Team:Heidelberg/Notebook/BSDesign/July

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Binding Site Design - July

05/07/2010 - 11/07/2010


Preperation of chemically competent cells E. coli Top10 and DH5alpha

  • plating of E. coli Top10 and DH5alpha on a agar plate (LB, without Amp); Preperation of competent cells according to the following protocol:

First, a 20 ml over night culture was inoculated in antibiotic free LB medium from a fresh single colony and transferred into 400 ml antibiotic free LB medium the next day. This culture was incubated at 37 °C while shacking until an OD600 of 0.5 – 0.6 was achieved. The culture was than cooled down on ice, centrifuged (8 min, 4 °C, 3500 rpm), the supernatant discarded and the pellet resuspended in 10 ml 100 mM CaCl2. After addition of further 190 ml 100 mM CaCl2 the suspension was incubated on ice for 30 min. The suspension was than again centrifuged (8 min, 4 °C, 3500 rpm), the supernatant discarded, the pellet resuspended in 20 ml 82.5 mM CaCl2 with 17.5 % glycerol and aliquoted. The aliquots were flash frozen in liquid nitrogen and than stored at -80 °C until usage.

Cell Culture Starting

  • thawing of Huh-7, HeLa p4 and HEK-293 cells according to the following protocol
  • vials from liquid nitrogen were thawn at 37 °C
  • once, the probe was nearly completely thawn, cells were thrown into pre-warmed DMEM (10 % FCS, L-Glut, P/S) and gentely mixed
  • cells were spinned down at 800 rpm, 3 min; supernatant was discarded
  • the pellet was resuspended in 10 ml DMEM an plated on a p100 cell culture dish in the following media according to the different cell lines:


Media for Hela and Hek cells:

  • DMEM with 10 % FCS, 1 % L-Glut and 1 % P/S

Media for HUH-7 cells:

  • DMEM with 10 % FCS, 1 % L-Glut and 1 % P/S and 1 % non-essential amino acids


from now on, cells were kept constantly in culture during the whole iGEM for passaging cells, the cells were split according to the following protocol:

  • remove media
  • wash cells one time in PBS (10 ml for p100 dish)
  • remove PBS; add 1-3 ml of trypsin-EDTA solution and incubate cells for 5 min at 37 °C
  • add 5 ml of the according media
  • take 1/10th of the cell suspension and plate out on the according dish (either p100 dish, 6 well plate or T-flask)




12/07/2010 - 19/07/2010


Preperation of RNA extracts for miRNA profiling


  • Hela, Hek and HUH were plated on p100 dishes in their according media (10E6 cells/dish) and grown to 60-70 % confluence
  • Infection of Hela p4, HUH-7 and HEK cells with AAV serotype 2 (GFP) and incubation for 48 h
  • afterwards, RNA Extraction was performed according to the following protocol:

Protocol

  • Samples were afterwards analyzed for miRNA expression by using the FEBIT miRNA profiling service


  • pSB1AC3 from the registry was transformed into Top10 cells according to the standard transformation protocol; a day later, a 5 ml LB culture was inocculated and incubated for 8 hours; plasmid was extracted by applying the Qiagen MiniPrep Protocol


design of diraPCR oligos


  • a diraPCR Designer tool (called miRACLE Designer) was programmed for enabling quick&easy design of diraPCR oligos. The program takes any microRNA guiding strand sequence of choice and constructs synthetic microRNA binding site oligos. Those oligos have the following properties:
  • they have a 5' and 3' anealing sequence which is inerte (has no natural microRNA target)
  • the microRNA binding site of choice with randomized nucleotides at position 9-12 and a missmatch introduced at position 0
  • an inerte spacer sequence of 0, 5 10 or 15 bp length


The miRACLE Designer constructs a set of 8 ready-to-order oligos and prints them out in the common FASTA format. When performing diraPCR, binding sites will be concatomerized with spacer sequences in between 15 and 30 bp length.

