- Fusion PCR: purifaction gel electrophoresis

- gel electrophoresis:

- 50 µl DNA
- 10 µl Loading Dye
- 0,7 % Agarose gel
- 6,6kb fragment
- 1h with 80 V

- purifaction with the Promega Purification Kit
- final concentration: 45,7 ng/µL

- test gel of PCR with IDT fragments of yesterday:
IAAH-PP7 - IAAM-MS2 - LacI - TaC1 - TaC2 - TaC3 - Ddx4-YFP

- only IAAH-PP7 and TaC3 bands are okay
- gel purification: PP7: 40,7 ng/µL
- TaC3: 27,3 ng/µL
- second PCR with other fragments, used three different temperatures for annealling for every fragment:

- Tip from Fabian: next time more gradient Temperature distance!
- fragments from left to right (Temperatures are alaso from left to right) : MS2, LacI, TaC1, TaC2, YFP

- MS2 / 9 band correct
- YFP / 6 and 7 bands are correct
- LacI no bands, TaC1 almost no bands, TaC2 bands incorrect
- gel run of MS2/9 and YFP/ 6,7 and put cut gel slices in the fridge for extraction tomorrow
- test gel of 4 uL (10 ng/uL) of IDT-fragments: LacI, TaC1, TaC2 with 6 uL H2O und 2 uL Dye to see if there's something wrong with the IDT fragments

- TaC1 and YFP show correct bands
- TaC2 correct and wrong band (maybe low concentration?) --> Nanodrop result: 11,4 ng/uL; problem that DNA concentration of desired
DNA is too low for restriction?

- Gel and PCR clean up (Promega kit)

- MS2: 240mg gel; final concentration: 16,6 ng/µL
- YEP 6: 250mg gel; final concentration: 19,6 ng/µL
- YEP 7: 200mg gel; final concentration: 10,9 ng/µL

Gibbson Assembly "NEBuilder® HiFi DNA Assembly Master Mix"
https://www.neb.com/protocols/2014/11/26/nebuilder-hifi-dna-assembly-reaction-protocol

Trafo
https://www.neb.com/protocols/2015/02/17/nebuilder-hifi-dna-assembly-chemical-transformation-protocol-e2621

- Gibbson Assembly (5 µl) + competen cells (C2987)
- plate cells: 100µl and 200µl

- Gibson Assembly worked, we have colonies but they are useless (see below)
- colony PCR following the protocol (beware that the protocol has been updated in the lab),
annealing Temperature: 52°C wiht Q24 and Q18 and 10 colonies
- negative control: IG_C_P1 miniprep
- negative/Gibson 1-10 and TaC3

- negative results for all reactions except the last onw which is just the gel purified TaC3
- excpept it isnt because the band cleearlyc shwows a sifferent size and is more likely to be IAAAH-PP7 (a suspicion of Sarah who wasn't sure if the tubes were swapped) which explains the negative results in the Gibson assembly
- Gibson assembly was done again withcorrect fragments:

- pSB4A5 miniprep: 2,75 uL (18 ng/µL)
- IAAM-MS2 6,1 uL (10,6 ng/µL)
- IAAH-PP7 1,9 uL (27,3 ng/µL)
- MasterMix 10,77 µL (fragments to Mastermix : 1:1)

- two Trafos were done with already used competent cells and new competent cells (always use the cells we got from - the Gibson Kit for Gibson assembly!) and plated with 200 uL and centrifuged
- repeated PCR to amplify IDT-fragments with TaC1, TaC2 and LacI (always as 50 uL reactions):

- 3 different concentrations and temperatures for each fragment:

from left to right: Marker- TaC1/ 1-9 - one empty lane - TaC2/1-4 - Marker Marker - TaC2/5-9 - LacI/ 1-9 (but not 5!) - Marker - 6LacI/5

low concentrations worked best, results at Tac1/1, TaC2/3 and LacI/1 were best and gel purified

- Tac1: 5,8 ng/µL
- Tac2: 9,2 ng/µL
- LacI: 12,9 ng/µL

Colony-PCR of P4 with Q24 and Q18 (see protocol and note the changes in the folder!)

