pur 2 A
9RBS gel pur 2 B
10BIG gel pur 2 A
11BIG gel pur 2 B
121kB Ladder

Strange bands, but sent several clones for sequencing anyway.

Digestion and Ligation of P18+P63 and P75+P63

Done in tandem and side by side with Christina (except for digestion).

Digestion of P18, P63, and P75 8/4

' P63 P75b P18
DNA30 uL6 uL11 uL
100x BSA0.5 uL0.25 uL0.25 uL
10x Buffer5 uL Buffer 22.5 uL Buffer 22.5 uL Buffer 2
RE 1EcoRI 1 uLEcoRI 1 uLEcoRI 1 uL
RE 2SpeI 1 uLXbaI 1 uLXbaI 1 uL
Water12.5 uL14.25 uL9.25 uL
Volume50 uL25 uL25 uL


Gel of Digestion 8/5

8-5-08 testlig al.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
11 kB Ladder
2Christina\'s Vector (CE)
3Christina\'s Insert (CI)
4Christina\'s Vector (IE)
5Christina\'s Insert (IE)
6P75 EX
7P63 ES
8P18 EX

Ligation of P18+P63 and P75+P63 8/5

Used dephosphorylated and undephosphorylated vector.

Plate Results 8/6

Plate # Colonies Notes
pUC19 Amp I 31
Negative controls:..
AmpI just cells0
AmpI ligC dephos. IE vector only8
AmpI ligC Ephos IE vector only v+i 1
AmpI ligC G8 SP just vector6
AmpC ligC G8 SP just vector7
AmpC ligC dephos IE vector only5
DNA Positive controls:.
AmpC ligC G8 + G10>200
AmpI ligC G8 + G1081
AmpI ligI G8 + G1078
AmpC ligI G8 + G10127
whole thing:.
AmpI ligC CE CG103
AmpI ligC CE dephos CG45
AmpC ligC CE dephos57
AmpC ligC CE CG224
uh oh:.
AmpI ligC IE CG3
AmpC ligC IE CG7
AmpC ligC IE dephos V + I46
iGEM DNA.
AmpI (-) 3
AmpI (- Dephos)0
Kan 63+7564
Kan 63 + 75 Dephos0
AmpI 63+ 18100+
AmpI 63+18 dephos40

Digestion and Ligation of P63 + cI857 (Both Primer Sets)

Digestion of cI857 PCR product and P63 8/5

' P63 EX cI857 RBS (GP) ES cI857 BIG (GP) ES cI857 RBS (PP) ES cI857 BIG (PP) ES P104 EX
DNA10 uL3 uL7 uL10 uL10 uL10 uL
100X BSA0.25 uL0.25 uL0.25 uL0.25 uL0.25 uL0.25 uL
10X Buffer 22.5 uL2.5 uL2.5 uL2.5 uL2.5 uL2.5 uL
EcoRI1 uL1 uL1 uL1 uL1 uL1 uL
Enzyme 21 uL XbaI1 uL SpeI1 uL SpeI1 uL SpeI1 uL SpeI1 uL XbaI
Water10.25 uL17.25 uL13.25 uL10.25 uL10.25 uL10.25 uL
Volume25 uL25 uL25 uL25 uL25 uL25 uL

Christina digested the same samples of P63, cI857 RBS GP and PP, and cI857 BIG GP and PP with EcoRI buffer. P104 was cut 8/6 in the morning.

Gel results 8/6

8-6-08 p104and63 al.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
11 kB Ladder
2P63
3P63c
4P104
51 kB Ladder

Ligation of P63, P63c, and P104 with cI857 8/6

Accidentally mixed P63c and P104 so plated each of those ligations in Amp and Kan selective plates.

