Part:BBa_K4160015

GEMS receptor construct containing HA-tag as affinity domain

This composite part encodes for a Generalized Extracellular Molecule Sensor (GEMS) receptor construct. This part was developed by replacing the RR120 VHH affinity domain of BBa_K4160008 with a HA (BBa_K1150016) as affinity domain (Figure 1) containing a linker of 8 amino acids.
The DNA sequence of this part was used as a template for mRNA

A HA-tag is fused to the erythropoietin receptor (EpoR) (BBa_K4160001), a transmembrane receptor that forms the foundation of the GEMS receptor. At the intracellular side of the EpoR, the intracellular signal transduction domain IL-6RB (BBa_K4160002) is attached. Sensing and binding of ligand anti-PR3 to the affinity domain should induce dimerization of the EpoR. As a result, the IL-6RB domain should activate downstream signaling of the Janus kinase (JAK)/Signal Transducer and Activator of Transcription (STAT) pathway. In this part, an Igκ secretion signal (BBa_K4160000) is incorporated. This signal localizes the GEMS receptor to the membrane of mammalian cells. Furthermore, at the C-terminus of the part, a bovine growth Hormone polyadenylation (bGH poly A) signal is located which medicates efficient transcription termination and polyadenylation.¹

Usage & biology

This GEMS receptor construct is based on the GEMS system that is developed by Scheller et al., 2018.² The authors developed this highly modular synthetic receptor construct that allows for the coupling of an extracellular input to an intracellular signaling pathway.² The modularity of this receptor allows the designing of GEMS platforms that sense and respond to a wide variety of extracellular molecules.²

The TU-Eindhoven team 2022 developed this part to investigate whether the GEMS receptor would be expressed properly on the cellular membrane of HEK293T cells. This part was expressed using mRNA

Characterization

To investigate the binding of anti-HA antibodies to the HA-tag, an initial flow cytometry experiment was conducted. The mRNA encoding for the GEMS receptor construct containing HA-tag as affinity domain was transfected into HEK293T cells. Since the optimal expression of mRNA and the receptor induction was hard to estimate beforehand, incubation steps of 24 and 48 hours were performed. Subsequently, the HEK293T cells were collected and stained with a primary anti-HA antibody with Alexa Fluor 488. Flow cytometry experiments were performed using a FACS instrument (Figure 3).

The green shading and percentages shown in the graphs depict the number of cells with a higher fluorescence intensity in the Alexa Fluor 488 channel than the negative control. A percentage of 11.6% and 9,7% for incubation after 24 and 48 hours, respectively, indicating the percentage of HEK293T cells that have bound anti-HA via their GEMS receptor construct was obtained (Figure 3).

This initial experiment demonstrated that successful expression of the receptor was obtained since an increase in binding between both antibodies and the GEMS receptor construct compared to the negative control was seen. Due to limited time, no optimizations could be done. However, these initial results are promising, as antibody binding to the affinity domain of the GEMS receptor construct was obtained.

References

1. Wang XY, Du QJ, Zhang WL, et al. Enhanced Transgene Expression by Optimization of Poly A in Transfected CHO Cells. Front Bioeng Biotechnol. 2022;10. doi:10.3389/FBIOE.2022.722722/FULL
2. Scheller L, Strittmatter T, Fuchs D, Bojar D, Fussenegger M. Generalized extracellular molecule sensor platform for programming cellular behavior. Nat Chem Biol. Published online 2018. doi:10.1038/s41589-018-0046-z
3. Expression vector pLeo619, complete sequence - Nucleotide - NCBI. Accessed September 8, 2022. https://www.ncbi.nlm.nih.gov/nuccore/MG437012