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VIABILITY PCR

Rapid & Sensitive Detection of Viable Microbes

Dead cell-specific dyes covalently modify DNA, allowing selective PCR amplification from live cells
PMAxx™ is our newest v-PCR dye, with improved live/dead discrimination compared to our original PMA
Easily get started with viability PCR, with any cell type
Improve PMA & PMAxx™ modification of dead gram-negative bacteria
PMA-Lite™ 2.0 LED Photolysis Device for sample tubes
Everything you need for v-PCR of common strains

A Powerful PCR-Based Method for Analyzing Microbial Viability


Introduction to Viability PCR (v-PCR)

Reliable detection of living microbes and viruses is of widespread interest across numerous sectors including basic research, food safety, agriculture, and public health. However, traditional methods of measuring microbial viability rely on time-consuming culturing, colony counting, or microscopic observation. In addition, certain organisms cannot be cultured with current technology. Consequently, these viable but non-culturable (VBNC) species require molecular measures of viability. Viability PCR (v-PCR) is a reliable and culture-free method that offers sensitive and rapid detection of viable microorganisms. Since 2006, Biotium has pioneered the field of v-PCR with the development of PMA (Propidium Monoazide) and the improved PMAxx™ v-PCR dye. These photoreactive, membrane-impermeant, DNA binding dyes offer superior dead cell selectivity over traditional culture-based methods and the previous EMA (Ethidium Monoazide) v-PCR dye.

Advantages of v-PCR with PMA & PMAxx™

  • Sensitive and rapid viability analysis without time-consuming culturing, microscopy, or colony counting
  • Allows strain-specific viability analysis
  • Validated and published for dozens of bacteria, fungi and viral species
  • Compatible with Next-Generation Sequencing applications
  • Suitable for complex sample types including soil, feces, water/wastewater, biological specimens, and food

An Industry Leader in v-PCR

PMA is the v-PCR dye of choice among industry leaders, and has been validated in hundreds of peer-reviewed publications and numerous strains of bacteria, fungi, and viruses. Early studies focused on v-PCR in bacteria, validating the procedure in dozens of different bacterial strains such as E. coli, Listeria, Legionella, Lactobacillus, M. tuberculosis, Chlamydia, H. pylori, and many other strains with relevance to human health. v-PCR has been most widely used in bacteria, but there are also dozens of publications using v-PCR in yeast and fungi, viruses, as well as a variety of other cell types such as archaea, amoeba, and parasites.

Published Applications for Viability PCR

  • Microbiome Studies
  • Environmental Testing
  • Probiotic Research
  • Clinical Testing
  • Food & Water Sanitation
  • Wine Fermentation
  • Microbial Sequencing

 

 

Measuring Bacterial Viability in Environmental Samples?

Sign up to our e-newsletter to download our Literature Digest: Monitoring Viable Bacteria in the Environment with PMA & PMAxx™.

In this digest we have provided summaries and takeaways for three publications on the use of v-PCR with PMA and PMAxx™ for monitoring bacterial viability in samples taken from wastewater, fresh water, and drinking water treatment plants.

Looking to Study Viral Integrity with PMA or PMAxx™?

v-PCR is a proven method for monitoring capsid integrity for dozens of viral strains, including SARS-CoV-2.

The figure below displays the genus and strain number of viruses investigated for using v-PCR to monitor capsid integrity in peer-reviewed studies in the last decade (2009 to 2021) in the fields of food safety and environmental virology.

Genus and strain number of viruses investigated for employing capsid integrity qPCR in peer-reviewed studies in the last decade (2009 to 2021) in the fields of food safety and environmental virology (number of peer-reviewed studies in parentheses). In cases where no strain name was listed, the virus is referred to as ‘not specified’. Adapted from: M. Leifels, et al. https://doi.org/10.1016/j.wroa.2020.100080 reproduced under the Creative Commons license.

Sign up to our e-newsletter to download our Literature Digest: Viral Integrity with PMA & PMAxx™.

In this digest, we have selected three publications with summaries and takeaways on the use of PMA or PMAxx™ combined with qPCR  for sensitive, accurate, and rapid detection of intact viral capsids.

How v-PCR works

The infographic below shows the basic mechanism of v-PCR. PMAxx™ and PMA are photoreactive dyes with high affinity for DNA. The dyes intercalate into dsDNA and form a covalent linkage upon exposure to intense visible light. The reaction inhibits PCR amplification of modified DNA templates by a combination of removal of modified DNA during purification and inhibition of template amplification by DNA polymerases. Because the dyes are cell membrane-impermeable, when a sample containing both live and dead bacteria is treated with dye, only dead bacteria with compromised cell membranes are susceptible to DNA modification. In a qPCR reaction, dead cell DNA will show delayed amplification and higher Ct than live cells.