Plate results 8/7

Plate Final Insert Size Marker # Colonies
E1 P63 + RBS PP770Amp28 big
E1 P63 + RBS GPC770Amp25 big, 25 small
E1 P63 + BIG PP1695Amp50 big, 50 small
E1 P63 + BIG GPC1695Amp25 big, 25 small
E1 P63c + RBS PP770Amp50 big, 50 small
E1 P63c + RBS GPC770Amp25 big, 25 small
E1 P63c +BIG PP1695Amp25 big, 50 small
E1 P63c + BIG GPC1695Amp10 big, 25 small
E1 P63 + RBS PP 6:2770Amp~50
E1 P63 + RBS PP 4:4770Amp11
E1 P63 + BIG PP (No dephos)1695 or 1600Amp0
E1 P63 Dephos onlyN/aAmp0
E1 P63c Dephos onlyN/aAmp10 big, 25 small
E1 P104 No dephos1020Amp0
E1 P104 Dephos onlyn/aAmp75-100
E1 P104 + RBS GP1695Amp50
E1 P104 + RBS PP1695Amp50
E1 P104 + BIG GP2620Amp0
E1 P104 + BIG PP2620Amp0
E1 P104 + RBS GPC1695Amp3
E1 P104 + RBS PPC1695Amp5
E1 P104 + BIG GPC2620Amp0
E1 P104 + BIG PPC2620Amp4
puc 19 (+) ctrlN/aAmp50-75
(-) ctrl just cellsN/aKan0
E1 P63c + RBS PP770Kan~20
E1 P63c + RBS GPC770Kan3 big (2mm)
E1 P63c +BIG PP1695Kan0
E1 P63c + BIG GPC1695Kan0
E1 P63c Dephos onlyN/aKan0
E1 P104 No dephos1020Kan0
E1 P104 Dephos onlyn/aKan0
E1 P104 + RBS GP1695Kan0
E1 P104 + RBS PP1695Kan16 big (2mm)
E1 P104 + BIG GP2620Kan0
E1 P104 + BIG PP2620Kan0
E1 P104 + RBS GPC1695Kan1
E1 P104 + RBS PPC1695Kan0
E1 P104 + BIG GPC2620Kan0
E1 P104 + BIG PPC2620Kan0

Colony PCRs of 8/6 Ligations 8/7

8-8-08 colonypcr al 1.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
11 kB ladder
2E1 P63 + RBS PP A
3E1 P63 + RBS PP B
4E1 P63 + RBS PP 4:4 A
5E1 P63 + RBS PP 4:4 B
6E1 P63 + RBS PP 4:4 B (well leaked)
7E1 P63 + RBS PP 6:2 A
8E1 P63 + RBS PP 6:2 B
9E1 P63 + RBS GPC A
10E1 P63 + RBS GPC B
11E1 P63c + RBS PP A
12E1 P63c + RBS PP B
13E1 P63 + RBS GPC A
8-8-08 colonypcr al 2.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
1E1 P63 + RBS GPC B
2E1 P104 + RBS PP A
3E1 P104 + RBS PP B
4E1 P104 + RBS GP A
5E1 P104 + RBS GP B
6E1 P104 + RBS PPC A
7E1 P104 + RBS PPC B
8E1 P104 + BIG GPC B
9E1 P104 + BIG GPC A
10E1 P104 Dephos only A
111 kB Ladder
12E1 P104 Dephos only B
13E1 P63c Dephos only A
14E1 P63c Dephos only B
15E1 P63 + BIG PP A
16E1 P63 + BIG PP B
17E1 P63 + BIG GPC A
18E1 P63 + BIG GPC B
19E1 P63c +BIG PP A
20E1 P63c +BIG PP B
8-8-08 colonypcr al 3.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
1E1 P63c + BIG GPC A
2E1 P63c + BIG GPC B
3E1 P104 + BIG PPC A
4E1 P104 + BIG PPC B
5E1 P104 + RBS GPC A
6E1 P63c + RBS GPC A
7E1 P63c + RBS GPC B
8E1 P104 + RBS PP A
9E1 P104 + RBS PP B
10E1 P104 + RBS PP C
11E1 P104 + RBS PP D
12E1 P104 + RBS PP E
13E1 P63c + RBS PP A
14E1 P63c + RBS PP B
15E1 P63c + RBS PP C
16E1 P63c + RBS PP D
17E1 P63c + RBS PP E
18E1 P63c + RBS PP F
19E1 P63c + RBS PP G
201 kB Ladder

E1 P63 + RBS PP B to be sequenced Monday. All of the bands in the third gel indicated re-ligated vector.

Ligation of P63, P63c, and P104 with cI (repeat) 8/7

Ligations were re-done with newly digested vector because of mishap in 8/6 ligations.

Digestions of P63, P63c, and P104 8/6

' P63 EX P63c EX P104 EX
DNA10 uL10 uL10 uL
100X BSA0.25 uL0.25 uL0.25 uL
10X Buffer 2.5 uL of Buffer 22.5 uL of EcoRI Buffer2.5 uL of Buffer 2
EcoRI1 uL1 uL1 uL
Enzyme 21 uL XbaI1 uL XbaI1 uL XbaI
Water10.25 uL10.25 uL10.25 uL
Volume25 uL25 uL25 uL

Gel of Digestion 8/7

8-7-08 p104and63 digest al.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
11 kB Ladder
2P63
3P63c
4P104
51 kB Ladder

Bands were extracted, purified, and dephosphorylated.

