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30 Years of Bioluminescent Technology Innovations

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Celebrating 30 Years of Innovation and Discovery using Bioluminescent Technology

Bringing Luciferase from Nature to the Benchtop

The glowing tail of a firefly or the blue waves of the ocean are a first exposure to the wonder of bioluminescence in nature. This phenomenon was recognized as a powerful platform to develop biological assays by researchers in the early years of biochemistry and molecular biology. In 1991 Promega released our first luciferase assay products, starting a program of further innovations that now includes a wide assortment of different assays built through continued research and innovation of bioluminescent systems. Here we detail the progression of research methods through the years and the amazing scientific advances made by innovative scientists and the power of bioluminescence. 
Read Feature Article: Shining Light on Molecular Darkness
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Bioluminescence as a natural phenomenon is widely experienced with amazement and delight at the prospect of living organisms creating their own light.
Keith V. Wood, 1998.
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September 13th–16th

Explore the possibilities of bioluminescent tools and how they're applied to advance our understanding in important therapeutic areas such as Targeted Protein Degradation and Kinase Biology.

Register for Discover Glo

Research and Product Spotlight

Caspase-Glo® 3/7 Assay Systems

In addition to using the firefly luciferase reaction to measure the amount of luciferase or ATP in a sample, it is also possible to measure changes in substrate (luciferin) concentration. By coupling the reaction with pro-luciferin substrates containing protecting groups that can be reacted upon by different enzyme classes, sensitive add-and-read assays have been created to measure the activity of various proteases and metabolizing enzymes, where the amount of light produced is proportional to enzyme activity. The Caspase-Glo® 3/7 Assay System was an early example of this approach, allowing for a simple, sensitive method to detect cells undergoing apoptosis. The ability to easily measure apoptotic cell death has allowed oncology researchers to efficiently screen for and characterize potential therapeutic approaches that can lead to the removal of cancer cells. Recently, this approach has been further adapted to enable the measurement of apoptosis in 3D culture systems, allowing scientists to study induction of apoptosis in model systems that more accurately mimic tumor cell growth.

Read how a research team from Innsbruck, Austria used the Caspase-Glo® 3/7 Assay to characterize potential treatments for Neuroblastoma ›

Learn more about measuring apoptosis in 3D culture systems ›

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Dual-Luciferase® Assay System Spotlight
The Dual-Luciferase® Reporter Assay System (DLR) was the first reagent to integrate firefly and Renilla luciferases as co-reporters, allowing for sequential detection of two reporters from the same sample. In contrast to other dual-reporter options, the DLR™ assay and Renilla luciferase control provided researchers with a simple internal normalization method for firefly luciferase that offered the same speed, sensitivity, and linearity of detection for both the experimental and control reporters. The DLR™ assay also offered significant handling improvements since both reporters could be detected from the same sample with the add-read-add-read (“Stop & Glo”) assay format, removing the requirement to split lysates and detect the normalization reporter using a separate assay system. 
The DLR™ assay has been used over the last 20+ years to help researchers advance our understanding of the genomic elements that regulate gene expression and can be found in some of the foundational work done to understand important transcriptional regulators such as Hif1A (hypoxia response) and NF-kB (inflammation and immune response). The dual-luciferase® concept has evolved to include the Dual-Glo® Luciferase Assay System to provide more stable signals for both reporters and the Nano-Glo® Dual-Luciferase® Reporter Assay System that allows NanoLuc and firefly luciferases to be used as co-reporters. However, the DLR™ assay continues to be used in applications today in fields as far ranging as drug development to crop production to virology. See how scientists are applying DLR™ assay ›
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Read how Nobel laureate Gregg L. Semenza used dual-reporter assays to advance our understanding of hypoxic gene regulation.

Read About Semenza's Work
Luciferase Assay System (LAR) Spotlight

The Luciferase Assay System (LAR) was the first luciferase detection reagent introduced by Promega in 1991 along with the firefly luciferase, luc, reporter gene. The LAR assay still provides one of the brightest firefly luciferase detection solutions with flash signal kinetics that require injector delivery.  Over the last 30 years the LAR reagent has been used in thousands of research projects to advance our understanding of topics ranging from regulation of gene expression to functional analysis of genetic polymorphisms.  Today researchers are finding reagents like LAR to be critical tools in our efforts to identify vaccines and treatments for SARS-CoV-2 infection.

Learn more about Luciferase Assay System
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Blast from the Past

Read our first review and announcement about luciferase reporters in its original formfrom 1990.