design of measurement standard


  • in order to design an appropriety standard respecting all the rules according to the standard of mammalian synthetic biology (RFC12), we developed a dual reporter measurement construct with the following properties:
  • bidirectional CMV promoter driving both reporter genes
  • distabilized EGFP and EBFP2 as reporter genes, as they are really similar in their whole structure and amino-acid sequence
  • BBB prefix and suffix cloned behind the EGFP for easy swapping of binding site patterns
  • unique BamHI and HindIII binding sites introduced behind the EBFP2 reporter for introducing a reference binding site
  • strong SV40 terminators behind both reporters
  • vector backbone, containing an Amp resistance, Hygromycin resistance, pBR322 origin and an FRT site for stable integration

please, find more information about the measurement standard design in the measurment standard page




20/07/2010


Dilution of raPCR-Oligos

  • oligos (hsa_miR_886_3p_sp0...) and stop oligo (miRaPCR_Stop_fw_Ecori and miRA_PCR_Stop_rev) diluted to a concentration of 100 um
  • Set up raPCR-reactions with different amounts of oligos being pooled
  • 2 ul of each hsa_miR_886_3p oligo
  • 1.0, 2 or 4 ul of each stop oligo
  • 25 ul of Phusion PCR MasterMix
  • add water to a total volume of 50 ul


Seven-Cyle PCR

  • run seven-cycle PCR under the following conditions


................................................

95 °C/ 5 min

................................................

95 °C/ 30 sec
55 °C/ 45 sec
72 °C/ 30 sec

................................................ (7x)

4 °C/ forever

................................................

  • PCR purification of the PCR-product (elution in 42 ul of water)


25-cycle PCR

MiR-886-3p optimization.png
  • run construct amplification PCR according to the following protocol


  • 20 ul of purified PCR product
  • 1 ul of each stop oligo
  • 3 ul of water
  • 25 ul of Phusion PCR MasterMix


................................................

95 °C/ 5 min

................................................

95 °C/ 30 sec
65 °C/ 45 sec
72 °C/ 30 sec

................................................ (25x)

72 °C/ 5 min

................................................

4 °C/ forever

................................................
Gel Electrophoresis

  • PCR products from the 25 cycle PCR were analyzed on a Gel. Therefor, 5 ul of PCR product were mixed with 1 ul of 6x-loading dye and loaded on a 1.5 % agarose gel. The gel ran at 135 V for 55 min.




21/07/2010

  • optimization of cycle number and oligo concentration for raPCR


  • 0.5 (BS0.5), 1 (BS1) or 1.5 (BS1.5) ul of each binding site oligo
  • 0 (Stop0), 0.5 (stop0.5) or 1 (stop1) ul of each stop oligo
  • 25 ul of Phusion PCR MasterMix
  • add water to total volume of 25 ul


12-cycle PCR

  • run 12-cycle PCR according to the following program


................................................

95 °C/ 5 min

................................................

95 °C/ 30 sec
57 °C/ 45 sec
72 °C/ 45 sec

................................................ (12x)

4 °C/ forever

................................................

  • add 1 ul of each stop oligo to reactions "Stop0"
  • run 3-cycle PCR with the "Stop0" reaction according to the following protocol

................................................

95 °C/ 5 min

................................................

95 °C/ 30 sec
65 °C/ 45 sec
72 °C/ 45 sec

................................................ (3x)

4 °C/ forever

................................................

  • PCR purify all products


25-cycle PCR

MiR-886-3p longer fragments.png
MiR-886-3p longer fragments2.png
  • run 25-cycle PCR in order to amplify constructs


  • 20 ul of purified PCR product
  • 1 ul of each stop oligo
  • 3 ul of water
  • 25 ul of Phusion PCR MasterMix


  • for construct Stop0.5/BS1 set up an addition reaction as follows


  • 1 ul of purified PCR product
  • 1 ul of each stop oligo
  • 22 ul of water
  • 25 ul of Phusion PCR MasterMix


  • run 25-cycle PCR according to the following protocol


................................................

