Team:Warsaw/Calendar-Main/9 July 2008

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<h3>Cloning of protein Z DNA to <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pET15b%2BOmpA-omega>pET15b-OmpA-alpha</a> in place of OmpA</h3><h4>Piotr, Antoni</h4>
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<p><ol><li><a href="https://2008.igem.org/Wiki/Team:Warsaw/igem_notebook.htm#digest">Digest</a> of <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pET15b%2BOmpA-alpha>pET15b-OmpA-alpha</a> and Z (in <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pGeneart_Z>Geneart vector</a>) with NdeI and NotI (Orange buffer).</li>
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<li><a href="https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#DNA_isolation_from_agarose_gel">Gel-out</a> of Z (~200 bp band).</li>
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<li>Overnight <a href="https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#ligation">ligation</a> of Z into digested <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pET15b%2BOmpA-alpha>pET15b-OmpA-alpha</a>.</li>
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<p>'''Preparation of constructs with OmpA protein fusions'''<br>
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1. Colony PCR on colonies from plates with transformations OmpA_omega and OmpA_alpha <br>
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</ol></p>
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<br>
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<h3>Preparation of construct <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pKSII+A>pKS with A protein</a></h3>
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<h4>Michał L., Marcin</h4>
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<p><ol>
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<li> Gradient PCR (achieving multiple copies of gene coding A protein):<br>
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template DNA pDRIVE-TAPtag - 1 µl<br>
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primer
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<a href="https://2008.igem.org/Wiki/Team:Warsaw/primers#AP+NotI">AP+NotI</a></html> - 2 µl<br><html>
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primer
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<a href="https://2008.igem.org/Wiki/Team:Warsaw/primers#AL+SacI">AL+SacI</a> - 2 µl<br>
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Pfu buffer with Mg<sup>2+</sup> - 5 µl<br>
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10 mM dNTPs - 1 µl<br>
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Pfu Turbo polymerase - 0.5 µl<br>
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H2O - 38.5 µl<br>
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<br><html>
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Program:<br>
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1. 94&deg;C, 3 min<br>
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2. 94&deg;C, 30 sec<br>
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3. 62 to 74&deg;C, 45 sec<br>
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4. 72&deg;C, 45 sec<br>
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5. Repeat of elongation step 25X<br>
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6. 72&deg;C, 10 min<br>
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7. Hold at 4 &deg;C<br>
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</li><br>
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<li> Gel electrophoresis of PCR product.</li>
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<li> <a href="https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#DNA_isolation_from_agarose_gel">Isolation</a> of proper band (470 bp) from the gel.</li>
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<li> Overnight <a href="https://2008.igem.org/Wiki/Team:Warsaw/igem_notebook.htm#digest">digest</a> of isolated PCR product and <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pKSII%2B>pKS</a> vector with NotI and SacI; to the reaction mix with <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pKSII%2B>pKS</a> added 0.5 µl of <a href="https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#removing">CIAP</a>. </li>
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</ol>
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</p>
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<h3>Preparation of constructs: OmpA_alpha and OmpA_omega #2</h3><h4>Michał K.</h4>
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<p><ol>
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<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>.
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</li><li> Gel electrophoresis. (<a href="https://2008.igem.org/Team:Warsaw/Calendar-Main/9_July_2008#fig1">Fig. 1. </a> and <a href="https://2008.igem.org/Team:Warsaw/Calendar-Main/9_July_2008#fig2">Fig. 2.</a>).</li>
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<li> Confirmed transformant colonies inoculated to liquid LB with kanamycin.
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</li></ol></p>
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<a name="fig1"><img src="https://static.igem.org/mediawiki/2008/3/36/Kolonijny_ompa%2Balfa_omegoa_pci1_04_08_2008.jpg" width=300 /></a><var><b>Fig. 1. </b>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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<a name="fig2"><img src="https://static.igem.org/mediawiki/2008/f/fb/July_9_th.jpg" width=300 /></a><var><b>Fig. 2.</b> 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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Latest revision as of 17:42, 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 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.

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. and Fig. 2.).
  3. Confirmed transformant colonies inoculated to liquid LB with kanamycin.

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