A375-iRFP-Neo
Species | Human |
Cell Type | Melanoma |
Transgene | Near-infrared fluorescent protein (iRFP; ex/em 690/713nm) |
Selection Gene | Neomycin resistance (Neo) |
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Description
A375-iRFP-Neo is a polyclonal population of the human malignant melanoma cell line A375 (ATCC® CRL-1619™). To achieve stable reporter expression in the polyclonal population, parental A375 cells were transduced with LV-iRFP-P2A-Neo (LV033) and selected using G418. LV-iRFP-P2A-Neo encodes the near-infrared fluorescent protein (iRFP) cDNA linked to the neomycin resistance gene (Neo) via a P2A cleavage peptide under the spleen focus-forming virus (SFFV) promoter.
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This cell line has been tested for mycoplasma contamination and is certified mycoplasma free.
The parental A375 cell line has been authenticated and certified free of interspecies cross contamination by short tandem repeat (STR) profiling with 9 STR loci.
Replication Competent Lentivirus (RCL) Test (including a test report) is available for this cell line at an added cost. Contact us to learn more.
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Characterization
Morphology
Low and high density cell morphology (200X)
iRFP Expression
A375-iRFP-Neo (red) or control (A375-Fluc-Puro; grey) cells were fixed with paraformaldehyde and analyzed by flow cytometry (20,000 events).
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Growth Conditions
Complete Growth Medium: DMEM supplemented with 10% FBS, 1X Penicillin/Streptomycin, and 0.6 µg/mL G418.
The addition of G418 to the complete growth medium maintains high reporter expression over continued passage of the cells. It is highly recommended, especially if the cells undergo multiple passages prior to being used for studies.
These cells should be grown in the indicated medium and passaged when they reach confluency. For routine passaging, cells are recommended to be split at a 1:10 ratio every 3-4 days.
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Usage Information
These cells are suitable for in vitro and in vivo experimentation. A375 cells are a xenograft model for malignant melanoma and form tumors post-implantation into immunosuppressed mice1. The iRFP transgene facilitates in vivo and ex vivo fluorescence imaging of implanted cells. To reduce background autofluorescence, mice should be fed an alfalfa-free diet for at least a week prior to imaging.
The cells can be amplified in vitro and used to generate additional frozen stocks. Cryopreservation of low passage stocks is recommended. Frozen stocks should be preserved in a designated cryopreservation medium.
These cells were generated via lentiviral vector transduction. The lentiviral vector used for transduction was a self-inactivating (SIN) vector in which the viral enhancer and promoter have been deleted. Transcription inactivation of the LTR in the SIN provirus increases biosafety by preventing mobilization by replication competent viruses and enables regulated expression of the genes from the internal promoters without cis-acting effects of the LTR2. Nevertheless, all work with these cells should be performed under biosafety-level 2 (BSL2) conditions by trained personnel. Institutional requirements may permit handling of these cells under BSL1 conditions if certain criteria are met.
References:
1Gershwin et al. J Natl Cancer Inst 1977. 58:1455-1461.
2Miyoshi et al. J Virol 1998. 72:8150-8157. -
Datasheet/COA
Lot Number CL-IM85