Team:Newcastle/12 July 2010

From 2010.igem.org

(Difference between revisions)
(Conditions)
(Research)
 
(24 intermediate revisions not shown)
Line 1: Line 1:
{{Team:Newcastle/mainbanner}}
{{Team:Newcastle/mainbanner}}
-
=LacI BioBrick Construction=
+
=Research=
-
[[Image:P7120450.JPG|300px|thumb|right]]
+
-
==Aims==
+
-
To use PCR to extract lacI (promoter, ribosome-binding site (RBS) & coding sequence (CDS)) from plasmid pMutin4 and ligate into vector pSB1AT3 in front of red fluorescent protein (RFP).
+
-
Summary:
+
We continued with our research on urease pathway in ''Bacillus subtilis'' 168.
-
# Colony PCR
+
-
# Streak plate
+
-
# Miniprep PCR - of colonies that worked
+
-
==Materials==
+
#Garnett J, Baumberg S, Stockley PG and Phillips SEV. (2007)."Structure of the C-terminal effector-binding domain of AhrC bound to its corepressor L-arginine". ''Acta crystallographica. Section F, Structural biology and crystallization communications''. 63(Pt 11). 918-21. International Union of Crystallography.
 +
#Garnett J, Marincs F, Baumberg S, Stockley PG and Phillips SEV. (2008). "Structure and function of the arginine repressor-operator complex from Bacillus subtilis". ''Journal of molecular biology''. 379(2. 284-98.
-
* PCR reagents
 
-
* Agar plates
 
-
* Gloves
 
-
* Wire loop
 
-
 
-
==Colony PCR==
 
-
 
-
Of the 11 plates with colonies grown 7 were used for colony PCR and Streak plating. Colony PCR is less accurate than the mini prep however results can be seen quicker whereas the miniprep has a 1 day wait. The colonies selected selected were satellite colonies because ampicillin degraded'''???'''
 
-
 
-
7 Tubes were labelled 1-7 (+ a control)
 
-
 
-
The quantities for the PCR are as follows:
 
-
[[Image:P7120427.JPG|200px|thumb|right]]
 
-
===Materials and Protocol===
 
-
 
-
Please refer to [[Team:Newcastle/PCR|PCR]]. The melting temperature, Tm, of this experiment is 54°C.
 
-
 
-
 
-
'''Note''' There are 2 possible reasons for red colonies formed:
 
-
 
-
# partial digest - rejoins without insert
 
-
# with insert 
 
-
 
-
We need to tell the difference between the two.
 
-
 
-
'''Note''' PCR is best when everything is kept on ice!
 
-
 
-
'''Note''' Melting temperatures of primers is important and can have a big effect on the product formed (Temperature used see Thursday)
 
-
 
-
==Spread Plates==
 
-
{|
 
-
|-
 
-
|[[Image:P7120408.JPG|thumb]]
 
-
|[[Image:P7120409.JPG|thumb]]
 
-
|[[Image:P7120418.JPG|thumb]]
 
-
|}
 
-
 
-
==Overnight culture==
 
-
The seven colonies that grew on the plates were cultured overnight. The protocol for [[Team:Newcastle/Growing_an_overnight_cultures| growing an overnight culture]] was followed.
 
-
 
-
==Tommorrow==
 
-
 
-
We are going to take one of the colonies that have worked and possibly a whole plasmid prep.
 
{{Team:Newcastle/footer}}
{{Team:Newcastle/footer}}

Latest revision as of 19:32, 25 October 2010

iGEM Homepage Newcastle University BacillaFilla Homepage Image Map

Research

We continued with our research on urease pathway in Bacillus subtilis 168.

  1. Garnett J, Baumberg S, Stockley PG and Phillips SEV. (2007)."Structure of the C-terminal effector-binding domain of AhrC bound to its corepressor L-arginine". Acta crystallographica. Section F, Structural biology and crystallization communications. 63(Pt 11). 918-21. International Union of Crystallography.
  2. Garnett J, Marincs F, Baumberg S, Stockley PG and Phillips SEV. (2008). "Structure and function of the arginine repressor-operator complex from Bacillus subtilis". Journal of molecular biology. 379(2. 284-98.


Newcastle University logo.png    Newcastle cbcb logo.pngNewcastle Biomedicine logo.gif    Team Newcastle CEG logo.gif
Newcastle iww logo.jpg  UNIPV Pavia Logo.gif  Newcastle BBSRC.gif    Newcastle Genevision logo.png Newcastle WelcomeTrust.jpg
FaceBook Icon
Retrieved from "http://2010.igem.org/Team:Newcastle/12_July_2010"