Difference between revisions of "Part:BBa K3610010"
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+ | ==Characterization== | ||
+ | |||
+ | ===Usage with split-NanoLuc=== | ||
+ | We fused this part to the SmallBit part of the NanoBit system, a split luciferase (CORE:SBit). We managed to express the CORE:SBit together with the ectodomain of the plant PRR BAK1 which was fused to the LargeBit part of the split NanoLuc protein (eBAK1:LBit). We were able to express both constructs in <i>S. cerevisiae</i>. For a more detailed description see the parts: [[Part:BBa K3610038]] and [[Part:BBa K3610051]]. | ||
+ | |||
+ | After transfection of the cells with the two plasmids, we tested whether the split-NanoLuc proteins would be able to interact, which would reconstitute its functionality. We further were interested in the interaction between the CORE and BAK1 ectoomain. CORE and BAK1 naturally interact upon binding of csp22. Should both receptors be expressed properly in the cell membrane of <i>S. cerevisiae</i>, the ligand will be able to bind to the CORE ectodomain. If this is sufficient to drive dimerization of the two receptor in <i>S. cerevisiae</i>, then the NanoLuc parts will be more likely to interact as well, which would lead to a higher amount of functional luciferase proteins in the cell. | ||
+ | |||
+ | To test for dimerization of the luciferase parts and also the two receptors, an assay with a luminometer was performed. | ||
+ | |||
+ | ====Luminescence assay==== | ||
+ | Samples with cells which were transfected with the two mentioned plasmids (eBAK1 and eCORE) and samples containing <i>S. cerevisiae</i> cells that were not transfected with any plasmids (UT). | ||
+ | |||
+ | Optical densities (OD600) of all samples were adjusted to 0.34.<br> | ||
+ | For each type of sample, three types of measurements were made: | ||
+ | *1 µL of deionized water added (no elicitor) | ||
+ | *1 µL of epitope elf18 added | ||
+ | *1 µL of epitope csp22 added | ||
+ | |||
+ | Each measurement was done four times with sample size 50µL. To each well 50 µL NanoGlo solution was added (50:1 buffer to furimazine)<br> | ||
+ | |||
+ | The average values of the four measurements are displayed in the plot below. | ||
+ | [[File:T--UZurich--NanoLuc CORE.png|600px|thumb|none|Figure 1: Average Luminescence over time]] | ||
+ | |||
+ | eBAK1 coexpressed with eCORE showed an increase in luminescence, although the effect was much smaller when compared with eEFR. The results again suggest, that addition of the bacterial elicitor csp22, which initiates interaciton between CORE and BAK1 does not increase the luminescence levels as samples without csp22 added showed greater luminescence than samples which were treated with this bacterial epitope. | ||
+ | |||
+ | These results led us to the conclusion that our plasmids get expressed. It further has been shown that the NanoBit parts fused to the receptors are able to interact and reconstitute their functionality as a funcitonal NanoLuc protein which catalyzes the reaction of furimazine to furimamide, which gives a luminescent output. In our case, however, receptor-specific bacterial epitopes did not increase luminescence levels when the receptors were expressed in S. cerevisiae. | ||
+ | It seems that there is no or very little csp22-driven dimerization of the two receptor-ectodomains CORE and BAK1. | ||
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Revision as of 23:12, 22 October 2020
CORE ectodomain from S. lycopersicum
This part compromises the cell surface receptor CORE of S. lycopersicum and contains the ectodomain and the transmembrane domain, including the juxtamembrane domain. It does not, however, include the native signal sequence in order to make it easier to express the CORE ectodomain in different organisms that do not recognize the signal sequence.
Usage and Biology
The cold shock protein receptor (CORE) is a plant pattern recognition receptor (PRR) and as such activates host innate immunity through detection of pathogen-associated molecular patterns (PAMPs). CORE is a leucine-rich repeat receptor-like kinase with 22 LRRs, there additionally is a 6 amino acid insert at LRR 11. It consists of an extracellular domain that perceives an epitope, csp22, from the highly conserved nucleic acid binding motif RNP-1 of bacterial cold-shock proteins (CSPs), which are highly abundant proteins found in the cytosol of bacteria. Further domains are a single pass transmembrane domain and an intracellular kinase domain (The sequence encoding the kinase domain is not in this part). Interaction of CORE with brassinosteroid-associated kinase (BAK)1 is necessary for inducing an immune response in the plant. The dimerization of CORE and BAK1 depends on the csp22, the ligand of CORE. The function of CORE in S. lycopersicum has been confirmed by expressing the receptor in A. thaliana, which made the plant responsive to csp22, a PAMP that is otherwise not perceived by PRRs from A. thaliana.
In our project we use this part to coexpress it together with the ectodomain of BAK1 in S. cerevisiae. The N-terminus of both parts are fused to a split-protein in order to visualize the interaction of the two LRR receptors, used as system for a visual output to confirm dimerization were split-mCherry and split-NanoLuc.
Characterization
Usage with split-NanoLuc
We fused this part to the SmallBit part of the NanoBit system, a split luciferase (CORE:SBit). We managed to express the CORE:SBit together with the ectodomain of the plant PRR BAK1 which was fused to the LargeBit part of the split NanoLuc protein (eBAK1:LBit). We were able to express both constructs in S. cerevisiae. For a more detailed description see the parts: Part:BBa K3610038 and Part:BBa K3610051.
After transfection of the cells with the two plasmids, we tested whether the split-NanoLuc proteins would be able to interact, which would reconstitute its functionality. We further were interested in the interaction between the CORE and BAK1 ectoomain. CORE and BAK1 naturally interact upon binding of csp22. Should both receptors be expressed properly in the cell membrane of S. cerevisiae, the ligand will be able to bind to the CORE ectodomain. If this is sufficient to drive dimerization of the two receptor in S. cerevisiae, then the NanoLuc parts will be more likely to interact as well, which would lead to a higher amount of functional luciferase proteins in the cell.
To test for dimerization of the luciferase parts and also the two receptors, an assay with a luminometer was performed.
Luminescence assay
Samples with cells which were transfected with the two mentioned plasmids (eBAK1 and eCORE) and samples containing S. cerevisiae cells that were not transfected with any plasmids (UT).
Optical densities (OD600) of all samples were adjusted to 0.34.
For each type of sample, three types of measurements were made:
- 1 µL of deionized water added (no elicitor)
- 1 µL of epitope elf18 added
- 1 µL of epitope csp22 added
Each measurement was done four times with sample size 50µL. To each well 50 µL NanoGlo solution was added (50:1 buffer to furimazine)
The average values of the four measurements are displayed in the plot below.
eBAK1 coexpressed with eCORE showed an increase in luminescence, although the effect was much smaller when compared with eEFR. The results again suggest, that addition of the bacterial elicitor csp22, which initiates interaciton between CORE and BAK1 does not increase the luminescence levels as samples without csp22 added showed greater luminescence than samples which were treated with this bacterial epitope.
These results led us to the conclusion that our plasmids get expressed. It further has been shown that the NanoBit parts fused to the receptors are able to interact and reconstitute their functionality as a funcitonal NanoLuc protein which catalyzes the reaction of furimazine to furimamide, which gives a luminescent output. In our case, however, receptor-specific bacterial epitopes did not increase luminescence levels when the receptors were expressed in S. cerevisiae. It seems that there is no or very little csp22-driven dimerization of the two receptor-ectodomains CORE and BAK1.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21INCOMPATIBLE WITH RFC[21]Illegal BglII site found at 1467
Illegal BamHI site found at 100
Illegal BamHI site found at 1492
Illegal BamHI site found at 1844 - 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]