Team:Evry/Interlab Study/tests

From 2014.igem.org

Revision as of 20:24, 17 October 2014 by ALOUIS (Talk | contribs)

IGEM Evry 2014

Interlab study - Aim & Results

Chassis
Conference
Transposons
Workshops
Target
Hackathons
IGEM Evry 2014

Interlab study - Aim & Results

The goal of the interlab study is to obtain GFP fluorescence data from the iGEM teams all around the world for about twenty constructions. This will permit to observe the result repeatability across technics, strains and teams.

There were two sub-parts in this study:
  • The mandatory one: obtain fluorescence data for three specific genetic devices expressing GFP and compare them.
  • The Extra Credit assignments: we choose to study the entire Anderson library of constitutive prokaryotic promoters (J23100 to J23119).
    This library corresponds to 19 constitutive promoters containing some nucleotide mutations on the -35 and the -10, as shown Used Biobricks and plasmids . The idea is to compare the expression strength of promoters according to mutations, from the maximum amount of fluorescence data in order to have significant results.

Required Devices


IMAGE

IMAGE


The three required constructions shown various fluorescence intensity at OD 600 nm = 0.5, as shown on graph and bar chart below. As shown on corrected GFP fluorescence intensity according to OD 600 nm, the relationship between corrected GFP fluorescence and OD 600 nm is linear that corresponded to the expected profile for a constitutive promoter.

Theoritically constructions I20260 and J3101 were similar, constructions and alignments in sillico matched perfectly. The difference between these constructions lies on the assembly way. However we obtained, as some other teams (University of Oxford, Paris-Bettencourt and ITESM-CEM), significant GFP expression difference. There is probably a Biobrick standard construction problem, which relates to the traited question on our Phylosophy subsection.

Entire Anderson library of constitutive promoters (J23100-J23119)


IMAGE

IMAGE


Our team achieved the 19 constructions of the Anderson library. Constructions were first designed in a software(Geneious v. 6.1.6)and then relized on web lab using iGEM 2014 Distribution kit. Verifications were made by eletrophoresis gel analytic PCR amplification and sequencing. Glycerol stock of 3 colonies per constructions were conserved and used for the measurments of GFP expression.
Unfortunatly, we did not collect satisfying data for the 19 constructions,although assays were repeated several times. The data profile was repeatable under people, apparatus and strain. Strain carrying promotorless vector seemed to had higher fluorescence intensity than strain containing constructions from the Anderson library, that explains negative curve on Corrected GFP fluorescence intensity according to OD 600 nm graph. However exploitable data were collected for 5 constructions (100, 104, 105, 107 and 118) for which the relationship between corrected GFP fluorescence and OD 600 nm was linear that corresponded to the expected profile for a constitutive promoter (See graph Corrected GFP fluorescence intensity according to OD 600 nm). Corrected GFP fluorescence intensity at OD 600 nm = 0.45 of these 5 constructions were presented on bar chart above and compared with registry data on table below.


IMAGE

Ratio were calculated dividing constructions corrected GFP fluorescence at 0.45 OD 600 nm by construction 100 corrected GFP fluorescence at 0.45 OD 600 nm.

Results were similar to registry results for the 100, 105 and 107 constructions contrary to constructions 104 and 118 for which data were significantly divergent.

Possible approach to overcome data acquisition problems:
  • Using M9 medium instead of LB medium to minimize the basal medium fluorescence
  • Using another E. coli strain that has a smaller natural fluorescence
  • Changing of dilution and gain to find the optimal one
  • Choosing a TECAN with a lower detection limits to collect data for weak promoters




Used Devices IGEM Evry 2014

Interlab study - Used devices

Construction way


IMAGE


Constructions were built using classical Biobrick restriction sites.

  • Required device 1: originally this device was carried by PSB1K3 and was sud-cloned onto PSB1C3.
    • Vector: digestion of PSB1C3 and PSB1K3 carrying I20260 via EcoRi and PstI
    • Insert: digestion of PSB1K3 carrying I20260 via EcoRi and PstI
    • Ligation with T4 DNA ligase (New England Biolabs)

  • Required device 2, 3 and the 19 constructions for the entire Anderson library: promoters were inserted into PSB1C3 carrying E0240. Process is described on following figure 1.
    • Vector: digestion of PSB1C3 carrying E0240 via EcoRI and XbaI
    • Insert: digestion of PSB1C3 carrying K823012* and J61002 carrying J23100 to J23119 via EcoRI and SpeI
    • Ligation with T4 DNA ligase (New England Biolabs)
* BBa_K823012 corresponds to BBa_J23115 that contains 2 missmatched basepairs.

Constructions were first designed in a software(Geneious v. 6.1.6), Plasmid 1 and 2 below, and then relized on web lab using iGEM 2014 Distribution kit. Verifications were made by eletrophoresis gel analytic PCR amplification and sequencing. Glycerol stock of 3 colonies per constructions were conserved and used for the measurments of GFP expression.

IMAGE

Plasmid map 1: Final construction of PSB1C3 containing E0240 and J23113( EcoRI, PstI, SpeI and XbaI). Constructions carrying J23100 to J23119 and K823012 were similar to this.

IMAGE
Plasmid map 2: Final construction of PSB1C3 containing I20260( EcoRI, PstI, SpeI and XbaI).


Analysis protocol


Our team decided to test the fluorescence with a TECAN infiniteM200 in 96 well plates. Each assay were performed after a 16 - 18 h preculture on 5 ml of LB medium at 37°C with 220 rpm agitation. Cultures were distributed 200 µl per well. Three strains per constructions were tested in five replicates. Two controls were added on plates: LB with chloramphenicol and the strain carrying the promoterless vector on LB with chloramphenicol.
Fluorescence data were analyzed via following formula that come from 2010 De Jong et al Experimental and computational validation of models of fluorescent and luminescent reporter genes in bacteria .

IMAGE

Equation A: A(t) is the corrected absorbance of DH5 alpha with the functional reporter system, Au(t)the uncorrected absorbance of DH5 alpha with the functional reporter system and Ab(t)the background absorbance corresponding to LB with chloramphenicol medium absorbance.
Equation B: B(t) is the absorbance of the strain carrying the promoterless vector, Iu(t) the uncorrected fluorescence intensity of DH5 alpha with the functional reporter system and Ib(t) the background fluorescence intensity of LB chloramphenicol medium with the DH5 alpha carrying the promoterless vector.


Used Biobricks and plasmids


IMAGE

Plasmid map 3: BBa_J61002 plasmid map with restriction sites and J23101 promoter ( EcoRI, PstI, SpeI and XbaI). Plasmids carrying J23100 to J23119 were similar to this.
IMAGE
Plasmid map 4: PSB1C3 carrying BBa_E0240 map with restriction sites and J23101 promoter ( EcoRI, PstI, SpeI and XbaI).





Sequencing results


Device I20260 Forward

AGTCAGTGAGCGAGGAAGCCTGCATAACGCGAAGTAATCTTTTCGGTTTTAAAGAAAAAGGGCAGGGTGGTGACACCTTGCCCTTTTTTGCCGGACTGCAGCGGCCGCTACTAGTATATAAACGCAGAAAGGCCCACCCGAAGGTGAGCCAGTGTGACTCTAGTAGAGAGCGTTCACCGACAAACAACAGATAAAACGAAAGGCCCAGTCTTTCGACTGAGCCTTTCGTTTTATTTGATGCCTGGCTCTAGTATTATTATTTGTATAGTTCATCCATGCCATGTGTAATCCCAGCAGCTGTTACAAACTCAAGAAGGACCATGTGGTCTCTCTTTTCGTTGGGATCTTTCGAAAGGGCAGATTGTGTGGACAGGTAATGGTTGTCTGGTAAAAGGACAGGGCCATCGCCAATTGGAGTATTTTGTTGATAATGGTCTGCTAGTTGAACGCTTCCATCTTCAATGTTGTGTCTAATTTTGAAGTTAACTTTGATTCCATTCTTTTGTTTGTCTGCCATGATGTATACATTGTGTGAGTTATAGTTGTATTCCAATTTGTGTCCAAGAATGTTTCCATCTTCTTTAAAATCAATACCTTTTAACTCGATTCTATTAACAAGGGTATCACCTTCAAACTTGACTTCAGCACGTGTCTTGTAGTTCCCGTCATCTTTGAAAAATATAGTTCTTTCCTGTACATAACCTTCGGGCATGGCACTCTTGAAAAAGTCATGCTGTTTCATATGATCTGGGTATCTCGCANAGCATTGAACACCATAACCGAAAGTAGTGACAAGTGTTGGCCATGGAACAGGTAGTTTTCCAGTAGTGCAAATAAATTTAAGGGTAAGTTTTCCGTATGTTGCATCACCTTCACCCTCTCCACTGACAGAAAATTTGTGCCCATTAACATCACCATCTAATTCAACAAGAATTGGGACAACTCCAGTGAAAAGTTCTTCTCCTTTACGCATCTAGTACTTTCCTGTGTGACTCTAGTAGCTAGCATAATACCTAGGACTGAGCTNNNTGTAAACTCTNNNANCGGCC 

