Team:Exeter/lab book/gibs/wk3

From 2012.igem.org

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     <!<p><b>**Tuesday 24.7.12**</b></p><p>Mary, Freddie, Becca and Alex B.</p><br><p><b>9am</b></p><p>3A assembly of Pbad weak-RBS, Pbad strong-RBS and PlacI-RBS</p><p>
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     <!<p><b>**Tuesday 24.7.12**</b></p><p>Mary, Freddie, Becca and Alex B.</p><br><p><b>9am</b></p><p>3A assembly of Pbad weak-RBS, Pbad strong-RBS and PlacI-RBS</p><br><p>
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Upstream Pbad W (211.4 ng/µl) Pbad S (130.4 ng/µl) PlacI (299.2 ng/µl) MM
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<u>Upstream</u></p><p>
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DNA (500ng) 2.37 µl 3.83 µl 1.67 µl -
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For 500ng DNA:</p><p>
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EcoRI-HF 0.5 µl 0.5 µl 0.5 µl 2 µl
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<ul>Pbad Weak - (211.4 ng/µl)=2.37 µl</p><p>Pbad Strong -(130.4 ng/µl) =3.83 µl </p><p>PlacI - (299.2 ng/µl)=1.67 µl</ul></p><p>
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SpeI 0.5 µl 0.5 µl 0.5 µl 2 µl
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EcoRI-HF0.5 µl (master mix volume 2 µl)</p><p>
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10X NEBuffer 2 2.5 µl 2.5 µl 2.5 µl 10 µl
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SpeI: 0.5 µl (master mix volume 2 µl)</p><p>
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100X BSA 0.25 µl 0.25 µl 0.25 µl 1 µl
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10X NEBuffer 22.5 µl (master mix volume 10 µl)</p><p>
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H2O (to 25 µl) 18.88 µl 17.42 µl 19.58 µl -
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100X BSA0.25 µl (master mix volume 1 µl)</p><p>
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H2O (to 25 µl):</p><p>
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<ul>Pbad Weak =18.88 µl</p><p>
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Pbad Strong =17.42 µl</p><p>
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PlacI =19.58 µl</ul></p><br>
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Downstream RBS (77.4 ng/µl)
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<p><u>Downstream</u></p><p>
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DNA (500ng) 6.46 µl
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RBS (77.4 ng/µl)</p><p>
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XbaI 0.5 µl
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DNA (500ng)6.46 µl</p><p>
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PstI 0.5 µl
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XbaI0.5 µl</p><p>
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10X NEBuffer 2 2.5 µl
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PstI0.5 µl</p><p>
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100X BSA 0.25 µl
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10X NEBuffer 22.5 µl</p><p>
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H2O to 25 µl 14.79 µl
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100X BSA0.25 µl</p><p>
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H2O to 25 µl14.79 µl</p><br><p>
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Destination plasmid
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<u>Destination plasmid</u></p><p>
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MM
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DNA 250ng</p><p>
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DNA 250ng -
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EcoRI-HF0.5 µl (master mix vol. 2 µl)</p><p>
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EcoRI-HF 0.5 µl 2
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PstI0.5 µl (master mix vol. 2 µl)</p><p>
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PstI 0.5 µl 2
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10X NEBuffer 22.5 µl (master mix vol. 10 µl)</p><p>
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10X NEBuffer 2 2.5 µl 10
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100X BSA0.25 µl (master mix vol. 1 µl)</p><p>
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100X BSA 0.25 µl 1
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H2O to 25 µl</p><p>
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H2O to 25 µl
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-
</p><p>
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Incubated 36 °C for 10 minutes</p><p>
Incubated 36 °C for 10 minutes</p><p>
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Heat inactivated at 80 °C for 20 minutes</p><p>
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Heat inactivated at 80 °C for 20 minutes</p><br><p>
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Ligation:
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<u>Ligation:</u></p><p>
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Upstream part digest 2 µl
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Upstream part digest2 µl</p><p>
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Downstream part digest 2 µl
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Downstream part digest2 µl </p><p>
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Destination plasmid digest 2 µl
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Destination plasmid digest2 µl</p><p>
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10X T4 DNA ligase buffer 2 µl
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10X T4 DNA ligase buffer2 µl</p><p>
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T4 DNA ligase 1 µl
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T4 DNA ligase1 µl</p><p>
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H2O 11 µl
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H2O11 µl</p><br><p>
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</p><p>
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Incubated at room temperature for 10 minutes</p><p>Heat inactivated at 80 °C for 20 minutes</p><p>Stored at -20°C prior to afternoon transformation</p><p>2.45pm</p><p>
Incubated at room temperature for 10 minutes</p><p>Heat inactivated at 80 °C for 20 minutes</p><p>Stored at -20°C prior to afternoon transformation</p><p>2.45pm</p><p>
Resuspended DNA according to IDT resuspension protocol (Alex B. and Becca then transformed them</p><p>
Resuspended DNA according to IDT resuspension protocol (Alex B. and Becca then transformed them</p><p>
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Transformation of 3A assembled Pbad strong-RBS and PlacI-RBS</p><p>
Transformation of 3A assembled Pbad strong-RBS and PlacI-RBS</p><p>
<ul><b><i>1.</i></b>2 µl DNA added to 50 µl top10 competent cells</p><p>
<ul><b><i>1.</i></b>2 µl DNA added to 50 µl top10 competent cells</p><p>
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<ul><b><i>2.</i></b>Incubated on ice 30 minutes</p><p>
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<b><i>2.</i></b>Incubated on ice 30 minutes</p><p>
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<ul><b><i>3.</i></b>Heat shocked 42 °C, 30 seconds</p><p>
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<b><i>3.</i></b>Heat shocked 42 °C, 30 seconds</p><p>
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<ul><b><i>4.</i></b>Ice 2 minutes</p><p>
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<b><i>4.</i></b>Ice 2 minutes</p><p>
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<ul><b><i>5.</i></b>Aseptically added 250 µl S.O.C. medium</p><p>
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<b><i>5.</i></b>Aseptically added 250 µl S.O.C. medium</p><p>
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<ul><b><i>6.</i></b>Shaken 220 rpm, 37 °C, 1 hour</p><p>
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<b><i>6.</i></b>Shaken 220 rpm, 37 °C, 1 hour</p><p>
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<ul><b><i>7.</i></b>Spread plates of 20 µl and 100 µl made on LB(tetracycline) plates</p><p>
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<b><i>7.</i></b>Spread plates of 20 µl and 100 µl made on LB(tetracycline) plates</p><p>
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<ul><b><i>8.</i></b>Plates incubated at 37 °C overnight</p><br>
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<b><i>8.</i></b>Plates incubated at 37 °C overnight</ul></p><br>
<b>**Thursday 26.7.12**</b></p><br><p>
<b>**Thursday 26.7.12**</b></p><br><p>

