Difference between revisions of "Team:Valencia UPV/Notebook"

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−
−	18/05/2016
−	Take glycerinated cultures of C58 Agrobacterium with dsRED from GoldenBraid Collection. Prepare broth culture (5 mL LB + 5 μL kanamycin + 5 μL Rifampin) 1:1000 and incubate overnight at 28 ºC.
−	19/05/2016
−	Refresh previously made culture by inoculating 10 μL in a new culture medium.
−	20/05/2016
−	Agroinfiltration in Nicotiana benthamiana of C58 with dsRED. (ENLACE)
−	06/06/2016
−	Take from the glycerinates of Goldenbraid Collection:
−	Plasmid
−	GB Code
−	pD6B3  α1
−	GB0015
−	pD6B3  α2
−	GB0017
−	pD6B3  Ω1
−	GB0019
−	pD6B3  Ω2
−	GB0021
−	pUPD2
−	GB0307
−
−	Prepare liquid culture (3 mL LB + 3 μL antibiotic) 1:1000. Incubate at 37 ºC overnight.
−	Experiment with snails:
−	Two experiments: one with infiltrated Nicotiana benthamiana and another with not infiltrated N.benthamiana (negative control). Lettuce leafs haven’t been correctly infiltrated and it seems that the expression level is low.
−	Let both N. benthamiana leafs with snails overnight at room temperature in separated boxes. We will observe if snails eat the leafs and if appears fluorescence.
−	15/06/2016
−	Experiment is over due to snails haven’t eaten leafs enough so we haven’t been able to see fluorescence.
−	30/06/2016
−	Orange DNA Genome Extraction protocol (ENLACE)
−	Take  from the glycerinates of GoldenBraid Collection:
−	Plasmid
−	GB Code
−	Promoter 35S : Cas9 : nopaline synthase terminator (T-nos)
−	GB0639
−	Luciferase (Luc)
−	GB0096
−	T-nos
−	GB0037
−
−
−	01/07/2016
−	Miniprep with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of:
−	Promoter 35S : Cas9 : T-nos
−
−	Luciferase and nopaline synthase terminator cultures haven’t succeed. Repeat Luc and Tnos cultures.
−
−	Primers IG16JUN01 and IG16JUN02 have arrived.
−
−	Finish orange DNA Genome Extraction and check DNA concentration with NanoDrop. Concentration is very low so extraction will be done again.
−	02/07/2016
−	Miniprep with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of Luc and Tnos.
−
−	Check orange DNA genome concentration with NanoDrop.
−	Sample
−	DNA concentration (ng / μL)
−	Clemenules 1
−	3153.8
−	Clemenules 2
−	4527.9
−
−	Perform a PCR to bind linker with luciferase
−	Reagent
−	Volume (μL)
−	Program
−	Luciferase pUPD
−	1
−	Temperature
−	Time
−	Buffer HF
−	10
−	98 ºC
−	5 minutes
−	dNTPs
−	2
−	98 ºC
−	35x
−	30 seconds
−	IG16JUN01
−	2.5
−	70 ºC
−	30 seconds
−	IG16JUN02
−	2.5
−	72 ºC
−	1 minute 30 seconds
−	Taq phusion
−	0.5
−	72 ºC
−	10 minutes
−	H2O milli-Q
−	31.5
−	16 ºC
−	∞
−
−	04/07/2016
−	Run electrophoresis gel of Clemenules DNA (agarose 1 %). 45 mL agarose gel at 1 % 0.45 g of agarose with 45 mL of TAE 1X. Voltage used is 100 V.
−
−
−	Rice DNA Genome Extraction Protocol (ENLACE)
−
−	Run electrophoresis gel of Luciferase PCR product. 45 mL agarose gel at 1 % 0.45 g of agarose with 45 mL of TAE 1X. Voltage used is 100 V.
−
−	Ligate linker: Luciferase into a pUPD2 and transform E.coli DH5α with it. The method that is necessary to carry out this procedure is explained in protocols.
−
−	Check DNA concentration with NanoDrop.
