QuantiGene Plex Gene Expression Assay

The QuantiGene Plex Gene Expression Assay is a hybridization-based assay using xMAP Luminex beads and performed in 96- or 384-well plates. The assay is based on direct quantification of the RNA targets for multiplexing of 3 to 80 RNA targets and branched DNA (bDNA) signal amplification technology. On the first day the sample is lysed to release the RNAs and incubated overnight with target specific probe sets and Luminex capture beads. On the second day the signal amplification tree is built via sequential hybridization of Pre-amplifier, Amplifier, and Label Probe. Each amplification unit provides a 400x signal amplification and there are six amplification units per target RNA copy resulting in a 2,400x signal amplification per copy RNA. The signal is detected by using the fluorescent reporter molecule, phycoerythrin, on a Luminex instrument for readout and analysis.

The QuantiGene Plex 384-well assay format enables multiplex gene expression analysis in a high throughput format. The assay uses target-specific probes to capture the RNA of interest and branched DNA technology to amplify fluorescent signals which are read with the FLEXMAP 3D, Luminex platform. Automation and batch processing options for this assay format increase sample throughput and decrease hands-on time while allowing for fast time to results for screening projects.

The QuantiGene Plex 384-well Assay Kit (Cat. No. QP1016) contains all the necessary reagents, buffers, and plates to perform QuantiGene Plex assays in 384-well plates. Design your target-specific QuantiGene Plex panel with our Panel Configuration Tool or contact your local Technical Sales Specialist for more information.
 

The QuantiGene Plex 384-well assay is designed to increase sample throughput and decrease hands-on time while allowing for fast time to results for screening projects. Below is example data that was generated using the 384-well format using the recommended equipment listed below.

Stimulation of cytokine production in HeLa cells
Cytokine production in cultured HeLa cells was stimulated using a Cell Stimulation Cocktail and monitored for various time points up to 24 hours. In this experiment, a full 80-plex panel was used for screening purposes focused on cytokine, and chemokine biomarkers.

The normalized gene expression of various targets in HeLa cells at different time points post stimulation with a Cell Stimulation cocktail reveals the degree of up- or downregulation. The average normalized expression (y-axis) represents the level of gene induction for the mRNA targets listed on the x-axis, while the time points of stimulation are shown on the z-axis. Of note, for example IL1B, IL8 and TGFB1 show pronounced relative gene expression at various time points of stimulation. While TGFB1 relative expression seems to gradually increase over time, peak expression for IL1B is seen at later time points around 24h. Table 1 shows normalized gene expression and fold change of various targets in HeLa cells at different time points post stimulation with a Cell Stimulation cocktail.

Table 1 and 2. Normalized gene expression and fold change of various targets in HeLa cells at different time points post stimulation with a Cell Stimulation cocktail. 

1. Danahay et. al. (2015) Notch2 Is Required for Inflammatory Cytokine-Driven Goblet Cell Metaplasia in the Lung. Cell Reports 10:239-252.
2. Ferrer et al. (2014) A multiplex high-throughput gene expression assay to simultaneously detect disease and functional markers in induced pluripotent stem cell-derived retinal pigment epithelium. Stem Cells Transl Med 2:911-922.
3. Severyn et al. (2016) Development of a High-Throughput Gene Expression Screen for Modulators of RAS-MAPK Signaling in a Mutant RAS Cellular Context. J Biomol screen 9:989-997.
4. Neilsen et al. (2020) High-throughput identification of protein functional similarities using a gene-expression-based siRNA screen. Sci Data 7:27.
    

Find instrumentation and equipment to make every step of your QuantiGene Plex 384-well workflow easy. For detailed options and recommendations for batch processing, refer to the QuantiGene Plex 384-well manual or contact your local Technical Sales Specialist.

