Revision as of 14:02, 17 August 2010

Lab notes (8/9 - 8/15)

Group: Photosensor

pfu PCR of B0015 and PCR purification

date: 17/8 Protocols: CP1.1 and GFX easy protocol
Notes:
2 uL PCR product of B0015 (no. 43 white) was used as template for each PCR reaction.3 PCR reactions were prepared.
Premix for 4 PCR reactions:

25uL	pfu bf. + MgSO4
7,5uL	dNTP's
7,5uL	VF2
7,5uL	VR
190uL	H20
2uL	pfu Polymerase enzyme

48uL premix is distrubuted into each PCR tube. PCR tubes are marked B0015.A-C
PCR program:

Start	95C	3min
Denaturating	95C	2min
Annealing	55C	30s
Elongation	72C	45s
Go to	2	29x
End	72C	2min
Hold	4C

5uL of PCR sample is loaded onto a 2% agarose gel. Generuler 100bp DNA ladder (blue) is used as marker.

Results:

Analysis: PCR product is OK and B0015 DNA is purified from the PCR product according to protocol. DNA is eluted in 20uL H2O. Purified samples are stored in the jumblebox (hotchpotch), marked as B0015-1 and B0015-2.

Group: Retinal

Characterization of Beta-carotene

Start date: 10/8
Methods: ON, sonication, UV-vis spectroscopy
Protocols: CC.1.1[1]

Colony PCR on transformants using ninaB fwd and rw primers

Date: 10/8
Done by: Christian & Tommy
Methods: ON
protocos:

Notes:
ON was made from 4 colonies:
Top 10 - on insert -> OD = 0,008 (100 x diluted)
Top 10 - with K274210 biobrick insert -> OD = 0,011 (100 x diluted)
MG1655 - on insert -> OD = 0,020 (100 x diluted)
Mg1655 - with K274210 biobrick insert -> OD = 0,017 (100 x diluted)
ON was made in 110 ml LB media. colonies with K274210 biobrick insert was grown in media containing ampicillin.
alle the ON cultures was grown for 20 hours at 37 °C.
After 16 hours, ml of the ON colonies was transferred in to 110 LB media and grown for 4 hours to the exponential phase:
Top 10 - on insert -> OD = 0,049 (100 x diluted)
Top 10 - with K274210 biobrick insert -> OD = 0,044 (100 x diluted)
MG1655 - on insert -> OD = 0,007 (100 x diluted)
Mg1655 - with K274210 biobrick insert -> OD = 0,009 (100 x diluted)
Colonies with K274210 biobrick insert was grown in media containing ampicillin.

Harvesting, sonication and UV-vis spektroscopy

Date: 11/8
Done by: Christian & Tommy
Methods: Cell harvesting, sonication and UV-vis messurements
protocos: none

Notes:
100 mL Cell cultures was centrifuged for 5 min at 14000 RPM. the supernantant was discarded and cells were resuspended in 5 mL acetone (99,9%), except the top 10 with the K274210 biobrick insert wicht was resuspended in 10 mL acetone (suorce of error.). The resuspended cells were sonicated for 5 min. the samples were spun down and the supernantant were transferrede to new tubes, cell bebri was discarded.
A standart curve was made from pure Beta-carotene,
The samples and the standarts were first measured at a fixed wavelengt of 456 nm. The standarts:

Concentration	Absorbance
1 mM	4,000
100 µM	2,260
50 µM	4,000
25 µM	0,155
10 µM	0,893
5 µM	0,440
1 µM	0,075
100 nM	0,015
10 nM	0,038
1 nM	0,005
100 pM	0,024

The samples:

	Top 10 cells (Absorbance)	MG1655 E. coli mutant (Absorbance)
Stationary phase control	0,034	0,024
Stationary phase with K274210 biobrick insert	0,319	1,549
Expotential phase control	0,020	0,024
Expotential phase with K274210 biobrick insert	0,034	0,033

@@ Line 124: / Line 124: @@
 mL Cell cultures was centrifuged for 5 min at 14000 RPM. the supernantant was discarded and cells were resuspended in 5 mL acetone (99,9%), except the top 10 with the K274210 biobrick insert wicht was resuspended in 10 mL acetone (suorce of error.). The resuspended cells were sonicated for 5 min. the samples were spun down and the supernantant were transferrede to new tubes, cell bebri was discarded.<br>
 A standart curve was made from pure Beta-carotene,<br>
+The samples and the standarts were first measured at a fixed wavelengt of 456 nm.
+The standarts:<br>
+<table style="text-align: left; width: 100%;" border="1"
+ cellpadding="2" cellspacing="2">
+    <tr>
+      <td>Concentration</td>
+      <td>Absorbance</td>
+    </tr>
+    <tr>
+      <td>1 mM</td>
+      <td>4,000</td>
+    </tr>
+    <tr>
+      <td>100 µM</td>
+      <td>2,260</td>
+    </tr>
+    <tr>
+      <td>50 µM</td>
+      <td>4,000</td>
+    </tr>
+    <tr>
+      <td>25 µM</td>
+      <td>0,155</td>
+    </tr>
+    <tr>
+      <td>10 µM</td>
+      <td>0,893</td>
+    </tr>
+    <tr>
+      <td>5 µM&nbsp;</td>
+      <td>0,440</td>
+    </tr>
+    <tr>
+      <td>1 µM</td>
+      <td>0,075</td>
+    </tr>
+    <tr>
+      <td>100 nM</td>
+      <td>0,015</td>
+    </tr>
+    <tr>
+      <td>10 nM</td>
+      <td>0,038</td>
+    </tr>
+    <tr>
+      <td>1 nM</td>
+      <td>0,005</td>
+    </tr>
+    <tr>
+      <td>100 pM</td>
+      <td>0,024</td>
+    </tr>
+</table>
+The samples:<br>
+<table style="text-align: left; width: 100%;" border="1"
+ cellpadding="2" cellspacing="2">
+    <tr>
+      <td></td>
+      <td>Top 10 cells (Absorbance)</td>
+      <td>MG1655 E. coli mutant (Absorbance)</td>
+    </tr>
+    <tr>
+      <td>Stationary phase control </td>
+      <td>0,034</td>
+      <td>0,024</td>
+    </tr>
+    <tr>
+      <td>Stationary phase with K274210 biobrick insert</td>
+      <td>0,319</td>
+      <td>1,549</td>
+    </tr>
+    <tr>
+      <td>Expotential phase control</td>
+      <td>0,020</td>
+      <td>0,024</td>
+    </tr>
+    <tr>
+      <td>Expotential phase with K274210 biobrick insert</td>
+      <td>0,034</td>
+      <td>0,033</td>
+    </tr>
+</table>

Team:SDU-Denmark/labnotes5

From 2010.igem.org