Gel 101001-1. Digestion of miniprep no. 8, 9, 14 and 16 with EcoRI and PstI. Odd lanes are undigested controls, even lanes are digested minis
repressor construct:
colony 8, 9, 14 and 16 were chosen for miniprep. They consist of the complete TetR construct in pBS 1C3
digestion of the minis with EcoRI and PstI for cloning into Template:Part, SAP of Template:Part, digestion was tested on gel and proven positive (see Gel 101001-1)
nucleotide removal, then ligation of TetR8 and TetR14 equimolar with SAPed backbone, TetR9 and TetR16 2:1 with not-SAPed backbone, transformation with TOP10 cells (10µl on 50µl E. coli)
Screening 1: shRNA10 single binding sites
Screening 2: shRNA10 single binding sites
Screening of the binding sites cloned into the constructs K3 and K4 containing shRNA10 in pSB1A3 on the previous day. 16 colonies were picked for each perfect, rand9-12 and rand9-22 binding site and colony-PCR was performed according to the colony-PCR standard protocol (Primers Luc2_bs_screen_seq and sh10_ape_xma_screen_rc). The results are shown on the gels Screening1 and Screening 2. Indicated are the construct numbers (either K3 or K4, which differ in the promoter driving the Luc2 gene) and the binding site property (perfect, 9-12 randomized or 9-22 randomized). Almost all clones show a positive band, although only some have a really bright band at the size of ~ 250 bp. LB cultures for 10 clones for each constructs K3 and K4 were inocculated.
02/10/2010
Gel 101002-1. Colony PCR. All lanes with right amplified fragment except on lane 3, 10, 11, 15 and 23. Lane 1 & 14: 1kb Plus Ladder (Invitrogen)
Gel 101002-2. Test digestions of repressor construct. Upper pattern: EcoRI & PstI. Lower pattern: BamHI. All bands revealing positive results except in the first column (negative control from lane 3 of gel 101002-1). Lane 1 and Lane 10: 1kb Plus Ladder (Invitrogen). Lane 16, 17, 18: incomplete digestion
Miniprep of the LB cultures (constructs K3 and K4 with shRNA10 and the corresponding binding sites) were done and used for transfection of Hek-293 cells
once or twice the binding site in each of the T1 constructs, respectively
once the binding site for the T2 construct
re-trial of ligation for two binding sites in T2
planned transfection into HeLa and HUH cells (non-liver and liver to prove ON-targeting) in ratio 6:1 = repressor:operator(tuning) as recommended in the [http://tools.invitrogen.com/content/sfs/manuals/trexsystem_man.pdf T-Rex manual]
new approach:
purification of PCR amplified shRNA-like miRNA against hAAT ("shhAAT")
digestion of shhAAT and Q2 and Q3 with HindIII and AflII (for backbones sequential because of two inner AflII cutting sites)
ligation in triplicates (using 70 ng of backbone and 10, 15 or 20 ng of insert, respectively)
transformation, over-night growth on selective agar plates (ampicillin)
06/10/2010
waiting for colonies from previous night, which did not grow after all
07/10/2010
repetition of shhAAT cloning
touch-down PCR setup: 8.5 µl ddH2O, 0.5 µl template DNA (pcDNA5, 50 ng/µl), 0.5 µl each primer (i.e. D7 & D16, 10 µl Phusion PCR MasterMix (2x)
touch-down PCR protocol: like this but with increase of annealing temperature from 68°C to 61°C (i. e. 0.2°C per cycle)
go on like 05/10/2010 but growth on freshly prepared plates
08/10/2010
mini-prep and submission for sequencing for the only promising colony of Q2 containing shhAAT for sequencing
09/10/2010
sequencing yesterday was fine but construct contains TetO2, thus: maybe Q2 and Q3 were confused
that would explain why measurements with TetR constructs are not working properly even though sequences were fine
cloning of binding sites for shhAAT (perfect binding site generated via annealing, and randomized ones PCR amplified)
touch-down PCR setup: 17 µl ddH2O, 4 µl each oligo (i.e. respective forward primer + second strand oligo D121), 25 µl Phusion PCR MasterMix (2x)
touch-down PCR protocol: like this but with increase of annealing temperature from 70°C to 62°C (i. e. 0.5°C per cycle, 16x) and four additional cycles with 62°C
annealing of perfect binding against shhAAT sites with an oligo-based strategy following the protocol from the 3rd October
digestion of PCR amplified binding sites with AgeI and XhoI, digestion of Q2 backbone containing the shhAAT with XhoI and XmaI, afterwards heat inactivation, nucleotide removal and ligation following standard protocol recommendations
transformation and over-night growth on selective agar plates (ampicillin)
10/10/2010
Gel 101010-1. Colony PCR for construct containing shhAAT and binding sites. Expected is an amplified fragment a bit smaller than 300 bp which can be seen on lane 3, 4, 6, 7, 8 (perfect binding sites), 12, 13, 14, 16 and 17 (randomized binding sites). Lane 1 and Lane 26: 1kb Plus Ladder (Invitrogen)
