Team:NTU-Singapore/Notebook/11 June 2008

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(Wednesday 11 June)
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***Gel electrophoresis for overnight digested products. Please refer to [https://2008.igem.org/wiki/index.php?title=Team:NTU-Singapore/Notebook/10_June_2008 10 June 2008 notebook]<br>(''Reminder'': the ratio of loading dye to test sample is 1:5)<br><br>'''Result:'''<br>+ RBS 32 and 34 that were digested with XbaI and SpeI showed correct bands at 2kb. Control experiments (RBS 32 and 34 digested with EcoRI and PstI) also showed correct bands at 2kb.<br>+ E7-1 PCR insert that was digested with XbaI and SpeI did not show any band, thus unsuccessful.
***Gel electrophoresis for overnight digested products. Please refer to [https://2008.igem.org/wiki/index.php?title=Team:NTU-Singapore/Notebook/10_June_2008 10 June 2008 notebook]<br>(''Reminder'': the ratio of loading dye to test sample is 1:5)<br><br>'''Result:'''<br>+ RBS 32 and 34 that were digested with XbaI and SpeI showed correct bands at 2kb. Control experiments (RBS 32 and 34 digested with EcoRI and PstI) also showed correct bands at 2kb.<br>+ E7-1 PCR insert that was digested with XbaI and SpeI did not show any band, thus unsuccessful.
***Gel extraction of E7-0 insert ([[Image:xxx|digested with XbaI and SpeI on Tuesday 10 June]]), RBS 32 and RBS 34 empty plasmid vectors ([[Image:upload later|digested with XbaI and SpeI on Tuesday 11 June]]) using QIAgen Gel Extraction Kit.
***Gel extraction of E7-0 insert ([[Image:xxx|digested with XbaI and SpeI on Tuesday 10 June]]), RBS 32 and RBS 34 empty plasmid vectors ([[Image:upload later|digested with XbaI and SpeI on Tuesday 11 June]]) using QIAgen Gel Extraction Kit.
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***Gel electrophoresis for confirmation after Gel extraction.
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***Gel electrophoresis for confirmation after Gel extraction (together with gel electrophoresis of T7 promoter).<br>'''Result:'''All the products showed correct 2kb bands. Also, as expected, T7 promoter didn't show any additional band as the pT7 gene is too small and probably run out of the gel.<br>
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***Ligation of E7-0 insert into RBS 32 empty plasmid vector.<br>  
***Ligation of E7-0 insert into RBS 32 empty plasmid vector.<br>  
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Revision as of 08:33, 13 June 2008

Wednesday 11 June

  • Morning:
    • Choon Kit, Hung:
      • Gel electrophoresis for overnight digested products. Please refer to 10 June 2008 notebook
        (Reminder: the ratio of loading dye to test sample is 1:5)

        Result:
        + RBS 32 and 34 that were digested with XbaI and SpeI showed correct bands at 2kb. Control experiments (RBS 32 and 34 digested with EcoRI and PstI) also showed correct bands at 2kb.
        + E7-1 PCR insert that was digested with XbaI and SpeI did not show any band, thus unsuccessful.
      • Gel extraction of E7-0 insert (digested with XbaI and SpeI on Tuesday 10 June), RBS 32 and RBS 34 empty plasmid vectors (digested with XbaI and SpeI on Tuesday 11 June) using QIAgen Gel Extraction Kit.
      • Gel electrophoresis for confirmation after Gel extraction (together with gel electrophoresis of T7 promoter).
        Result:All the products showed correct 2kb bands. Also, as expected, T7 promoter didn't show any additional band as the pT7 gene is too small and probably run out of the gel.
      • Ligation of E7-0 insert into RBS 32 empty plasmid vector.
Insert 1 E7-0 PCR insert 16ul
Vector 2 empty plasmid vector(from RBS 32) 2ul
ligase buffer T4 ligase buffer 2ul
ligase enzyme T4 ligase 1ul
Total 21ul
(After adding above amounts, incubate the mixtures at 4oC for at least 4-5 hours)
      • Transform ligated E7 (new biobrick part) into Top10 competent cells.
      • Transform LacI-GFP into BL-91 as control.