DNA

Part:BBa_K4181014

Designed by: Junzhi Yan   Group: iGEM22_SJTU-BioX-Shanghai   (2022-09-20)
Revision as of 09:12, 12 October 2022 by JunzhiYan (Talk | contribs)


cotE protein DNA sequence

We added a Linker sequence to the end of the cotE protein sequence to facilitate the production of cotE with a further binding peptide to function with the cotB protein.


Usage and Biology

cotB and cotE proteins are both innate proteins of B.subtilis which will express when sporulation is induced. They help organize the outer spore surface and therefore can be chosen as the anchoring proteins used in the spore display system, fused with exogeneous proteins to display them on the spore surface. Firstly, since cotB and cotE proteins are bacteriophage surface proteins of Bacillus subtilis and their coding genes are available in their genome, we extracted the genome of Bacillus subtilis strain WB800N, and then used this genome as a template to PCR the gene sequences corresponding to cotE and cotB proteins from the genome. With the design of PCR primers, we added the cotE to the homologous arm of the pHT01 plasmid sequence.A RBS sequence was added to the 5' end of the cotE gene sequence, and the stop codon was removed at its 3' end and the linker sequence was added; the homologous arm of the tyrosinase coding sequence and the RBS sequence were added to the 5' end of the cotB gene sequence, and the stop codon was removed at its 3' end. The stop codon was removed at the 3' end and the FLAG tag was added.

2022-SJTU-Biox-Shanghai-1.png
Figure 1. Electrophoresis results after PCR of cotE and the first PCR electrophoresis results of cotB. The picture indicates a positive result.

Next, PCR the cotB gene sequence again, and add 4B4 melanin-binding peptide and the stop codon to the 3' end of this sequence by designing your primers for this PCR.

2022-SJTU-Biox-Shanghai-2.png
Figure 2. Electrophoresis results of cotB after the second PCR and Dsup-encoded gene after PCR. The picture indicates a positive result.
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
    COMPATIBLE WITH RFC[25]
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Illegal SapI.rc site found at 493

Characterization

cotE and cotB proteins are closely related to tyrosinase activity.Tyrosinase and the melanin-binding-peptide were the next to be demonstrated because of their display on the spore surface, and the process of sporulation has been mentioned above. Because there was his-tag linking with our tyrosinase protein, we decided to use immunofluorescence to detect it. The following is the result of our immunofluorescence test:

2022-SJTU-Biox-Shanghai-3.png
Figure 3. Immunofluorescence assay on tyrosinase anchoring on the spore surface. Groups: Samples containing plasmid with IPTG induced; Samples containing plasmid without IPTG induced; WB800N wildtype.
.

Flow Cytometry

FCM was also conducted by similar procedures and the results are as below:

2022-SJTU-Biox-Shanghai-4.png
Figure 4. Results of flow cytometry for the detection of tyrosinase.

From the results, compared with the control group, samples with IPTG-induced plasmids showed more positive signals, whilst nearly no signals had been detected in the negative controls, suggesting a similar results as the immunofluoresecnce results. However, the peak of positive signals is just by the side of the negative peak, indicating a weak fluorescence intensity. From the result of FCM, it is more obvious that the total expression proportion of the target protein is relatively low. After discussion, we thought this was caused by several reasons. Firstly, during the growth and propagation of B.subtilis, the plasmid may be lost and thus no proteins can be generated. Secondly, as we could observe a large amount of spores under the phase-contract microscopy, it reminded us that we added IPTG for induction at the time when the OD of becteria was ranging from 0.6-0.8. This concentration was before the log-growth phase so that the bacteria would still propogate after IPTG induction. With the mother cells absorbing IPTG, less IPTG is left for daughter cells so that the bacteria produced by binary fissions later could not exposed to suffient amount of IPTG. Of course, as it can be indicated by fig20, B.subtilis would go through a quick propagation after transferred into sporulation medium, the concentration of ITPG at that stage of experiment could went even lower since no extra IPTG was added given its negative effects on the bacteria. Therefore, the concentration might be too low to induce the later produced bacteria generating proteins. Thirdly, we thought this might be caused by competitions between endogeneous cot proteins and the ones we introduced by exogeneous plasmid. As it is mentioned in our design, we cloned cotB and cotE proteins directly form the bacterial genome. So, there’re intrinsic prioteins to express under the regulation of sporulation signals naturally and thus compete with our exogeneous proteins to occupy the space on the spores’ outer surface. According to our results from Western blot, the expression level of our target priteins was not so much. In this regard, an unclear competitive advantage of exogeneous introduced proteins over the endogeneous ones might lead to the low anchoring rate of target proteins displayed in the outer surface. Generally, these results suggested we had successfully induced the expression and anchoring of tyrosinase on the spore surface. And there was notable expression disparity between the bacteria with IPTG-induced plasmid and the bacteria with no IPTG-induced plasmid and the wildtype.

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