−	SAMPLE
−	DNA Concentration (ng / μL)
−	Rice Gleva 1
−	22.8
−	Rice Gleva 2
−	17.3
−
−	05/07/2016
−
−	Run electrophoresis gel of Gleva rice DNA. We have checked that there isn’t DNA.
−
−	Repeat: Rice DNA Genome Extraction
−
−	Check DNA concentration with NanoDrop.
−	SAMPLE
−	DNA Concentration (ng / μL)
−	Rice Gleva 1
−	294.9
−	Rice Gleva 2
−	193.7
−
−	Run electrophoresis gel of Gleva rice DNA. It observed that genome extraction is correctly done.
−	06/07/2016
−	Take glycerinated cultures:
−	GB part
−	Plasmid
−	Antibiotic
−	Number GB
−	psgRNA
−	pUPD
−	Ampicillin
−	0645
−	U6-26
−	pUPD
−	Ampicillin
−	1001
−
−	07/07/2016
−	Miniprep with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of psgRNA and U6-26
−
−	Primers IG16JUL01, IG16JUL02, IG16JUL03, IG16JUL04, IG16JUL05, IG16JUL06, IG16JUL07 and IG16JUL08 arrived.
−
−	gBlocks of - promoter 35S : 5’ region - have arrived.
−
−	We perform a PCR of orange and rice Genome Extraction.
−
−	Sample
−	Initial concentration (ng/μL)
−	Final concentration (ng/μL)
−	Initial volume (μL)
−	Final volume (μL)
−	Clemenules 1
−	3153.8
−	150
−	4.756
−	100
−	Clemenules 2
−	4527.9
−	150
−	3.31
−	100
−	Gleva 1
−	294.9
−	150
−	50.8647
−	100
−	Gleva 2
−	193.7
−	150
−	77.44
−	100
−
−	REAGENT
−	VOLUME (μL)
−	PROGRAM
−	Clemenules DNA
−	1
−	TEMPERATURE
−	TIME
−	Buffer HF
−	10
−	98ºC
−	5 minutes
−	dNTPs
−	2
−	98ºC
−	35x
−	30 seconds
−	IG16JUL01 (TFL_For)
−	2.5
−	64ºC
−	30 seconds
−	IG16JUL02 (TFL_Rev)
−	2.5
−	72ºC
−	30 seconds
−	Taq phusion
−	0.5
−	72ºC
−	10 minutes
−	H2O milli-Q
−	31.5
−	16ºC
−	∞
−
−	REAGENT
−	VOLUME (μL)
−	PROGRAM
−	Gleva DNA
−	1
−	TEMPERATURE
−	TIME
−	Buffer HF
−	10
−	98ºC
−	5 minutes
−	dNTPs
−	2
−	98ºC
−	35x
−	30 seconds
−	IG16JUL03 (Ga20_for)
−	2.5
−	72ºC
−	30 seconds
−	IG16JUL02 (Ga20_rev)
−	2.5
−	72ºC
−	30 seconds
−	Taq phusion
−	0.5
−	72ºC
−	10 minutes
−	H2O milli-Q
−	31.5
−	16ºC
−	∞
−
−
−	Ligate promoter 35S : 5’ region in pUPD2. Following ligation protocol, BsmbI enzyme is used in this reaction.
−	08/07/2016
−	Run electrophoresis gel of Clemenules and Gleva PCR products. 45 mL agarose gel at 1 % 0.45 g of agarose with 45 mL of TAE 1X. Voltage used is 120 V.
−
−	Transform E.coli with the construction: promoter 35S : 5’ region (electroporation 2.5KV). Plating it.
−
−	Take glycerinated culture for Georgia collaboration. The construction is promoter 35S : GFP : Tnos (α1 and kanamycin)
−	09/07/2016
−	Miniprep with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of promoter 35S : GFP : Tnos
−
−	No colonies have grown in 35S : 5’ region petri dishes. Repeat transformation procedure and plating again.
