pRL-Luc Adenovirus (Ad-pRL-Luc)

SKU:BHV21600320
Overview
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Replication-defective Ad5 adenovirus encoding Luc under the pRL promoter. Commonly used in cell biology for transduction-efficiency benchmarking and reporter assays.
Transgene Luc
Promoter pRL
Reporter/Tag RLuc
Plasmid Backbone Human Adenovirus Type5 (dE1/E3)
Application Reporter assay
Available Options

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

  • Options: Titer: 1x10^10 PFU/ml; Volume: 200 µL.
  • Lead time: in stock; ships within 1–2 business days. Custom production typically requires 4–6 weeks.
  • Storage: -80°C.
  • Shipping: cold-chain shipment (typically with dry ice or ice packs).
  • Upon receipt: store at −80 °C as soon as possible; aliquot before first use to minimize freeze-thaw cycles (≤ 3 cycles for quantitative work).
  • Sales terms and conditions: Please review prior to ordering.
Options selector
Catalog no. Titer Volume
1671 1x10^10 PFU/ml
Field Specification
Form Liquid
Function
  • Adenovirus
  • Over-Expression
  • Luciferase Reporters
Plasmid Backbone Human Adenovirus Type5 (dE1/E3)
Product Type
  • Vectors & Viruses
  • Adenovirus
Production System
  • HEK293 (E1-complementing helper)
Promoter pRL
Reporter RLuc
Storage -80°C

Overview

Ad-pRL-Luc is a replication-defective recombinant Ad5 adenovirus expressing the Luc reporter gene under the pRL promoter. Reporter adenoviruses are commonly used to benchmark transduction efficiency, titrate MOI in new cell or animal models, and as transduction-load controls for paired over-expression vectors.

Key elements and design rationale

  • Backbone: Human adenovirus type 5 (Ad5) with E1 and E3 deleted (dE1/E3). Replication-incompetent in standard cells; replication-competent helper cells (HEK293) are required for amplification.
  • Promoter (pRL): the promoter governs cell-type and strength of expression.
  • Transgene: Luc (RLuc tag).
  • Titer & format: 1×1010 PFU/ml in storage buffer (DMEM, 2% BSA, 2.5% glycerol or equivalent), supplied as a 200 µL aliquot.

Biological background

In this recombinant adenovirus, the Renilla Luciferase (RLuc) is under the control SV40 early promoter/enhancer (derived from pRL-SV40 vector).

Research relevance and current trends

  • Decision-relevant for researchers studying Reporter Vectors.
  • Adenovirus-mediated delivery is well-established in primary cells, organoids, and small-animal models.

Common research applications

  • Transduction-efficiency benchmarking in new cell lines or animal models.
  • MOI titration as a positive control before switching to a transgene of interest.
  • Promoter-activity readout for transcriptional studies.

Notes for experimental interpretation

  • Adenoviral delivery is episomal and non-integrating; expression dilutes with cell division and typically lasts 1–2 weeks in dividing cells (longer in non-dividing cells such as hepatocytes, neurons, and cardiomyocytes).
  • Pre-existing anti-Ad5 neutralizing antibodies are common in human and primate hosts and can reduce in vivo transduction; this is less relevant in inbred laboratory mouse strains.
  • MOI optimization is essential — over-dosing can cause cytopathic effects; under-dosing yields incomplete transduction. A 3–5× MOI titration in your specific cell or animal model is recommended.
  • Replication-defective Ad5 vectors are typically handled at BSL-2; consult your institutional biosafety officer for specific transgenes and routes of use.

The Adenovirus Genome

The adenovirus genome is a linear double-stranded DNA molecule of 26–46 kb that encodes 23–46 proteins (Figure 1). These genes are split into two functional categories:

  • Early genes (E1–E4): encode proteins involved in viral transcription, viral DNA replication, and suppression of the host immune response.
  • Late genes (L1–L5): encode viral capsid components and proteins required for capsid assembly.

These genes are flanked by inverted terminal repeats (ITRs) that initiate viral DNA replication and serve as binding sites for transcription factors.

Schematic of the linear double-stranded DNA adenovirus type 5 genome showing early genes E1 through E4 and late genes L1 through L5 flanked by inverted terminal repeats.
Figure 1. The adenovirus genome. Early genes (E1–E4) and late genes (L1–L5) are shown on the adenovirus type 5 genome.

Adenovirus Capsid and Serotypes

The adenovirus capsid is a non-enveloped icosahedral protein shell of approximately 70–90 nm in diameter, built from three major capsid proteins — hexon, penton base, and fiber — together with the minor proteins IIIa, VI, VIII, and IX (Figure 5). The 240 hexon trimers form the 20 triangular facets of the icosahedron, while 12 penton complexes occupy each vertex; each penton consists of a penton base anchored in the capsid and a trimeric fiber projecting outward. The fiber knob mediates initial attachment to host cell receptors, and the penton base then engages cellular integrins to drive internalization.

