Difference between revisions of "Part:BBa K1648002:Experience"

 
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This experience page is provided so that any user may enter their experience using this part.<BR>Please enter
 
This experience page is provided so that any user may enter their experience using this part.<BR>Please enter
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===Applications of BBa_K1648002===
 
===Applications of BBa_K1648002===
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This part is designed for <b>homologous recombination</b> to introduce the large magnetosome forming operon into <i>Azotobactor vinelandii</i>.
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This part is introduced into <i>A. vinelandii</i> genome via <b>random integration</b> before full operon sequences to be transformed into <i>A. vinelandii</i>.
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This Part were verified by double digestion (Fig. 1) and sequencing.
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[[File:K16480001GEL.jpg|400px]]
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Fig 1. Checking of recombinant plasmid using double digestion.
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L: DNA ladder.
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Lane 1-3: Recombination Template for mamAB Operon with Promotor and Terminator (BBa_K1648002) without digestion, with single digestion at XbaI site, with double digestion cut at XbaI and PstI site.
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This part was introduced into Azotobacter vinelandii by stable genomic integration. Every coding parts of it were successfully expressed. The expression of proteins was shown in SDS-PAGE (Fig .2).
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[[File:BBa_K1648002 SDS.jpg|450px]]
  
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Fig 2. SDS-PAGE showing expression of Recombination Template for mamAB Operon with Promotor and Terminator (BBa_K1648002) in Azotobacter vinelandii. L: Protein ladder. Lane 1: Wild-type Azotobacter vinelandii. Lane 2: transformed Azotobacter vinelandii. Lane 2 shows 3 more bands compared to lane 1, in which the ~25 kDa band is the protein coded by chloramphenicol resistant gene in BBa_K1648002, the ~15 kDa and ~ 13kDa bands are the protein coded by Recombination Template for mamAB Operon.
 
===User Reviews===
 
===User Reviews===
 
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Revision as of 05:11, 20 September 2015

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_K1648002

This part is designed for homologous recombination to introduce the large magnetosome forming operon into Azotobactor vinelandii.


This part is introduced into A. vinelandii genome via random integration before full operon sequences to be transformed into A. vinelandii.

This Part were verified by double digestion (Fig. 1) and sequencing. K16480001GEL.jpg
Fig 1. Checking of recombinant plasmid using double digestion. L: DNA ladder. Lane 1-3: Recombination Template for mamAB Operon with Promotor and Terminator (BBa_K1648002) without digestion, with single digestion at XbaI site, with double digestion cut at XbaI and PstI site.

This part was introduced into Azotobacter vinelandii by stable genomic integration. Every coding parts of it were successfully expressed. The expression of proteins was shown in SDS-PAGE (Fig .2).

BBa K1648002 SDS.jpg

Fig 2. SDS-PAGE showing expression of Recombination Template for mamAB Operon with Promotor and Terminator (BBa_K1648002) in Azotobacter vinelandii. L: Protein ladder. Lane 1: Wild-type Azotobacter vinelandii. Lane 2: transformed Azotobacter vinelandii. Lane 2 shows 3 more bands compared to lane 1, in which the ~25 kDa band is the protein coded by chloramphenicol resistant gene in BBa_K1648002, the ~15 kDa and ~ 13kDa bands are the protein coded by Recombination Template for mamAB Operon.

User Reviews

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