Human Clival Chordoma Tumor Cell Line (UM-Chor1)

Overview

This novel human clival chordoma cell line is isolated from primary diseased tissue showing phenotypic characteristics of classical chordomaphysaliferous cells. Cells were sorted using the neural cell adhension molecule (NCAM).

Key elements and design rationale

• Model identity: Human Clival Chordoma Tumor Cell Line (UM-Chor1) is supplied as a tumor cell line derived from Human bone.
• Growth properties: Adherent
• Growth conditions: Use of Applied Cell Extracellular Matrix (G422) is required for cell adhesion to the culture vessel. 4:1 ratio mixture of PriGrow V (TM015) and PriGrow II medium (TM002) + 10% FBS(Regular*) + 1X NEAA + 1% Penicillin/Streptomycin Solution (G255), 37.0°C, 5% CO₂. *Do not heat-inactivate
• Product format: Frozen, BSL-2

This cell-based model is generally used in neurobiology, differentiation, and cell signaling studies. Donor/background information is available for contextual interpretation.

Biological background

These cells can be grown in animal models are useful for chordoma related research. Donor/background information provided for this product: Clival Chordoma.

Research relevance and current trends

• Cell-line models continue to be used for tumor phenotype comparison, pathway perturbation studies, and assay development in controlled in vitro systems.
• Engineered and subtype-defined tumor lines are often used to compare growth behavior, reporter output, and response patterns across matched experimental conditions.
• When metastatic or lineage features are described, investigators commonly interpret results alongside morphology, passage history, and culture environment.

Common research applications

• Neurobiology-focused studies of growth state, differentiation-associated morphology, and cell signaling changes in culture.
• Cell-based assays that compare experimental perturbations across defined media and substrate conditions.
• Phenotype tracking using morphology, marker expression, or reporter output where applicable.

Changes in morphology, growth rate, viability, or reporter signal are typically interpreted together with passage history, culture matrix, and the specified growth conditions for the model.

Notes for experimental interpretation

• Morphology, doubling behavior, and reporter or marker output can shift with passage number, substrate choice, and medium composition; these variables should be recorded alongside experimental readouts.
• Matched controls such as parental cells, untreated cultures, or parallel cultures maintained under identical conditions help distinguish background effects from biology of interest.

Culture and product details

• Growth Conditions: Use of Applied Cell Extracellular Matrix (G422) is required for cell adhesion to the culture vessel. 4:1 ratio mixture of PriGrow V (TM015) and PriGrow II medium (TM002) + 10% FBS(Regular*) + 1X NEAA + 1% Penicillin/Streptomycin Solution (G255), 37.0°C, 5% CO₂. *Do not heat-inactivate
• Seeding Density (cells/cm²): 40,000

Cell line sourcing and selection (species, tissue, and disease model matching) · Stable cell line engineering (overexpression, knockdown, knockout via CRISPR/Cas9, shRNA, sgRNA) · Reporter gene integration (GFP, RFP, luciferase, fluorescent/bioluminescent constructs) · Genome editing and knockin (point mutations, tagged endogenous proteins, conditional alleles) · Inducible expression systems (Tet-On/Off and regulatable constructs) · Drug resistance marker selection (puromycin, G418, hygromycin, and others) · Custom growth and media optimisation for specific assay requirements · Scale-up production for high-throughput screening campaigns · Authentication and QC services (STR profiling, mycoplasma testing, viability assessment). Talk to a Scientist or contact support@biohippo.com.