Difference between revisions of "Part:BBa K562008:Experience"
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<I>iGEM Dundee 2011</I> | <I>iGEM Dundee 2011</I> | ||
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| − | This part was seen work in practice. Synthesis of the | + | This part was seen work in practice. Synthesis of the five encoded polypeptides in very small scale cultures (1 ml) was observed by 35-S-Methionine labelling (Figure 1). |
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| + | ===Results=== | ||
| + | <i>E. coli</i> was transformed with <partinfo>BBa_K562008</partinfo> expressed from pT7.5, and the plasmid pGP1-2 encoding T7 polymerase, and grown aerobically for 3 hours in LB medium. T7 polymerase synthesis was induced by heat shock before all native transcription in <i>E. coli</i> was halted by the addition of rifampicin. 10 minutes later 1 ml of cells was then collected and spiked with 35-S-labelled Methionine. Following a 10 minute incubation the cell pellet was harvested and resuspended in Laemmli disaggregation buffer. Protein labelling was analysed by SDS-PAGE and autoradiography. | ||
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| + | This very small scale and sensitive technique reveals all polypeptides being expressed from the plasmid. | ||
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| + | [[Image:2008.jpg]] | ||
| + | :Figure 1: Transcription and translation of gene products produced from <partinfo>BBa_K562008</partinfo>. Radiolabelled revealed bands of the corresponding sizes to the PduA, PduN, PduT and PduU proteins. PduB can be expressed as a smaller PduB' variant from an alternative translation start site. The RED ARROW points to the lane producing polypeptides from BBa_K562008. | ||
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Latest revision as of 12:37, 1 October 2011
This experience page is provided so that any user may enter their experience using this part.
Please enter
how you used this part and how it worked out.
Applications of BBa_K562008
User Reviews
UNIQ4e15a435a966f4b2-partinfo-00000000-QINU
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•••
iGEM Dundee 2011 |
This part was seen work in practice. Synthesis of the five encoded polypeptides in very small scale cultures (1 ml) was observed by 35-S-Methionine labelling (Figure 1). |
Results
E. coli was transformed with BBa_K562008 expressed from pT7.5, and the plasmid pGP1-2 encoding T7 polymerase, and grown aerobically for 3 hours in LB medium. T7 polymerase synthesis was induced by heat shock before all native transcription in E. coli was halted by the addition of rifampicin. 10 minutes later 1 ml of cells was then collected and spiked with 35-S-labelled Methionine. Following a 10 minute incubation the cell pellet was harvested and resuspended in Laemmli disaggregation buffer. Protein labelling was analysed by SDS-PAGE and autoradiography.
This very small scale and sensitive technique reveals all polypeptides being expressed from the plasmid.
- Figure 1: Transcription and translation of gene products produced from BBa_K562008. Radiolabelled revealed bands of the corresponding sizes to the PduA, PduN, PduT and PduU proteins. PduB can be expressed as a smaller PduB' variant from an alternative translation start site. The RED ARROW points to the lane producing polypeptides from BBa_K562008.
UNIQ4e15a435a966f4b2-partinfo-00000004-QINU