- 10 colonies
- masterplate
- did a test gel (1 % Agarose) (actualy did two beacuse of missing marker in the first one, see lab book)
- gel picture shows: all fragments have expected length
- no miniprep culturs inoculated because colonies were too small -> To do tomorrow

Gibbson assembly of P5 (IAA-RBP in pSB4A5) (see online protocol from NEB) Transformation of P5 into Jm109

- for tomorrow: inoculate miniprep cultures of positive clones on masterplate for P4, Colony-PCR and test gel for P5

Colony PCR of P5 (low copy plasmid, see protocol) with Q19 and Q20
- gel picture: all clones okay
- inoculated three precultures for minipreps tomorrow (10 ml, 37 °C shaker)
- also inoculated three precultures of P4 for miniprep tomorrow (10 ml, 37 °C shaker)

- Eppis named like this: "IG_C_P4_2_Mini"
- test digests:
P4:

- P5 looks good on both digests,
- P4 only one band but probably just two bands which semm ike one so it should be fine
- glycerol stock was put in -80 °C of P4 2,4 and 8 and P5 1 and P5 3

- diluted P4 / 2,4,8 and P5/ 1,3 to 100 ng/µl and Q21/q22 to 5 µM
- sent fo rsequencing as follows:

- prepared 2 ml over night culture for glycerol stocks

- IG_C_P4 clone 2, 4 and 8
- IG_C_P5 clone 1 and 3

- Preparation for Gibson assembly: PCR with Q5 polymerase for P5 (to amplify LacI-dCas9 with overhangs to P4) and P4 (to open the plasmid)

- prepared dilutions of 1 ng/µl for each template:

- PCR programs (name in Torsten: P4_P5_PCR-vor-Gibson)
- PCR programs how they should be: - amplified fragment size

- P4: 7309 bp - P5: 5680 bp

P5		P4	cycles
98°C 30s		62.5
98°C 10s	30	6.25	30
57°C 30s	30	62°C 30s	30
72°C 170s	30	72°C 220s	30
72°C 2 min		72°C 2 min

Wednesday, 09/06/17



Thursday, 09/07/17

component	volume in µl
Mastermix (Q5 2x)	25
Q25	2.5
Q26	2.5
IAAH-PP7	1
ddH2O	19

component	volume in µl
ddH2O	92,3
Q18	11.7
Q24	11.7
Taq Polymerase	144.3

Friday, 09/08/17

- Gel picture see lab book

Monday, 09/11/17

component	volume in µl
IG_c_P1 linearized (18 ng/µL)	2,75
IAAM-MS2 (10,6 ng/µL)	6,1
IAAH-PP7 (19,8 ng/µL)	2,7
	11,55

Tuesday, 09/12/17

temperature in °C	time in sec
95	60
95	15
52	15
72	11

- 30 cycles


Wednesday, 09/13/17

temperature in °C	time in sec
98	30
98	10
71	30
72	120
72	120
10

- 35 cycles
- second PCR

temperature in °C	tube
60,1	1,10
60,9	2,11
61,8	3,12
63,1	4,13
64,4	5,14
65,6	6,15
66,9	7,16
68,2	8,17
69,1	9,18

Friday, 09/15/17

- prepared P5 for shipping to iGEM HQ
- used Q37/Q38
- PCR program: dCas9 iGEM

temperature in °C	time in sec
98	30
98	10
65	15
72	1:50 min
72	2 min

Monday, 09/18/17

component	volume in µl
Q5 Master mix	25
IG_C_Q26 (10µM)	2,5
IG_C_Q39 (10µM)	2,5
IaaH-PP7 IDT (1:10)	1
water	19
sum	50

component	volume in µl
Assembly Master mix	15.65
IaaM-MS2 (10.6 ng/µl)
IG_C_Q39 (10µM)IaaH-PP7 (7.8 ng/µl)	6.8
pSB4A5 (IG_C_P1 linearized, 18 ng/µl)	2.75
sum	31.3

component	volume in µl
Cutsmart	1
EcoRI	1.5
PstI	1.5
LacI-dCas9 (400 ng)	4.18
water	1.82
sum	10

component	volume in µl
T4 DNA Ligation Buffer	2.5
	1
LacI-dCas9 (10.2 ng/µl)	10.7
pSB1C3 (12.5 ng/µl)	8
water	2.8
sum	25

