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From 2008.igem.org

Revision as of 10:15, 28 July 2008 (view source) Ylzouyilong (Talk | contribs) ← Older edit		Revision as of 10:15, 28 July 2008 (view source) Ylzouyilong (Talk | contribs) Newer edit →
Line 32:		Line 32:
	Primer 1             10uM                 1   2		Primer 1             10uM                 1   2
	Primer 2             10um                 1   2		Primer 2             10um                 1   2
-	Template DNA     changeable                 0.5   1	+	Template DNA       changeable                 0.5   1
	MgCl2             0.2M                 0.5   1		MgCl2             0.2M                 0.5   1
	ddH2O                 ---                 40.5 81		ddH2O                 ---                 40.5 81

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Revision as of 10:15, 28 July 2008

Although this page is still in heavy construction, every guest is welcomed to left your trace on the "Doodle Board".

             Our Team       Project   Parts      Experiments        Communication Links     Doodle Board

Our Team

      Luying Jia                      Yuanfan Yang 
      Gechong Ruan                Shan Lin
      Xin Rong                       Yicheng Long
      Ziying Liu                       Yuemeng Wang 
      Yilong Zou                     Zi Wang
      He Yang
      Yongqiang Gou                 Chao Wang
      Junjie Luo                    Cong Liu

Project

  This year we are trying to work at the motility of bacteria. E.coli senses some chemicals and moves toward or stays still, this behavior is called chemotaxis. Any modification of the pathway from the sensor to the motile apparatus will cause into different chemotactic effcts.

Parts

Communication

Experiment and Protocol

   1   PCR
    
   1.1 Gold Faster 	Taq system:
   
   Reagent	           Concentration/Activity	50ul 	100ul
   GF taq buffer     	    10x	                         5       10
   GF taq		                                 0.5	  0.5
   dNTPmix	            10mM each	                 1	  2
   Primer 1 	            10uM	                 1	  2
   Primer 2	            10um	                 1	  2
   Template DNA	      changeable	                 0.5	  1
   MgCl2	            0.2M	                 0.5	  1
   ddH2O	                ---	                40.5	 81

   1.2 The program under Gold faster taq system

   Progress	     Program I	                 Program 2
   Predenaturing    95℃         2-5 min	         95℃   2-5 min
   Denaturing	     95℃        10-20sec	         95℃   10-20sec
   Annealing	     (Tm-5) ℃   2-5 sec	         68℃   10-15sec/1kb
   Extension	     72℃        10-15sec/1kb	

25-30cycle 25-30cycle

   Last extension	  1-2min or skipped	       1-2min or skipped

   2 	Restriction cut:

           Reagent	        Concentration/Activity	 Volume(50ul system)
           Restriction cut buffer	10x	           5ul
           Enzyme 1	                --	           2.5ul
           Enzyme 2	                --	           2.5ul

 Incubate at 37℃, 1.5 hrs or longer
 (Enzymes from Takara Co., Ltd)

     3  Ligation:
              Reagent	    Volume(10ul system)
              Solution I	5ul
              DNA fragment	3.5ul
              Vector	        1.5ul

   Incubate at 16-18℃,1hr or longer
   (Ligation kit from Takara)

Links

 Tsinghua University: http://www.tsinghua.edu.cn/qhdwzy/index.jsp

 Parts: http://partsregistry.org

 iGEM Headquarter: hq@igem.org

 Beijing Normal University:https://2008.igem.org/Team:Beijing_Normal 

 ETH_Zurich:https://2008.igem.org/Team:ETH_Zurich

 Nature:http://www.nature.com

 Science:http://www.sciencemag.org

 System and Synthetic Biology:http://www.springer.com/biomed/journal/11693 

Doodle Board

 Oh, My E.coli, where are you!        Yilong 08.7.11

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