Difference between revisions of "Part:BBa K5237101"
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<li class="toclevel-2 tocsection-7"><a href="#4.2"><span class="tocnumber">4.2</span class="toctext"> The Truncated and Mutated Form of Cathepsin B Was Poorly Expressed in HEK293T Cells</span></a></li> | <li class="toclevel-2 tocsection-7"><a href="#4.2"><span class="tocnumber">4.2</span class="toctext"> The Truncated and Mutated Form of Cathepsin B Was Poorly Expressed in HEK293T Cells</span></a></li> | ||
− | <li class="toclevel-2 tocsection-8"><a href="#4. | + | <li class="toclevel-2 tocsection-8"><a href="#4.3"><span class="tocnumber">4.3</span class="toctext"> Conclusion</span></a> |
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Revision as of 09:07, 29 September 2024
Truncated and Mutated Form of Cathepsin B
Cathepsin B is a lysosomal protease involved in the progression of various cancer types. Here, we present a truncated and mutated form of cathepsin B (Δ1-20, D22A, H110A, R116A). This form of cathepsin B lacks an N-terminal signal peptide responsible for co-translational targeting of cathepsin B to the lumen of the endoplasmic reticulum. Additionally, we introduced three point mutations into the amino acid sequence of cathepsin B to increase its catalytic activity at higher pH values. We investigated cathepsin B induced cleavage of different peptide linkers via a fluorescence readout assay indicating that the truncated and mutated form of cathepsin B was not active in the cytosol. Western blotting further confirmed that our truncated and mutated form of cathepsin B was only poorly expressed in HEK293T cells.
1. Sequence Overview
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21INCOMPATIBLE WITH RFC[21]Illegal BglII site found at 566
Illegal BglII site found at 665 - 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal NgoMIV site found at 67
Illegal NgoMIV site found at 919
Illegal AgeI site found at 751 - 1000COMPATIBLE WITH RFC[1000]
2. Usage and Biology
Cathepsin B is a cysteine protease typically located in lysosomes or secreted outside the cell, where it degrades proteins of the extracellular matrix (Ruan et al., 2015). To facilitate lysosomal escape of cathepsin B, cells were treated with low concentrations of doxorubicin. As an alternative strategy, we created a cytosolic single-chain version of cathepsin B. Full-length human cathepsin B has an N-terminal signal peptide facilitating targeting and translation of cathepsin B into the rough endoplasmic reticulum (Ni et al., 2022). Procathepsin B is then transported into the lysosome where it matures into its active form by cleavage into a light and heavy chain (Szulc-Dąbrowska et al., 2020).
3. Assembly and Part Evolution
We designed a fluorescence readout assay in HEK293T cells based on expression of mCherry induced by the transactivator VP64. VP64 was conjugated to the DNA-binding domain (DBD) of Gal4 through the GFLG linker (BBa_K5237020). Binding of Gal4-DBD upstream of a gene encoding the fluorescence protein mCherry induces overexpression of mCherry by VP64. Consequently, separation of Gal4-DBD and VP64 by cathepsin B cleavage of the GFLG linker reduces mCherry expression (see Fig. 1).
We transfected our genetic constructs into HEK293T cells. The negative control was not transfected with the plasmid encoding cathepsin B. We investigated two different test conditions, in which we either transfected 30 ng or 60 ng of the plasmid encoding cathepsin B. The fluorescence intensity of mCherry was measured 48 hours after transfection. Our initial tests did not result in the unambiguous identification of a cathepsin B-cleavable peptide linker (see Fig. 2). For all linkers, we did not observe a large decrease in fluorescence intensity between the negative control and test conditions. In some conditions, the fluorescence intensity even increased between the negative control and test conditions.
Since cathepsin B is a lysosomal protease that is normally only active in the lysosome and the extracellular environment but not in the cytosol, we decided to change the native amino acid sequence of cathepsin B. The first modification we made to the gene encoding for human cathepsin B, was the deletion of the first twenty amino acids. This N-terminally truncated version of cathepsin B had previously been observed to have catalytic activity even in the absence of lysosomal proteases like pepsin (Müntener et al., 2005). Furthermore, we introduced three point mutations into the polypeptide chain of cathepsin B (D22A, H110A, and R116A). This has been shown to increase the activity of cathepsin B at higher pH values by disrupting the interactions of an occluding loop with the substrate binding pocket of cathepsin B (Nägler et al., 1997).
4. Results
4.1 The Truncated and Mutated Form of Cathepsin B Is not Catalytically Active in Vivo
We performed the same fluorescence readout assay in HEK293T cells that we also used for wild-type cathepsin B (BBa_K5237100). The fluorescence intensity of mCherry was measured 48 hours after transfection. However, we observed no decrease in fluorescence between our negative control and test conditions, indicating that Gal4-DBD-Linker-VP64 was not cleaved (see Fig. 3).4.2 The Truncated and Mutated Form of Cathepsin B Was Poorly Expressed in HEK293T Cells
Figure 4 shows a western blot of the wild-type (wt) version of cathepsin B as well as the truncated and mutated version of cathepsin B (Δ1-20, D22A, H110A, R116A). Cells of both cathepsin B versions were treated with 500 nM doxorubicin (dox) 24 hours post-transfection and incubated for additional 24 hours. For each condition, three replicates were blotted. We observed no differences in protein expression levels between the dox-treated and untreated wt versions of cathepsin B. For the truncated and mutated version of cathepsin B, however, only the untreated samples showed the corresponding band at approximately 36 kDa expected for this version of cathepsin B. Additionally, the bands of the truncated and mutated version appeared much weaker than the ones of the wt, indicating poorer protein expression.
4.3 Conclusion
Our results indicate that the truncated and mutated form of cathepsin B was poorly expressed in HEK293T cells. Therefore, we continued to use the wild-type form of cathepsin B for further experiments. After consulting the literature, we decided to treat cells with the cytostaticum doxorubicin to induce lysosomal escape of cathepsin B, as had been previously reported (Bien et al., 2004).
5. References
Müntener, K., Willimann, A., Zwicky, R., Svoboda, B., Mach, L., & Baici, A. (2005). Folding Competence of N-terminally Truncated Forms of Human Procathepsin B*. Journal of Biological Chemistry, 280(12), 11973-11980. https://doi.org/10.1074/jbc.M413052200
Nägler, D. K., Storer, A. C., Portaro, F. C. V., Carmona, E., Juliano, L., & Ménard, R. (1997). Major Increase in Endopeptidase Activity of Human Cathepsin B upon Removal of Occluding Loop Contacts. Biochemistry, 36(41), 12608-12615. https://doi.org/10.1021/bi971264+
Ni, J., Lan, F., Xu, Y., Nakanishi, H., & Li, X. (2022). Extralysosomal cathepsin B in central nervous system: Mechanisms and therapeutic implications. Brain Pathol, 32(5), e13071. https://doi.org/10.1111/bpa.13071
Ruan, H., Hao, S., Young, P., & Zhang, H. (2015). Targeting Cathepsin B for Cancer Therapies. Horiz Cancer Res, 56, 23-40.
Szulc-Dąbrowska, L., Bossowska-Nowicka, M., Struzik, J., & Toka, F. N. (2020). Cathepsins in Bacteria-Macrophage Interaction: Defenders or Victims of Circumstance? Front Cell Infect Microbiol, 10, 601072. https://doi.org/10.3389/fcimb.2020.601072