Device J23101 Forward

 ATAAAANTNGGCGTNTCACGAGGCAGAATTTCAGATAAAAAAAATCCTTAGCTTTCGCTAAGGATGATTTCTGGAATTCGCGGCCGCATCTAGAGTTTACAGCTAGCTCAGTCCTAGGTATTATGCTAGCTTCTAGAGTCACACAGGAAAGTACTAGATGCGTAAAGGAGAAGAACTTTTCACTGGAGTTGTCCCAATTCTTGTTGAATTAGATGGTGATGTTAATGGGCACAAATTTTCTGTCAGTGGAGAGGGTGAAGGTGATGCAACATACGGAAAACTTACCCTTAAATTTATTTGCACTACTGGAAAACTACCTGTTCCATGGCCAACACTTGTCACTACTTTCGGTTATGGTGTTCAATGCTTTGCGAGATACCCAGATCATATGAAACAGCATGACTTTTTCAAGAGTGCCATGCCCGAAGGTTATGTACAGGAAAGAACTATATTTTTCAAAGATGACGGGAACTACAAGACACGTGCTGAAGTCAAGTTTGAAGGTGATACCCTTGTTAATAGAATCGAGTTAAAAGGTATTGATTTTAAAGAAGATGGAAACATTCTTGGACACAAATTGGAATACAACTATAACTCACACAATGTATACATCATGGCAGACAAACAAAAGAATGGAATCAAAGTTAACTTCAAAATTAGACACAACATTGAAGATGGAAGCGTTCAACTAGCAGACCATTATCAACAAAATACTCCAATTGGCGATGGCCCTGTCCTTTTACCAGACAACCATTACCTGTCCACACAATCTGCCCTTTCGAAAGATCCCAACGAANAGAGAGACCACATGGTCCTTCTTGAGTTTGTAACAGCTGCTGGGATTACACATGGCATGGATGAACTATACAAATAATAATACTAGAGCCAGGCATCANATAAAACGAAAGGCTCAGTCGAAAGACTGGGCCTTTCGTTTTATCTGTTGTTTGTCGGTGAACGCTCTCTACTAGAGTCACACTGGCTCACCTTCGGGTGGGCCTTTCTGCGTTTATATACTAGTAGCGGCCGCTGCAGTCCGGCAANANAGGGCAAGGTGTCACCACCCTGCCCTTTTTCTTTAAAACCGANAAGATTACTTCGCGTTATGCAGGCTTNCTCGCTCACTGACTCGCTGCGCTCGGTCGTTCGGCTGCGGCGAACGG
Device K823012 Forward

  
TTACTATAAANTAGGCGTATCACGAGGCAGAATTTCAGATAAAAAAAATCCTTAGCTTTCGCTAAGGATGATTTCTGGAATTCGCGGCCGCTTCTAGAGTTTATAGCTAGCTCAGTCCTAGGTACAATGCTAGCTACTAGAGCACACAGGAAAGTACTAGATGCGTAAAGGAGAAGAACTTTTCACTGGAGTTGTCCCAATTCTTGTTGAATTAGATGGTGATGTTAATGGGCACAAATTTTCTGTCAGTGGAGAGGGTGAAGGTGATGCAACATACGGAAAACTTACCCTTAAATTTATTTGCACTACTGGAAAACTACCTGTTCCATGGCCAACACTTGTCACTACTTTCGGTTATGGTGTTCAATGCTTTGCGAGATACCCAGATCATATGAAACAGCATGACTTTTTCAAGAGTGCCATGCCCGAAGGTTATGTACAGGAAAGAACTATATTTTCAAAGATGACGGGAACTACAAGACACGTGCTGAAGTCAAGTTTGAAGNNGATACCCTTGTTAATAGAATCGAGTTAAAAGGTATTGATTTTAAAGAAGATGGAAACATTCTTGGACACANATTGNAATACAACTATAACTCACACAATGTATACATCATGGCAGACAANCNNNAGAATGNAATCAAANTTAACTTCAAAATTANACACAACA
Device I20260 Reverse
TAGGCGTATNANGAGGCAGAATTTCAGATAAAAAAAATCCTTAGCTTTCGCTAAGGATGATTTCTGGAATTCGCGGCCGCTTCTAGAGTTTACAGCTAGCTCAGTCCTAGGTATTATGCTAGCTACTAGAGTCACACAGGAAAGTACTAGATGCGTAAAGGAGAAGAACTTTTCACTGGAGTTGTCCCAATTCTTGTTGAATTAGATGGTGATGTTAATGGGCACAAATTTTCTGTCAGTGGAGAGGGTGAAGGTGATGCAACATACGGAAAACTTACCCTTAAATTTATTTGCACTACTGGAAAACTACCTGTTCCATGGCCAACACTTGTCACTACTTTCGGTTATGGTGTTCAATGCTTTGCGAGATACCCAGATCATATGAAACAGCATGACTTTTTCAAGAGTGCCATGCCCGAAGGTTATGTACAGGAAAGAACTATATTTTTCAAAGATGACGGGAACTACAAGACACGTGCTGAAGTCAAGTTTGAAGGTGATACCCTTGTTAATAGAATCGAGTTAAAAGGTATTGATTTTAAAGAAGATGGAAACATTCTTGGACACAAATTGGAATACAACTATAACTCACACAATGTATACATCATGGCAGACAAACAAAAGAATGGAATCAAAGTTAACTTCAAAATTAGACACAACATTGAAGATGGAAGCGTTCAACTAGCAGACCATTATCAACAAAATACTCCAATTGGCGATGGCCCTGTCCTTTTACCAGACAACCATTACCTGTCCACACAATCTGCCCTTTCGAAAGATCCCAACGAANAGAGAGACCACATGGTCCTTCTTGAGTTTGTAACAGCTGCTGGGATTACACATGGCATGGATGAACTATACAAATAATAATACTAGAGCCAGGCATCAAATAAAACGAAAGGCTCAGTCGAAAGACTGGGCCTTTCGTTTTATCTGTTGTTTGTCGGTGAACGCTCTCTACTAGAGTCACACTGGCTCACCTTCGGGTGGGCCTTTCTGCGTTTATATACTAGTAGCGGCCGCTGCAGTCCGGCAAAAAAGGGCAAGGTGTCACCACCCTGCCCTTTTTCTTTAAAACCGAAAANATTACTTCNCGTTATGCAGGCTTCCTCGCTCACTGACTCGCTGCGCTCGGTCGTTCGGCTGCGGCGNACGG
Device J23101 Reverse

 
Device K823012 Reverse

  

IGEM Evry 2014

Interlab study - Notebook

Picture

The three required devices

IMAGE


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23101 - PSB1C3+E0240+J23104
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (09h00-16h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23119:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (09h00-16h00)
IMAGE DU PLAN DE PLAQUE

Oct 11
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23110 - PSB1C3+E0240+J23107
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (09h00-16h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23106:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (09h00-16h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23108 - PSB1C3+E0240+J23118 - PSB1C3+E0240+J23111
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (14h00-21h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23102:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (14h00-21h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23101 - PSB1C3+E0240+J23104 - PSB1C3+E0240+J23119:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.

Oct 10
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23109 - PSB1C3+E0240+J23117
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (11h00-18h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23114:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (11h00-18h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23115 - PSB1C3+E0240+J23116
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (16h00-23h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23105:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (16h00-23h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23110 - PSB1C3+E0240+J23107 - PSB1C3+E0240+J23106:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.

PSB1C3+E0240+J23108 - PSB1C3+E0240+J23118 - PSB1C3+E0240+J23111 - PSB1C3+E0240+J23102:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.

Oct 09
Picture

Construction n°1: PSB1C3 with I20260




Construction n°2: PSB1C3 with J23101-E1010




Construction n°3: PSB1C3 with K823012-E1010


Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (12h00-17h00)
IMAGE DU PLAN DE PLAQUE


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (12h00-17h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23112 - PSB1C3+E0240+J23103 - PSB1C3+E0240+J23113:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (17h00-00h00)
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23109 - PSB1C3+E0240+J23117 - PSB1C3+E0240+J23114:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.

PSB1C3+E0240+J23115 - PSB1C3+E0240+J23116 - PSB1C3+E0240+J23105:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.

Oct 08
Picture

Construction n°1: PSB1C3 with I20260


Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (12h00-19h00)
IMAGE DU PLAN DE PLAQUE



Construction n°2: PSB1C3 with J23101-E1010


Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM. (12h00-19h00)
IMAGE DU PLAN DE PLAQUE



Construction n°3: PSB1C3 with K823012-E1010


Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.

Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.

Oct 07
Picture

Construction n°1: PSB1C3 with I20260



Construction n°2: PSB1C3 with J23101-E1010


Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.


Construction n°3: PSB1C3 with K823012-E1010


Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h at 37°C.