Tuesday, 09/19/17

component	volume in µl
water	100,8
Q17	9,6	-> annealing Tm 52°C, binds to backbone
Q20	9,6	-> annealing Tm 52,6°C, binds to dCas9
Red Taq	120

component	volume in µl
water	100,8
Q18	9,6
Q24	9,6
Red Taq	120

component	volume in µl
water	48
Q39	8
Q26	8
Q5 master mix	80

Wednesday, 09/20/17

Cas-4	47
Cas-7	66,2
Cas-8	48,9
Cas-10	64,4
Cas-10	64,4
P4-1	129,5
P4-6	158,2
P4-8	140,2
P4-10	173,7

Thursday, 09/21/17

tube	annealing temp.
1	60,0°C
2	63,7°C
3	65,8°C
4	68,1°C

temperature in °C	time in sec
95	60
95	15
52	15
72	108
75	5 min

- 30 cycles
- gel: all clones negative


Friday, 09/22/17

- Gibson assembly of IAAH-PP7 (corr.) with IAAM-MS2

component	volume in µl
IAAH-PP7	0,7
IAAM-MS2	3,4
H2O	5,9
Hifi DNA Assembly Master Mix	10

component	volume in µl
IAAM-MS2-IAAH-PP7 (17 ng\µl)*	6.86
IG_C_P1 lin. (18 ng/µl)	2.75
H2O	0.39
Hifi DNA Assembly Master Mix	10

Friday, 09/29/17

-colony PCR for LacI-dCas9 in pSB1C3
-4 clones, all negative
-amplification of P1 and IAA-fusion for assembly of P4:
Q40/Q41:
- amplification of P1 creating new overhangs for Gibson assembly --> 3,4 kb
Q42/Q43:
- amplificaton of IAA-fusion creating new overhangs for Gibson assembly --> 4 kb
Q44/Q45:
- amplification of IAA-fusion creating overhangs for restriction enzymes to cut more efficiently
-made 50uL reactions and ran test gel (left 4 bands are colony PCR then 40/42/44)


-only 42 has correct band
-gel extraction: 33,7 ng/ul
-named Eppi "IAA-fusion for Gibson"
-gradient PCR for 40 and 44:

well	temperature in °C
1	52
4	55
5	57
6	59
7	61
8	63
9	65
12	68

-10 µL reaction and gel run
-40/1,4,5,6 and 44/1 were positive --> a PCR-clean-up has to be done
-repeat PCR from 27.07.2017:
A2: 1µl Template 59°C
A4: 1µl Template 63,3°C
A5: 1µl Template 66,5°C
B4 0,1µl Template 63,3°C
(A2, A4, A5 and B5 are the names of the original well names of the gradient PCR)
-just A 5 was positive -> a gel clean up has to be done the next day

