Fluorescence and Luciferase Dual Reporter Lentivirus

SKU:BHV19400181
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    Overview
    Click light‑blue chips for details
    The Fluorescence and Luciferase Dual Reporter Lentivirus stably co-expresses a luciferase and a fluorescent protein from one transcript via self-cleaving peptides, giving each labeled cell both a bioluminescent and a fluorescent tag. Supplied as ultra-purified, high-titer particles, it efficiently transduces primary and difficult-to-transfect cells for longitudinal in vivo imaging of tumor growth and metastasis alongside flow cytometry and FACS-based analysis of the tumor microenvironment.
    Reporter GFP, RFP, Luc
    Selection Blasticidin, Puromycin
    Promoter CMV, CMV+PGK, EF1α, PGK
    Application In Vivo & In Vitro Dual Imaging
    Titer 3×10⁸ VP/mL
    Format 3rd Gen, VSV-G Pseudotyped
    Available Options

    Select the lentiviral variant that best fits your experiment. Availability and lead time may vary by option.

    • Options:
      • Vector Layout: LFV-V1a; Component Arrangement: CMV-Luc-T2A-GFP-P2A-Puro; Amount TU: 2x10^6 — LFV-V1a construct featuring CMV-driven co-expression of luciferase and GFP with puromycin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V1a; Component Arrangement: CMV-Luc-T2A-RFP-P2A-Puro; Amount TU: 2x10^6 — LFV-V1a construct featuring CMV-driven co-expression of luciferase and RFP with puromycin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V1a; Component Arrangement: CMV-Luc-T2A-GFP-P2A-BSD; Amount TU: 2x10^6 — LFV-V1a construct featuring CMV-driven co-expression of luciferase and GFP with blasticidin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V1a; Component Arrangement: CMV-Luc-T2A-RFP-P2A-BSD; Amount TU: 2x10^6 — LFV-V1a construct featuring CMV-driven co-expression of luciferase and RFP with blasticidin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V1b; Component Arrangement: CMV-GFP-T2A-Puro-P2A-Luc; Amount TU: 2x10^6 — LFV-V1b construct featuring CMV-driven co-expression of luciferase and GFP with puromycin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V1b; Component Arrangement: CMV-RFP-T2A-Puro-P2A-Luc; Amount TU: 2x10^6 — LFV-V1b construct featuring CMV-driven co-expression of luciferase and RFP with puromycin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V1b; Component Arrangement: CMV-GFP-T2A-BSD-P2A-Luc; Amount TU: 2x10^6 — LFV-V1b construct featuring CMV-driven co-expression of luciferase and GFP with blasticidin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V1b; Component Arrangement: CMV-RFP-T2A-BSD-P2A-Luc; Amount TU: 2x10^6 — LFV-V1b construct featuring CMV-driven co-expression of luciferase and RFP with blasticidin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V1a; Component Arrangement: EF1α-Luc-T2A-GFP-P2A-Puro; Amount TU: 2x10^6 — LFV-V1a construct featuring EF1α-driven co-expression of luciferase and GFP with puromycin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V1a; Component Arrangement: EF1α-Luc-T2A-RFP-P2A-BSD; Amount TU: 2x10^6 — LFV-V1a construct featuring EF1α-driven co-expression of luciferase and RFP with blasticidin resistance via T2A/P2A peptides; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V3; Component Arrangement: PGK-GFP-P2A-Luc; Amount TU: 2x10^6 — LFV-V3 construct featuring PGK-driven co-expression of luciferase and GFP via P2A peptide; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V3; Component Arrangement: PGK-RFP-P2A-Luc; Amount TU: 2x10^6 — LFV-V3 construct featuring PGK-driven co-expression of luciferase and RFP via P2A peptide; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V4; Component Arrangement: EF1α-Luc-P2A-GFP; Amount TU: 2x10^6 — LFV-V4 construct featuring EF1α-driven co-expression of luciferase and GFP via P2A peptide; supplied as 2x10^6 TU.
      • Vector Layout: LFV-V4; Component Arrangement: EF1α-Luc-P2A-RFP; Amount TU: 2x10^6 — LFV-V4 construct featuring EF1α-driven co-expression of luciferase and RFP via P2A peptide; supplied as 2x10^6 TU.
    • Lead time: typically ships in ~7 business days; timing may vary by selected option.
    • Storage: store at -80°C
    • Shipping: Ships on dry ice
    • Upon receipt: store at the recommended temperature as soon as possible; avoid repeated freeze–thaw cycles.
    • Sales terms and conditions: Please review prior to ordering.
    Options selector
    Catalog no. Vector Layout Selection Amount (TU)
    LFV-0001-01 CMV-Luc-GFP-Puro
    LFV-0001-02 CMV-Luc-RFP-Puro
    LFV-0001-03 CMV-Luc-GFP-BSD
    LFV-0001-04 CMV-Luc-RFP-BSD
    LFV-0001-05 CMV-GFP-Puro-Luc
    LFV-0001-06 CMV-RFP-Puro-Luc
    LFV-0001-07 CMV-GFP-BSD-Luc
    LFV-0001-08 CMV-RFP-BSD-Luc
    LFV-0001-09 EF1α-Luc-GFP-Puro
    LFV-0001-10 EF1α-Luc-RFP-BSD
    LFV-0001-11 PGK-GFP-P2A-Luc
    LFV-0001-12 PGK-RFP-P2A-Luc
    LFV-0001-13 EF1α-Luc-P2A-GFP
    LFV-0001-14 EF1α-Luc-P2A-RFP
    LFV-0001-16 CMV-GLuc-RFP-BSD
    LFV-0001-15 CMV-GLuc-GFP-Puro
    LFV-0001-18 CMV-GLuc-RFP-Puro
    LFV-0001-17 CMV-GLuc-GFP-BSD
    LFV-0001-19 CMV-rFLuc-RFP-BSD
    LFV-0001-20 CMV-GLuc-ZsG-BSD
    Field Specification
    Product Type
    • Lentiviral Vector
    • Dual Reporter Lentivirus
    Promoter CMV, CMV+PGK, EF1α, PGK
    Reporter GFP, RFP, Luc
    Selection Marker Blasticidin, N/A, Puromycin
    Shipping Ships on dry ice; store at -80°C

