U2OS-ZFN-SNAP-Nup107 Cells

USD$800.00*

Products are shipped frozen on dry ice in cryotubes. Each cryotube typically contains 3 × 10⁶ cells for adherent lines or 5 × 10⁶ cells for suspension lines (refer to the batch CoA for details).

Prices excl. taxes plus shipping costs

cryovial

Product number: 300294

Safety data sheet

Product sheet

Certificate of Analysis (CoA)

Description	The U-2 OS-ZFN-SNAP-Nup107 cell line represents a specialized variant of the widely used human osteosarcoma cell line U-2 OS. This particular model has been engineered to express the SNAP-tagged version of the nucleoporin Nup107, a pivotal component of the nuclear pore complex, which is essential for the transport of molecules between the nucleus and the cytoplasm. The integration of the SNAP-tag technology allows for the biorthogonal labeling and visualization of Nup107 in live or fixed cells, providing a powerful tool for studying nucleocytoplasmic transport and nuclear pore complex architecture under physiological conditions. The U-2 OS background offers several advantages, including robust growth rates and a well-characterized karyotype, which support high-throughput screening applications and genomic studies. The ZFN (Zinc Finger Nuclease) technology used in this cell line facilitates targeted genome editing, enhancing the precision with which researchers can investigate the genetic contributions to nuclear transport and other cellular processes. This cell line is particularly useful for studies aimed at elucidating the dynamics and regulation of nuclear pore complexes in cancer biology and cellular physiology. Due to the specialized nature of the U-2 OS-ZFN-SNAP-Nup107 no.294 cell line, it is highly suited for advanced imaging techniques, including super-resolution microscopy, to explore nucleoporin functions at unprecedented detail. It is also a valuable resource for developing therapeutic strategies targeting nuclear transport pathways implicated in various diseases, including cancer. The SNAP-tag component adds versatility for further biochemical and proteomic analyses, making it an indispensable tool in the field of cellular and molecular biology.
Organism	Human
Tissue	Bone
Disease	Osteosarcoma

Age	15 years
Gender	Female
Ethnicity	Caucasian
Growth properties	Adherent

Citation	U-2 OS-ZFN-SNAP-Nup107 (Cytion catalog number 300294)
Biosafety level	1
NCBI_TaxID	9606
CellosaurusAccession	CVCL_B7FM
Depositor	The Ellenberg Lab (EMBL)
GMO Status	GMO-S1: This human osteosarcoma cell line (U2OS-ZFN-SNAP-Nup107 no.294) contains a ZFN-mediated SNAP-Nup107 gene fusion, supporting selective labeling of the Nup107 nuclear pore subunit. The modification is stably present. This classification applies only within Germany and may differ elsewhere.

Protein expression	SNAP-Nup107 (nuclear pore complex protein 107, SNAP-tag)

Culture Medium	McCoys 5a, w: 3.0 g/L Glucose, w: stable Glutamine, w: 2.0 mM Sodium pyruvate, w: 2.2 g/L NaHCO3 (Cytion article number 820200a)
Supplements	Supplement the medium with 10% FBS, 3.0 g/L Glucose, stable Glutamine, 2.0 mM Sodium pyruvate, 2.2 g/L NaHCO3, 1% NEAA
Dissociation Reagent	Accutase
Subculturing	Remove the old medium from the adherent cells and wash them with PBS that lacks calcium and magnesium. For T25 flasks, use 3-5 ml of PBS, and for T75 flasks, use 5-10 ml. Then, cover the cells completely with Accutase, using 1-2 ml for T25 flasks and 2.5 ml for T75 flasks. Let the cells incubate at room temperature for 8-10 minutes to detach them. After incubation, gently mix the cells with 10 ml of medium to resuspend them, then centrifuge at 300xg for 3 minutes. Discard the supernatant, resuspend the cells in fresh medium, and transfer them into new flasks that already contain fresh medium.
Fluid renewal	2 to 3 times per week
Freeze medium	As a cryopreservation medium, we use complete growth medium (including FBS) + 10% DMSO for adequate post-thaw viability, or CM-1 (Cytion catalog number 800100), which includes optimized osmoprotectants and metabolic stabilizers to enhance recovery and reduce cryo-induced stress.
Thawing and Culturing Cells	Confirm that the vial remains deeply frozen upon delivery, as cells are shipped on dry ice to maintain optimal temperatures during transit. Upon receipt, either store the cryovial immediately at temperatures below -150°C to ensure the preservation of cellular integrity, or proceed to step 3 if immediate culturing is required. For immediate culturing, swiftly thaw the vial by immersing it in a 37°C water bath with clean water and an antimicrobial agent, agitating gently for 40-60 seconds until a small ice clump remains. Perform all subsequent steps under sterile conditions in a flow hood, disinfecting the cryovial with 70% ethanol before opening. Carefully open the disinfected vial and transfer the cell suspension into a 15 ml centrifuge tube containing 8 ml of room-temperature culture medium, mixing gently. Centrifuge the mixture at 300 x g for 3 minutes to separate the cells and carefully discard the supernatant containing residual freezing medium. Gently resuspend the cell pellet in 10 ml of fresh culture medium. For adherent cells, divide the suspension between two T25 culture flasks; for suspension cultures, transfer all the medium into one T25 flask to promote effective cell interaction and growth. Adhere to established subculture protocols for continued growth and maintenance of the cell line, ensuring reliable experimental outcomes.
Incubation Atmosphere	37°C, 5% CO₂, humidified atmosphere.
Shipping Conditions	Cryopreserved cell lines are shipped on dry ice in validated, insulated packaging with sufficient refrigerant to maintain approximately −78 °C throughout transit. On receipt, inspect the container immediately and transfer vials without delay to appropriate storage.
Storage Conditions	For long-term preservation, place vials in vapor-phase liquid nitrogen at about −150 to −196 °C. Storage at −80 °C is acceptable only as a short interim step before transfer to liquid nitrogen.

Sterility	Mycoplasma contamination is excluded using both PCR-based assays and luminescence-based mycoplasma detection methods. To ensure there is no bacterial, fungal, or yeast contamination, cell cultures are subjected to daily visual inspections.