colony pcr reveals some positive clones (see gel 101010-1) from previous day
inoculation of 5 ml LB Amp cultures for mini-prep over night
11/10/2010
mini-prep of ten cultures from yesterday and direct transfection to test the system
amount: each 100 µl (c=2.5 ng/µl)
measurement construct for single binding sites:
PCR-based generation of binding sites against miR122 (perfect and randomized)
touch-down PCR setup:
17 µl ddH2O,
4 µl each oligo (i.e. respective forward primer D71, D62 or D5 + second strand oligo D13),
25 µl Phusion PCR MasterMix (2x)
touch-down PCR protocol:
like this but with increase of annealing temperature from 70°C to 62°C (i. e. 0.5°C per cycle, 16x)
and four additional cycles with 62°C, elongation time only 10 seconds
digestion of generated binding sites and the pSMB_miMeasure backbone with EcoRI and PstI, then nucleotide removal
ligation with ~ 70 ng vector and between 7.5 ng and 15 ng insert
colony pcr of each eight of load of colonies + two negative controls (sum: 50 samples)
protocol: 16 cycles touch-down pcr from 70°C to 62°C of annealing temperature, then 19 additional cycles with 62°C annealing temperature
elongation time: 90''
no positive results, maybe due to insufficient screening primers (one for BBb standard, the other one for CMV resulting in an 1300 bp fragment)
as a consequence: repetition of entire cloning with [http://www.fermentas.com/templates/files/tiny_mce/coa_pdf/coa_ef0511.pdf SAP] treated backbone tomorrow
note: vector concentration of pSMB_miMeasure is okay but after digestion and nucleotide removal it is always pretty low
(loss of 75% of DNA on average whereas other DNA yields to 90% of purified DNA as compared to digested amount)
14/10/2010
cloning of 47 - 58 into pSB_H1
cloning of tuning constructs for in vivo measurement:
cloning of binding sites of miRNA haat with perfect and several imperfect binding
oligo annealing following the standard protocol
digestion of backbone pbsU6 with NotI and XhoI
ligation and transformation
15/10/2010
Screening of M1 to M11 constructs, 4 clones were picked from each plate. 300bp band marks positive clones
Screening of M12 to M22 constructs, 4 clones were picked from each plate. 300bp band marks positive clones
Screening of measurement standard with perfect, 9-12 and 9-22 randomized binding sites. constructs, 8 clones were picked from each plate. 300bp band marks positive clones
screening of plates M1 to M11 of the transformation with the construct pBSU6_SV40_Luc2 with 11 different binding sites for sh hAAT. Four clones from each plate were screened by colony pcr, positives give a band at 300bp. Primers Luc2_bs_screen_seq_fw and reverse primerse are the reverse binding site oligos for the binding sites.
inoculation of miniprep cultures for one positive from each plate.
transformation of miRsAg and mir122 expression constructs
screening of measurement standart cloning from 13th with perfect, 9-12 randomized and 9-22 randomized binding sites for miRNA 122. primers mir122_mimeasure_screen_rev and pSMB_miMeasure_screen_fw. Positives give a band at 300bp.
inoculation of miniprep cultures for positive clones
screening of plates M12 to M22 of the transformation with the measurement plasmid with 11 different binding sites for miRsAg. Four clones from each plate were screened by colony pcr, positives give a band at 300bp. Primers pSMB_miMeasure_Sequencing_rev and forward primerse are the forward primer oligos for the binding sites.
inoculation of miniprep cultures for one positive from each plate.
16/10/2010
mini Prep of mimeasure colonies (4 each)
mini prep of haat constructs
inoculation of miRsAg and mir122 expression constructs
Maxi Preps of constructs M1 till M10
inoculation for Maxipreps of Adenovirus 5, AAV8 rep and cap genes and pBSU6 H1 haat construct
inoculation for Maxiprep of constructs M11 an M23-29
cloning of on targeting constructs with a new strategy...
17/10/2010
annealing of eleven sAg binding sites using oligos
protocol:
5 µl of each oligo, 5 µl of Buffer 2 (NEB), 35 µl H2O
95°C, 5'
cool down to room temperature for 2h
incubation on ice, 10'
use 1 µl for ligation with ~ 40 ng of backbone (i. e. with NotI and XhoI digested pBS_U6 containing hAAt cDNA)
transformation and growth on selective plates (ampicillin)
18/10/2010
colony-PCR of 4 colonies for each plate of previous day transformations using reverse binding site oligo and forward hAAT primer expecting a fragment round about 1300 bp
gel 101018-1 reveals almost positive samples except two (data not yet shown)
19/10/2010
mini-preps of cloned shAAT constructs
dilution and co-transfection with miRsAg expressing construct into HeLa cells for ELISA measurements