95 °C/ 5 min

................................................

95 °C/ 30 sec
65 °C/ 45 sec
72 °C/ 50 sec

................................................ (25x)

72 °C/ 5 min

................................................

4 °C/ forever

................................................

Gel Electrophoresis

  • PCR products from the 25 cycle PCR were analyzed on a Gel. Therefor, 5 ul of PCR product were mixed with 1 ul of 6x-loading dye and loaded on a 1.5 % agarose gel. In addition, 2.5 ul of the 7-cycle PCR (07/21/2010) and 12-cycle PCR were loaded as well. The gel ran at 135 V for 55 min.






22/07/2010


  • the PCR products from the previous days' raPCR were loaded on a 1 % agarose gel and the brightest 200, 400, 700 and 1400 bp bands were gel extracted using the Qiagen Gel Extraction Kit (elution in 32 ul of nuclease free water)
  • Vector pSB1AC3 (500 ng) and the gel extraction products were digested with EcoRI and SpeI according to the standard digestion protocol
  • PCR purification was performed for the digested raPCR products and a gel-extraction was performed for the ~ 3 kb vector band of pSB1AC3 (elution in 32 ul of nuclease-free water each)
  • 12 ligation reactions were performed using 5 or 10 ul of insert and 5 ul of vector in each reaction; standard ligation was performed




23/07/2010


  • transformation of ligation product (previous day) into E. coli Top10 cells according to the standard transformation protocol




26/07/2010


  • of 21 colonies, 7 of each hsa-mir-886_3p 200, 400 and 700 bp band cloning product and inocculation of Miniprep LB cultures


single binding site synthesis


In order to construct a database of synthetic single binding sites, we developed and optimized a standardized single binding site synthesis protocol;

The band at ~60 bp shows the synthesized single binding sites. For mir-886 and mir-122 there were some unspecific products or multimers obtained.
  • Protocol 1:
set up the following reaction
  • 1 ul of each single binding site oligo (100 uM) has-mir-886-3p, hsa-mir-886-3p(perf), hsa-mir-769-5p, hsa-mir-769-5p(perf), hsa-mir-122, hsa-mir-122(perf)
  • 1 ul of SBSSSS_EcoRI primer (reverse strand synthesis primer)
  • 23 ul of water
  • 25 ul of Phusion PCR MasterMix

PCR protocol:
................................................

95 °C/ 5 min

................................................

95 °C/ 30 sec
60 °C/ 45 sec
72 °C/ 30 sec

................................................ (30x)

72 °C/ 5 min

................................................

4 °C/ forever

................................................

  • analysis of the result on a 2 % agarose gel, run 45 min @ 135 V



27/07/2010


The 200, 400 and 1000 bp cloning products were analyzed in an analytic PCR. Only The very first sample of the 200 bp product seems to be positive, as it shows a higher band (~ 300 bp) compared to the religated vector product band at ~ 200 bp
  • Miniprep of the LB cultures inocculated the previous day
  • analytic PCR for detecting positive clones was set up according to the following protocol


  • 3 ul of Miniprep product
  • 0.5 ul of each standard sequencing primer VF and VR
  • 21 ul of water
  • 25 ul of PCR Phusion Mastermix


PCR protocol:
................................................

95 °C/ 5 min

................................................

95 °C/ 30 sec
60 °C/ 45 sec
72 °C/ 30 sec

................................................ (30x)

72 °C/ 5 min

................................................

4 °C/ forever

................................................

  • PCR products were analyzed on a 1 % agarose gel, run for 45 min @ 135 V





Single Binding Site Synthesis - Optimization

  • Further optimization of the single binding site synthesis protocol
The unspecific or multimer side products were clearly reduced, but there is still sime unwanted, longer product in case of mir-122.
  • Protocol 2:
set up the exact same reaction as on the day before, but using an anealing temperature of 65 °C
  • analysis of the result on a 2 % agarose gel, run 45 min @ 135 V
















28/07/2010

Nearly no unspecific/longer products can be seen. Thus, the synthesis protocol has been perfectly optimized.


