IGEM:Cambridge/2008/Notebook/Turing Pattern Formation/2008/07/30: Difference between revisions

Revision as of 04:35, 5 September 2008

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Wet Work

Checking our big stock of biobricks and PNZ plasmid

We did big culture of biobricks and PNZ8901 plasmid to be able to make stocks. We want to check them before making stocks.

- Plamsid miniprep (for I746001, I746101 and PNZ8901 from big flasks

- Measure DNA concentration in our samples to decide the volume of DNA we have to add in our preparation

	260/280	DNA concentration (ng/nl)
I746001	1.79	50.5
I746101	1.87	54.3
PNZ8901	1.84	87

- Digest

For I746001 and I746101	For PNZ8901 plasmid
14μL of SDW	14μL of SDW
2μL of 10X Fast Digest Buffer	2μL of Buffer 3 (Biolabs)
2μL of DNA of biobricks	2μL of DNA of PNZ8901
1μL of EcoRI	1μL of PstI
1μL of SpeI	1μL of SalI

- Gel

Results from this gel

Lane 9 : I746001
Lane 10 : I746101
Lane 11 : PNZ8901
Lane 12 : HyperladderI

Everthing is really too big! There is a problem, either dimerization, either contamination, either a problem in our work. So we are going to run a new gel.

New gel to check

- Miniprep plasmid from growth bottles (I746001, I746101 and PNZ8901); from plates (I746001, I746101 and PNZ8901).

- Do single digest for PNZ8901 (one with PstI, one with SalI)

- Run a gel with : PNZ8901 from friday, PNZ8901 digest with PstI, PNZ8901 digest with SalI, 3 samples from growth bottles, 3 samples from plates (to check the size of the uncut vectors)

Result from this second gel

The ladders are really bad! But the size of our biobricks and plasmid are too big! So we can not trust these big cultures. They is a problem. With tests from the first week, we know that biobricks are right, so we are going to grow new cultures from these first cultures, to make stocks.

Concerning the vectors, they are from last year, so we are not sure of what they are. Since we ordered new well defined vectors (we should receive them on friday), we will use them in the next steps to be sure of our work.

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 {|{{table}} width="800"
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-|style="background-color: #EEE"|[[Image:IgemCam.jpg|200px]]<span style="font-size:22px;"> Turing Pattern Formation</span>
+|style="background-color: #444444"|[[Image:Signalling_button.gif|200px|center]]
 |style="background-color: #F2F2F2" align="center"|<html><img src="/images/9/94/Report.png" border="0" /></html> [[{{#sub:{{FULLPAGENAME}}|0|-11}}|Main project page]]<br />{{#if:{{#lnpreventry:{{FULLPAGENAME}}}}|<html><img src="/images/c/c3/Resultset_previous.png" border="0" /></html>[[{{#lnpreventry:{{FULLPAGENAME}}}}{{!}}Previous entry]]<html>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;</html>}}{{#if:{{#lnnextentry:{{FULLPAGENAME}}}}|[[{{#lnnextentry:{{FULLPAGENAME}}}}{{!}}Next entry]]<html><img src="/images/5/5c/Resultset_next.png" border="0" /></html>}}
 |-
@@ Line 13: / Line 13: @@
 ==Wet Work==
-* '''Transforming Bacillus Subtilis with medium A and medium A + tryptophan'''
-Medium A
-{|class="wikitable" style="text-align:center" border="1"
-|-
-! Time (min) !! 0 !! 20 !! 40 !! 60 !! 73 !! 85 !! 95 !! 105
-|-
-| OD650 || 0.1394 || 0.1370 || 0.1660 || 0.2304 || 0.2778 || 0.3138 || 0.3373 || 0.3583
-|-
-|}
-For this medium, the curb stop to increase logarithmically at 100min.
-Medium A + tryptophan
-{|class="wikitable" style="text-align:center" border="1"
-|-
-! Time (min) !! 0 !! 20 !! 40 !! 60 !! 73 !! 85 !! 95
-|-
-| OD650 || 0.1493 || 0.1636 || 0.2080 || 0.2909 || 0.3512 || 0.4002 || 0.4165
-|-
-|}
-For this medium, the curb stop to increase logarithmically at 90min.
-- Incubate 90min at 37°C by shaking
-- Prepare 7 tubes for medium A and 7 tubes for medium A + tryptophan : add 0.45mL of prewarmed medium B and 0.05mL of culture and incubate 90min at 37°C by shaking.
-- Transform B.S. by adding DNA and incubate 30min at 37°C
-We have one transformation with ppL82 (add 7.5μL of DNA), one with PNZ8901 (add 10μL of DNA) and one negative control without DNA.
-- Plate 500μL on Cm plate (35μg/mL)
-- For the remaining tubes, in one, add 60μL of glycerol and keep it in the freezer and keep the other one on the bench (for each medium)
 * '''Checking our big stock of biobricks and PNZ plasmid'''
-We didbig culture of biobricks and PNZ8901 plasmid to be able to make stocks. We want to check them before making stocks.
+We did big culture of biobricks and PNZ8901 plasmid to be able to make stocks. We want to check them before making stocks.
 - Plamsid miniprep (for I746001, I746101 and PNZ8901 from big flasks
@@ Line 107: / Line 65: @@
 * '''Results from this gel'''
+* Lane 9 : I746001
+* Lane 10 : I746101
+* Lane 11 : PNZ8901
+* Lane 12 : HyperladderI
+[[Image:photob.gif|300px|center]]
 Everthing is really too big! There is a problem, either dimerization, either contamination, either a problem in our work. So we are going to run a new gel.
@@ Line 119: / Line 84: @@
 * '''Result from this second gel'''
+[[Image:photoc.gif|300px|center]]
 The ladders are really bad! But the size of our biobricks and plasmid are too big! So we can not trust these big cultures. They is a problem.  With tests from the first week, we know that biobricks are right, so we are going to grow new cultures from these first cultures, to make stocks.

IGEM:Cambridge/2008/Notebook/Turing Pattern Formation/2008/07/30: Difference between revisions

Revision as of 04:35, 5 September 2008

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