Viability PCR dyes like PMAxx™ or PMA are membrane-impermeant, which makes them dead cell specific. Once inside of a dead cell, they bind to DNA. Exposure to intense visible light renders the dyes reactive, and causes them to covalently attach to the DNA. This DNA modification prevents amplification in subsequent PCR reactions.

v-PCR Workflow

The basic workflow for v-PCR is shown in the infographic below (detailed protocols can be found on product pages). It is adaptable for many different sample types and experimental set-ups. For a small number of cultures, the samples can be prepared in microcentrifuge tubes, and exposed to light in the PMA-Lite™ 2.0 LED Photolysis Device (See lower on this page for more information).

Workflow Modifications

Many publications have used modifications of the basic protocol for specialty applications. For example, for large, dilute volumes, samples can be filtered onto a membrane, followed by dye treatment and photolysis on the membrane itself. Opaque, complex samples such as soil or feces generally need a higher dye concentration and longer light exposure; sample dilution can also help. And some users choose to perform qPCR directly on bacterial lysates, instead of purifying the DNA first.

The basic v-PCR workflow involves the following 5 steps: dye addition, incubation, light exposure, DNA extraction, and qPCR.
PMAxx technology is covered by granted and/or pending US and international patents.

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PMA & PMAXX™: THE INDUSTRY STANDARD FOR VIABILITY PCR


PMA is validated in hundreds of journal articles for a wide variety of strains

Since Biotium first developed PMA, there have been hundreds of publications on the use of the dye in many sample types including dozens of bacterial strains, biofilms, yeast, fungi, viruses, and eukaryotic cells. It has been used in such applications as food and water safety and environmental testing, and has been used in conjunction with qPCR, NextGen Sequencing (NGS), Sanger sequencing, and Loop-mediated Isothermal Amplification (LAMP).

PMAxx™ is a superior alternative to PMA

While PMA is generally effective at differentiating between live and dead bacteria by qPCR, it does not completely eliminate PCR products from dead cell DNA. This could potentially give false positive results. PMAxx™ was designed by Biotium scientists to be a superior alternative to PMA. PMAxx™ is much more effective at eliminating PCR amplification of dead cell DNA, and therefore provides the best discrimination between live and dead bacteria. Learn more about viability PCR with PMA and PMAxx™ with links to our flyer and our full list of references below.

 

Live or dead bacteria treated with either PMA or PMAxx™ prior to qPCR. Dead bacteria treated with either PMA or PMAxx™ show delays in amplification compared to either live cells, or untreated dead cells. Bacteria treated with PMAxx™ show a larger delay than those treated with PMA. Therefore PMAxx™ is better able to differentiate live vs dead bacteria by viability PCR.
Product Name Catalog No. Features
PMAxx™, 20 mM in H2O 40069 •    Next-generation v-PCR dye
•    Gives the best live/dead discrimination
PMA Dye 40013 •    Original v-PCR dye developed at Biotium
•    Validated in hundreds of publications and a wide variety of organisms
PMA Dye, 20 mM in H2O 40019

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STARTER KITS FOR V-PCR


The customizable Viability PCR Starter Kits contain the materials that you need for selective detection of viable cells using either PMA or PMAxx™ viability dye and qPCR. These kits can be used with any cell type of your choosing (see the PMA/PMAxx™ Reference List and Validated Bacterial Strains List for published validated cell types). All of the kits contain Forget-Me-Not™ EvaGreen® qPCR Master Mix, and your choice of PMA or PMAxx™ dye. You also have the choice of selecting a kit with or without the Enhancer for Gram Negative Bacteria (not to be used with other cell types). The user will need to supply their own primers to amplify their species of interest (see this blog post for primer design considerations). Each kit contains reagents sufficient to treat 80 bacterial cultures and perform 200 PCR reactions.

Kits include:

• PMA dye OR PMAxx™ dye
• Forget-Me-Not™ EvaGreen® qPCR Master Mix
• ROX reference dye
• PMA Enhancer (gram-negative strains only)

Not included but required:

• primers to amplify your cell type of interest
• DNA extraction kit or reagents


Product Name Catalog No. Viability Dye Target Cell Type
Viability PCR Starter Kit with PMA 31075 PMA Any cells
Viability PCR Starter Kit with PMAxx™ 31075-X PMAxx™ Any cells
Viability PCR Starter Kit with PMA and Enhancer 31076 PMA Gram-negative bacteria
Viability PCR Starter Kit with PMAxx™ and Enhancer 31076-X PMAxx™ Gram-negative bacteria

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PMA ENHANCER FOR GRAM-NEGATIVE BACTERIA


PMA Enhancer for Gram Negative Bacteria was designed to improve discrimination between live and dead gram-negative bacteria during viability PCR. PMA Enhancer is provided as a 5X solution, and is added to a sample before the addition of viability dye. When a sequence from a gram-negative bacteria is amplified by PCR, samples pre-treated with Enhancer show a decrease in the signal from dead cells, with no change in the signal from live cells. PMA Enhancer is compatible with PMAxx™ as well as PMA. PMAxx™ plus Enhancer is the optimal way to perform viability PCR on gram-negative bacteria. PMA Enhancer is available as a stand-alone product, and is also a component of our PMA Bacterial Viability Kits (gram-negative strains only) (see below).