−	11/07/2016
−	Pick a single E. coli DH5α (promoter 35S : 5’ region in pUPD2) colony from the plate that has been incubated overnight. Inoculate a starter culture of 4 ml of LB medium with 4 μL of chloramphenicol in a 50 ml tube with the colony and incubate it overnight at 37ºC with shaking.
−
−	Check Georgia miniprep concentration with NanoDrop (promoter 35S : GFP : Tnos)
−	Sample
−	DNA Concentration (ng / μL)
−	DNA Concentration (ng)
−	1
−	105.2
−	5035.2
−	2
−	104.6
−
−	Targets ligations ( Orange Clemenules and Rice Gleva)
−	Following ligation protocol, BsmbI enzyme is used in this reaction.
−	12/07/2016
−	Pick a single E. coli DH5α (target Gleva in pUPD2 and target Clemenules in pUPD2) colony from the plate that has been incubated overnight. Inoculate a starter culture of 4 ml of LB medium with 4 μL of chloramphenicol in a 50 ml tube with the colony and incubate it 16 hours at 37ºC.
−
−	Miniprep with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of:
−	Promoter 35S : 5’region in pUPD2
−
−	Digestion of minipreps with NotI. Incubate 1 hour at 37ºC
−
−	Run electrophoresis gel of the construction: promoter 35S : 5’ region in pUPD2. We remain the samples 1 and 3.
−
−	Miniprep with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of:
−	Rice Gleva target in pUPD2
−	Orange Clemenules target in pUPD2
−
−	Digestion of minipreps with NotI. Incubate 1 hour at 37ºC.
−
−	Run electrophoresis gel of the same construction:
−	Rice Gleva target in pUPD2
−	Orange Clemenules target in pUPD2
−
−	Ligation using Golden Braid assembly of the next construction:
−	Promoter 35S : 5’ region : Target : LUC : Tnos in α1
−	13/07/2016
−	E.coli Transformation with the construction:
−	Promoter 35S : 5’ region : Target : LUC : Tnos in α1
−
−	E. coli plating in plates with Kanamycin (antibiotic). Incubate overnight at 37ºC
−	14/07/2016
−	Pick a single E. coli DH5α (promoter 35S : 5’ region) colony from the plate that has been incubated overnight. Inoculate a starter culture of 4 ml of LB medium with 4 μL of chloramphenicol in a 50 ml tube with the colony and incubate it 16 hours at 37ºC.
−
−	Primers IG16JUL09, IG16JUL10, IG16JUL11, IG16JUL12, IG16JUL13, IG16JUL14, IG16JUL15 and IG16JUL16 arrived.
−
−	Ligation using Golden Braid assembly of the next constructions:
−	Promoter 35S : 5’Region : Clemenules target control + : Luc : Tnos
−	Promoter 35S : 5’Region : Gleva target control + : Luc : Tnos
−	Promoter 35S : 5’Region : Clemenules target consensus : Luc : Tnos
−	Promoter 35S : 5’Region : Gleva target consensus : Luc : Tnos
−	Promoter U6-26 : sgRNA Clemenules : psgRNA (scaffold)
−	Promoter U6-26 : sgRNA Gleva : psgRNA (scaffold)
−
−	Step 1: Annealing of oligonucleotides. Received primers are at 1μM. It is necessary taking to 10 μM.
−	Mix in an Eppendorf:
−	18 μL of H2O milli-Q
−	1 μL forward primer
−	1 μL reverse primer
−	Step 2: Ligation reaction
−	Reagent
−	Volume (μL)
−	Clemenules target control + / Gleva target control + / Clemenules target consensus / Gleva target consensus
−	1
−	Promoter 35S : 5’ region
−	1
−	Luciferase
−	1
−	Tnos
−	1
−	α1
−	1
−	BSA10X
−	1.2
−	Ligase Buffer
−	1.2
−	BsaI
−	1
−	T4 ligase
−	1
−	H2O milli-Q
−	2.6
−
−	Reagent
−	Volume (μL)
−	sgRNA Clemenules / sgRNA Gleva
−	1
−	Promoter U6 -26
−	1
−	psgRNA (scaffold)
−	1
−	α1
−	1
−	BSA10X
−	1.2
−	Ligase Buffer
−	1.2
−	BsaI
−	1
−	T4 ligase
−	1
−	H2O milli-Q
−	3.6
−
−	E.coli Transformation with the constructions previously explained.