Other constructions of the Anderson library of constitutive promoters


Oct 06
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM.
OVERFLOW
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23107:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (19h00-02h00).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23109:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP < 80nM.
OVERFLOW
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

Oct 04
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 80-500nM.
OVERFLOW
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23107:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (19h00-02h00).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23109:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP < 80nM.
OVERFLOW
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

Oct 04
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 60-250nM.
OVERFLOW
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23105:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (17h00-00h00).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23107:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23109:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 60-250nM.
OVERFLOW
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23117:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (17h00-00h00).
IMAGE DU PLAN DE PLAQUE
OVERFLOW

Oct 03
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 60-100nM.
TECAN FAILED
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23105:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23107:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 60-100nM.
OVERFLOW

PSB1C3+E0240+J23109:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23117:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

Oct 02
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23107:
Measure of the cells' growth and fluorecence on TECAN infiniteM200.
OVERFLOW

PSB1C3+E0240+J23109:
Measure of the cells' growth and fluorecence on TECAN infiniteM200.
TECAN FAILED

PSB1C3+E0240+J23111:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (17h00-00h00).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23117:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (9h00-16h00).
IMAGE DU PLAN DE PLAQUE

Oct 01
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200.
OVERFLOW

PSB1C3+E0240+J23105:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 40-100nM (10h30-17h30).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23107:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23109:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23111:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23117:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

Sep 30
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23105:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23109:
The pre-culture didn't grow.

Sep 29
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23109:
PCR colony of 8 colonies for each construction following protocol table 1 and 2. gel
Pre-culture from colony 1 for glycerol stock and TECAN in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23114:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 20-60nM (15h00-22h00).
IMAGE DU PLAN DE PLAQUE

Sep 28
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200.
OVERFLOW

PSB1C3+E0240+J23108:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 60-20nM (14h00-21h00).
IMAGE DU PLAN DE PLAQUE

Sep 27
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200.
OVERFLOW
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23107:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 40-100nM (10h30-17h30).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23114:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (9h30-16h30).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23108:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23118:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 5-40nM (18h30-1h30).
IMAGE DU PLAN DE PLAQUE

Sep 26
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200.
OVERFLOW
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23107:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 REPORTED.
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23110:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 40-100nM (15h00-22h00).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23112:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 60-20nM (15h00-22h00).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23114:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23118:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

Sep 25
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Measure of the cells' growth and fluorecence on TECAN infiniteM200.
OVERFLOW
New pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23107:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23110:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23112:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

Sep 24
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23101:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 40-100nM (19h30-2h30).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23113:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 10-40nM (10h-17h).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23119:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 with rank of GFP 40-80nM (20h40-3h40).
IMAGE DU PLAN DE PLAQUE

Sep 23
Picture


Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23101:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23107:
Measure of the cells' growth and fluorecence on TECAN infiniteM200.
OVERFLOW

PSB1C3+E0240+J23113:
Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23118:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (Xh00-Xh00).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23119:
Measure of the cells' growth and fluorecence on TECAN infiniteM200.
TECAN FAILED

Sep 22
Picture

Construction n°1: PSB1C3 with I20260




Construction n°2: PSB1C3 with J23101-E1010




Construction n°3: PSB1C3 with K823012-E1010


Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23100:
  • Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.
  • Measure of the cells' growth and fluorecence on TECAN infiniteM200 (18h30-2h30).
    OVERFLOW

PSB1C3+E0240+J23104:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (1h30-8h30).
PLAN DE PLAQUE

PSB1C3+E0240+J23105:
  • Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.
  • Measure of the cells' growth and fluorecence on TECAN infiniteM200 (18h30-2h30).
    Plaque

PSB1C3+E0240+J23107:
Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

PSB1C3+E0240+J23115:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (10h50-17h50).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23116:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (11h00-18h00).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23117:
Measure of the cells' growth and fluorecence on TECAN infiniteM200 (1h00-8h00).
IMAGE DU PLAN DE PLAQUE

PSB1C3+E0240+J23118:
Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.
Sep 19
Picture

Construction n°1: PSB1C3 with I20260




Construction n°2: PSB1C3 with J23101-E1010




Construction n°3: PSB1C3 with K823012-E1010


Measure of the cells' growth and fluorecence on TECAN infiniteM200 (00h-07h).
PLAN DE PLAQUE

Other constructions of the Anderson library of constitutive promoters


PSB1C3+E0240+J23101:
  • Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.
  • Measure of the cells' growth and fluorecence on TECAN infiniteM200 (16h43-23h43).
    PLAN DE PLAQUE

    PSB1C3+E0240+J23102:
  • Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.
  • Measure of the cells' growth and fluorecence on TECAN infiniteM200 (16h30-23h30).
    PLAN DE PLAQUE

    PSB1C3+E0240+J23104:
    Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    PSB1C3+E0240+J23105:
    glycerol stock preparation from LB culture of the 17th September.

    PSB1C3+E0240+J23107:
    glycerol stock preparation from LB culture of the 17th September.

    PSB1C3+E0240+J23110:
    Pre-culture does'nt grow. The TECAN measure is reported.

    PSB1C3+E0240+J23115:
    Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    PSB1C3+E0240+J23116:
    Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    PSB1C3+E0240+J23117:
    Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    PSB1C3+E0240+J23114:
    • PCR colony of 5 colonies for each construction following protocol table 1 and 2.
      IMAGE
      GEL 1: 1% agarose gel. PCR product of 5 colonies of the PSB1C3+E0240+J23114 construction.

    A pre-culture was made with one colony to make a glycerol stock.

    Sep 18
  • Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010


    Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    Other constructions of the Anderson library of constitutive promoters


    PSB1C3+E0240+J23100:
    Measure of the cells' growth and fluorecence on TECAN infiniteM200 (11h-16h).
    OVERFLOW

    PSB1C3+E0240+J23101:
    Measure of the cells' growth and fluorecence on TECAN infiniteM200.
    TECAN FAILED

    PSB1C3+E0240+J23103:
    Measure of the cells' growth and fluorecence on TECAN infiniteM200 (16h30-23h30).
    PLAN DE PLAQUE

    PSB1C3+E0240+J23105:
    pre-culture of the colony 5 in LB+Cam (1:1000) according to the result of PCR of 13th September. Incubation overnight at 37°C.

    PSB1C3+E0240+J23107:
    pre-culture of the colony 5 in LB+Cam (1:1000) according to the result of PCR of 13th September. Incubation overnight at 37°C.

    PSB1C3+E0240+J23110:
    Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    PSB1C3+E0240+J23115:
    Measure of the cells' growth and fluorecence on TECAN infiniteM200 (12h-19h).
    PLAN DE PLAQUE

    PSB1C3+E0240+J23104, PSB1C3+E0240+J23112, PSB1C3+E0240+J23113: PCR colony of 6 colonies for each construction following protocol table 1 and 2.
    Migration of the PCR products
    PCR purification of clones with the good construction
    IMAGE
    GEL : 1% agarose gel. PCR product of 1 colony of the PSB1C3+E0240+J23104, PSB1C3+E0240+J23112 and PSB1C3+E0240+J23113 constructions.
    A pre-culture was made for each colony to make a glycerol stock.

    Sep 17
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    PSB1C3+E0240+J23100:
    Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    PSB1C3+E0240+J23101:
    Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    PSB1C3+E0240+J23102:
    • glycerol stock preparation from LB culture from the 14th September.
    • Measure of the cells' growth and fluorecence on TECAN infiniteM200.(18h30-1h30):
    IMAGE DU PLAN DE PLAQUE

    PSB1C3+E0240+J23106:
    • glycerol stock preparation from LB culture from the 14th September.
    • Measure of the cells' growth and fluorecence on TECAN infiniteM200.(2h-9h):
    IMAGE DU PLAN DE PLAQUE
    PSB1C3+E0240+J23115 - PSB1C3+E0240+J23115:
    • PCR colony of 5 colonies for each construction following protocol table 1 and 2.
      IMAGE
      GEL 1: 1% agarose gel. PCR product of 5 colonies of the PSB1C3+E0240+J23116 and PSB1C3+E0240+J23115 constructions.

    A pre-culture was made with one colony for each construction to make a glycerol stock.

    PSB1C3+E0240+J23117 - PSB1C3+E0240+J23119:
    • PCR colony of 6 colonies for each construction following protocol table 1 and 2.
      IMAGE
      GEL 2: 1% agarose gel. PCR product of 6 colonies of the PSB1C3+E0240+J23117 and PSB1C3+E0240+J23119 constructions.

    A pre-culture was made with one colony for each construction to make a glycerol stock.


    Sep 16
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010


    Pre-culture from glycerol stock in LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    Other constructions of the Anderson library of constitutive promoters


    PSB1C3+E0240+J23100:
    Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    PSB1C3+E0240+J23106:
    Pre-culture from glycerol in 3mL of LB+Cam (1:1000). Incubation 16h-18h at 37°C.

    Sep 15
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    PSB1C3+E0240+J23101:
    Measure of the cells' growth and fluorecence on TECAN infiniteM200.
    TECAN FAILED

    PSB1C3+E0240+J23106:
    pre-culture of the colony 3 in LB+Cam (1:1000) according to the result of PCR of 13th September. Incubation 16h at 37°C.

    Sep 14
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    PSB1C3+E0240+J23101:
    pre-culture of the colony 3 in LB+Cam (1:1000). Incubation 16h at 37°C.