Revision as of 13:03, 14 September 2012

ExiGEM2012 Lab Book Gibs wk3

Operon Construction: 23rd - 27th July 2012

 **Tuesday 24.7.12**

Mary, Freddie, Becca and Alex B.


9am

3A assembly of Pbad weak-RBS, Pbad strong-RBS and PlacI-RBS


Upstream

For 500ng DNA:

    Pbad Weak - (211.4 ng/µl)=2.37 µl

    Pbad Strong -(130.4 ng/µl) =3.83 µl

    PlacI - (299.2 ng/µl)=1.67 µl

EcoRI-HF: 0.5 µl (master mix volume 2 µl)

SpeI: 0.5 µl (master mix volume 2 µl)

10X NEBuffer 2: 2.5 µl (master mix volume 10 µl)

100X BSA: 0.25 µl (master mix volume 1 µl)

H2O (to 25 µl):

    Pbad Weak =18.88 µl

    Pbad Strong =17.42 µl

    PlacI =19.58 µl


Downstream

RBS (77.4 ng/µl)

DNA (500ng): 6.46 µl

XbaI: 0.5 µl

PstI: 0.5 µl

10X NEBuffer 2: 2.5 µl

100X BSA: 0.25 µl

H2O to 25 µl: 14.79 µl


Destination plasmid

DNA 250ng

EcoRI-HF: 0.5 µl (master mix vol. 2 µl)