−
−	E. coli plating in 6 plates (6 ligation reactions) with Kanamycin (antibiotic). Incubate overnight at 37ºC.
−
−	Miniprep with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of:
−	Promoter 35S : 5’ region : CL target : Luc : Tnos (3α1)
−	Promoter 35S : 5’ region : A target : Luc : Tnos (3α1)
−
−	Digestion of minipreps with EcoRI. Incubate 1 hour at 37ºC
−	15/07/2016
−	Ligation using Golden Braid assembly of the next construction:
−	Promotor 35S : Cas9 : Tnos – Promotor 35S : 5’ region : CL target : Luc : Tnos
−	Promotor 35S : Cas9 : Tnos – promotor 35S : 5’ region : A target : Luc : Tnos
−
−	E. coli Transformation with the constructions previously explained.
−
−	Run electrophoresis gel of the products from the digestion of minipreps. The constructions are:
−	Promoter 35S : 5’ region : CL target : Luc : Tnos (3α1)
−	Promoter 35S : 5’ region : A target : Luc : Tnos (3α1)
−
−	Sequencing products:
−	Promotor 35S : 5’ region in pUPD2 → correct
−	16/07/2016
−
−	E.coli transformations with:
−	Promoter 35S : 5’ region : CL target : Luc : Tnos (3α1)
−	Promoter 35S : 5’ region : A target : Luc : Tnos (3α1)
−
−	Plating the last constructions in 2 plates with Agrobacterium C58. Incubate 2 days at 28ºC.
−
−	Minipreps (2 samples for each construction) with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of:
−	Promoter 35S : 5’Region : Clemenules target control + : Luc : Tnos
−	Promoter 35S : 5’Region : Gleva target control + : Luc : Tnos
−	Promoter 35S : 5’Region : Clemenules target consensus : Luc : Tnos
−	Promoter 35S : 5’Region : Gleva target consensus : Luc : Tnos
−	Promoter U6-26 : sgRNA Clemenules : psgRNA (scaffold)
−	Promoter U6-26 : sgRNA Gleva : psgRNA (scaffold)
−
−	Ligation using Golden Braid assembly of the next construction:
−	Promotor 35S : Cas9 : Tnos –U6 : CL sgRNA : psgRNA (scaffold) (Ω1)
−	Promotor 35S : Cas9 : Tnos –U6 : A sgRNA : psgRNA (scaffold) (Ω1)
−	Reagent
−	Volume (μL)
−	Promotor 35S : Cas9 : Tnos
−	1
−	U6-26 : CL sgRNA : psgRNA /                  U6-26 : A sgRNA : psgRNA
−	1
−	3Ω1
−	1
−	BSA10X
−	1.2
−	Ligase Buffer
−	1.2
−	BsmbI
−	1
−	T4 ligase
−	1
−	H2O milli-Q
−	4.6
−
−	Digestion of the minipreps with EcoRI which have been done before. Incubate 1 hour at 37ºC. There is a total of twelve minipreps. It has been followed the Miniprep digestion protocol.
−
−	Run electrophoresis gel of the digestion products.
−
−	Lanes
−	Samples
−	Verification
−	1
−	1 Kb molecular weight marker
−
−	2
−	gRNA Ga20ox 1
−
−	3
−	gRNA Ga20ox 2
−
−	4
−	Ga20ox consensus 1
−
−	5
−	Ga20ox consensus 2
−
−	6
−	Ga20ox knock-out 1
−
−
−	7
−	Ga20ox knock-out 2
−
−	8
−	TFL consensus 1
−
−
−	9
−	TFL consensus 2
−
−
−	10
−	TFL knock-out 1
−
−	11
−	TFL knock-out 2
−
−	12
−	TFL gRNA 1
−
−	13
−	TFL gRNA 2
−
−	14
−	1 Kb molecular weight marker
−
−
−	Pick a single E. coli DH5α colony from the plates that have been incubated overnight. The constructions are:
−	Promotor 35S : TFL Knock-out : Luc : Tnos (4 samples)
−	Promoter U6-26 : A sgRNA : psgRNA (2 samples)
−	Inoculate a starter culture of 4 ml of LB medium with 4 μL of chloramphenicol in a 50 ml tube with the colony and incubate it 16 hours at 37ºC.