    PSB1C3+E0240+J23105, PSB1C3+E0240+J23106 and PSB1C3+E0240+J23107:
    • PCR colony of 7 colonies for each construction following protocol table 1 and 2.
      IMAGE
      GEL 1: 1% agarose gel. PCR product of 7 colonies of the PSB1C3+E0240+J23107 construction. PCR product of 8 colonies of the PSB1C3+E0240+J23106 construction.

      A pre-culture was made with one colony for each construction to make a glycerol stock.

      IMAGE
      GEL 2: 1% agarose gel. PCR product of 7 colonies of the PSB1C3+E0240+J23105 construction.

    A pre-culture was made with one colony for each construction to make a glycerol stock.

    Sep 13
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    PSB1C3+E0240+J23101 and PSB1C3+E0240+J23118:
    glycerol stock preparation from LB culture from the 11th September.
    Sep 12
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    PSB1C3+E0240+J23101, PSB1C3+E0240+J23118, PSB1C3+E0240+J23105, PSB1C3+E0240+J23106 and PSB1C3+E0240+J23107:
    • Transformation plate from the 10th September observation. There were 50 colonies for each constructions.


    PSB1C3+E0240+J23101 and PSB1C3+E0240+J23118,
    • PCR colony of 3 colonies for each construction following protocol table 1 and 2.
      IMAGE
      GEL 1: 1% agarose gel.
      Lane 1 to 3: PCR product of 3 colonies of the PSB1C3+E0240+J23101 construction.
      Lane 4 to 6: PCR product of 3 colonies of the PSB1C3+E0240+J23118 construction.
    • PCR purification of sample 1 and 4 of the Gel 1 were purified with the NucleoSpin kit (Macherey Nagel). DNA was quantify by Nanodrop 2000.
    • Preparation of samples to sequencing. N° XX
    • Preparation of 3 ml cultures LB Cam. Incubation overnight at 37°C.


    PSB1C3+E0240+J23100, PSB1C3+E0240+J23102, PSB1C3+E0240+J23103, PSB1C3+E0240+J23104 and PSB1C3+E0240+J23118,
    • PCR colony of 1 colony for each construction following protocol table 1 and 2.
      IMAGE
      GEL 2: 1% agarose gel.
      Lane 1: PCR product of 1 colonies of the PSB1C3+E0240+J23100 construction.
      Lane 2: PCR product of 1 colonies of the PSB1C3+E0240+J23102 construction.
      Lane 3: PCR product of 1 colonies of the PSB1C3+E0240+J23103 construction.
      Lane 4: PCR product of 1 colonies of the PSB1C3+E0240+J23104 construction.

      A pre-culture was made for each colony to make a glycerol stock.

      Sep 11
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    Miniprep disgestion of PSB1C3+E0240 plasmid.
    • 1 µl EcoRI
    • 1 µl XbaI
    • 2 µl buffer 2.1
    • 0.2 µl BSA
    • 5 µl template (miniprep)
    • 10.8 µl miliQ watter

    Miniprep disgestion of BBa_J61002+J23101, BBa_J61002+J23118, BBa_J61002+J23105, BBa_J61002+J23106 and BBa_J61002+J23107 plasmids.
    • 1 µl EcoRI
    • 1 µl SpeI
    • 2 µl buffer 2.1
    • 0.2 µl BSA
    • 5 µl template (miniprep)
    • 10.8 µl miliQ watter
    Incubation 45 minutes at 37°C. Denaturation step 20 minutes at 80 °C.

    Ligation to obtain constructions PSB1C3+E0240+J23101, PSB1C3+E0240+J23118, PSB1C3+E0240+J23105, PSB1C3+E0240+J23106 and PSB1C3+E0240+J23107.
    • 1 µl T4 DNA ligase
    • 6 µl Insert (digested BBa_J61002+J23101, BBa_J61002+J23118, BBa_J61002+J23105, BBa_J61002+J23106 and BBa_J61002+J23107)
    • 2 µl vector (digested PSB1C3+E0240)
    • 2 µl buffer
    • 9 µl miliQ watter
    Incubation 45 minutes at room temperature.
    Transformation in E. coli DH5 alpha with the protocol of the 15th of August. Bacteria were plated on Chloramphenicol agar plates and incubated at 37°C overnight.

    Sep 10
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    Sep 09
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    Sep 07
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    PSB1C3+E0240+J23111:
    PCR colony of 7 colonies for each construction following protocol table 1 and 2. gel
    Pre-culture of colony 2 for grycerol stock
    Sep 06
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    Sep 05
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    Sep 04
    Picture

    Construction n°1: PSB1C3 with I20260




    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    Sep 03
    Picture


    Construction n°1: PSB1C3 with I20260


    Analyse of sequencing results. The two constructions were ok although the colony 4 had a better match. So we decided to keep this colony to perform promoter activity assays.
    26DJ96
    GTCAGTGAGCGAGGNAAGCCTGCATAACGCGAAGTAATCTTTTCGGTTTTAAAGAAAAAGGGCAGGGTGGTGACACCTTGCCCTTTTTTGCCGGACTGCAGC GGCCGCTACTAGTATATAAACGCAGAAAGGCCCACCCGAAGGTGAGCCAGTGTGACTCTAGTAGAGAGCGTTCACCGACAAACAACAGATAAAACGAAAGGCCCAGT CTTTCGACTGAGCCTTTCGTTTTATTTGATGCCTGGCTCTAGTATTATTATTTGTATAGTTCATCCATGCCATGTGTAATCCCAGCAGCTGTTACAAACTCAAGAAG GACCATGTGGTCTCTCTTTTCGTTGGGATCTTTCGAAAGGGCAGATTGTGTGGACAGGTAATGGTTGTCTGGTAAAAGGACAGGGCCATCGCCAATTGGAGTATTTT GTTGATAATGGTCTGCTAGTTGAACGCTTCCATCTTCAATGTTGTGTCTAATTTTGAAGTTAACTTTGATTCCATTCTTTTGTTTGTCTGCCATGATGTATACATTG TGTGAGTTATAGTTGTATTCCAATTTGTGTCCAAGAATGTTTCCATCTTCTTTAAAATCAATACCTTTTAACTCGATTCTATTAACAAGGGTATCACCTTCAAACTT GACTTCAGCACGTGTCTTGTAGTTCCCGTCATCTTTGAAAAATATAGTTCTTTCCTGTACATAACCTTCGGGCATGGCACTCTTGAAAAAGTCATGCTGTTTCATAT GATCTGGGTATCTCGCANAGCATTGAACACCATAACCGAAAGTAGTGACAAGTGTTGGCCATGGAACAGGTAGTTTTCCAGTAGTGCAAATAAATTTAAGGGTAAGT TTTCCGTATGTTGCATCACCTTCACCCTCTCCACTGACAGAAAATTTGTGCCCATTAACATCACCATCTAATTCAACAAGAATTGGGACAACTCCAGTGAAAAGTTC TTCTCCTTTACGCATCTAGTACTTTCCTNNGTGACTCTAGTAGCTANCCATAANNCCTAGGAACTGANCTAGCTG

    26DJ97
    GATTACTANNAATAGGCGTATCACGAGGCAGAATTTCAGATAAAAAAAATCCTTAGCTTTCGCTAAGGATGATTTCTGGAATTCGCGGCCGCTTCTAGAGTT TACAGCTAGCTCAGTCCTAGGTATTATGCTAGCTACTAGAGTCACACAGGAAAGTACTAGATGCGTAAAGGAGAAGAACTTTTCACTGGAGTTGTCCCAATTCTTGT TGAATTAGATGGTGATGTTAATGGGCACAAATTTTCTGTCAGTGGAGAGGGTGAAGGTGATGCAACATACGGAAAACTTACCCTTAAATTTATTTGCACTACTGGAA AACTACCTGTTCCATGGCCAACACTTGTCACTACTTTCGGTTATGGTGTTCAATGCTTTGCGAGATACCCAGATCATATGAAACAGCATGACTTTTTCAAGAGTGCC ATGCCCGAAGGTTATGTACAGGAAAGAACTATATTTTTCAAAGATGACGGGAACTACAAGACACGTGCTGAAGTCAAGTTTGAAGGTGATACCCTTGTTAATAGAAT CGAGTTAAAAGGTATTGATTTTAAAGAAGATGGAAACATTCTTGGACACAAATTGGAATACAACTATAACTCACACAATGTATACATCATGGCAGACAAACAAAAGA ATGGAATCAAAGTTAACTTCAAAATTAGACACAACATTGAAGATGGAAGCGTTCAACTAGCAGACCATTATCAACAAAATACTCCAATTGGCGATGGCCCTGTCCTT TTACCAGACAACCATTACCTGTCCACACAATCTGCCCTTTCGAAAGATCCCAACGAAAAGAGAGACCACATGGTCCTTCTTGAGTTTGTAACAGCTGCTGGGATTAC ACATGGCATGGATGAACTATACAAATAATAATACTAGAGCCAGGCATCAAATAAAACGAAAGGCTCAGTCGAAAGACTGGGCCTTTCGTTTTATCTGTTGTTTGTCG GTGAACGCTCTCTACTAGAGTCACACTGGCTCACCTTCGGGTGGGCCTTTCTGCGTTTATATACTAGTAGCGGCCGCTGCAGTCCGGCAAANAAGGGCAAGGTGTCA CCACCCTGCCCTTTTTCTTTAAAACCGAAAANATTACTT