Ligation of P63, P63c, and P104 with cI 857 8/7

Vector backbones were ligated with cI857 digested 8/5.

Plate Results 8/8

Plate Final Insert Size Marker # Colonies (After 1 Day) # Colonies After 1 Day
E1 P63 (Buffer 2) + RBS GPAmp0N/a
E1 P63 (Buffer 2) + BIG PPCAmp5 1-1.5mm coloniesN/a
E1 P63c + RBS GPAmp1 1.5mm colonyN/a
E1 P63c +BIG PPCAmp6 1-1.5mm coloniesN/a
E1 P63 (2) Dephos onlyAmp2 1mm colonies on edgeN/a
E1 P63c Dephos onlyAmp1 1.5mm colonyN/a
E1 P104 + RBS GP 6:2Kan3 colonies, no fluor3 2-3mm colonies, 6 1mm colonies
E1 P104 + RBS GPKan8 colonies, no fluor8 2-3mm colonies, 3 1mm colonies
E1 P104 + RBS PPKan30 colonies, 10 fluor, rest no fluor30 big 2-3mm colonies, 2 1mm colonies.
E1 P104 + BIG GPKan4 small 0.25 colonies?4 1mm colonies.
E1 P104 + BIG PPKan0 colonies5 small 0.25mm colonies.
E1 P104 + RBS GPCKan3 1.5mm colonies, no fluor3 big 3mm colonies, 2 1mm colonies.
E1 P104 + RBS PPCKan1 0.5mm colony1 2mm colony, no fluor, and 2 1mm colonies.
E1 P104 + BIG GPCKanLots of small 0.25mm colonies100 0.5-1mm colonies, no fluor.
E1 P104 + BIG PPCKan0 colonies1 0.5mm colony
E1 P104 + BIG PPC 6:2Kan0 colonies0
E1 P104 Dephos onlyKan1 colony on edge of plate 1.5 mm2mm colony on edge, and 3 0.5-1mm colonies.
puc 19 (+) ctrlAmp100-200 1.5mm coloniesN/a
Kan (-) ctrlKan01 1mm colony
Amp (-) ctrlAmp0N/a

Restreaked some non-fluor colonies from RBS ligations/ transformations to see if repressor is being repressed-- grew in 37 and 42 degrees. No perceived difference in fluor/ no induction.

Colony PCR of Ligations 8/8

8-9-08 colonypcr 1 al.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
11 kB Ladder
2E1 P63 (Buffer 2) + RBS GP
3E1 P63 (Buffer 2) + BIG PPC A
4E1 P63 (Buffer 2) + BIG PPC B
5E1 P63 (Buffer 2) + BIG PPC C
6E1 P63c +BIG PPC A
7E1 P63c +BIG PPC B
8E1 P63c +BIG PPC C
9E1 P104 + RBS GP 6:2 A
10E1 P104 + RBS GP 6:2 B
11E1 P104 + RBS GP 6:2 C
12E1 P104 + RBS GP A
8-9-08 colonypcr 2 al.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
1E1 P104 + RBS GP B
2E1 P104 + RBS GP C
3E1 P104 + RBS GP D
4E1 P104 + RBS PP A
5E1 P104 + RBS PP B
6E1 P104 + RBS PP C
71 kB ladder
8E1 P104 + RBS PP D
9E1 P104 + RBS PP E
10E1 P104 + RBS PP F
11E1 P104 + RBS GPC A
12E1 P104 + RBS GPC B

3 bands in second gel indicate re-ligated vector.

Ligation of P104 and P63+P18 with cI RBS from TOPO

Digestion of cI RBS from TOPO and P18+P63 8/8

P18+ P63 not confirmed by sequencing yet.