−
−	17/07/2016
−	DH5α E.coli transformations with:
−	Promotor 35S : Cas9 : Tnos –U6 : CL sgRNA : psgRNA (scaffold) (Ω1)
−	Promotor 35S : Cas9 : Tnos –U6 : A sgRNA : psgRNA (scaffold) (Ω1)
−
−	Plating E.coli transformations in plates with LB + agar + IPTG + XGal and incubate it overnight at 37ºC.
−
−	Miniprep with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of:
−	Promoter U6-26 : A sgRNA : psgRNA
−	Promoter 35S : 5’ region : TFL Knock-out : Luc : Tnos (3α1)
−
−	Digestion of the minipreps with EcoRI which have been done before. Incubate 1 hour at 37ºC. There is a total of six minipreps. It has been followed the Miniprep digestion protocol.
−
−	Run electrophoresis gel of the digestion products.
−	Lanes
−	Samples
−	Verification
−	1
−	1 Kb molecular weight marker
−
−	2
−	gRNA Ga20ox 1
−
−	3
−	gRNA Ga20ox 2
−
−	4
−	gRNA Ga20ox 3
−
−	5
−	gRNA Ga20ox 4
−
−	6
−	TFL knock-out 1
−
−	7
−	TFL knock-out 2
−
−	8
−	1 Kb molecular weight marker
−
−
−	However, despite the fact that electrophoresis gel have correctly run, we have decided to repeat the ligation reactions. We haven’t get the expected results for a gRNA.
−
−	Ligation using Golden Braid assembly of the next constructions:
−	Promoter 35S : 5’Region : Clemenules target control + : Luc : Tnos
−	Promoter 35S : 5’Region : Gleva target control + : Luc : Tnos
−	Promoter 35S : 5’Region : Clemenules target consensus : Luc : Tnos
−	Promoter 35S : 5’Region : Gleva target consensus : Luc : Tnos
−	Promoter U6-26 : sgRNA Clemenules : psgRNA (scaffold)
−	Promoter U6-26 : sgRNA Gleva : psgRNA (scaffold)
−	Reagent
−	Volume (μL)
−	Reagent
−	Volume (μL)
−	TFL/Ga20ox gRNA
−	1
−	Promotor35S :5’region
−	1
−	U6-26
−	1
−	TFL / Ga20ox consensus          TFL / Ga20ox knock-out
−	1
−	psgRNA
−	1
−	luciferase
−	1
−	3α1
−	1
−	Tnos
−	1
−	BSA10X
−	1.2
−	3Ω1
−	1
−	Ligase Buffer
−	1.2
−	BSA10X
−	1.2
−	BsaI
−	1
−	Ligase Buffer
−	1.2
−	T4 ligase
−	1
−	BsmbI
−	1
−	H2O milli-Q
−	3.6
−	T4 ligase
−	1
−
−
−
−
−	H2O milli-Q
−	2.6
−
−	18/07/2016
−	DH5α E.coli transformations with ligation products (consensus targets and knock-out targets of TFL and Ga20ox as well as their gRNAs)
−
−	Plating E.coli transformations in plates with LB + agar + IPTG + XGal and incubate it overnight at 37ºC.
−
−	Pick a single Agrobacterium C58 colony from the plates that have been incubating since 16/06/2016. The constructions are:
−	Promoter 35S : 5’ region : CL target : Luc : Tnos (3α1)
−	Promoter 35S : 5’ region : A target : Luc : Tnos (3α1)
−	Incubate it 48 hours at 28ºC.