PstI: 0.5 µl (master mix vol. 2 µl)

10X NEBuffer 2: 2.5 µl (master mix vol. 10 µl)

100X BSA: 0.25 µl (master mix vol. 1 µl)

H2O to 25 µl

Incubated 36 °C for 10 minutes

Heat inactivated at 80 °C for 20 minutes


Ligation:

Upstream part digest: 2 µl

Downstream part digest: 2 µl

Destination plasmid digest: 2 µl

10X T4 DNA ligase buffer: 2 µl

T4 DNA ligase: 1 µl

H2O: 11 µl


Incubated at room temperature for 10 minutes

Heat inactivated at 80 °C for 20 minutes

Stored at -20°C prior to afternoon transformation

2.45pm

Resuspended DNA according to IDT resuspension protocol (Alex B. and Becca then transformed them

    1.2 µl of DNA from Pbad S-RBS and PlacI-RBS ligations added to 25 µl top10 competent cells

    2.Incubated on ice for 30 minutes

    3.Heat shocked 42 °C 30 seconds

    4.Placed on ice for 2 minutes

    5.Aseptically added 250 µl S.O.C. medium (pre-warmed)

    6.Shaken at 220 rpm, 37 °C, 1 hour

    7.Spread plates of 20 and 100 µl made

    8.incubated at 37 °C overnight


**Wednesday 25.7.12**

Mary and Freddie


9.45 am

Biobricking attempt 2

To make Pbad Strong-RBS and PlacI-RBS (n.b. placI-RBS relevant only to 3 gene part of project)

3A assembly

Upstream Pbad S (130.4 ng/µl) PlacI (299.2 ng/µl) MM DNA (500ng) 3.8 µl 1.7 µl - EcoRI-HF 1 µl 1 µl 3 µl SpeI 1 µl 1 µl 3 µl 10X NEBuffer 2 5 µl 5 µl 15 µl 100X BSA 0.5 µl 0.5 µl 1.5 µl H2O (to 50 µl) 38.7 µl 40.8 µl - Downstream RBS (77.4 ng/µl) MM DNA (500ng) 6.5 µl - XbaI 0.5 µl 3 PstI 0.5 µl 3 10X NEBuffer 2 2.5 µl 15 100X BSA 0.25 µl 1.5 H2O 6.7 µl - Destination plasmid (tetracycline) pSB1T3 (linear) MM DNA 250ng 20 µl - EcoRI-HF 1 µl 3 PstI 1 µl 3 10X NEBuffer 2 5 µl 15 100X BSA 0.5 µl 1.5 H2O to 50 µl 22.5 µl - Incubated 36 °C for 10 minutes

Heat inactivated at 80 °C for 20 minutes

Ligation: Upstream part digest 2 µl Downstream part digest 2 µl Destination plasmid digest 2 µl 10X T4 DNA ligase buffer 2 µl T4 DNA ligase 1 µl H2O 11 µl Incubated at room temperature for 10 minutes

Heat inactivated at 80 °C for 20 minutes

Stored at -20°C prior to afternoon transformation

Standard assembly run in parallel to 3A

Upstream Pbad S PlacI MM DNA (500ng) 15.3 µl 6.7 µl - EcoRI-HF 1 µl 1 µl 3 µl SpeI 1 µl 1 µl 3 µl 10X NEBuffer 2 5 µl 5 µl 15 µl 100X BSA 0.5 µl 0.5 µl 1.5 µl H2O (to 40 µl) 17.2 µl 25.8 µl - Downstream RBS 2 (77.4 ng/µl) RBS 4 (63.0 ng/µl) MM DNA (500ng) 25.8 µl 31.7 µl - EcoRI-HF 1 µl 1 µl 3 XbaI 1 µl 1 µl 3 10X NEBuffer 2 5 µl 5 µl 15 100X BSA 0.5 µl 0. 5 µl 1.5 H2O 6.7 µl 0.8 - Digested for 1 hour at 36 °C

DNA cleanup from enzymatic reactions using microcentrifuge and Quiagen column

For RBS 2 and RBS 4 plasmids (post-digestion)

    1.40 µl digest + 120 µl QG buffer + 40 µl isopropanol mixed and transferred to column (n.b. RBS 2 may not have been adequately mixed before being transferred to column)

    2.Centrifuged for 1 minute, 13000 rpm, room temp.