' cI857 RBS TOPO ES 1 cI857 RBS TOPO ES 2 cI857 RBS TOPO ES 3 cI857 RBS TOPO ES 5 P18+ P63 ES 1 P18+ P63 ES 2 P18+ P63 ES 3 P18+ P63 ES 4 E1 P63 + RBS PP B E1 P104 + RBS PP A E1 P63c + RBS PP G
DNAFill inFill inFill inFill inFill inFill inFill inFill inFill inFill inFill in
100X BSA0.25 uL0.25 uL0.25 uL0.25 uL0.25 uL0.25 uL0.25 uL0.25 uL0.25 uL0.25 uL0.25 uL
10X Buffer 22.5 uL2.5 uL2.5 uL2.5 uL2.5 uL2.5 uL2.5 uL2.5 uL2.5 uL of Buffer 32.5 uL of Buffer 32.5 uL of Buffer 3
EcoRI1 uL1 uL1 uL1 uL1 uL1 uL1 uL1 uL1 uL XbaI1 uL XbaI1 uL XbaI
Enzyme 21 uL SpeI1 uL SpeI1 uL SpeI1 uL SpeI1 uL XbaI1 uL XbaI1 uL XbaI1 uL XbaI1 uL PstI1 uL PstI1 uL PstI
WaterFill inFill inFill inFill inFill inFill inFill inFill inFill inFill inFill in
Volume25 uL25 uL25 uL25 uL25 uL25 uL25 uL25 uL25 uL25 uL25 uL

Gel results 8/9

8-9-08 digests al.jpg 1% agarose gel visualized using EtBr/UV
Lane Sample
11 kB Ladder
2cI857 RBS TOPO ES 1
3cI857 RBS TOPO ES 2
4cI857 RBS TOPO ES 3
5cI857 RBS TOPO ES 5
6
71 kB Ladder
8P18+ P63 EX 1
9P18+ P63 EX 2
10P18+ P63 EX 3
11P18+ P63 EX 4
121 kB Ladder
13E1 P63 + RBS PP B
14E1 P104 + RBS PP A
15E1 P63c + RBS PP G

RBS TOPO 1,3, and 5, and P18+ P63 EX 1-4 were extracted and purified.

Update: At least P18+ P63 1-2 have been sequence confirmed.

Digest of P104 and P63 8/9

' P63 EX P104 EX
DNA5 uL15 uL
100X BSA0.25 uL0.25 uL
10X Buffer 2.5 uL of Buffer 22.5 uL of Buffer 2
EcoRI1 uL1 uL
Enzyme 21 uL XbaI1 uL XbaI
Water15.25 uL5.25 uL
Volume25 uL25 uL

Gel of Digestion 8/10

Extracted and purified 8/10.

mtrB, P97, P63 digests 08/06

We digested mtrB with ES and XP so that we can put it into the P63 (terminator) and P97 (RBS) vectors. We also digested P97 with SP (and dephosphorylated it).

Ligation transformation results 08/07

Plasmid Ligation time Ligation ratio (vector:insert) Strain No. of Colonies
mtrB not BB+P1 not BB old10 min2:6DH5-alpha1
mtrB not BB+P1 not BB10 min2:6DH5-alpha4
mtrB not BB+P1 not BB5 min2:6TOP1088
mtrB not BB+P3 not BB old10 min2:6DH5-alpha0
mtrB not BB+P3 not BB10 min2:6DH5-alpha8
mtrB not BB+P3 not BB5 min2:6TOP1040
mtrB+P6310 min2:6TOP1048
mtrB+P6310 min1:7DH5-alpha5
mtrB+P9710 min2:6DH5-alphaTMTC
mtrB+P9710 min1:7DH5-alpha200
P105+P1 not BB old10 min2:6DH5-alpha5
P105+P1 not BB10 min2:6DH5-alpha1
P105+P1 not BB5 min2:6TOP102
P105+P3 not BB old10 min2:6DH5-alpha1
P105+P3 not BB10 min2:6DH5-alpha8
P105+P3 not BB5 min2:6TOP1055

Colony PCR

Ladders (end of each block) alternate as low range (100, 200, 400, 800, 2000bp) and 1kb plus. Expected band sizes indicated. (Lanes rearranged from 2% agarose 96 well E-gel)

1-16

1.png

Lane 1: Plasmid control P85 (2.3kb)
Lane 2: Colony control P88 (2.2kb)
Lanes 3-16: P105+P3 ligation colony PCR (2.5kb)

4, 6, 14 look like they have potentially correct products, so liquid cultures were grown up.

14 is incorrect- it's just P1 in pSB3K3.

17-24: P105+P1 ligation colony PCR (2.5kb)

2.png

None appear to be correct.

25-48: mtrB+P63 ligation colony PCR (2.2kb)

3.png

27, 28 picked.

RE digests 08/09

8-10 gel 1 MXHTA.jpg

Lane 1: 1 kb ladder

Lane 2: mtrB+63 #28 cut XP (~2200+3.1kb)

Lane 3: E1P3A-P38+51C cut SP (4155)

Lane 4: E1P3A-P38+51D cut SP (4155)

Lane 5: E1P3A-P38+51B cut SP (4155)

49-64: mtrB+P97 ligation colony PCR (2.1kb)

4.png

51 picked.