  • Further optimization of the single binding site synthesis protocol
set up the following reaction
  • 1 ul of each single binding site oligo (100 uM) has-mir-886-3p, hsa-mir-122
  • 0.5 ul of SBSSSS_EcoRI primer (reverse strand synthesis primer)
  • 23 ul of water
  • 25 ul of Phusion PCR MasterMix


  • negative controls were performed with either the SBSSSS_EcoRI primer or the binding site oligos


  • run PCR under the follwing different conditions
a) 30 cycles, annealing temperature 68 °C constant
b) touchdown PCR 68 °C (- 0.5°C each cycle)
c) incubation for 1 h @ 37 °C, then 30 cycle PCR with annealing temperature @ 65 °C


  • The PCR product was analyzed on a 2 % agarose gel, run for 45 min @ 135 V



raPCR for the construction of anti miRsAg-shRNA sponges

In order to vary the length of the constructed sponges, three parameters were varied in the different PCRs:
a) the stop oligos were either added before or after the 12 cycle PCR
b) we used different amounts of binding site oligos (0.5, 1 or 1.5 ul each)
c) different amounts of 12 cycle PCR product were used in the second, 25 cycle PCR (either 1 or 20 ul)
  • the reaction was set up according to the standard miRACLE protocol; either 0.5, 1 or 1.5 ul of each binding site oligo were used. 0.5 ul were either added to the first and second PCR reaction or were not present in the first, but the second PCR. For analysis, 5 ul of each PCR product were loaded on a 1 % agarose gel, run @ 135 V for 45 min





31/07/2010


  • ready-to-use vector pSB1A3 from the registry (25 ng/ul) digestion with EcoRI/PstI (NEB Buffer EcoRI + BSA, volume: 40 ul)
  • PCR purification of digestion product
  • subsequent digestion with DpnI (NEB Buffer 4, volume: 40 ul)
  • 5 ul of digestion product was analyzed on a 1 % agarose gel; unfortunately, there was no digestion product detectable (data not shown)


  • transformation of pSB1A3-1 vector (Tom Knight, 2004) from the registry into Top10 cells according to the following protocol:
  • 10 ul of nuclease-free water was pipetted into well C1 of Spring 2010 distribution plate 1
  • incubation for 10 min at room temperature
  • Top10 cells were thawn on ice (10 min) and 2 ul of DNA was added
  • incubation on ice for 15 min
  • 1 min heat-shock at 42 °C
  • incubation on ince for 2 min
  • adding 500 ul of LB media; mixing
  • centrifugation of the cells (5 min, 6000 rpm)
  • supernatant was removed, pellet resuspended in 50 ul LB media and cells were plated on a LB-Amp plate


  • digestion of the 200 bp, 400 bp and 700 bp band from the previous day (corresponding to hsa-mir-886-3p microRNA binding site patterns constructed via diraPCR
  • no digestion product was detectable on the gel; therefor raPCR was repeated


diraPCR for constructing hsa-886-3p binding site patterns


  • the diraPCR was pipetted according to the following protocol in three repeats:
  • 1 ul of each binding site oligo
  • 0.5 ul of each stop oligo
  • 25 ul of Phusion MasterMix
  • add water to final volume of 50 ul


  • 12 cycle PCR was performed according to the standard miRACLE PCR protocol
  • after PCR purification the subsequent PCR reaction was pipetted as follows:
  • 5, 10 or 20 ul of 12 cycle PCR prodcut
  • 0.5 ul of each stop oligo
  • 25 ul of Phusion MasterMix
  • add water to final volume of 50 ul


  • the 25 cycle PCR was performed according to the standard miRACLE PCR protocol