Team:Warsaw/Calendar-Main/21 July 2008

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<h3>Cloning omega-A fusion on <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pKSII%2B>pKS</a> (second attempt)</h3>
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<h4>Michał L., Ewa, Marcin</h4>
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<p>We have finally got rid of evil phage infection and we are able to work with <i>E. coli</i> again. Hurray!</p>
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<ol>
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<li>Since the phage is gone we can continue this cloning:</li>
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<li>Restriction <a href="https://2008.igem.org/Wiki/Team:Warsaw/protocols#digest">digest</a> of PCL product and <A HREF=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pKSII%2B>pKS</a> vector with SacI and NotI (BamHI buffer) .</li>
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<li><a href="https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#ligation">Ligation</a> of omega-A fusion with <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pKSII%2B>pKS</a> vector.</li>
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<li><a href="https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#chemotransform">Transformation</a> of Top10 with ligation product.</li>
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<p>'''Cloning of protein A DNA to OmpA constructs''' <br>
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1. Colony PCR on colonies from plates with transformations pACYC177+OmpA_A_omega. Primers used:
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<a href="https://2008.igem.org/Wiki/Team:Warsaw/primers#AL+SacI">AL+SacI</a> and <a href="https://2008.igem.org/Wiki/Team:Warsaw/primers#AP+NotI">AP+NotI</a>
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2. Confirmed transformant colonies inoculated to liquid LB with kanamycin. <br>
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3. Isolation of plasmids from cultures inocluated on previous day (pACYC177+OmpA_A_alpha). <br>
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4. Control digest of isolated plasmids with BamHI and SacI .
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<p>Paweł: restriction analysis of plasmids isolated from overnight cultures. Result: none of isolated plasmids contain insert</p>
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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-omega</a> in place of OmpA</h3><h4>Paweł</h4>
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<p><ol><li>Result of ligation of <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pET15b%2BOmpA-omega>pET15b-OmpA-omega </a> with protein Z DNA: 4 colonies grown.</li>
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<li>Each colony cultured overnight in LB + ampicilin.</li>
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</p>
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<h3>Cloning of protein A DNA to OmpA constructs</h3><h4>Michał K.</h4>
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<p><ol>
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<li> <a href="https://2008.igem.org/Wiki/Team:Warsaw/protocols#digest">Digest</a> of <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pKSII+A>pKS-A</a> plasmid, <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> with NotI and SacI (BamHI buffer). pACYC177 vectors were also <a href="https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#removing">dephosphorylated (with CIAP)</a>.</li>
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<li> Gel electrophoresis and <a href="https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#DNA_isolation_from_agarose_gel">gel-out</a> of proper bands (420 bp - <A href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pKSII+A>pKS-A</a> lane, 4050 bp - <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pACYC177%2BompA-omega>pACYC177+OmpA_omega</a> lane and 4300 bp <a href=https://2008.igem.org/Wiki/Team:Warsaw/vectors/pACYC177%2BompA-alpha>pACYC177+OmpA_alpha</a> lane) (<a href="https://2008.igem.org/Team:Warsaw/Calendar-Main/21_July_2008#fig1">Fig. 1.</a>).</li>
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<li> <a href="https://2008.igem.org/wiki/index.php?title=Wiki/Team:Warsaw/protocols#ligation">Ligation</a> of A DNA fragment with both pACYC177 vectors.</li>
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<li> <a href="https://2008.igem.org/Wiki/Team:Warsaw/protocols#electrotransform">Transformation</a> of <i>E. coli</i> <a href="https://2008.igem.org/Wiki/Team:Warsaw/igem_notebook.htm#top10">TOP10</a>  strain with ligations. </li>
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<li>Transformants plating on LB + kanamycin. </li></ol>
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</p>
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<a name="fig1"><img src="https://static.igem.org/mediawiki/2008/a/ae/Mis_gogo.jpg" width=220/></a> <var><b>Fig. 1. </b>SacI/NotI digests of plasmids<br>
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1. Marker<br>
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2. digested pACYC177_OpmA_omega <br>
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3. digested pKSA <br></var>
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Latest revision as of 16:51, 29 October 2008

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Cloning omega-A fusion on pKS (second attempt)

Michał L., Ewa, Marcin

We have finally got rid of evil phage infection and we are able to work with E. coli again. Hurray!

  1. Since the phage is gone we can continue this cloning:
  2. Restriction digest of PCL product and pKS vector with SacI and NotI (BamHI buffer) .
  3. Ligation of omega-A fusion with pKS vector.
  4. Transformation of Top10 with ligation product.

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

Paweł

  1. Result of ligation of pET15b-OmpA-omega with protein Z DNA: 4 colonies grown.
  2. Each colony cultured overnight in LB + ampicilin.

Cloning of protein A DNA to OmpA constructs

Michał K.

  1. Digest of pKS-A plasmid, pACYC177+OmpA_omega and pACYC177+OmpA_alpha with NotI and SacI (BamHI buffer). pACYC177 vectors were also dephosphorylated (with CIAP).
  2. Gel electrophoresis and gel-out of proper bands (420 bp - pKS-A lane, 4050 bp - pACYC177+OmpA_omega lane and 4300 bp pACYC177+OmpA_alpha lane) (Fig. 1.).
  3. Ligation of A DNA fragment with both pACYC177 vectors.
  4. Transformation of E. coli TOP10 strain with ligations.
  5. Transformants plating on LB + kanamycin.

Fig. 1. SacI/NotI digests of plasmids
1. Marker
2. digested pACYC177_OpmA_omega
3. digested pKSA