    26DJ98
    AGTCAGTGAGCGAGGAAGCCTGCATAACGCGAAGTAATCTTTTCGGTTTTAAAGAAAAAGGGCAGGGTGGTGACACCTTGCCCTTTTTTGCCGGACTGCAGC GGCCGCTACTAGTATATAAACGCAGAAAGGCCCACCCGAAGGTGAGCCAGTGTGACTCTAGTAGAGAGCGTTCACCGACAAACAACAGATAAAACGAAAGGCCCAGT CTTTCGACTGAGCCTTTCGTTTTATTTGATGCCTGGCTCTAGTATTATTATTTGTATAGTTCATCCATGCCATGTGTAATCCCAGCAGCTGTTACAAACTCAAGAAG GACCATGTGGTCTCTCTTTTCGTTGGGATCTTTCGAAAGGGCAGATTGTGTGGACAGGTAATGGTTGTCTGGTAAAAGGACAGGGCCATCGCCAATTGGAGTATTTT GTTGATAATGGTCTGCTAGTTGAACGCTTCCATCTTCAATGTTGTGTCTAATTTTGAAGTTAACTTTGATTCCATTCTTTTGTTTGTCTGCCATGATGTATACATTG TGTGAGTTATAGTTGTATTCCAATTTGTGTCCAAGAATGTTTCCATCTTCTTTAAAATCAATACCTTTTAACTCGATTCTATTAACAAGGGTATCACCTTCAAACTT GACTTCAGCACGTGTCTTGTAGTTCCCGTCATCTTTGAAAAATATAGTTCTTTCCTGTACATAACCTTCGGGCATGGCACTCTTGAAAAAGTCATGCTGTTTCATAT GATCTGGGTATCTCGCANAGCATTGAACACCATAACCGAAAGTAGTGACAAGTGTTGGCCATGGAACAGGTAGTTTTCCAGTAGTGCAAATAAATTTAAGGGTAAGT TTTCCGTATGTTGCATCACCTTCACCCTCTCCACTGACAGAAAATTTGTGCCCATTAACATCACCATCTAATTCAACAAGAATTGGGACAACTCCAGTGAAAAGTTC TTCTCCTTTACGCATCTAGTACTTTCCTGTGTGACTCTAGTAGCTAGCATAATACCTAGGACTGAGCTNNNTGTAAACTCTNNNANCGGCC

    26DJ99
    TAGGCGTATNANGAGGCAGAATTTCAGATAAAAAAAATCCTTAGCTTTCGCTAAGGATGATTTCTGGAATTCGCGGCCGCTTCTAGAGTTTACAGCTAGCTC AGTCCTAGGTATTATGCTAGCTACTAGAGTCACACAGGAAAGTACTAGATGCGTAAAGGAGAAGAACTTTTCACTGGAGTTGTCCCAATTCTTGTTGAATTAGATGGT GATGTTAATGGGCACAAATTTTCTGTCAGTGGAGAGGGTGAAGGTGATGCAACATACGGAAAACTTACCCTTAAATTTATTTGCACTACTGGAAAACTACCTGTTCCA TGGCCAACACTTGTCACTACTTTCGGTTATGGTGTTCAATGCTTTGCGAGATACCCAGATCATATGAAACAGCATGACTTTTTCAAGAGTGCCATGCCCGAAGGTTAT GTACAGGAAAGAACTATATTTTTCAAAGATGACGGGAACTACAAGACACGTGCTGAAGTCAAGTTTGAAGGTGATACCCTTGTTAATAGAATCGAGTTAAAAGGTATT GATTTTAAAGAAGATGGAAACATTCTTGGACACAAATTGGAATACAACTATAACTCACACAATGTATACATCATGGCAGACAAACAAAAGAATGGAATCAAAGTTAAC TTCAAAATTAGACACAACATTGAAGATGGAAGCGTTCAACTAGCAGACCATTATCAACAAAATACTCCAATTGGCGATGGCCCTGTCCTTTTACCAGACAACCATTAC CTGTCCACACAATCTGCCCTTTCGAAAGATCCCAACGAANAGAGAGACCACATGGTCCTTCTTGAGTTTGTAACAGCTGCTGGGATTACACATGGCATGGATGAACTA TACAAATAATAATACTAGAGCCAGGCATCAAATAAAACGAAAGGCTCAGTCGAAAGACTGGGCCTTTCGTTTTATCTGTTGTTTGTCGGTGAACGCTCTCTACTAGAG TCACACTGGCTCACCTTCGGGTGGGCCTTTCTGCGTTTATATACTAGTAGCGGCCGCTGCAGTCCGGCAAAAAAGGGCAAGGTGTCACCACCCTGCCCTTTTTCTTTA AAACCGAAAANATTACTTCNCGTTATGCAGGCTTCCTCGCTCACTGACTCGCTGCGCTCGGTCGTTCGGCTGCGGCGNACGG

    26EA00
    Impossible to read

    26EA01
    Impossible to read

    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010



    Other constructions of the Anderson library of constitutive promoters


    Miniprep cultures from the 2cnd of september was purified with the NucleoSpin Plasmid kit (Macherey-Nagel). DNA was quantify with the Nanodrop 2000.
    Glycerol stock were prepared started from the 16 cultures from the 2cnd of september (750 µl of culture + 750 µL of 10% glycerol) and stored at -80°C. Sep 02
    Picture


    Other constructions of the Anderson library of constitutive promoters


    PCR colony were performed on colonies from transformations of the 29th August. Used protocol was the same as Table 1 and 2 with the Q5 high fidelity enzyme.
    PCR product of first colony of each transformation was loaded on 1% agarose gel and gel run 45 minutes at 110 mV.
    IMAGE
    PCR product of BBa_J61002 plasmids containing promoters results.
    3 ml LB culture were started from tested colonies which presented the right PCR product profile. Cultures were incubated overnight at 37°C. Sep 01

    Picture


    Other constructions of the Anderson library of constitutive promoters


    Aug 31
    Picture


    Other constructions of the Anderson library of constitutive promoters


    Transformation plates observation.
    IMAGE
    Colony number according to plasmid including promoters.
    PCR colony were performed on 8 colonies per transformation plate. PCR products were loaded on 1% agarose gel and gel ran one 45 minutes. There were nothing on gel, reason is probably a mix and temperature problem.
    Aug 30
    Picture

    Construction n°1: PSB1C3 with I20260


    Selected colonies PCR products from the 28/08/2014 were purified with the NucleoSpin kit (Macherey Nagel). DNA was quantify by Nanodrop 2000.
    • Colony n°2: 30.7 ng/µl and A260/280 1.92
    • Colony n°4: 52.3 ng/µl and A260/280 1.75
    • Colony n°7: 26.1 ng/µL and A260/280 1.72

    Samples were send to sequencing. N° 26DJ96, 26DJ97, 26DJ98, 26DJ99, 26EA00 and 26EA01.

    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: PSB1C3 with K823012-E1010


    Selected colonies PCR products from the 28/08/2014 were purified with the NucleoSpin kit (Macherey Nagel). DNA was quantify by Nanodrop 2000.
    • Colony n°2: 41.4 ng/µl
    • Colony n°3: 65.8 ng/µl
    • Colony n°4: 27.4 ng/µL

    Colony n°3 was sent to sequence with the identification 26AE07 (VF2) and 26AE08 (VR)

    Other constructions of the Anderson library of constitutive promoters


    Transformation in DH5 alpha chemocompetent E. coli as doing on 21th August, with ampicilline LB agar plates
    Incubation overnight at 37°C.

    Aug 29
    Picture



    Contruction n°2: PSB1C3 with J23101-E1010




    Contruction n°3: PSB1C3 with K823012-E1010


    PCR colony was done on 7 colonies:
    1. Steril H2O:34,5µL
    2. 5X Q5 Reaction buffer: 10µL
    3. Template:2µL
    4. 10mM dNTP: 1µL
    5. 10µM Primer forward VF2: 1µL
    6. 10µM Primer reverse VR: 1µL
    7. Q5 DNA Polymerase: 0,5µL

    A migration of PCR product was done. We expect to observe in each wells a band of 1176bp:
    image not found

    6 colonies have a band at 1200 bp around so we decided to choose colonies n°2, 3 and 4.

    Other constructions of the Anderson library of constitutive promoters


    Promoters were resuspended from 2014 distribution kit plates with 10 µl of sterile MiliQ watter and stored at -20°C.
    IMAGE
    Table: Additional promoters of the Interlab Study. In grey, plasmids already resuspended, transformed, sequenced and stock glycerol existed.