    3.Flow through discarded

    4.500 µl buffer QG added to column

    5.Centrifuged for 1 minute, 13000 rpm, room temp.

    6.Flow through discarded

    7.750 µl buffer PE added to column

    8.Centrifuged for 1 minute, 13000 rpm, room temp.

    9.Flow through discarded

    10.Centrifuged for 1 minute, 13000 rpm, room temp.

    11.Moved column to fresh 1.5 ml eppendorf

    12.30 µl water added

    13.Left to stand for 1 minute

    14.Centrifuged 13000 rpm, 1 minute, room temp.

    15.DNA stored at -20 °C after analysis with a nanodrop spectrophotometer


Transformation of 3A assembled Pbad strong-RBS and PlacI-RBS

    1.2 µl DNA added to 50 µl top10 competent cells

    2.Incubated on ice 30 minutes

    3.Heat shocked 42 °C, 30 seconds

    4.Ice 2 minutes

    5.Aseptically added 250 µl S.O.C. medium

    6.Shaken 220 rpm, 37 °C, 1 hour

    7.Spread plates of 20 µl and 100 µl made on LB(tetracycline) plates

    8.Plates incubated at 37 °C overnight


**Thursday 26.7.12**


Suspended sequencing primers (according to manufacturer’s instructed volumes) and prepared 50 µl aliquots for later

Resuspended BBa_I0500 (large pbad promoter - selected as alternative to pbad strong due to sequence match with Gibson primers) in 10 µl water

Left to stand for 5 minutes

Transferred to eppendorf

Centrifuged for 5 secs

    1.2 µl DNA added to 50 µl top10 competent cells (remaining DNA stored at -20 °C)

    2.Incubated on ice 30 minutes

    3.Heat shocked 42 °C, 30 seconds

    4.Ice 2 minutes

    5.Aseptically added 250 µl S.O.C. medium

    6.Shaken 220 rpm, 37 °C, 1 hour

    7.Spread plates of 20 µl and 100 µl made on LB(kanamycin) plates

    8.Plates incubated at room temperature over weekend


Transferred colonies from plates prepared 25.7.12 into 5 ml LB(tetracycline) broth (1:1000)

Incubated overnight at 220 rpm, 37 °C


**Friday 27.7.12**


9 am Miniprep of 3A assembled plasmid (from 25.7.12)

    1.Transferred broth to fresh falcon tubes to remove pipette tips (tips and original tubes stored in fridge until same day streak-plates made)

    2.Centrifuged 5 minutes, 3901 rcf, 4 °C

    3.Supernatant discarded

    4.250 µl resuspension solution added

    5.Pipetted to mix and transferred to clean 1.5 ml eppendorf

    6.250 µl lysis solution added

    7.Inverted ~6 X

    8.350 µl neutralisation solution added

    9.Inverted ~6 X

    10.Centrifuged 5 mins, 13000 rpm, room temperature

    11.Transferred supernatant to spin column

    12.Centrifuged for 1 minute, 13000 rpm, room temperature

    13.Discarded flow-through

    14.500 µl wash solution added

    15.Centrifuged 1 minute, 13000 rpm, room temperature

    16.Discarded flow-through

    17.500 µl wash solution added

    18.Centrifuged 1 minute, 13000 rpm, room temperature

    19.Discarded flow-through

    20.Centrifuged 1 minute, 13000 rpm, room temperature

    21.Transferred column to clean 1.5 ml eppendorf

    22.50 µl water added

    23.Centrifuged 1 minute, 13000 rpm, room temperature

    24.5 µl water added

    25.Centrifuged 1 minute, 13000 rpm, room temperature

    26.Column discarded, DNA concentration measured and DNA stored in eppendorf at -20 °C

(n.b. digest gel was run for analysis, but for this part of the project is considered irrelevant due to inconclusive results from small fragment size and because BBa-I0500 was decided to be more useful for this part of the project)


Streak plates made from dregs of overnight culture (see above)

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