Difference between revisions of "Part:BBa K371014:Design"
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In the previous literature,most of research work on pdu BMC(or pdu MCP) focus on ''Citrobacter Freundii'' and ''Salmonella enterica''. Taking all of the factors together, we choose Citrobacter Freundii as the orgin of gene in our project. Because the whole genome of Citrobacter Freundii has not been decoded yet, we use the reference sequence sent to NCBI by Martin J.Warren group(GenBank: AM498294.1). | In the previous literature,most of research work on pdu BMC(or pdu MCP) focus on ''Citrobacter Freundii'' and ''Salmonella enterica''. Taking all of the factors together, we choose Citrobacter Freundii as the orgin of gene in our project. Because the whole genome of Citrobacter Freundii has not been decoded yet, we use the reference sequence sent to NCBI by Martin J.Warren group(GenBank: AM498294.1). | ||
− | In order to make the new parts compatible to new standard, we firstly check the sequence of pduP, which we get from GenBank(GenBank: AM498294.1), with the new four restriction enzymes site EarI, SapI,SacI and BglII. Luckily, none of these site were find in the 192bp sequence of pduP. Then we use the following primers to get the pduP64 from ''Citrobacter Freundii'' genome. The final part consist of cds of | + | In order to make the new parts compatible to new standard, we firstly check the sequence of pduP, which we get from GenBank(GenBank: AM498294.1), with the new four restriction enzymes site EarI, SapI,SacI and BglII. Luckily, none of these site were find in the 192bp sequence of pduP. Then we use the following primers to get the pduP64 from ''Citrobacter Freundii'' genome. The final part consist of cds of pduP64 with meta-prefix and meta-suffix in its sides |
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<div style="padding-left:25px;background-color:#FFFACD"> | <div style="padding-left:25px;background-color:#FFFACD"> | ||
− | <p>forward primer:5'- | + | <p>forward primer:5'-GTTTCTCTTCAATGAACACTTCAGAACTTGAAACCCTT-3'</p> |
− | <p>reverse primer:5'- | + | <p>reverse primer:5'-GTTTCTCTTCAACCTCGCAGGGCGTTAATGATGG-3'</p> |
</div> | </div> | ||
</html> | </html> | ||
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===Source=== | ===Source=== |
Latest revision as of 07:41, 27 October 2010
pduP1-64
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]
Design Notes
The present BioBrick assembly standard RFC does not support Protein fusion. In our project, we propose a new BioBrick assembly standard BBF RFC53---MetaPart Assembly Standard, which extending RFC 10 to Enable Scarless Protein Fusion with Type IIS Restriction Enzyme EarI and SapI.
In the previous literature,most of research work on pdu BMC(or pdu MCP) focus on Citrobacter Freundii and Salmonella enterica. Taking all of the factors together, we choose Citrobacter Freundii as the orgin of gene in our project. Because the whole genome of Citrobacter Freundii has not been decoded yet, we use the reference sequence sent to NCBI by Martin J.Warren group(GenBank: AM498294.1).
In order to make the new parts compatible to new standard, we firstly check the sequence of pduP, which we get from GenBank(GenBank: AM498294.1), with the new four restriction enzymes site EarI, SapI,SacI and BglII. Luckily, none of these site were find in the 192bp sequence of pduP. Then we use the following primers to get the pduP64 from Citrobacter Freundii genome. The final part consist of cds of pduP64 with meta-prefix and meta-suffix in its sides
forward primer:5'-GTTTCTCTTCAATGAACACTTCAGAACTTGAAACCCTT-3'
reverse primer:5'-GTTTCTCTTCAACCTCGCAGGGCGTTAATGATGG-3'
Source
Citrobactor freudii, the strain was bought from NITE Biological Resource Center (NBRC). NBRC NO. is 12681. History:IFO 12681 <- Ajinomoto Co., Inc. (AJ 2619) <- ATCC 8090 <- C.H. Werkm