Team:Freiburg/Notebook/26 July

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This is the wiki page
of the Freiburger student
team competing for iGEM 2011.
Thank you for your interest!


Contents

blue light receptor

Gibson-Assembly

Investigators: Sandra, Sophie

Planned Gibson-Assembly for Lov-tap and Not-Gate. Need to order NAD. We will start an thursday.


Precipitator

Ligation


Name: Ruediger Date: 26.07
Continue from Date Name

Experiment Digestion 25.07 Ruediger

Project Name:GFPPbd

Procedure


PCR tube:

total volume 20 μl


  1. add H2O (17 μl -X-Y-Z)
  2. add 2 μl Ligase Buffer 10x
  3. add Insert 1, Insert 2(when proceeding from 3A digestion use 2 μl of each)
  4. add Vector (20ng needed. When proceeding from 3A digestion use 2 μl)
  5. Add 1 μl T4-DNA Ligase
  6. Incubate 10-30 min at room temperature
  7. heat for 20 minutes at 80°C
  8. store at -20°C or directly proceed to transformation


Part name Volume (μl) Part name Volume (μl)
S39 2 S43 2
P18 1,8 P18 1,8
Psb1T3 2 Psb1T3 2
S39 2 S43 2
P19 1,8 P19 1,8
Psb1T3 2 Psb1T3 2
S39 2 S43 2
P20 1,8 P20 1,8
Psb1T3 2 Psb1T3 2

Added 12,2 μl to every sample


Documentation:

Why are you doing this experiment? Where are your parts stored? Name the parts for ligation etc.


See digestion yesterday

3A assembly combination as shown in table.


Transformation


Name: RT Date: 26.07
Continue from Date Name

Experiment Ligation 26.07 Ruediger

Project Name: GFPPbd

Procedure


  1. take cells from -80°C freezer and put them on ice! (every eppi contains about 400 μl cells)
  2. thaw cells on ice 20 minutes
  3. pipette 50 μl cells and 2 μl DNA into eppi still on ice!
  4. Incubate for 30 minutes on ice
  5. Heat at 42°C for 60 sec
  6. Incubate on ice for 5 minutes
  7. Add 200 μl LB Broth
  8. Incubate for 2 hours at 37°C (cells with lysis cassette at 30°C!!)
  9. Plate 50 μl and 200μl on two different LB/Agar plates with appropriate antibiotic resistance

Documentation:

Why are you doing this experiment? Name of the sample? Where are they stored? Name the vector with inserts, antibiotika resistance etc.


Had only 6 tet plates -> put 100 μl of each sample on each plate

Incubator overnight for 30°C


S39-P18

S39-P19

S39-P20


S43-P18

S43-P19

S43-P20


Lysis cassette

Sequencing of Quickchange-modified Lysis Repressor Part (modified K098995)

Right-click to download the annotated ape (.gb) file


3A Assembly (K098995 + K124017)

Digestion of 3A Assembly


Name: Theo Date: 26.07.2011
Continue from Experiment : Quickchange V.3
Project Name: Lysis Cassette V.2 (3A assembly of quickchange-modified K098995 with Lysis genes K124017)

Procedure


  1. add H2O (38μl-DNA )
  2. 5 μl NEB4 buffer (stored at iGEM’s, -20°C)
  3. 5 μl 10x BSA (used 1:10 diluted sample stored at iGEM’s, -20°C)
  4. DNA (500 ng) (Vector:Insert ratio 1:3 in following Ligation)
  5. 1 μl restriction enzymes (stored at iGEM’s, -20°C)
  6. heat for 1-2 hours 37°C (6 hours if time)
  7. heat for 20 minutes 80°C (inactivation of enzymes)
  8. keep at 4°C if you cannot continue

Restriction enzymes you need to cut the vector, insert1 and insert 2:


Components
Vector (μl)
Insert1 -K098995- and 2 - K124017-(μl)
DNA (500ng) 10 5 7
BSA (10x) (5μl)
NEB4 Buffer (5μl)
Enzyme 1 (1μl) EcoRI + DpnI EcoRI XbaI
Enzyme 2 (1μl) PstI SpeI PstI
H2O (38 μl- DNA) 27 33 31
In total 50 μl

Documentation:

Why are you doing this experiment? Where are the samples stored? Antibiotica resistance, vector used etc.


3A assembly of quickchange-modified K098995 with Lysis genes K124017.

Quickchange-modified K098995: 132,8ng/µl (Amp)

Lysis genes K124017: (Amp+Kan)

*Parts were run on the gel and verified that the inserts were cut, image accidentaly not saved*

Vector: pSB1T3 + DpnI Digestion

Stored in Theos Box



Ligation


Name: Theo Date: 26.07.2011
Continue from: 26.07.2011 Lysis Cassette V.2 Digestion
Project Name: Lysis Cassette V.2 (3A assembly of quickchange-modified K098995 with Lysis genes K124017)

Procedure


PCR tube:

total volume 20 μl


  1. add H2O (17 μl -X-Y-Z)
  2. add 2 μl Ligase Buffer 10x
  3. add Insert 1, Insert 2(when proceeding from 3A digestion use 2 μl of each)
  4. add Vector (20ng needed. When proceeding from 3A digestion use 2 μl)
  5. Add 1 μl T4-DNA Ligase
  6. Incubate 10-30 min at room temperature
  7. heat for 20 minutes at 80°C
  8. store at -20°C or directly proceed to transformation


Name of part Ratio Insert:Vector

= 3:1 or 1:1

Volume (μl)
X insert 1 Modif. K098995 3:1 (1,5*3) 4,5
Y insert 2 K124017 3:1 (2*3) 6
Z vector pSB1T3 1:3 (1) 1
H2O 5,5

Documentation:

Why are you doing this experiment? Where are your parts stored? Name the parts for ligation etc.


Ligation step of 3A assembly.


How to calculate ratios --> e.g. for K124017

Length of pSB1T3= ca 2200bp

Length of K124017+Vector= ca 4500bp

4500/2200= ca 2

So 2*3 µl (since 3:1 is needed) = 6 µl





Transformation


Name: Theo Date:
Continue from : 26.07.2011 Lysis Cassette V.2 Ligation



Project Name: Lysis Cassette V.2 (3A assembly of quickchange-modified K098995 with Lysis genes K124017)

Procedure


  1. take cells from -80°C freezer and put them on ice! (every eppi contains about 400 μl cells)
  2. thaw cells on ice 20 minutes
  3. pipette 50 μl cells and 2 μl DNA into eppi still on ice!
  4. Incubate for 30 minutes on ice
  5. Heat at 42°C for 60 sec
  6. Incubate on ice for 5 minutes
  7. Add 200 μl LB Broth
  8. Incubate for 2 hours at 37°C (cells with lysis cassette at 30°C!!)
  9. Plate 50 μl and 200μl on two different LB/Agar plates with appropriate antibiotic resistance

Documentation:

Why are you doing this experiment? Name of the sample? Where are they stored? Name the vector with inserts, antibiotika resistance etc.


New Composite Part in pSB1T3 Vector with quickchange-modified K098995 and Lysis genes K124017



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