Team:UTP-Panama/Week 16

From 2011.igem.org

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(WET LAB)
 
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==September 19==
==September 19==
===WET LAB===
===WET LAB===
-
(Objetives or Title):
+
====I. DIGESTION====
-
--ESCRIBIR Y MEJORAR LAB--
+
For each Eppendorf PCR was added the following:<br>
 +
1. 10µL DNA (residue of mini prep)<br>
 +
2. 32.5 µL water ultra-pure distilled water<br>
 +
3. 5µL buffer (P2)  <br>
 +
4. 0.5µL BSA<br>
 +
5. 1µL enzyme 1 (EcoRI)<br>
 +
6. 1µL enzyme 2 (Spel)<br>
 +
____________<br>
 +
Total 50µL<br>
 +
 
 +
[[File:19sep dig.jpg|center]]<br>
 +
 
 +
There was added the 6 components to the small tube of PCR. <br>
 +
Note: Make sure to mix all the components in the centrifuge <br>
 +
 
 +
7. Two (2)eppendorf tubes were incubated in the thermocycler during 1 hour at 37°C : <br>
 +
a. UPSTREAM (GaTech) <br>
 +
b. DOWNSTREAM (Bristol)<br>
 +
8. Once again, tubes were incubated in the thermocycler during 20 minutes at 80°C<br>
 +
9. We stored at -20°C until it is used for ligation.<br>
 +
 
 +
==== Transformation of Competent Cells====
 +
A.
 +
4 petri dishes were filled with 5mL of solid LB
 +
3 positive controls and 1 negative control.
 +
[[File:calculo 19sept.jpg]]
 +
 
 +
Total: '''19.36µL para 20µL de LB'''<br>
 +
 
 +
''''Content of controls:'''' <br>
 +
Positive Control: 50µL competent cells + 2µL BBa_K410000 is resuspended.<br>
 +
Negative Control: 50µL competent cells  <br>
 +
 
 +
1. In 3 eppendorf tubes was added the specified amount in positive control and were resuspended.<br>
 +
2. Tubes in previous step remained settled in ice during 30 minutes.<br>
 +
3. Afterwards, cold shock carried out, the 4 eppendorf are set in water bath for a minute. (T=42°C)<br>
 +
4. Right after the water bath, it remained in ice during 5 minutes.<br>
 +
5. Added 200µL cold SOC to each eppendorf tube, then resuspended<br>
 +
6. Every petri dish was sealed with parafilm and was appropriately labeled; afterwards they were put in the incubator<br>
 +
 
 +
==September 20==
-
==September 20==}
 
===Scientific Comunication Activities===
===Scientific Comunication Activities===
-
Presentation (by the students of iGEM UTP-Panama) in the Electrical Faculty  of:<br>
+
Tree sessions: <br>
-
What's SynBio?<br>
+
Session 1: Civil Engineering Faculty (morning)
 +
Session 2: Electrical Engineering Faculty (afternoon)
 +
Session 3: Civil Engineering Faculty (afternoon)
 +
Presentation (by the students of iGEM UTP-Panama) about the following topics:<br>
 +
What's SynBio? <br>
 +
Applications of SynBio <br>
What's iGEM?<br>
What's iGEM?<br>
What are we doing? (our project) <br>
What are we doing? (our project) <br>
-
The applications of SynBio.
+
Future projects
-
===WET LAB===
+
====WET LAB====
-
(Objetives or Title):
+
 
-
--ESCRIBIR Y MEJORAR LAB--
+
 
 +
Objetives or Title:<br>
 +
In the picture of the result of the electrophoresis of Biobrick BBa-K381001, neither the patron nor the plasmids could be observed, for this reason the protocol was repeated the next day.<br>
 +
          1  2    3  4
 +
[[File:igem utp 20-09-2011.jpg]]
 +
 
