Team:Stockholm/12 October 2010

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(Difference between revisions)

Latest revision as of 11:09, 26 October 2010

Nina

Gel clean up

I loaded samples in an agarose gel 1 % and ran at 80 V.

Samples:

Protein A_TAT_N, _Tra10_N and _LMWP_N
Fusion_CPP1, TAT_C ans _CPP3
Fusion_TAT_N, _Tra10_N and _LMWP_N

The procedure was according to the description in protocols.

Weight of all samples: 200 mg

200 * 3 = 600 ul QXI

In step 3 I added 10 ul of QIAEXII to each sample.

Polyacrylamide gel

I ran a gel of the purified SOD.His (N terminal) to check if there had been any purification of the protein.

Ladder: PageRuler Unst. Protein Ladder

Arrangement on the gel:

Gel:

The gel was incubated in coomassie blue staining and destained on shake.

Unfortunately there were no bands representing SOD.His (~17 kDa) on the gel, which must mean that there was too small culture (12 ml) and that the cells have not been lysed properly. I will redo this work but with more start culture and lyse the cells in a more effiecient way.

The polyacrylamide gel was prepared by the SDS-PAGE mixtures described in protocols.

Andreas

Removal of insertion in BioBrick suffixes

Transformation results

Good colony yield on all plates. A few red colonies discovered on all plates, indicating that some partly digested pSB1C3 vector, still containing the RFP insert, had been excised during gel extraction.

Colony PCR

From 11/10 transformations'

pSB1C3.IgGp A-C
pSB1C3.bFGF A-C
pSB1C3.ProtA A-C
pSB1C3.yCCS A-C
pSB1C3.SOD A-C

Standard colony PCR settings
- 1:15 elongation time

Gel verification

Gel 1. Colony PCR gel verification of cloned with insertion removed.
3 μl λ; 5 μl sample.
λ = O'GeneRuler 1 kb DNA ladder.

Gel 2. Colony PCR gel verification of cloned with insertion removed.
3 μl λ; 5 μl sample.
λ = O'GeneRuler 50 bp DNA ladder.

Gel 1: 1 % agarose, 140 V
Gel 2: 1 % agarose, 160 V

Expected bands

pSB1C3.IgGp: 1262 bp
pSB1C3.bFGF: 794 bp
pSB1C3.ProtA: 506 bp
pSB1C3.yCCS: 1076 bp
pSB1C3.SOD: 791 bp

Results

All clones correct.
All clones correct.
All clones correct.
Correct size for clone C, weak band for clone B. Clone A probably carrying an RFP insert.
All clones correct.

ON cultures

5 ml LB + Cm 25; 37 °C, 225 rpm
- 1C, 2C, 3C, 4C, 5C

BL21 transformation and growth test

Testing BL21 cells with/without CPP expression by transforming and inducing with IPTG.

50 μl 0.1 M IPTG
40 μl competent cells
- pEX.SOD⋅His
- pEX.nTra10⋅SOD⋅His
- pEX.nTAT⋅SOD⋅His
- pEX.nLMWP⋅SOD⋅His

Mimmi

SOD activity assay

Kits?
- Biosite/trevigen 6000sek
- Biovision/labinova 3000sek, ca 1week delivery time
- Cayman
- Cellbiolabs
- Merch
- Abcam 3600sek
- Probior
- Sigma-Aldrich 3000sek
- T-cell technology inc.

Kit from Sigma-Aldrich
- sponsored with a very good offer

The Faculty of Science at Stockholm University

Swedish Vitiligo association (Svenska Vitiligoförbundet)

@@ Line 32: / Line 32: @@
 Gel:
-PICTURE!!
+[[Image:Aq19.jpg|300px]]
 The gel was incubated in coomassie blue staining and destained on shake.
-Unfortunately there were no bands on the gel, which must mean that there was too small culture (12 ml) and that the cells have not been lysed properly. I will redo this work but with more start culture and lyse the cells in a more effiecient way.
+Unfortunately there were no bands representing SOD.His (~17 kDa) on the gel, which must mean that there was too small culture (12 ml) and that the cells have not been lysed properly. I will redo this work but with more start culture and lyse the cells in a more effiecient way.
 The polyacrylamide gel was prepared by the SDS-PAGE mixtures described in protocols.
 ==Andreas==
@@ Line 91: / Line 91: @@
 **pEX.nTAT&sdot;SOD&sdot;His
 **pEX.nLMWP&sdot;SOD&sdot;His
+== Mimmi ==
+=== SOD activity assay ===
+*Kits?
+**Biosite/trevigen  6000sek
+**Biovision/labinova 3000sek, ca 1week delivery time
+**''Cayman''
+**''Cellbiolabs''
+**''Merch''
+**Abcam 3600sek
+**Probior
+**Sigma-Aldrich 3000sek
+**''T-cell technology inc.''
+*Kit from Sigma-Aldrich
+**sponsored with a very good offer
+{{Stockholm/Footer}}