    Aug 28
    Picture

    Contruction n°1: pSB1C3 with I20260




    Contruction n°2: pSB1C3 with J23101-E1010




    Contruction n°3: pSB1C3 with K823012-E1010


    At the end of the day, there were 3 colonies that have grown

    Aug 27
    Picture

    Construction n°1: PSB1C3 with I20260


    Loading of the PSB1C3 digestion by EcoRI and PstI from the 25th August, on a 1% agarose gel. The 40 µl were loaded with 8 µl of loading dye 6X. Migration was performed 1 hour at 110 mV.
    IMAGE
    Figure 6: 1% agarose gel of colony PCR products for BBa_E0240 and BBa_I20260. Lane 2 and 3: digestion product of PSB1C3 by EcoRI and PstI, Lane 4: Purple 2-Log ladder NEB



    Construction n°2: PSB1C3 with J23101-E1010




    Construction n°3: pSB1C3 with K823012-E1010


    Digestion of the insert pSB1C3 (J23115) with EcoRI and XbaI:
    • Steril H2O: 10,8µL
    • Buffer 2.1 NEB : 2µL
    • BSA: 0,2µL
    • DNA: 5µL
    • EcoRI-HF: 1µL
    • XbaI: 1µl

    Digestion of the vector pSB1C3(E0240) with EcoRI and SpeI:
    • Steril H2O: 10,8µL
    • Buffer 2.1 NEB : 2µL
    • BSA: 0,2µL
    • DNA: 5µL
    • EcoRI-HF: 1µL
    • SpeI: 1µl

    Mix were incubated at 37°C during 45mn then at 80°C during 20 mn

    Ligation:
    • Steril H2O: 9µL
    • Insert (J23115):6µL
    • Vector (E0240): 2µL
    • 10X T4 DNA ligase reaction buffer: 2µL

    Mix was incubated at 10mn at room temperature then at 80°C during 20mn before the transformation in DH5a chimiocompetent with 3µL of the ligation product with the same protocol
    Aug 26
    Picture


    Aug 25
    Picture


    Aug 24
    Picture

    Contruction n°1: PSB1C3 with I20260


    Digestion of PSB1C3 and PSB1K3-I20260 by EcoRI and PstI
    • 1 µl EcoRI-HF
    • 1 µl PstI
    • 2 µl buffer
    • 0.2 µl BSA
    • 13.7 or 76 µl respectively for I20260 and PSB1C3
    • 10.8 µl miliQ watter

    Incubation 45 minutes at 37°C. Denaturation step 20 minutes at 80 °C.
    Loading on a 1% agarose gel to perform an extraction from gel

    Contruction n°2: PSB1C3 with J23101-E1010


    Aug 23
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010


    Transformation plate observation:
    - BBa_J23101: 11 isolated colonies
    - BBa_K823012: 100-150 isolated colonies

    A PCR was performed with 8 colonies for BBa_K823012 and for BBa_J23101 following the protocol Table 3 and 4.
    To verify PCR products, 10 µl was loaded on a 1% agarose gel with 2 µl of loading dye 6X.

    IMAGE
    1% agarose gel of PCR products. Lane 1 to 8: BBa_K823012 PCR products and Lane 9: Purple 2-Log. ladder NEB

    We expected to obtain a band between 300 and 400 bp. So we decided to amplify the colony n°8. The colony was seed in 5 ml of LB medium and 5 µl of chloramphenicol. Culture was incubated overnight at 37°C with 200 rpm agitation.
    IMAGE
    1% agarose gel of PCR products. Lane 10 to 17: BBa_J23101 PCR products and Lane 9: Purple 2-Log ladder NEB


    We expected to obtain a band around 1200 bp. So we decided to amplify the colony n°2 corresponding to lane 11. The colony was seed in 5 ml of LB medium and 5 µl of chloramphenicol. Culture was incubated overnight at 37°C with 200 rpm agitation.

    Aug 22
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010


    Transformations of registry parts (BBa_K823012 and J23101) were performed to obtain colonies with plasmid containing parts for future amplifications.
    The transformation was performed on DH5 alpha E. coli, as followed:

    1. Remove E. coli competent tubes from -80°C and keep it on ice
    2. Add 3 µl of template (here solubilized plasmids from the registry distribution kit) and mix gently
    3. Incubate 10 minutes on ice
    4. Perform an heat shock 30 seconds at 42°C
    5. Incubate 2 minutes on ice
    6. Add 2 ml of LB medium and incubate 60 minutes at 37°C with an agitation at 200 rpm
    7. Plate 200 µl of BBa_K823012 or BBa_J23101 on a chloramphenicol LB agar plate.
    8. Incubate plate overnight at 37°C

    Aug 21
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010

    Miniprep cultures from the 19th August was purified with the NucleoSpin Plasmid kit (Macherey-Nagel). DNA was quantify with the Nanodrop 2000. DNA concentrations and A260/280 were respectively for BBa_E0240 and BBa_I20260: 42 ng/µl and 1.91 ; 13.7 ng/µl and 1.71.
    A glycerol stock was prepared for each culture and stored at -80°C.

    Aug 20
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010

    Preparation of a 1% agarose gel: 1.01 g of Top Vision agarose (Thermo Scientific) + 100 ml of TAE 1X. Microwave 30s by 30s until agarose total dissolution Gel was cooling down until to be lukewarm, one BET drop was added. Gel was loaded with 10µl per sample previously added with 2 µl of loading dye 6X, and 5 µl for ladders. Gel running 45 minutes at 100 mV in TAE 1X buffer.

    IMAGE
    Figure 6: 1% agarose gel of colony PCR products for BBa_E0240 and BBa_I20260. Lane 1 and 10: Purple 2-Log ladder NEB, Lane 2 to 9: BBa_E0240 PCR products, Lane 11 to 17: BBa_I20260 PCR products
    We expected one band at 1200 bp for both BioBrick. So we decided to amplify the colony 1 for BBa_E0240 and colony 1 for BBa_I20260. PCR products were purified with the GeneJET purification kit (Thermo Scientific) followed by DNA quantification with the NanoDrop 2000 (Thermo Scientific). BBa_E0240 purified PCR product: 61 ng/µl and BBa_I20260 purified PCR product: 37.8 ng/µl.
    Purified PCR product aliquot was send to sequencing. The sequencing number were 26DJ68, 69, 70, 71.
    Preparation of miniprep culture of BBa_I20260 and BBa_E0240 selected colonies in 5 ml of LB with respectively 5 µl of Kana or chloramphenicol solution stock. Incubation overnight at 37°C and 300 rpm.

    Aug 19
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010

    Sequencing results were received for BBa_J23101 (26DJ62 and 26DJ63) and BBa_K823012(26DJ64 and 26DJ65) PCR products.
    26DJ62

    TCAGANNAAAAAAATCCTTAGCTNNCGCTAAGGATGANNTCTGGAATTCGCGGCCGCTTCTAGAGTTTACAGCTAGCTCAGTCCTAGGTATTATGCTAGCTACTAGTAG CGGCCGCTGCAGTCCGGCAAAAAAGGGCAAGGTGTCACCACCCTGCCCTTTTTCTTTAAAACCGAAAAGATTACTTCGCGTTATGCAGGCTTCCTCGCTCACTGACTC GCTGCGCTCGGTCGTTCGGCTGCGGCGAGCGGTATCAGCTCACTCAGAG


    26DJ63

    GAGCGCANCGAGTCAGTGAGCGAGGAAGCCTGCATAACGCGAAGTAATCTTTTCGGTTTTAAAGAAAAAGGGCAGGGTGGTGACACCTTGCCCTTTTTTGCCGGACTG CAGCGGCCGCTACTAGTAGCTAGCATAATACCTAGGACTGAGCTAGCTGTAAACTCTAGAAGCGGCCGCGAATTCCAGAAATCATCCTTAGCGAAAGCTAAGGATTTTT TTTATCTGAAATTCTGCCTCGTGATACGCCTATTTTTATAGGTTAATGTCATGATAATAATGGTTTCTTAGACGCAAGGTGGCAAA


    26DJ64

    TCAGANNAAAAAAATCCTTAGCTNNCGCTAAGGATGATTTCTGGAATTCGCGGCCGCTTCTAGAGGTTTATAGCTAGCTCATCCTAGGTACAATGCTAGCTACTAG TAGCGGCCGCTGCAGTCCGGCAAAAAAGGGCAAGGTGTCACCACCCTGCCCTTTTTCTTTAAAACCGAAAAGATTACTTCGCGTTATGCAGGCTTCCTCGCTCACTGAC TCGCTGCGCTCGGTCGTTCGGCTGCGGCGAGCGGTATCAGCTCACTCAGG


    26DJ65

    CNGCGAGTCAGTNAGCGAGGAAGCCTGCANNACGCGAAGTNATCTTTTTCGGTTTTAAAGAAAAAGGGCAGGGTGGTGACACCTNGCCCTTTTTTGCCGGACTGCAGC GGCCGCTACTAGTAGCTAGCATTGTACCTAGGACTGAGCTAGCTATAAACTCTAGAAGCGGCCGCGAATTCCAGAAATCATCCTTAGCGAAAGCTAAGGATTTTTTTTA TCTGAAATTCTGCCTCGTGATACGCCTATTTTTATAGGTTAATGTCATGATAATAATGGTTTCTTAAC


    The mapping was perfect for BBa_J23101 for BBa_K823012.