 +
1, 2 : BBa_K381001 (positive control)
 +
 
 +
3, 4 : BBa_K381001 (negative control)
==September 21==
==September 21==
===WET LAB===
===WET LAB===
-
(Objetives or Title):
+
[[File:3CONTROLES 21SEPT CONTRASTE INVERTIDO Bristol.jpg]]
-
--ESCRIBIR Y MEJORAR LAB--
+
-
==September 22==
+
This day the electrophoresis test was performed to the obtained plasmids with BBa-K381001 in Sept 14, 2011.<br>
-
===WET LAB===
+
Also were transformed competent cells with BBa-K672000 (RENBO); Sept 21, 2011.<br>
-
(Objetives or Title):
+
-
--ESCRIBIR Y MEJORAR LAB--
+
==September 23==
==September 23==
===WET LAB===
===WET LAB===
-
(Objetives or Title):
+
We carried out a '''dirty mini prep protocol''' to BBa-K672000 to send 250ng DNA in 10µL TE. A sample was preserved for electrophoresis.
-
--ESCRIBIR Y MEJORAR LAB--
+
==September 24==
==September 24==
===GENERAL SESSION ===
===GENERAL SESSION ===
-
Morning: Talikng about WET LAB final activities.
+
Afternoon: Talikng about WET LAB final activities.
-
Design of the '''"SB UTP 1.0"''' and '''"SB UTP Project 1.0"'''
+
Design of the '''"SB UTP 1.0"''' and '''"SB UTP Project 1.0"'''<br>
 +
Discussion about remake the experiments with the Bristol and Gatech Biobricks (experience).

Latest revision as of 05:00, 29 September 2011

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Week 16: September 19 to 24

September 19

WET LAB

I. DIGESTION

For each Eppendorf PCR was added the following:
1. 10µL DNA (residue of mini prep)
2. 32.5 µL water ultra-pure distilled water
3. 5µL buffer (P2)
4. 0.5µL BSA
5. 1µL enzyme 1 (EcoRI)
6. 1µL enzyme 2 (Spel)
____________
Total 50µL

19sep dig.jpg

There was added the 6 components to the small tube of PCR.
Note: Make sure to mix all the components in the centrifuge

7. Two (2)eppendorf tubes were incubated in the thermocycler during 1 hour at 37°C :
a. UPSTREAM (GaTech)
b. DOWNSTREAM (Bristol)
8. Once again, tubes were incubated in the thermocycler during 20 minutes at 80°C
9. We stored at -20°C until it is used for ligation.

Transformation of Competent Cells

A. 4 petri dishes were filled with 5mL of solid LB 3 positive controls and 1 negative control. Calculo 19sept.jpg

Total: 19.36µL para 20µL de LB

'Content of controls:'
Positive Control: 50µL competent cells + 2µL BBa_K410000 is resuspended.
Negative Control: 50µL competent cells

1. In 3 eppendorf tubes was added the specified amount in positive control and were resuspended.
2. Tubes in previous step remained settled in ice during 30 minutes.
3. Afterwards, cold shock carried out, the 4 eppendorf are set in water bath for a minute. (T=42°C)
4. Right after the water bath, it remained in ice during 5 minutes.
5. Added 200µL cold SOC to each eppendorf tube, then resuspended
6. Every petri dish was sealed with parafilm and was appropriately labeled; afterwards they were put in the incubator

September 20

Scientific Comunication Activities

Tree sessions:
Session 1: Civil Engineering Faculty (morning) Session 2: Electrical Engineering Faculty (afternoon) Session 3: Civil Engineering Faculty (afternoon) Presentation (by the students of iGEM UTP-Panama) about the following topics:
What's SynBio?
Applications of SynBio
What's iGEM?
What are we doing? (our project)
Future projects

WET LAB

Objetives or Title:
In the picture of the result of the electrophoresis of Biobrick BBa-K381001, neither the patron nor the plasmids could be observed, for this reason the protocol was repeated the next day.

         1   2    3   4

Igem utp 20-09-2011.jpg

1, 2 : BBa_K381001 (positive control)

3, 4 : BBa_K381001 (negative control)

September 21

WET LAB

3CONTROLES 21SEPT CONTRASTE INVERTIDO Bristol.jpg

This day the electrophoresis test was performed to the obtained plasmids with BBa-K381001 in Sept 14, 2011.
Also were transformed competent cells with BBa-K672000 (RENBO); Sept 21, 2011.

September 23

WET LAB

We carried out a dirty mini prep protocol to BBa-K672000 to send 250ng DNA in 10µL TE. A sample was preserved for electrophoresis.

September 24

GENERAL SESSION

Afternoon: Talikng about WET LAB final activities. Design of the "SB UTP 1.0" and "SB UTP Project 1.0"

Discussion about remake the experiments with the Bristol and Gatech Biobricks (experience).
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