More than 50 human adenovirus serotypes have been characterized and are organized into seven species (A–G) based on hemagglutination, sequence homology, and receptor usage. Serotype determines tropism and primary receptor:

  • Species C (e.g., Ad2, Ad5): bind the coxsackievirus and adenovirus receptor (CAR); broad tropism with strong transduction of liver and many epithelial cell types. Ad5 is the most widely used backbone in research and gene-delivery applications.
  • Species B (e.g., Ad3, Ad11, Ad35): use CD46 as the primary receptor, giving access to cell types that express low levels of CAR.
  • Species D: several members use sialic acid; some serotypes are associated with ocular tropism.

The replication-defective recombinant adenoviruses used as research vectors are typically derived from Ad5, with E1 (and often E3) deleted to render the virus non-replicative and to create space for transgene insertion.

Diagram of the icosahedral adenovirus capsid showing hexon trimers forming the facets, penton bases at the vertices, and trimeric fibers projecting outward with terminal knob domains.
Figure 5. Adenovirus capsid structure.
What is this product?

Ad-pRL-Luc is a replication-defective recombinant Ad5 expressing the Luc reporter gene under the pRL promoter. Reporter adenoviruses are commonly used for transduction-efficiency benchmarking, MOI titration in new cell lines or animal models, and as transduction-load controls for paired over-expression vectors.

How should I store and handle the virus?

Stocks are supplied at 1×1010 PFU/ml in storage buffer (typically 10 mM Tris pH 8.0, 2 mM MgCl2, 4% sucrose or similar). Store at −80 °C upon receipt, and aliquot before first use to minimize freeze-thaw cycles — recombinant adenovirus loses ~10–20% of infectious titer per freeze-thaw and should be limited to ≤3 cycles for quantitative work. Thaw on ice and dilute into pre-warmed culture medium immediately before infection.

Biosafety: Replication-defective Ad5 vectors are typically handled at BSL-2; consult your institutional biosafety officer for the specific transgene and route of use.

What MOI should I start with?

Optimal MOI varies by cell type, but useful starting ranges are:

  • Most cell lines (HEK293, HeLa, U2OS, HepG2, etc.): MOI 10–100
  • Primary cells (hepatocytes, cardiomyocytes, fibroblasts): MOI 50–500
  • Resistant or low-CAR cells (some lymphocytes, hematopoietic): MOI 500–2000 (may give limited transduction; consider Ad5/35 fiber modification if available)

Worked example. To infect 1×106 cells at MOI 100 from a 1×1010 PFU/ml stock: PFU needed = 100 × 106 = 1×108 PFU; volume needed = 10 µl of stock. Always run a 3–5× MOI titration in your specific cell model to identify the dose that gives near-100% transduction without cytopathic effect.

When can I expect expression / activity?

Transgene expression is typically detectable within 24 hours post-infection, peaks at 48–72 hours, and remains elevated for 1–2 weeks in dividing cells (the episomal Ad genome dilutes with cell division). In non-dividing cells (hepatocytes, neurons, cardiomyocytes), expression can persist for several weeks. Plan endpoint assays around the 48–72 hour window for peak expression.

What controls should I run?

For experiments using this reporter to quantify transduction:

  • Mock-infected cells — baseline autofluorescence / background signal.
  • Ad-CMV-Null or Ad-Blank — capsid/dose control matching for non-specific viral effects.
  • Untransduced cells — for separating transduction effects from any culture-condition effects.

Can't find the adenovirus you need—or require a custom design and packaging service? We offer end-to-end adenoviral support for diverse research needs, including vector design and cloning, adenovirus construction for over-expression (from your plasmid, sequence, or RefSeq#), shRNA-silencing adenoviruses (from a working shRNA or via shRNA screening when you only have the target gene), and gRNA adenoviruses (from a gRNA cassette or sequence). Custom plasmid construction typically takes ~2 weeks, with viral packaging, purification, and QC adding another 2–4 weeks. Final stocks are CsCl-purified and PFU-titered, with deliverables of approximately 1×1012 viral particles (1×1010–1×1011 PFU). We also provide amplification and CsCl purification services at medium scale (~1×1010–5×1010 PFU/IFU in 2 mL, ~2 weeks; ideal for in vitro studies) and large scale (5×1012–1×1013 viral particles / 1–3×1011 PFU, ~2–3 weeks; ideal for in vivo studies) — including amplification of customer-supplied viral stocks. Click Talk to a Scientist to submit a request, email us at support@biohippo.com, or explore our Research Services for additional support. Our team will be in contact with you shortly.

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