    Sequencing results were received for BBa_E0240 (26DJ68 and 26DJ69) and BBa_I20260 (26DJ70 and 26DJ71) PCR products.
    26DJ68
    GAGCNCAGCGAGTCAGTGAGCGAGGAAGCCTGCATAACGCGAAGTAATCTTTTCGGTTTTAAAGAAAAAGGGCAGGGTGGTGACACCTTGCCCTTTTTTGCCGGACTG CAGCGGCCGCTACTAGTATATAAACGCAGAAAGGCCCACCCGAAGGTGAGCCAGTGTGACTCTAGTAGAGAGCGTTCACCGACAAACAACAGATAAAACGAAAGGCCC AGTCTTTCGACTGAGCCTTTCGTTTTATTTGATGCCTGGCTCTAGTATTATTATTTGTATAGTTCATCCATGCCATGTGTAATCCCAGCAGCTGTTACAAACTCAAGA AGGACCATGTGGTCTCTCTTTTCGTTGGGATCTTTCGAAAGGGCAGATTGTGTGGACAGGTAATGGTTGTCTGGTAAAAGGACAGGGCCATCGCCAATTGGAGTATTT TGTTGATAATGGTCTGCTAGTTGAACGCTTCCATCTTCAATTTGTGTCTAATTTTGAAGTTAACTTTGATTCCATTCTTTTGTTTGTCTGCCATGATGTATACATTGT GTGAGTTATAGTTGTATTCCAATTTGTGTCCAAGAATGTTTCCATCTTCTTTAAAATCAATACCTTTTAACTCGATTCTATTAACAAGGGTATCACCTTCAAACTTGA CTTCAGCACGTGTCTTGTAGTTCCCGTCATCTTTGAAAAATATAGTTCTTTCCTGTACATAACCTTCGGGCATGGCACTCTTGAAAAAGTCATGCTGTTTCATATGAT CTGGGTATCTCGCAAAGCATTGAACACCATAACCGAAAGTAGTGACAAGTGTTGGCCATGGAACAGGTAGTTTTCCAGTAGTGCAAATAAATTTAAGGGTAAGTTTTC CGTATGTTGCATCACCTTCACCCTCTCCACTGACAGAAAATTTGTGCCCATTAACATCACCATCTAATTCAACAAGAATTGGGACAACTCCAGTGAANAGTTCTTCTC CTTTACGCATCTAGTACTTTCCTGTGTGACTCTAGTAGCTAGCATAATACCTAGGACTGAGCTAGCTGTNAACTCTANAAGCGGCCGCGAATTCCAGAAATCATCCTT ANCNNAAGCTAAGGATTTTTTTTATCTGNAATTCTGCCTC

    26DJ69
    GATTACTATNAAATAGGCGTANNANGAGGCAGAATTTCAGATAAAAAAAATCCTTAGCTTTCGCTAAGGATGATTTCTGGAATTCGCGGCCGCTTCTAGAGTTTACAG CTAGCTCAGTCCTAGGTATTATGCTAGCTACTAGAGTCACACAGGAAAGTACTAGATGCGTAAAGGAGAAGAACTTTTCACTGGAGTTGTCCCAATTCTTGTTGAATT AGATGGTGATGTTAATGGGCACAAATTTTCTGTCAGTGGAGAGGGTGAAGGTGATGCAACATACGGAAAACTTACCCTTAAATTTATTTGCACTACTGGAAAACTACC TGTTCCATGGCCAACACTTGTCACTACTTTCGGTTATGGTGTTCAATGCTTTGCGAGATACCCAGATCATATGAAACAGCATGACTTTTTCAAGAGTGCCATGCCCGA AGGTTATGTACAGGAAAGAACTATATTTTTCAAAGATGACGGGAACTACAAGACACGTGCTGAAGTCAAGTTTGAAGGTGATACCCTTGTTAATAGAATCGAGTTAAA AGGTATTGATTTTAAAGAAGATGGAAACATTCTTGGACACAAATTGGAATACAACTATAACTCACACAATGTATACATCATGGCAGACAAACAAAAGAATGGAATCAA AGTTAACTTCAAAATTAGACACAACATTGAAGATGGAAGCGTTCAACTAGCAGACCATTATCAACAAAATACTCCAATTGGCGATGGCCCTGTCCTTTTACCAGACAA CCATTACCTGTCCACACAATCTGCCCTTTCGAAAGATCCCAACGAANAGAGAGACCACATGGTCCTTCTTGAGTTTGTAACAGCTGCTGGGATTACACATGGCATGGA TGAACTATACAAATAATAATACTAGAGCCAGGCATCAAATAAAACGAAAGGCTCAGTCGAAAGACTGGGCCTTTCGTTTTATCTGTTGTTTGTCGGTGAACGCTCTCT ACTAGAGTCACACTGGCTCACCTTCGGGTGGGCCTTTCTGCGTTTATATACTAGTAGCGGCCGCTGCAGTCCGGCNAAAAAGGGCAAGGTGTCACCACCNTGCCCTTT TTCTTTAAAACCGNAAA

    26DJ70
    AGCGAGTCAGTGAGCGAGGAAGCCTGCATAACGCGAAGTAATCTTTTCGGTTTTAAAGAAAAAGGGCAGGGTGGTGACACCTTGCCCTTTTTTGCCGGACTGCAGCGG CCGCTACTAGTATATAAACGCAGAAAGGCCCACCCGAAGGTGAGCCAGTGTGACTCTAGTAGAGAGCGTTCACCGACAAACAACAGATAAAACGAAAGGCCCAGTCTT TCGACTGAGCCTTTCGTTTTATTTGATGCCTGGCTCTAGTATTATTATTTGTATAGTTCATCCATGCCATGTGTAATCCCAGCAGCTGTTACAAACTCAAGAAGGACC ATGTGGTCTCTCTTTTCGTTGGGATCTTTCGAAAGGGCAGATTGTGTGGACAGGTAATGGTTGTCTGGTAAAAGGACAGGGCCATCGCCAATTGGAGTATTTTGTTGA TAATGGTCTGCTAGTTGAACGCTTCCATCTTCAATGTTGTGTCTAATTTTGAAGTTAACTTTGATTCCATTCTTTTGTTTGTCTGCCATGATGTATACATTGTGTGAG TTATAGTTGTATTCCAATTTGTGTCCAAGAATGTTTCCATCTTCTTTAAAATCAATACCTTTTAACTCGATTCTATTAACAAGGGTATCACCTTCAAACTTGACTTCA GCACGTGTCTTGTAGTTCCCGTCATCTTTGAAAAATATAGTTCTTTCCTGTACATAACCTTCGGGCATGGCACTCTTGAAAAAGTCATGCTGTTTCATATGATCTGGG TATCTCGCAAAGCATTGAACACCATAACCGAAAGTAGTGACAAGTGTTGGCCATGGAACAGGTAGTTTTCCAGTAGTGCAAATAAATTTAAGGGTAAGTTTTCCGTAT GTTGCATCACCTTCACCCTCTCCACTGACAGAAAATTTGTGCCCATTAACATCACCATCTAATTCAACAAGAATTGGGACAACTCCAGTGAAAAGTTCTTCTCCTTTA CGCATCTAGTACTTTCCTGTGTGACTCTAGAAGCGGCCGCGAATTCCAGAAATCATCCTTAGCGATGAATTCCAGAAATCATCCTTANCGAAAGCTNAGGATTTTTTT TATCTGNAATTCTGNCTCG

    26DJ71
    GATTAAACTATNAATAGGCGTATCACGAGGCAGAATTTCAGATAAAAAAAATCCTTAGCTTTCGCTAAGGATGATTTCTGGAATTCATCGCTAAGGATGATTTCTGGA ATTCGCGGCCGCTTCTAGAGTCACACAGGAAAGTACTAGATGCGTAAAGGAGAAGAACTTTTCACTGGAGTTGTCCCAATTCTTGTTGAATTAGATGGTGATGTTAAT GGGCACAAATTTTCTGTCAGTGGAGAGGGTGAAGGTGATGCAACATACGGAAAACTTACCCTTAAATTTATTTGCACTACTGGAAAACTACCTGTTCCATGGCCAACA CTTGTCACTACTTTCGGTTATGGTGTTCAATGCTTTGCGAGATACCCAGATCATATGAAACAGCATGACTTTTTCAAGAGTGCCATGCCCGAAGGTTATGTACAGGAA AGAACTATATTTTTCAAAGATGACGGGAACTACAAGACACGTGCTGAAGTCAAGTTTGAAGGTGATACCCTTGTTAATAGAATCGAGTTAAAAGGTATTGATTTTAAA GAAGATGGAAACATTCTTGGACACAAATTGGAATACAACTATAACTCACACAATGTATACATCATGGCAGACAAACAAAAGAATGGAATCAAAGTTAACTTCAAAATT AGACACAACATTGAAGATGGAAGCGTTCAACTAGCAGACCATTATCAACAAAATACTCCAATTGGCGATGGCCCTGTCCTTTTACCAGACAACCATTACCTGTCCACA CAATCTGCCCTTTCGAAAGATCCCAACGAANAGAGAGACCACATGGTCCTTCTTGAGTTTGTAACAGCTGCTGGGATTACACATGGCATGGATGAACTATACAAATAA TAATACTAGAGCCAGGCATCAAATAAAACGAAAGGCTCAGTCGAAAGACTGGGCCTTTCGTTTTATCTGTTGTTTGTCGGTGAACGCTCTCTACTAGAGTCACACTGG CTCACCTTCGGGTGGGCCTTTCTGCGTTTATATACTAGTAGCGGCCGCTGCAGTCCGGCAAANAAGGGCAAGGTGTCACCACCNTGCCCTTTTTCTTTAAAACCGNAA AGATTACTTCNNNGTTATGCAGGCTTCCTCGCTCACTGACTCGCTGCGCTCGGTCGTTCGGCT

    The mapping were correct for BBa_E0240 and BBa_I20260.