−	19/07/2016
−
−	Pick transformed E.coli colony from the incubated plates. The constructions are:
−	Promoter 35S : 5’Region : Clemenules target control + : Luc : Tnos
−	Promoter 35S : 5’Region : Gleva target control + : Luc : Tnos
−	Promoter 35S : 5’Region : Clemenules target consensus : Luc : Tnos
−	Promoter 35S : 5’Region : Gleva target consensus : Luc : Tnos
−	Promoter U6-26 : sgRNA Clemenules : psgRNA (scaffold)
−	Promoter U6-26 : sgRNA Gleva : psgRNA (scaffold)
−	Incubate it overnight at 37ºC.
−	20/07/2016
−
−	-          Miniprep with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of:
−	§  Promoter 35S : 5’Region : Clemenules target knockout : Luc : Tnos
−	§  Promoter 35S : 5’Region : Gleva target control knockout : Luc : Tnos
−	§  Promoter 35S : 5’Region : Clemenules target consensus : Luc : Tnos
−	§  Promoter 35S : 5’Region : Gleva target consensus : Luc : Tnos
−	§  Promoter U6-26 : sgRNA Clemenules : psgRNA (scaffold)
−	§  Promoter U6-26 : sgRNA Gleva : psgRNA (scaffold)
−
−	-          Digestion of the minipreps with EcoRI which have been done before. Incubate 1 hour at 37ºC. There is a total of six minipreps. It has been followed the Miniprep digestion protocol.
−
−	-          Run electrophoresis gel of the digestion products. We will keep the minipreps with “1”.
−	Lanes
−	Samples
−	Verification
−	1
−	1 Kb molecular weight marker
−
−
−	2
−	gRNA TFL 1
−
−
−	3
−	gRNA TFL 2
−
−
−	4
−	TFL consensus 1
−
−
−	5
−	TFL consensus 2
−
−
−	6
−	TFL knock-out 1
−
−
−	7
−	TFL knock-out 2
−
−
−	8
−	1 Kb molecular weight marker
−
−
−	9
−	gRNA Ga20ox 1
−
−
−	10
−	gRNA Ga20ox 2
−
−
−	11
−	Ga20ox consensus 1
−
−
−	12
−	Ga20ox consensus 2
−
−	13
−	Ga20ox knock-out 1
−
−
−	14
−	Ga20ox knock-out 2
−
−
−	15
−	1 Kb molecular weight marker
−
−
−
−	-          Ligation using Golden Braid assembly of the next constructions. Is used the restriction enzyme BsmbI.
−	§  Promoter 35s:Cas 9:T-nos – U6-26:TFL sgRNA: psgRNA
−	§  Promoter 35s:Cas 9:T-nos – U6-26:Ga20ox sgRNA: psgRNA
−	21/07/2016
−
−	-          E.coli transformations with:
−	§  Promoter 35s:Cas 9:T-nos – U6-26:TFL sgRNA: psgRNA
−	§  Promoter 35s:Cas 9:T-nos – U6-26:Ga20ox sgRNA: psgRNA
−	Incubate 2 hours at 37 ºC.
−	-          Plating E.coli transformation explained before and incubate it at 37ºC overnight.
−
−	-          Agrobacterium C58 transformation with:
−	§  Promoter 35S : 5’Region : Clemenules target knockout : Luc : Tnos
−	§  Promoter 35S : 5’Region : Gleva target control knockout : Luc : Tnos
−	§  Promoter 35S : 5’Region : Clemenules target consensus : Luc : Tnos
−	§  Promoter 35S : 5’Region : Gleva target consensus : Luc : Tnos
−	Incubate 48 hours at 28 ºC.
−
−	22/07/2016
−
−	-          Sequencing reaction
−	Reagent
−	Volume (μL)
−	Primer to sequence
−	3
−	Miniprep reaction
−	5
−	H2O milli-Q
−	6
−
−	TFL gRNA à 210.13.201
−	Ga20 gRNA à 210.13.202
−	-          Ordered the necessary primers to sequence:
−	TFL consensus, TFL knockout, Ga20ox consensus and Ga20ox knockout.