View luciferase review and announcement PDF ›

Firefly Luciferase Reporter Vectors Spotlight
The first commercially available firefly luciferase (Fluc) reporter vectors  (pGL2) used the native firefly luciferase gene, luc, as the reporter providing a useful new tool for researchers. However, it became clear that further genetic engineering could improve the performance of this reporter system.  The next generation of FLuc reporter (pGL3) introduced a new gene, luc+, with mammalian codon optimization for improved reporter expression and improvements to the vector backbone to reduce background expression. These engineering steps increased luciferase activity by 20- to 100-fold over what could be achieved with the pGL2 system.  These performance improvements were taken even further with the pGL4 vector series which introduced the luc2 reporter gene. This round of improvements included further codon optimization, removal of cryptic regulatory sequences, and the introduction of destabilized luciferase genes to improve response rates. The pGL4 design created a reporter system that expresses uniformly and optimally in mammalian host cells;  minimizes off-target responses and responds rapidly to transcriptional dynamics, providing even more possibilities for cell biology research and high-throughput screening drug discovery applications.  

Firefly Luciferase Sheds Light on Development of New Malaria Treatments

Read About Harnessing the Power of Firefly Luciferase
Dr Paul Horrocks

See how Dr. Paul Horrocks uses a firefly luciferase-based system to understand the dynamics of drug action in the development of new malaria treatments.

Watch Case Study
Bright-Glo™ and Steady-Glo® Luciferase Assay Systems Spotlight

First generation luciferase detection assays have very bright but short-lived signal and require lysate generation prior to addition of assay reagents. Although extremely powerful, the short signal duration and upstream processing requirements present challenges to researchers using bioluminescent reporters in high-throughput analysis. The second generation “Glow” reagents such as the Bright-Glo™ and Steady-Glo® Assay Systems overcame these limitations by extending the kinetics of the firefly luciferase reaction (30 minute and 5-hour respective half-lives) while also providing a single-addition reagent that is added directly to cells in culture to lyse the cell and provide all of the assay components. These “add-mix-measure” assays significantly simplified sample processing and brought compatibility to microplate workflows allowing researchers to batch process 10s to 100s of plates at a time, expanding the use of luciferase reporter assays to high-throughput screening applications.

Learn more about the differences between Flash and Glow assays

Read how researchers use the Bright-Glo™ Assay in a drug repurposing screen to identify potential SARS-CoV-2 treatments

CellTiter-Glo® Luminescent Cell Viability Assays Spotlight

ATP is well recognized as an indicator of metabolically active cells, making the measurement of total ATP levels an important tool in determining the impact of compound treatment on cell viability. The CellTiter-Glo® Luminescent Cell Viability Assay uses the cell as source of the ATP in the luciferase reaction, producing a bioluminescent signal that is proportional to the number of viable cells in a well. Similar to other “Glow”-type luciferase assays, the luminescent signal has an extended half-life ( > 5hr), and the reagent can be added directly to cells in culture making it ideal for automated high-throughput cell proliferation and cytotoxicity assays. The assay has been further optimized to reduce preparation time and simplify repeat use in the CellTiter-Glo® 2.0 assay and has also been adapted to measuring cellular ATP in 3D model systems for determining cell viability in these more complex physiological models.

Learn more about bioluminescent ATP Assays

See how Dr. Samantha Llewellyn uses CellTiter-Glo® 3D to assess toxicity of in physiologically relevant 3D liver models.

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Shining Light On Scientists & Their Innovations

Episode 1: Kyle Hooper Pt. 1

Episode 5: Kyle Hooper Pt. 2

Episode 2: Brian Hurwitz

Episode 3: Luigi Scotto

Episode 4: Hai Li

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Bioluminescence Applications Guide

Want to learn how to use NanoLuc® Luciferace (NLuc) and NLuc-derived technologies as protein reporter tags to answer your research questions about protein abundance, localization, modification and interaction? Preview Chapter 3, NanoLuc® Luciferase as a Protein Reporter, from our Bioluminescence Applications Guide.

Download PDF

A Glo-ing History of Innovation and Discovery

Looking back at 30 years of bioluminescent discovery, innovation, and ground breaking research. 

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1991 Glowing Firefly

Luciferase Assay System

The first luciferase detection reagent introduced by Promega providing the beginning of sensitive, non-radioactive reporter gene assays. The LAR assay still provides one of the brightest firefly luciferase detection solutions with flash signal kinetics that require injector delivery. LAR along with the firefly luciferase (luc) reporter gene, provided some of the first tools that allowed researchers to begin mapping regulators of gene expression.

Read about Bioluminescent Reporter Genes
1995 Dual-Luciferase Technology Glowing

Dual-Luciferase® Reporter Assay System (DLR)

DLR was the first reagent that allowed for sequential detection of a second reporter in a single sample. It provided a key advancement in improving reporter assay reliability by allowing for internal normalization of luciferase activity.

See how Scientists are Applying Dual-Luciferase

pGL Luciferase Reporter Vector Series

The pGL3 family of reporter vectors featured a modified firefly luciferase gene, luc+. This early example of engineering a reporter for performance improvements was later taken further for the pGL4 and luc2 reporters with even great improvements possible through bioinformatics and synthesis.

pGL4 Luciferase Reporter Vectors Tool
1999 Image of CellTiter-Glo Assay Technology

ENLITEN®/Ultra-Glo™ Recombinant Luciferase

Promega offered a recombinant firefly luciferase (Enliten) early on, but through an early example of directed evolution, a thermostable luciferase was engineered, called Ultra-Glo. The development of Ultra-Glo was key to making one-step, add-and-read assays with a variety of assay and storage conditions.

