Difference between revisions of "Part:BBa K1041002:Experience"
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Team NRP-UEA_Norwich 2013 created this part using biobricks [[BBa_K1041000]] and [[BBa_K1041001]]. These biobricks both contain a Nde1 site after their promoter sequence, enabling a restriction digest to be performed. The RFP coding gene was excised from BBa_K1041000 and ligated in front of the AntG promoter of BBa_K1041001 to create a new biobrick. | Team NRP-UEA_Norwich 2013 created this part using biobricks [[BBa_K1041000]] and [[BBa_K1041001]]. These biobricks both contain a Nde1 site after their promoter sequence, enabling a restriction digest to be performed. The RFP coding gene was excised from BBa_K1041000 and ligated in front of the AntG promoter of BBa_K1041001 to create a new biobrick. | ||
− | Due to the major research side of our project involving | + | Due to the major research side of our project involving actinomycetes not ''E.coli'' this part was cloned into an appropriate actinomycete-specific intergrative plasmid PMS82. This was to allow the reporter to be utilised in screening for antimycin producing actinomycetes. |
− | The plasmid containing the reporter sequence (Bba_K1041002)was transformed into specialised ''E.coli''strains: ET12567 and pUZ8002. These cells were then conjugated with spore stocks of | + | The plasmid containing the reporter sequence (Bba_K1041002)was transformed into specialised ''E.coli''strains: ET12567 and pUZ8002. These cells were then conjugated with spore stocks of actinomycetes cultivated from soil samples to transfer the active biosensor in the plasmid. |
====Characterisation==== | ====Characterisation==== |
Revision as of 11:18, 4 October 2013
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.
Team NRP-UEA_Norwich 2013
Team NRP-UEA_Norwich 2013 created this part using biobricks BBa_K1041000 and BBa_K1041001. These biobricks both contain a Nde1 site after their promoter sequence, enabling a restriction digest to be performed. The RFP coding gene was excised from BBa_K1041000 and ligated in front of the AntG promoter of BBa_K1041001 to create a new biobrick.
Due to the major research side of our project involving actinomycetes not E.coli this part was cloned into an appropriate actinomycete-specific intergrative plasmid PMS82. This was to allow the reporter to be utilised in screening for antimycin producing actinomycetes. The plasmid containing the reporter sequence (Bba_K1041002)was transformed into specialised E.colistrains: ET12567 and pUZ8002. These cells were then conjugated with spore stocks of actinomycetes cultivated from soil samples to transfer the active biosensor in the plasmid.
Characterisation
This involved sequencing, restriction digests and BLAST analysis.
Restriction Digest
Part Bba_K1041002 was digested with enzymes XbaI and NdeI and compared to uncut DNA Fig 1.The enzyme digest shows the NdeI restriction has been conserved after ligation of fragments from parts Bba_J04450 and Bba_K1041001.
Sequencing
The biobrick was sent off to a company for sequencing and the data we received back Fig 2,3,4 showed the DNA is good quality as strong peaks were produced throughout analysis of the sample.
BLAST Analysis
The data we recieved back from the sequencing company was aligned using BLAST with the expected DNA sequence Fig 5,6The sequencing with both the forward and reverse primers had over 96% matches.
User Reviews
UNIQ7a91f615b8295913-partinfo-00000000-QINU UNIQ7a91f615b8295913-partinfo-00000001-QINU