A New Covance Offering: zPREDICTA®’sReconstructed Bone (r-Bone), plate-based, 3-dimensional (3D) culture assay that mimics the tumor microenvironment found in myeloma, acute myelogenous leukemia and solid tumor metastasis.

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In order to provide a more reflective model of how tumor cells would respond to test agents in vivo, the tissue physiology where the tumor grows and proliferates needs to be recapitulated in vitro. This process has been accomplished using zPREDICTA’s organ-specific three-dimensional (3D) matrices that support long-term culture of carcinoma cells. Covance and zPREDICTA have worked together to develop tumor-specific 3D models, based on zPREDICTA’s proprietary 3D cell culture platform for preclinical testing and research studies in the biopharmaceutical industry. This tech spotlight highlights the characteristics of the Reconstructed Bone (r-Bone) model.

Growth of tumor cells within the bone marrow is a common phenomenon in hematologic malignancies. Thus, human myeloma cell linesRPMI 8226,NCI-H929, and U266B1 were utilized in proof-of-concept studies. As shown inFigure 1, U266B1 human myeloma cells were cultured in growth medium alone (2D) or in r-Bone matrix for 4 days. While the 2D culture becomes quickly overgrown and the cells maintain a morphology characterized by a single cell suspension, the r-Bone 3D culture supports the development of cell aggregates which proliferate into larger clusters more representative of tumor morphology. These cultures can be maintained for long periods with minor intervention by the researcher.

Figure 1: 2D vs Reconstructed Bone (r-Bone) 3D culture of U266B1 human myeloma cells
Figure 1: 2D vs Reconstructed Bone (r-Bone) 3D culture of U266B1 human myeloma cells

Figure 2shows cryo-electron microscopic images of r-Bone culture and ex vivo bone marrow seeded with metastatic breast cancer cells. The spatial and physical architecture of bone marrow stroma is maintained in the r-Bone extracellular matrix (ECM). The r-Bone ECM allows for co-culture of tumor cells with mesenchymal stem cells, fibroblasts, lymphoid, myeloid, andag亚博网站cells.

Cells can be isolated from the matrix after test agent exposure and analyzed by an appropriate downstream application, such asflow cytometry, RNASeq, or in situ imaging. Cytotoxicity assays such as CellTiter-Glo® can be performed in a high throughput format with the successful development of both 96 and 384-well assay formats. The platform is compatible with all drug classes tested, including biologics and small molecules.

Figure 2: Extracellular matrix architecture of r-Bone is indistinguishable from ex vivo tissue
Figure 2: Extracellular matrix architecture of r-Bone is indistinguishable from ex vivo tissue

Figure 3: Bortezomib is a standard of care agent for the treatment of multiple myeloma2。船尾er 4-day culture of NCI-H929, RPMI 8226, and U266B1 cells in r-Bone, bortezomib was added and the cells were returned to culture for an additional 4 days. (A) CellTiter-Glo® reagent was added and luminescence was quantified using a Cytation 3 imaging plate reader (Biotek Instruments). Four parameter nonlinear curve fitting analysis was normalized against the vehicle treated wells (n = 3 wells per concentration). (B) Representative images of U266B1 cells in r-Bone culture treated with vehicle (0.5% DMSO) or 20nM bortezomib. The red arrows indicate dead or dying cells in the cell clusters after 72hr exposure.

Figure 3: Bortezomib inhibition of myeloma cell proliferation in r-Bone culture
Figure 3: Bortezomib inhibition of myeloma cell proliferation in r-Bone culture

The r-Bone assay is a potential platform for studying multiple hematologic malignancies in vitro as well as the investigation of solid tumor metastasis, like breast and prostate carcinomas to the bone matrix.

zPREDICTAhas provided customized tumor-specific 3D cell culture models since 2014 and has been actively developing numerous organ-specific matrices to broaden the Covance preclinical tumor offerings since we've been working together.

Reconstructed mouse breast (r-mBreast) and human breast (r-Breast), lung (r-Lung), and prostate (r-Prostate), are currently being characterized and developed. These models will represent new early opportunities to screen test agents in a platform that will more closely mimic in vivo tissue microenvironments without investing in animal studies upfront. The potential to screen targeted chemical libraries in a high throughput 3D assay should be considered in early discovery efforts.

For more information on how these 3D model assays can be applied to yourpreclinical oncology and immuno-oncology research, contact thescientists at Covance Preclinical Oncology

References

1.埃德蒙森R,德布罗意JJ,爱德考克房颤,杨l .用力推ee-dimensional cell culture systems and their applications in drug discovery and cell-based biosensors.Assay Drug Dev Technol。2014;12(4):207–218.

2. Bortezomib Monograph for Professionals. Drugs.com. Retrieved 13 October 2019.