    Background

    Tracking the location, abundance, and behavior of defined cell populations is fundamental to cancer and immunology research. Bioluminescence imaging with luciferase enables sensitive, longitudinal monitoring of cell number in living animals, while fluorescent proteins allow single-cell identification by microscopy and flow cytometry. Combining both modalities in the same cell provides complementary readouts: luciferase for whole-body imaging of tumor growth and metastasis, and fluorescence for ex vivo histology, FACS-based isolation, and analysis of tumor-infiltrating immune cells. Stable, division-resistant labeling is essential for accurate longitudinal preclinical studies of tumor biology and the tumor microenvironment.

    Product Description & Applications

    The Fluorescence and Luciferase Dual Reporter Lentivirus constitutively co-expresses a luminescent reporter (firefly or secreted Gaussia luciferase) and a fluorescent protein (GFP or RFP) from a single transcript, using self-cleaving peptides for independent, equimolar protein production. Expression is driven by a CMV, PGK, or EF1α promoter, and a selection marker (puromycin or blasticidin) supports stable cell line generation. Stable integration ensures persistent dual-reporter expression, enabling longitudinal bioluminescence imaging of tumor growth and metastasis in vivo and parallel fluorescence-based identification, gating, or FACS sorting of tumor cells for flow cytometry, scRNA-seq, and proteomics. Multiple vector layouts optimize for stable line establishment or primary-cell labeling. Supplied as ultra-purified, high-titer lentiviral particles suitable for in vitro and in vivo use, including transduction of primary and cryopreserved cells.

    About This Product

    This lentivirus constitutively co-expresses a luciferase reporter and a fluorescent protein (GFP, RFP, Luc) from a strong CMV or EF1α promoter, using a self-cleaving P2A peptide to ensure equimolar, independent production of both reporters. A selection marker (Blasticidin, Puromycin) is co-encoded for stable cell line generation.

    The stable lentiviral integration ensures persistent, division-stable reporter expression in the target cell line, enabling longitudinal bioluminescence imaging (IVIS) of tumor burden in mouse models and parallel fluorescence-based readouts for ex vivo analysis. The dual-modality design provides built-in redundancy — luciferase for high-sensitivity whole-body imaging and fluorescence for histology, flow cytometry, and FACS — within a single stably engineered cell line.

    What is the difference between the fluorescent and luciferase reporters in this product?
    Is this product suitable for in vivo bioluminescence imaging?
    How do I establish a stable dual-reporter cell line?
    Which cancer cell lines and tumor models are most commonly used with this reporter?
    Can the two reporters be detected simultaneously without spectral overlap?

    Can't find the lentiviral construct you need, or want to adjust key design elements? Contact us to discuss custom LV design and optional add-ons.

    Common customization requests

    • Insert / payload: replace the gene/sequence, swap to a different isoform, add mutations, or optimize cloning features.
    • Expression design: change promoter (e.g., CMV/EF1α/PGK), add enhancers, or adjust regulatory elements.
    • Reporters: add/swap GFP/RFP/mCherry/luciferase (single or dual reporters where applicable).
    • Selection markers: add/swap puromycin/blasticidin/neomycin or fluorescent selection options.
    • Vector format: switch between OE, shRNA, CRISPR (sgRNA/Cas systems), or control vectors (where supported).

    Add-ons you can request

    • Control viruses: empty vector, non-targeting shRNA, reporter-only controls, or matched backbone controls.
    • Packaging / format: concentration options, aliquoting, or custom fill volume for screening workflows.
    • Documentation: construct map/sequence confirmation package (as available) and batch documentation.

    What to include in your request

    • Target cell type/model (cell line or primary cells) and intended readout (reporter, knockdown, OE, etc.)
    • Insert sequence (FASTA) or reference ID, plus any required tags/mutations
    • Promoter, reporter, and selection marker preferences
    • Desired scale and preferred format (aliquots / concentration requests)

    Email us at support@biohippo.com or use the Talk to a Scientist request form.

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