Monday, 10/02/17

-gel-clean-up LacI-dCas9 (A5) and PCR-clean-up 40/1 and 44/1 (40/4,5,6 were found in the waste, 40/4 was empty, because open cap, but 40/5,6 were also clean-up by PCR clean-up and purifien over one column but separated from 40/1 to not possibly destroy the one safe sample)
-concentration: 40/1: 19,7 ng/µl
-40/5,6: 31 ng/µl (but probably waste/just denatured DNA or something else)
-44/1: 30,6 ng/µl
-LacI-dCas9: 25,9 ng/µl
-Eppi-names: "IAA-Fusion for Restriction" name of 44/1 (is from PCR with Q44 and Q45)
-"P1 + overhangs 1" name of 40/1 and "P1 + overhangs 5,6" name of 40/5,6 (is from PCR with Q40 and Q41)
-Restriction of IAA-Fusion (is from PCR with Q44 and Q45):
10,2µl IAA-Fusion (19,7ng/µl) --> 200ng
1,5µl Eco-RI-HF
1,5µl PstI
1,5µl NEB2.1
0,3µl water
-total volume: 15µl
-final concentration of IAA-Fusion: 13,3ng/µl
-was incubated 1h 35min at 37°C
-Ligation of digested IAA-Fusion in pSB4A5 = P1
-176,7ng Insert = 13,25µl Iaa-Fusion digested (13,3 ng/µl)
-50ng backbone = 2,5µl pSB4A5 digested (with EcoRI and PstI) (19.8ng/µl)
-1,25µl water
-2µl Ligase-buffer
-1µl Ligase
-total volume: 20µl
-90 min at room temperature
-for ligation an insert-backbone-ratio of 3:1 was choosen
-IAA-Fusion (Insert): 4000bp
-pSB4A5 (backbone): 3395bp
-(4000bp/3395bp) * 50ng * 3 = 176,7ng = m(Insert)
-Restriction of LacI-dCas9 for iGEM-HQ of Part P5:
-digestion of 400ng LacI-dCas9 = 15,4µl LacI-dCas9
-15,4µl LacI-dCas9 (25,9ng/µl)
-2µl NEB2.1
-0,5µl EcoRI
-0,5µl PstI
-1,6µl H2O
-total volume: 20µl
-final concentration LacI-dCas9: 20ng/µl
-was incubated for 1h15min at 37°C
-Ligation of digested LacI-dCas9 in pSB1C3 for iGEM-HQ:
-Ligation was sheduled in a 1:1 Insert:backbone-ratio, because the insert is much bigger than the backbone and a very high concentration of insert would be needed to get this ratio in a 20µl reaction. Such a high concentration we don't have. But the concentration was this time at least high enough for a 1:1-ratio with 50ng of backbone.
-size Insert: 5700bp
-size backbone: 2000bp
-(5700bp/2000bp)*50ng*1 = 142,5ng
-142,5ng LacI-dCas9 (20ng/µl) = 7,1µl LacI-dCas9
-7,1µl LacI-dCas9 digested (20ng/µl; 142,5ng)
-4µl pSB1C3 digested (12,5ng/µl; 50ng)
-2µl Ligase-buffer
-1µl Ligase
-5,9µl H2O
-total volume: 20µl
-incubated 90 min at room temperature
-Gibbson-Assembly of IAA-Fusion with P1=pSB4A5:
-2,5µl pSB4A5 linearised (19,7ng/µl; 50ng; P1 with new overhangs from today PCR-clean-up, Eppi-name: P1 +overhangs 1") -> we used 40/1, because even if 5/6 has a higher concentration, 5/6 was the whole weekend not cooled in the waste and we can not be sure, that what we measured as concentration is really our DNA-fragment of interest, if this Gibbson-Assembly should not work we can try with 5/6 or better we check 5/6 on a gel before
-3,5µl IAA-Fusion for Gibbson (33,7ng/µl; 116,6ng; from Friday 29.09.)
-4µl water
-10µl Gibbson-Master-Mix
-total volume: 20µl
-IAA-Fusion + pSB4A5 reaction for 19 min at 50°C incubated
-Transformation of
-IAA-Fusion in pSB4A5 (Restriction-Ligation)
-IAA-Fusion in pSB4A5 (Gibbson-Assembly)
-LacI-dCas9 in pSB1C3 (Restriction-Ligation)
-in chemo-competent E.coli-cells (followed transformation protocol)
-Inactivation of ligase of the both ligase reactions after transformation for 10min at 65°C
-eppis with names "Ligation IAA-Fusion in pSB4A5" and "Ligation LacI-dCas9 in pSB1C3" stored at -20°C
-Gibbson-Assembly with eppi name: "Gibbson-Assembly IAA-Fusion in pSB4A5" stored at -20°C
-plating of the cells after 1h incubation at 37°C: 200µl and pellet, respectively

Tuesday, 10/03/17

-colony-PCR of IAA-fusion in psB4A5 (Gibson-Assembly) (primer: IG_C_Q17 and IG_C_Q23)
-no colony-PCR of restriction-ligation, because no colonies
-colony-PCR of LacI-dCas9 in psb1C3 (restriction-ligation) (primer: IG_C_Q17 and IG_C_Q20)












-minpreps of colonie 1 and 4 (IAA-fusion in pSB4A5)