Workflow step	Recommended equipment		Description
Sample incubation and target hybridization	Temperature regulated orbital shaker: MaxQ 4450 Benchtop Orbital Shakers		Versatile shaker ideal for incubating a small number of vessels and cell culture and many other applications.
Plate washes	Magnetic microplate washers		Automated magnetic microplate washer for 384-well plates.
Sample incubation	Plate sealer: ALPS 50 V-Manual Heat Sealer		Applies consistent, secure, tight seals around individual wells, eliminating sample loss through evaporation and cross contamination between wells.
Sample and plate additions	Versette Automated Liquid Handler		Compact liquid handler featuring user-friendly programming, reliable performance, and a choice of 96- or 384-channel pipetting heads.
Multiplex detection	Luminex FLEXMAP 3D Instrument System		Most advanced and multifunctional multiplex unit for simultaneous measurement of up to 80 tests in a single reaction volume.

1. What sample types are compatible with QuantiGene Plex assay?
   Whole blood, fresh tissue, cultured cells, and purified RNA are validated. Other sample types including Tempus blood, bacteria, H&E stained/unstained FFPE, and blood spots should also be applicable.
2. What data analysis software solutions are offered for the QuantiGene Plex assay?
   Analyze data using the QuantiGene cloud-based application from any computer, anywhere. For advanced analysis and visualize, data can be analyzed using the free desktop application software, Applied Biosystems Transcriptome Analysis Console (TAC) software.
3. Can the VorTemp™ 56 Shaking Incubator be used for hybridization?
   We highly recommend the MaxQ Shaking incubator for optimal assay performance. It is possible to use the Vortemp, but 800 rpm is recommended.
4. What is the recommended temperature for hybridization?
   The Day 1 temperature is 54°C while the Day 2 temperature is 50°C. Please use Quantigene Incubator Temperature Validation Kit (QS0517) to verify the incubator temperature.
5. What are the proper storage conditions for the QuantiGene Plex reagents?
   When the kit arrives, please follow the instructions to store individual components. The Preamp/Amp/LP Diluent, Bead Mix, SAPE, SAPE Diluent should be stored at 4°C, while probe set mix, Proteinase K, and blocking reagent should be stored at -20°C. Others are stored at room temperature. Refer to the product insert for details.
6. What reagents are included in the kit?
   The kit provides all necessary reagents to perform the assay except Target Probe and Bead mix which are ordered separately. See the user manual for a list of the reagents.
7. Can QuantiGene Plex 384-well assays be used for miRNA or DNA analysis?
   No. We have options with the QuantiGene Singleplex assay for miRNA and DNA.
8. Should any control/housekeeping genes be used in my panel
   Three or more control/housekeeping genes are recommended to normalize the gene expression results.
9. Can I use a heat sealer to seal the plate on day 2 of the assay
   No, manual sealing using the provided seal is recommended. Heat sealing would deform the plate causing problem in washing.
10. How do I dilute my samples?
    For cell lysate or blood lysate, please use Diluted Lysis Mix (DLM); for tissue homogenates, please use Homogenizing Solution.
11. How should I seal the Day 1 plate for Target Probe hybridization?
    The Day 1 plate can be sealed either manually or using a heat sealer. The pressure seal for manual sealing and the heat seal AB-0757 for Thermo Fisher ALPS 50 V (AB-1443A) are provided in the kit. If a different heat sealer will be used, please consult the manufacturer for suitable sealing.

• Factors affecting blood gene expression
• Defining a QuantiGene Plex panel

User manuals for use with assay kits QP1013, QP1014, QP1015 and QP1016

• QuantiGene Plex manual 3-64 plex and 65-80 plex assays
• QuantiGene Plex 384-well assays

QuantiGene sample processing

• Preparation of bacterial homogenates for use in QuantiGene Assays
• Cultured cells
• Fresh/frozen animal or plant tissues
• Blood samples
• FFPE tissue samples
• QuantiGene incubator temperature validation kit
• IKA plate shaker

• QuantiGene Application Guide
• New determination of gene signatures to subgroup melanoma patients using novel branched DNA hybridization assays
• Transcript regulation of 18 ADME genes by prototypical inducers in human hepatocytes using QuantiGene Plex Assays