−	-          E.coli transformations with:
−	§  Promoter 35s:Cas 9:T-nos – U6-26:TFL sgRNA: psgRNA
−
−	-          Plating the last construction in plates with Agrobacterium C58. Plates contain spec + IPTG + X-Gal. Incubate 2 days at 28ºC.
−
−	-          Pick a single E.coli DH5α (Promoter 35s:Cas 9:T-nos – U6-26:TFL sgRNA: psgRNA and Promoter 35s:Cas 9:T-nos – U6-26:Ga20ox sgRNA: psgRNA ) colony from the plates that has been incubated overnight. Inoculate a starter culture of 4 ml of LB medium with 4 μL of spectinomycin in a 50 ml tube with the colony and incubate it overnight at 37ºC with shaking.
−
−	23/07/2016
−
−	-          Minipreps (4 samples for each construction) with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of:
−	§  Promoter 35s:Cas 9:T-nos – U6-26:TFL sgRNA: psgRNA
−	§  Promoter 35s:Cas 9:T-nos – U6-26:Ga20ox sgRNA: psgRNA
−
−	-          Digestion of minipreps with BamHI following digestion protocol. Incubate 1 hour at 37ºC.
−
−	-          Run electrophoresis gel of the digestion products. We will keep the minipreps with the sample number 4 for TFL sgRNA and the sample number 2 for Ga20ox sgRNA.
−
−	-          Pick a single Agrobacterium C58 (Promoter 35s:Cas 9:T-nos – U6-26:TFL sgRNA: psgRNA and Promoter 35s:Cas 9:T-nos – U6-26:Ga20ox sgRNA: psgRNA ) colony from the plates that has been incubated overnight. Inoculate a starter culture of 5 ml of LB medium with 5 μL of spectinomycin and kanamycin in a falcon tube with the colony and incubate it overnight at 28ºC with shaking.
−
−	-          Agrobacterium C58 transformations with:
−	§  Promoter 35s:Cas 9:T-nos – U6-26:TFL sgRNA: psgRNA
−	§  Promoter 35s:Cas 9:T-nos – U6-26:Ga20ox sgRNA: psgRNA
−	24/07/2016
−
−	-          Store the next cultures at -80 ºC:
−	§  Promoter 35s:5’ region in pUPD2 (DH5α) à 1
−	§  Linker: luciferase in pUPD2 (DH5α) à 2
−	25/07/2016
−
−	-          Pick a single Agrobacterium C58 (Promoter 35s:Cas 9:T-nos – U6-26:TFL sgRNA: psgRNA in 3Ω1 and promoter 35s:Cas 9:T-nos – U6-26:Ga20ox sgRNA: psgRNA in 3Ω1 ) colony from the plates that has been incubated overnight. Inoculate a starter culture of 5 ml of LB medium with 5 μL of spectinomycin and kanamycin in a falcon tube with the colony and incubate it overnight at 28ºC with shaking.
−
−	Incubate it 48 hours at 28 ºC
−
−	-          Minipreps of Agrobacterium with E.Z.N.A.® Plasmid Mini Kit I, Q(capless) Spin of:
−	§  Promoter 35S : 5’Region : Clemenules target control + : Luc : Tnos
−	§  Promoter 35S : 5’Region : Gleva target control + : Luc : Tnos
−	§  Promoter 35S : 5’Region : Clemenules target consensus : Luc : Tnos
−	§  Promoter 35S : 5’Region : Gleva target consensus : Luc : Tnos
−
−	-          Digestion of minipreps with the restriction enzyme EcoRI. Incubate 1 hour at 37ºC.
−
−	-          Run electrophoresis gel of the digestion products.
−
−	Lanes
−	Samples
−	Verification
−	1
−	1 Kb molecular weight marker
−
−
−	2
−	Target Ga20ox consensus
−
−
−	3
−	Target Ga20ox Knockout
−
−
−	4
−	Target TFL consensus
−
−
−	5
−	Target TFL knockout
−
−
−	6
−	1 Kb molecular weight marker
	</p>		</p>

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Revision as of 16:39, 25 July 2016