    Colony PCRs were performed on 8 colonies for BBa_E0240 and BBa_I20260, form plates from the transformation of 16th August.
    IMAGE
    Table 3: PCR mix Preparation for One Taq PCR colony
    49 µl of mix were distributed in each PCR tubes. The One Taq PCR program was applied.
    IMAGE
    Table 4:IGEM One Taq PCR program termocycling conditions
    Aug 18
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010

    Colonies had grown on plates as followed:

    • LB agar: more than 1000 colonies for the two biobricks
    • LB agar kanamycin: 10 colonies for BBa_E0240 and >40 colonies for BBa_I20260
    • LB agar chloramphenicol: >50 colonies for BBa_E0240 and 3 colonies for BBa_I20260

    Plate storage at 4°C.

    Aug 17
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010

    Nothing had grown during the night on both plates. Taking into consideration different hypothesis, the transformation was repeated with a change on step 6 and 7. At step 6, only 1 ml of LB medium was added. To plate, 200 µl of BBa_E0240 and BBa_I20260 were plated on 3 plates: LB agar, LB agar kanamycin and LB agar chloramphenicol.

    Aug 16
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010

    BBa_E0240 and BBa_I20260 are respectively into a PSB1C3 and a PSB1K3 vector. In order to select colonies, LB complemented with kanamycin or chloramphenicol are necessary. 200 ml of LB agar medium was prepared with 7 g of LB Agar powder(Sigma) into 200 ml of miliQ water. After complete dissolution, the solution was sterilized in the Tuttmauer 2540ML apparatus, STE 20 minutes at 121°C and EXT+DRY 15 minutes. 50 µl of kanamycin stock solution (25 mg/L) was added to 50 ml of LB agar to pour 2 plates. 150 µl of chloramphenicol stock solution was added in the 150 LB agar remaining ml to pour 6 plates.
    The transformation was performed into DH5 alpha ''E. coli'', as followed:

    1. Remove E. coli competent tubes from -80°C and keep it on ice
    2. Add 1 µl of template (here solubilized plasmids from the registry distribution kit) and mix gently
    3. Incubate 10 minutes on ice
    4. Perform an heat shock 30 seconds at 42°C
    5. Incubate 2 minutes on ice
    6. Add 3 ml of LB medium and incubate 60 minutes at 37°C with an agitation at 200 rpm
    7. Plate 200 µl of BBa_E0240 on a chloramphenicol LB agar plate and BBa_I20260 on a Knamycin LB agar plate
    8. Incubate plate overnight at 37°C
    Aug 15
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010

    To amplify BBa_I20260 and BBa_0240, a PCR was perform with the mix described Table 1. The program IGEM Q5 PCR was applied, see Table 2. PCR products were cleaned with the GeneJET purification kit (Thermo Scientific)followed by DNA quantification with the NanoDrop 2000 (Thermo Scientific). Purified samples of I20260 and E1010 had respectively following concentration 30.9 ng/µl and 43.3 ng/µl.


    Preparation of a 1% agarose gel: 0.52 g of Top Vision agarose (Thermo Scientific) + 50 ml of TAE 1X. Microwave 30s by 30s until agarose total dissolution Gel was cooling down until to be lukewarm, one BET drop was added. Gel was loaded with 20 µl of BBa_E0240 PCR product and BBa_I20260 purified PCR product added with 4 µl of loading dye, at 10µl of the mix per well. Gel running 45 minutes at 100 mV in TAE 1X buffer.

    IMAGE
    Figure 4: 1% agarose gel of PCR products from 08.14.2014 after PCR clean up. Lane 1 and 5: Purple 2-Log ladder NEB, Lane 2, 3 and 4: BBa_E0240 purified PCR product, Lane 6,7 and 8: BBa_I20260 purified PCR product


    3 pieces of gel were sampled in four tubes to perform a DNA purification from gel. The DNA purification was made with the GeneJET purification kit (Thermo Scientific).
    A verification electrophoresis was performed on a 1% agarose gel.

    IMAGE
    Figure 5: 1% agarose gel of purified fragments from gel. Lane 1: Purple 2-Log ladder NEB, Lane 2: BBa_E0240 1200 bp purified fragment and Lane 3: BBa_I20260 1200 bp purified fragment

    The major part of the DNA was lost during the purification because the amount of was to weak to be purified from gel. So we decide do transform ''E. coli'' to isolate a colony containing the desired plasmid for BBa_E0240 and BBa_I20260.

    Aug 14
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010

    PCR products were cleaned with the GeneJET purification kit (Thermo Scientific)followed by DNA quantification with the NanoDrop 2000 (Thermo Scientific).
    Purified PCR product of BBa_J61002/J23101 and BBa_J61002/K823012 concentration were respectively: 53.9 ng/µl and 54.1 ng/µl.


    Preparation of a 1% agarose gel: 0.56 g of Top Vision agarose (Thermo Scientific) + 50 ml of TAE 1X. Microwave 30s by 30s until agarose total dissolution Gel was cooling down until to be lukewarm, one BET drop was added. Gel was loaded with 10µl per sample previously added with 2 µl of loading dye 6X, and 5 µl for ladders. Gel running 45 minutes at 100 mV in TAE 1X buffer.

    IMAGE
    Figure 2: 1% agarose gel of PCR products from 08.12.2014 after PCR clean up. Lane 1 and 7: Purple 2-Log ladder NEB, Lane 2: BBa_J23101 purified PCR product, Lane 3: BBa_K823012 purified PCR product, Lane 4: BBa_E0240 purified PCR product, Lane 5: BBa_I20260 purified PCR product and Lane 6: pBHR1 purified PCR product

    Profiles were same as before PCR clean up. To sequence the amplified parts, we decided to a purification of fragments from the gel as presented below.



    Preparation of a 1% agarose gel: 0.56 g of Top Vision agarose (Thermo Scientific) + 50 ml of TAE 1X. Microwave 30s by 30s until agarose total dissolution. Gel was cooling down until to be lukewarm, one BET drop was added. Gel was loaded with 30 µl of BBa_E0240 purified PCR product and BBa_I20260 purified PCR product added with 6 µl of loading dye, at 10µl of the mix per well. Gel running 45 minutes at 100 mV in TAE 1X buffer.

    IMAGE
    Figure 3: 1% agarose gel of PCR products from 08.12.2014 after PCR clean up. Lane 4 and 8: Purple 2-Log ladder NEB, Lane 1, 2 and 3: BBa_E0240 purified PCR product, Lane 5, 6 and 7: BBa_I20260 purified PCR product

    Four pieces of gel were sampled in four tubes to perform a DNA purification from gel.


    Aug 13
    Picture

    Contructions PSB1C3 with I20260, J23101-E1010 and K823012-E1010

    The 4 needed parts are: BBa_J23101, BBa_K823012, BBa_E0240 and BBa_I20260. Corresponding wells were located on 2014 Distribution kit plates and resuspended with 10 µL steril water. That permits to obtain a DNA concentration around 0.2 ng/µl (according to the registry. Solutions were transferred into 1 ml eppendorf tubes and stored at -20°C.
    To amplify fragments, a PCR was performed on the 4 constructions, with the mix described on table 1.

    IMAGE
    Table 1: PCR mix preparation

    Distribution of 49 µl of mix per PCR tube. Application of program IGEM Q5 PCR.

    IMAGE
    Table 2: IGEM Q5 PCR program thermocycling conditions

    Preparation of a 1% agarose gel: 0.56 g of Top Vision agarose (Thermo Scientific) + 50 ml of TAE 1X.Microwave 30s by 30s until agarose total dissolution. Gel was cooling down until to be lukewarm, one BET drop was added. Gel was loaded with 10µl per sample previously added with 2 µl of loading dye 6X, and 5 µl for ladders. Gel running 45 minutes at 100 mV in TAE 1X buffer.

    IMAGE
    Figure 1: 1% agarose gel of PCR products.

    Lane 1: BBa_K823012 PCR product, Lane 2: pBHR1 PCR product, Lane 3 and 6: Purple 2-Log ladder NEB, Lane 4: BBa_E0240 PCR product, Lane 5: BBa_I20260 PCR product, Lane 7: 1 Kb plus Ladder Ogene Ruller and Lane 8: BBa_J23101 PCR product

    We expected to obtain one band per PCR sample corresponding to the interesting amplified fragment. For Lane 2, 3 and 6 it was ok. We had the expected profile. By contrast 2 bands were visible, one at the expected size (around 1200 bp) and another around 600 bp. We decided to perform a purification on gel of each bands.

    Aug 12



    Retrieved from "http://2014.igem.org/Team:Evry/Interlab_Study/tests"