Team:TMU-Tokyo/Notebook/Assay 2 Protocol and Result

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Latest revision as of 02:22, 27 September 2012

■Experiment
1st week (8.13 - 8.19)
2nd week (8.20 - 8.26)
3rd week (8.27 - 9. 2)
4th week (9. 3 - 9. 9)
5th week (9.10 - 9.16)
6th week (9.17 - 9.23)
7th week (9.24 - 9.30)

■Protocols

■Assay
Assay0
Device1 Assay
Device2 Assay
Device3 Assay

Assay 2

■Assay2 Protocol

・Quantitative Analysis of Formaldehyde

Ⅰ Preparing a Standard Solution（Making a diluted solution of formaldehyde）

Add 1μl 20% formalin solution in DW399μl, diluted 400-fold. Make a 4000-fold dilution DW180μl take this and 20μl. I will continue to order from here a 2-fold dilution. This is the standard solution (diluted 4000,8000,16000,32000,64000,128000 fold dilution).

Ⅱ Making sample
1.The cells were cultured at 30 ℃ for 18 hours in medium
2.Centrifuged 10000 × g　5min
3.Remove the supernatant
4.Wash the fungus
Add dw and Centrifuged 10000 × g　5min
5.Remove the supernatant
6.E. coli disrupted by sonicator in buffer of 50mM Tris-HCl pH7.2 .
7.Centrifuged 11000 × g at 4 ℃ so that the enzyme is not deactivated, the supernatant was harvested as crude enzyme solution (If you want to save is stored at 4 ℃ in a cold room)

The reaction mixture are 50mM Tris-HCl ph7.2 0.8ml
There formaldehyde 20mM 0.1ml (2mM final concentration)
20mM NAD + 0.1ml
Incubated for 5 minutes at 37 ℃ put
I was allowed to react at 37 ℃ in the next, put 0.05ml crude enzyme solution.

Ⅲ Creating Standard Curves and Measured samples
Liquid, the sample and standard experiment in triplicate. Performed only once blind
(40μl = 400μl for blind = 360μl + 40μl × 3 × 3 lane:: each reagent = 120μl 40μl × 3 each consecutive sample)
- The calibration curve
Absorbance = the absorbance of the standard solution- absorbance of the standard solution of blind accurate
①Into 40μl of each sample into a 96-well sample, standard, and blind.
Mix coloring reagent 40μl and alkaline reagent 40μl.
Allowed to stand at room temperature for 15 minutes at 20 ~ 35 ℃.
②Add 40μl reagent oxidation , (about 15 seconds) until the shaking stops foaming
③ Measured at 550nm wavelength in a microplate reader to measure the absorbance.

■Assay2 Result
Standard Curves

concentration
BBa_K749024

Enzyme+NAD	NO enzyme	NO NAD
21.190	25.629	24.181

wt

Enzyme+NAD	NO enzyme	NO NAD
21.181	26.984	25.124

All samples Reaction time 60min

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 <Br>
 <B>■Assay</B><Br>
-Device1 Assay<Br>
+<A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Assay_0_Protocol_and_Result">Assay0</A><Br>
+<A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Assay_1_Protocol_and_Result">Device1 Assay</A><Br>
 Device2 Assay<Br>
-Device3 Assay<Br>
+<A Href="https://2012.igem.org/Team:TMU-Tokyo/Notebook/Assay_3_Protocol_and_Result">Device3 Assay</A><Br>
@@ Line 48: / Line 61: @@
 <p class="title">
 <Br>
-Assay 1
+Assay 2
 <Hr>
 </p>
@@ Line 54: / Line 67: @@
 <p class="description">
 <b>■Assay2 Protocol</b><Br>
-<Br><Br></p>
+<Br>・Quantitative Analysis of Formaldehyde<Br>
+<Br>
+Ⅰ Preparing a Standard Solution（Making a diluted solution of formaldehyde）<Br>
+<Br>
+Add 1μl 20% formalin solution in DW399μl, diluted 400-fold. Make a 4000-fold dilution DW180μl take this and 20μl. I will continue to order from here a 2-fold dilution. This is the standard solution (diluted 4000,8000,16000,32000,64000,128000 fold dilution).<Br>
+<Br>
+Ⅱ Making sample<Br>
+.The cells were cultured at 30 ℃ for 18 hours in medium<Br>
+.Centrifuged 10000 × g　5min<Br>
+.Remove the supernatant<Br>
+.Wash the fungus<Br>
+Add dw and Centrifuged 10000 × g　5min<Br>
+.Remove the supernatant<Br>
+.E. coli disrupted by sonicator in buffer of 50mM Tris-HCl pH7.2 .<Br>
+.Centrifuged 11000 × g at 4 ℃ so that the enzyme is not deactivated, the supernatant was harvested as crude enzyme solution (If you want to save is stored at 4 ℃ in a cold room)<Br>
+<Br>
+The reaction mixture are 50mM Tris-HCl ph7.2 0.8ml<Br>
+There formaldehyde 20mM 0.1ml (2mM final concentration)<Br>
+mM NAD + 0.1ml<Br>
+Incubated for 5 minutes at 37 ℃ put<Br>
+I was allowed to react at 37 ℃ in the next, put 0.05ml crude enzyme solution.<Br>
+<Br>
+Ⅲ Creating Standard Curves and Measured samples<Br>
+Liquid, the sample and standard experiment in triplicate. Performed only once blind<Br>
+(40μl = 400μl for blind  = 360μl + 40μl × 3 × 3 lane:: each reagent = 120μl 40μl × 3 each consecutive sample)<Br>
+- The calibration curve <Br>
+Absorbance = the absorbance of the standard solution- absorbance of the standard solution of blind accurate<Br>
+①Into 40μl of each sample into a 96-well sample, standard, and blind.<Br>
+Mix coloring reagent 40μl and alkaline reagent 40μl.<Br>
+Allowed to stand at room temperature for 15 minutes at 20 ~ 35 ℃.<Br>
+②Add 40μl reagent oxidation , (about 15 seconds) until the shaking stops foaming<Br>
+③ Measured at 550nm wavelength in a microplate reader to measure the absorbance.<Br>
+<Br></p>
 <p class="description">
 <b>■Assay2 Result</b><Br>
+Standard Curves<Br>
+<Br>
+<IMG Src="https://static.igem.org/mediawiki/2012/a/a3/Assay2tmu.JPG" Width="640" Height="480"><Br>
+<Br>
+<b>concentration</b>
+<Br>
+<b>BBa_K749024</b><Br>
+<table border>
+<tr>
+<td>Enzyme+NAD</td>
+<td>NO enzyme</td>
+<td>NO NAD</td>
+</tr>
+<tr>
+<td>21.190</td>
+<td>25.629</td>
+<td>24.181</td>
+</tr>
+</table>
+<Br>
+<Br>
+<b>wt</b><Br>
+<table border>
+<tr>
+<td>Enzyme+NAD</td>
+<td>NO enzyme</td>
+<td>NO NAD</td>
+</tr>
+<tr>
+<td>21.181</td>
+<td>26.984</td>
+<td>25.124</td>
+</tr>
+</table>
+<p class="description"><Br>All samples Reaction time 60min<Br>
 </p>
 <Br>