65-80: mtrB'+P3 ligation colony PCR (2.3kb)

5.png

65, 69, 70, 78, 79, 80 picked.

65 sequence did not read properly.

81-96: mtrB'+P1 ligation colony PCR (2.3kb)

6.png

82, 87, 95 picked.

82 is wrong- mystery sequence. 87 and 95 are BLAST to pHELLSGATE ?!

RE digests 08/07

8-08 gel 1 MXHTA.jpg

Lane 1: 1 kb ladder

Lane 2: E1P1+P17A cut EX (3652)

Lane 3: E1P1+P17C cut EX (3652)

Lane 4: E1P1+P17D cut EX (3652)

Lane 5: E2P1+P17A cut EX (3652)

Lane 6: E2P1+P17B cut EX (3652)

Lane 7: P108 cut SP (4155)

Lane 8: P45 cut XP (876; 2079)

Ligations 08/08

  • We ligated P17 in a p15A vector (P1 or P3) to P38 and P39. We used a vector to insert ratio of 1:7. We also prepared a ligation reaction with 1 μL vector (P17) and 7 μL water as a transformation control. We transformed 50 μL TOP10 cells with 7 μL DNA and 100 μL DH5α cells with 7 μL DNA. We also used 7 μL of the vector-only ligation to transform 7 μL DH5α cells.
  • To test the Lac QPI system, we ligated P45 (RBS+GFP+terminator) to P108. We used a vector to insert ratio of 2:6. We also prepared a ligation reaction with 1 μL vector (P108) and 7 μL water as a transformation control. We transformed 100 μL DH5α cells with 7 μL DNA and we also used 7 μL of the vector-only ligation to transform 7 μL DH5α cells.

Transformation results 08/09

Plasmid Amount of DNA Strain Ligation ratio (vector:insert by volume) Number of colonies
P108 (vector control)7 ul 100 ul DH5-alpha2 (vector)!6 (water)0
P45+1087 ul100 ul DH5-alpha2:61
P17 in p15A (vector control)7 ul100 ul DH5-alpha1 (vector):7 (water)188
(P17 in p15A)+P397 ul50 ul TOP101:71
(P17 in p15A)+P397 ul100 ul DH5-alpha1:70
(P17 in p15A)+P387 ul50 ul TOP101:73
(P17 in p15A)+P387 ul100 ul DH5-alpha1:70

Colony PCR 8/9

We picked all of the noncontrol colonies and one control colony for colony PCR using the BBp/sfx primers.

08-09 colony mxh.jpg 1.2% E-gel visualized using EtBr/UV
Lane Contents (approx. expected band size)
1P39+P17 in P1/3- col#1 (~940bp)
2-5P38+P17 in P1/3- col#2-5 (~940bp)
61kb ladder
8-9P108+P45 (same sample) (~2.3kb)
10ligation control (no insert)

Since the bands are at least plausible, the P38/39 in P1/3 samples were grown up and miniprepped.

Retransformation 8/9

We retransformed 5μL of the P39+17 in P1/3 ligation into 50μL DH5α and obtained two colonies.

Colony PCR shows that one of these does not contain the right construct. The other was set up in 5ml culture.

08-10 colpcr ta.jpg

1kb ladder, colony A, colony B (both should have ~950 products if correct)

New ligations and transformations 08/10

We retransformed our old P108+45 (2:6 vector to insert) ligation and the old vector control. We also did this ligation over with a 2:1 molecular ratio of insert to vector. Both P108 (4155 bp) and P45 (876 bp) were about 17 ng/μL. We used a ratio of 5.4:2.3 vector to insert by volume.

Transformation results

Plasmid Ratio (vector!insert) Strain Number of colonies
P108 vector control (old)2 ul P108!6 ul EBDH5-alpha0
P108+45 (old)2!6DH5-alpha0
P108+45 (old)2!6TOP104
P108 vector control (new)5.4 ul P108!2.3 ul EBDH5-alpha0
P108+45 (new)5.4 ul P108!2.3 ul EBDH5-alpha2
P108+45 (new)5.4 ul P108!2.3 ul EBDH5-alpha8

Transforming LacZ parts

We attempted to transform the following parts: I732017, E0435, E0435, I732005 into our competent DH5α. E0435 (on CM) had 0 colonies). The others (on Carb) had 10-20 extremely small colonies (after 16+hrs of incubation) each. We picked 2 of each for liquid culture, but none grew.

We requested the parts directly from MIT.