Team:Warsaw/Calendar-Main/9 July 2008

From 2008.igem.org

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<h3>Preparation of constructs with OmpA protein fusions</h3><h4>Michał K.</h4>
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<h3>Preparation of constructs: OmpA_alpha and OmpA_omega #2</h3><h4>Michał K.</h4>
<p><ol>
<p><ol>
<li> Colony PCR on colonies from plates with transformations <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pACYC177%2BompA-omega>pACYC177+OmpA_omega</a> and <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pACYC177%2BompA-alpha>pACYC177+OmpA_alpha</a>. Primers used:
<li> Colony PCR on colonies from plates with transformations <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pACYC177%2BompA-omega>pACYC177+OmpA_omega</a> and <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pACYC177%2BompA-alpha>pACYC177+OmpA_alpha</a>. Primers used:
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<a href="https://2008.igem.org/Wiki/Team:Warsaw/primers#OmpaL_N">OmpaL_N</a> and <a href="https://2008.igem.org/Wiki/Team:Warsaw/primers#OmpaP_link">OmpaP_link</a>.
<a href="https://2008.igem.org/Wiki/Team:Warsaw/primers#OmpaL_N">OmpaL_N</a> and <a href="https://2008.igem.org/Wiki/Team:Warsaw/primers#OmpaP_link">OmpaP_link</a>.
</li><li> Gel electrophoresis.(Fig. 1., Fig. 2.)</li>
</li><li> Gel electrophoresis.(Fig. 1., Fig. 2.)</li>
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<img src="https://static.igem.org/mediawiki/2008/3/36/Kolonijny_ompa%2Balfa_omegoa_pci1_04_08_2008.jpg" width=300 /><var>Fig. 1. Colony PCR on primers shown above (vector change from pET15b to pACYC177) <b></b><br>
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Upper gel:<br>
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1. Marker<br>
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2-12 PCR from colonies carrying probable Omp_A_alpha<br>
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Lower gel<br>
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1. Marker<br>
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2-5. PCR from colonies carrying probable Omp_A_alpha<br>
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6. negative control<br>
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7-12. PCR from colonies carrying probable Omp_A_omega<br></var>
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<img src="https://static.igem.org/mediawiki/2008/f/fb/July_9_th.jpg" width=300 /><var>Fig. 2. Colony PCR on primers shown above (vector change from pET15b to pACYC177) <b></b><br>
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1. Marker<br>
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2-10 PCR from colonies carrying probable Omp_A_omega<br></var>
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<li> Confirmed transformant colonies inoculated to liquid LB with kanamycin.
<li> Confirmed transformant colonies inoculated to liquid LB with kanamycin.
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</p>
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<img src="https://static.igem.org/mediawiki/2008/3/36/Kolonijny_ompa%2Balfa_omegoa_pci1_04_08_2008.jpg" width=300 /><var>Fig. 1. Colony PCR on primers shown above (vector change from pET15b to pACYC177) <b></b><br>
 
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Upper gel:<br>
 
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1. Marker<br>
 
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2-12 PCR from colonies carrying probable Omp_A_alpha<br>
 
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Lower gel<br>
 
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1. Marker<br>
 
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2-5. PCR from colonies carrying probable Omp_A_alpha<br>
 
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6. negative control<br>
 
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7-12. PCR from colonies carrying probable Omp_A_omega<br></var>
 
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<img src="https://static.igem.org/mediawiki/2008/f/fb/July_9_th.jpg" width=300 /><var>Fig. 2. Colony PCR on primers shown above (vector change from pET15b to pACYC177) <b></b><br>
 
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1. Marker<br>
 
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2-10 PCR from colonies carrying probable Omp_A_omega<br></var>
 
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Revision as of 16:35, 26 October 2008

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Cloning of protein Z DNA to pET15b-OmpA-alpha in place of OmpA

Piotr, Antoni

  1. Digest of pET15b-OmpA-alpha and Z (in Geneart vector) with NdeI and NotI (Orange buffer).
  2. Gel-out of Z (~200 bp band).
  3. Overnight ligation of Z into digested pET15b-OmpA-alpha.


Preparation of constructs: OmpA_alpha and OmpA_omega #2

Michał K.

  1. Colony PCR on colonies from plates with transformations pACYC177+OmpA_omega and pACYC177+OmpA_alpha. Primers used: OmpaL_N and OmpaP_link.
  2. Gel electrophoresis.(Fig. 1., Fig. 2.)
    3. Fig. 1. Colony PCR on primers shown above (vector change from pET15b to pACYC177)
    Upper gel:
    1. Marker
    2-12 PCR from colonies carrying probable Omp_A_alpha
    Lower gel
    1. Marker
    2-5. PCR from colonies carrying probable Omp_A_alpha
    6. negative control
    7-12. PCR from colonies carrying probable Omp_A_omega
     Fig. 2. Colony PCR on primers shown above (vector change from pET15b to pACYC177)
    1. Marker
    2-10 PCR from colonies carrying probable Omp_A_omega
  3. Confirmed transformant colonies inoculated to liquid LB with kanamycin.

Preparation of construct pKS with A protein

Michał L., Marcin

  1. Gradient PCR (achieving multiple copies of gene coding A protein):
    template DNA pDRIVE-TAPtag - 1 µl
    primer AP+NotI - 2 µl
    primer AL+SacI - 2 µl
    Pfu buffer with Mg2+ - 5 µl
    10 mM dNTPs - 1 µl
    Pfu Turbo polymerase - 0.5 µl
    H2O - 38.5 µl

    Program:
    1. 94°C, 3 min
    2. 94°C, 30 sec
    3. 62 to 74°C, 45 sec
    4. 72°C, 45 sec
    5. Repeat of elongation step 25X
    6. 72°C, 10 min
    7. Hold at 4 °C

  2. Gel electrophoresis of PCR product.
  3. Isolation of proper band (470 bp) from the gel.
  4. Overnight digest of isolated PCR product and pKS vector with NotI and SacI; to the reaction mix with pKS added 0.5 µl of CIAP.


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