Team:UCL/Labbook/Week12

Bacterial Lab

Monday 19th August

pSB1C3 streaked plates (well 23.O) were retrieved from 30C incubator. Colony growth visible indicating successful transformation. Colonies were expected to be red in colour, however this was not observed.

A single colony from each plate was then inoculated in LB in order to later prepare glycerol stocks.

iGEM 2012 boxes were searched for pSB1C3. Transformation was carried out, selective plates were spread, incubated at 37°C overnight.

Inoculations of the following were carried out in 2mL LB:

·IRRE+PC+RBS (pSB1C3) (2x in 2mL LB) -> 2ul and 5ul -> incu-shaker

·RFP+pSB1C3 (scooped from plates) (2x in 2mL LB) -> incu-shaker

1.5mL miniprep, 0.5mL glycerol stock for following day.

Tuesday 20th August

Plates taken from incubation:

Competent cells transformed with plasmid: Colony growth indicating cells have successfully taken up plasmid.

Negative control (only competent cells): Colony growth indicating likely problems with chloramphenicol.

Chloramphenicol will therefore be re-made.

take from incu-shaker:

IRRE+PC+RBS ( pSB1C3) -> 4x 200ul glycerols -> storage at -20°C.

RFP+PSB1C3 -> 4x 200ul glycerols -> glycerol storage at -20°C.

All 4 Falcons were minipreped. Subsequently ran gel showed no bands indicating no DNA presence.

Wednesday 21st August

Nanodrop of pDNA

10x chloramphenicol plates were made using supervisor Yanika Borg's chloramphenicol.

Meeting with Dr Darren Nesbeth:

The following Biobricks ordered were brought by our supervisor to be streaked onto the relevant antibiotic plates and inoculated in antibiotic+2mL LB. Incubate at 37°C overnight.

A PCR of Zeocin was performed, a gel was subsequently ran.

PCR tube:

1 - PCR zec bb F, R, 2ul template

2 - PCR zec bb F, R, 1ul template

3 - PCR zec F, R, 2ul template

4 - PCR zec F, R, 1ul template

5 - PCR negative control zec bb F, R,

6 - PCR negative control zec F, R

PCR was unsuccessful.

Thursday 22nd August

Results from Biobrick streaking and inoculation:

Glycerol stocks were made from the plates that displayed sufficient colony growth.

A second attempt at zeocin PCR was performed using Phusion DNA Polymerase.

1 - Zec bb F, R 2ul

2 - Zec bb F, R 1ul

3 - Zec F, R 2ul

4 - Zec F, R 1ul

5 - Negative control zec bb F, R

6 - Negative control zec F, R

A gel was run with 8ul of each of the 6 reactions. PCR was successful.

Restriction digest of the following samples:

A - K105028

B - K105027

C - K105030

D - K812014

E - J63009/8

Nanodrop of samples:

PCR Purification

1 - zeo bb F, R 2ul template

2 - zeo bb F, R 1ul template

^ stored in iGEM 2013 box

Preparative digest of K812014 (pSB1C3)

5ug sample = 44ul of 113.3 ng/ul

CMV PCR

Primers used: 2s + 6FW, 2s + bbRE

Friday 23rd August

Gel was ran with (lane):

(3) PCR purified zeo bb FR + 2ul template

(4) PCR purified zeo bb FR + 1ul template

(6) bwf + bb RE + 1ul template

(7) bwf + bb RE + 2ul template

(8) bwf + bb RE

Samples in lanes 3 & 4 failed, therefore a nanodrop was recorded:

Mammalian Lab

Monday 19th August Viable cell count data for HeLa growth curve, Day 1 : 0.1 x 10^-6 viable cells per mL

Disc 1 Disc 2

Split stock HeLa cells

Tuesday 20th August

Viable cell count data for HeLa growth curve, Day 1 : [0.17, 0.068 (anomaly), 0.23] x 10^-6 viable cells per ml

Disc 1 Disc 2

Wednesday 21st August

Viable cell count data for HeLa growth curve, Day 1 : [0.496, 0.244 (anomaly), 0.356] x 10^-6 viable cells per ml

Thursday 22nd August - Viable cell count data for HeLa growth curve, Day 1 : [0.79, 1.12, 1.19] x 10^-6 viable cells per ml