Difference between revisions of "Part:BBa K3888007"

 
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HupS Upstream Flanking region<br>
 
HupS Upstream Flanking region<br>
The HupS gene encodes a partial uptake hydrogenase subunit. Mutating the hupS gene inactivated the uptake hydrogenase enzyme, thus increasing hydrogen production. The experimental plan is to obtain a 1.3 KB DNA fragment containing hupS gene and about 0.5 KB upstream and downstream flanking region DNA fragment by PCR, and clone them into pJQ200SK plasmid. The engineered plasmid will then be transferred by e. coli S17-1 conjugation or electroporation into R. Palustris CGA009.
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The HupS gene encodes a partial uptake hydrogenase subunit. Mutating the hupS gene inactivated the uptake hydrogenase enzyme, thus increasing hydrogen production. The experimental plan is to obtain two 1KB upstream and downstream flanking region DNA fragment by PCR, and gibson with pK18mobsacB-Gm plasmid backbone.Then the plasmid was imported into R. palustris via elctrotransformation.
 
In our experiment, Hups upstream flanking region is a part of DNA fragment about 1 KB in length for the deletion.<br>
 
In our experiment, Hups upstream flanking region is a part of DNA fragment about 1 KB in length for the deletion.<br>
[[File:T--SJTang--Hups_knockout2.png]]
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[[File:Deletion Plasmid construction.png]]
 
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===Figure 1: Illustration  of the general form of plasmid used to create marked knockout strains of R. palustris. ===
 
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The origin of replication (ori), origin of transfer (oriT) and sacB (blue) are part of the delivery plasmid. The green sequence is inserted into the multiple cloning site of the delivery plasmid. The left and right fragments (green) are sequences amplified from the R. palustris genome and used in overlap extension PCR to generate a recombinant product containing (a deletion and a restriction site). The restriction site is used to introduce the resistance cassette (purple). This interrupts the gene even if no deletion is present, and allows selection of successful transformants. <br>
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According to this model, we constructed UppE knockout plasmid below.<br>
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[[ File:HupS Deletion Plasmid Map.png]]
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===Figure 2: Deletion plasmid of HupS constructed according to the method mentioned above.===
  
  

Latest revision as of 15:43, 21 October 2021


HupS Upstream Flanking Region

HupS Upstream Flanking region
The HupS gene encodes a partial uptake hydrogenase subunit. Mutating the hupS gene inactivated the uptake hydrogenase enzyme, thus increasing hydrogen production. The experimental plan is to obtain two 1KB upstream and downstream flanking region DNA fragment by PCR, and gibson with pK18mobsacB-Gm plasmid backbone.Then the plasmid was imported into R. palustris via elctrotransformation. In our experiment, Hups upstream flanking region is a part of DNA fragment about 1 KB in length for the deletion.
Deletion Plasmid construction.png

Figure 1: Illustration of the general form of plasmid used to create marked knockout strains of R. palustris.

The origin of replication (ori), origin of transfer (oriT) and sacB (blue) are part of the delivery plasmid. The green sequence is inserted into the multiple cloning site of the delivery plasmid. The left and right fragments (green) are sequences amplified from the R. palustris genome and used in overlap extension PCR to generate a recombinant product containing (a deletion and a restriction site). The restriction site is used to introduce the resistance cassette (purple). This interrupts the gene even if no deletion is present, and allows selection of successful transformants.
According to this model, we constructed UppE knockout plasmid below.
HupS Deletion Plasmid Map.png

Figure 2: Deletion plasmid of HupS constructed according to the method mentioned above.

Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    INCOMPATIBLE WITH RFC[25]
    Illegal NgoMIV site found at 121
    Illegal NgoMIV site found at 258
    Illegal NgoMIV site found at 690
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Illegal BsaI.rc site found at 414