ENLITEN® ATP Assay System

Bright-Glo™ (1999), Steady-Glo® (1998), Dual-Glo® (2001) Luciferase Assay Systems

Through the development of new ways to alter the signal kinetics of the firefly luciferase assay, Bright-Glo, Steady-Glo, and Dual-Glo allowed use of microtiter plates for assays. The add-and-read format simplified sample processing and allowed use of reporter gene assays in very high-throughput applications.

Find the Best Reporter Assay

CellTiter-Glo® Cell Viability Assay

With the development of UltraGlo luciferase, it was now possible to make an add-and-read ATP detection assay. ATP has been found to be a key indicator of cell health, making CellTiter-Glo a powerful assay for assessing cell viability especially in higher-throughput applications. The assay principle also lead to other platforms that measure ATP, notably Kinase-Glo (2004) and ADP-Glo (2009) enzyme assays used to study ATPases such as kinases.

See How CellTiter-Glo is being used in COVD-19 Research
2003 Caspase-Glo Assay Technology Example

Caspase-Glo® 3/7 Assay

In addition to measuring the amount of luciferase or ATP in a sample using the firefly luciferase reaction, it is possible to measure changes in substrate (luciferin) concentration. By coupling luciferin with protecting groups that can be reacted upon by different enzyme classes, sensitive, add-and-read assays are possible for these enymes. Examples include Caspases and other proteases, and Cytochrome P450s.

Using Caspase-Glo® Assay in Cancer Research Explore Caspase-Glo®
2007 Glowing Fireflies in Field

ONE-Glo™ Luciferase Assay System

With further understanding of the firefly luciferase reaction chemistry and a team of biologists and chemists at Promega, an improved luciferin was created to be better suited for use in typical reporter gene assay applications. This new substrate, fluoroluciferin, is an early example of novel substrate development.

Pseudotyped Viral Particles and Luciferase Discover ONE-Glo™
2012 NanoLuc Technology Application Glowing

NanoLuc® Luciferase

Experience in directed evolution and development of novel substrates came together to design a new luciferase reporter. system Adapted from a shrimp luciferase, the new NanoLuc luciferase was developed to be a small (19kDa) monomer with a unique substrate that offers approximately 100x great sensitivity than the already highly sensitive firefly or Renilla luciferase systems. This novel reporter would be used in many applications and serve as the basis for further technological development.

Researchers use NanoLuc Luciferase to Create Models of Cardiovascular Disease
2015 NanoBRET Glowing 3D Technology Image

NanoBRET™ Technology

The efforts to develop NanoLuc luciferase resulted in a versatile platform for further developments. The small size and very bright light output from NanoLuc was recognized to offer ideal characteristics as a protein tag. These traits also serve well as a donor for Bioluminescence Resonance Energy Transfer (BRET). A thorough study of a variety of energy-accepting fluorophores found options in the red spectrum that helped eliminate some of the challenges associated with BRET measurements. These fluorophores could be added to molecules such as protein ligands to measure engagement of a target protein or configured as HaloTag ligands to allow detection of protein:protein interactions in live cells.

Using NanoBRET to Better Understand the Kinome
2016 NanoBiT Glowing 3D Technology Image

NanoBiT® Technology

With the successful design of NanoLuc, scientists at Promega then endeavored to configure this reporter into a multi-subunit system. The resulting system, termed "NanoLuc Binary Technology" or NanoBiT, is a two part system consisting of an 11 amino acid small tag and a larger, further refined subunit of NanoLuc, LgBiT. Structurally complementation of both parts reconstitutes a bright luciferase enzyme. Affinity of the these subunits can be low as with SmBiT peptide, allowing for creation of protein interaction assays. Or it can be high, as with HiBiT, allowing for self assembly. HiBiT serves as an easily detected, highly sensitive protein tag that, when used with CRIPSR-based tagging, allows for the creation of endogenous reporter models.

Adapting NanoBiT to a Biochemical Assay Format
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Lumit™ Technology

Following on the development of NanoBiT technology, it was recognized that this system could be used to detect a wide variety of analytes through conjugation of components of immunoassays. The resulting platform, now called "Lumit", offers simplified immunoassays with high sensitivity.

Explore Lumit™ Technology
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Present, Meet the Past

The Turner TD-20/20 was one of the first luminometers to offer dual-injectors. This made it a useful instrument for performing the Dual-Luciferase Assay.

If you think this is cool, check out the tool that aided Promega's early bioluminescent protein research.

Read About the Spectrometer From Space

Helping Researchers Analyze Luminescence and Fluorescence Data

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A high performance luminometer captures the full performance of bioluminescence assays. 
Explore Our GloMax Solutions
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Want to learn more about measuring and optimizing bioluminescent assays?

Preview Chapter 8, Measuring Bioluminescent Assays with a Plate Reader, from our Bioluminescence Applications Guide.

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