Tag
PelB

Part:BBa_J32015

Designed by: Austen Heinz   Group: iGEM06_Duke   (2006-08-25)
Revision as of 12:38, 27 October 2017 by Zxjjdldb (Talk | contribs)


PelB leader sequence; directs protein to E. coli periplasmic membrane

The pelB leader sequence is a sequence of amino acids which when attached to a protein, directs the protein to the periplasmic membrane of E. coli, where the sequence is removed by pelB peptidase. It is used to direct coat protein-antigen fusions to the cell surface.

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 54
  • 1000
    COMPATIBLE WITH RFC[1000]


Improvement

When the 5 aspartate repeated sequence(5D) is added to the back of the pelB,its function will be improved. In order to verify the function of pelB-5D, we constructed piGEM2016-001, piGEM2016-002,piGEM2016-module01* and piGEM2016-module01. piGEM2016-001 and piGEM2016-002 are the expression vectors containing pelB-5D and PETase, the only difference between them is the immanent signal peptide of PETase with piGEM2016-002 was removed.piGEM2016-module01 and piGEM2016-module01* is a vector containing PETase and MHETase, the difference between them is that pelB-5D is added in the front of piGEM2016-module01s'MHETase. SDS-PAGE results of piGEM2016-001 and piGEM2016-002 show that the pelB-5D is working.Further more,SDS-PAGE result of piGEM2016-module01 is obviously better than that of piGEM2016-module01*. In short,All results show that pelB-5D can significantly enhance the secretion of extracellular protein.

T--UESTC-China--part21.jpg


Improvement By NEFU-China

To improve the function of this part, we made the codon optimization. In order to express and secret the recombinant CALB in E. coli, the 5’-terminal of the gene without its own translational initiation codon was combined with our improved PelB(BBa-K2302005). The fusion protein was expressed in E. coli BL21(DE3) using the pHis vector. Then we targeted CalB in the culture medium by western blot. To express and secret recombinant CAlB in E. coli, the 5’ terminal of the CALB gene without its own translational initiation codon was combined with the genes coding for the original Pelb signal sequence in Pelb-CALB#1, and Pelb-CALB#2 was combined with improved Pelb signal sequence. The gene of fusion protein was constructed in the pHis vector with tac promoter.

Results

To further demonstrate whether the CALB can secrete to the medium by the signal peptide Pelb, the supernatant was directly detected using western blot. CAlB was targeted by His-tag probe. 30ug of protein sample was added in every well. It was obvious that the bands were much more darker in figure B, which indicated the expression of Pelb-CALB#2 was higher than that of Pelb-CALB#1. The predicted molecular weight of fusion protein is different between Pelb-CALB#1 and Pelb-CALB#2, it maybe caused by the changed protein conformation after the codon optimization. Comparing the expression between A and B, it shows that the function of Pelb has been improved remarkablely.

NEFU-China_2017_PelB.png

Link

【1】https://parts.igem.org/Part:BBa_K2302005 【2】http://2017.igem.org/Team:NEFU_China/Basic_Part


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Categories
//proteindomain/localization
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