The mechanism by which Enhancer improves live/dead discrimination has not been determined. It may improve passive permeability of dead cell walls or membranes to the dye, and/or improve access of the dye to the dead cell DNA.

E. coli were killed with mild heat treatment (56°C for 3 hrs) and treated with PMAxx™ or PMAxx™ + Enhancer, followed by light exposure using PMA-Lite™, DNA purification, and qPCR with Fast EvaGreen® qPCR Master Mix. dCt values were calculated by subtracting the Ct without dye from the Ct with dye. Only dead cells treated with PMAxx™ + Enhancer showed a large dCt, indicating that the dye successfully inhibited PCR of dead cell DNA.

PMA Enhancer for Gram-Negative Bacteria

Product Name Catalog No. Features
PMA Enhancer for Gram Negative Bacteria, 5X Solution 31038 •    Improves live/dead discrimination in gram-negative strains

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PHOTOACTIVATION DEVICE


PMA-Lite™ 2.0 LED Photolysis Device

The PMA-Lite™ 2.0 LED Photolysis Device allows for time- and temperature-controlled light treatment of PMAxx™- or PMA-treated samples in microcentrifuge tubes. It is designed as an improved version over the previous PMA-Lite™ LED Photolysis Device by including an intuitive touch screen for programming and monitoring, in addition to offering more flexibility for photoactivation durations.

PMA-Lite™ 2.0 Features:

  • Provides even illumination to up to 18 microcentrifuge tubes
  • Internal fan keeps temperature < 37°C
  • Timer for 5-45 minutes of photoactivation
  • Long-lasting LED lights with 465-475 nm emission
  • Best results are achieved with PMAxx™ dye
PMA-Lite™ 2.0 LED Photolysis Device
PMA-Lite™ 2.0 LED Photolysis Device

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STRAIN-SPECIFIC V-PCR KITS


Strain-specific v-PCR kits are designed for selective detection of viable bacteria from a specific strain using PMAxx™ or PMA dye and real-time PCR. The kits contain PMA dye OR PMAxx™ dye, Forget-Me-Not™ EvaGreen® qPCR Master Mix, and validated PCR primers for detection of selected strains of bacteria that are of widespread interest to food safety, public health, and/or antibacterial research.

Don’t see your favorite bug? Let us know at techsupport@biotium.com

Kits include:

• PMA dye OR PMAxx™ dye
• Forget-Me-Not™ EvaGreen® qPCR Master Mix
• ROX reference dye
• PMA Enhancer (gram-negative strains only)
• Validated PCR primers for specific bacterial strain

PMA Real-Time PCR Bacterial Viability Kits are available for:

Salmonella enterica
Mycobacterium tuberculosis
Staphylococcus aureus
Staphylococcus aureus (methicillin-resistant)
Listeria monocytogenes
E. coli
E. coli O157:H7
Legionella pneumophila

Strain-Specific Bacterial Viability PCR Kits

Bacteria Strain Gene name Kit with PMA (catalog #) Kit with PMAxx™ (catalog #)
Salmonella enterica invA 31033 31033-X
Mycobacterium tuberculosis groEL2 31034 N/A
Staphylococcus aureus nuc 31035 N/A
MRSA mecA 31036 N/A
E. coli O157:H7 Z3276 31037 31037-X
E. coli uidA 31050 31050-X
Listeria monocytogenes hly 31051 31051-X
Legionella pneumophila mip 31053 N/A

 

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PMA Enhancer for Gram Negative Bacteria, 5X Solution

From: $92 Sizes: 16 mLCatalog #: 31038

PMA Real-Time PCR Bacterial Viability Kit – Listeria monocytogenes (hly)

From: $393 Sizes: 200 assaysCatalog #:
31051
, - 31051-XView allHide

PMAxx™ Dye, 20 mM in H2O

From: $159 Sizes: 100 uLCatalog #: 40069

PMA Real-Time PCR Bacterial Viability Kit – E. coli O157:H7 (Z3276)

From: $426 Sizes: 200 assaysCatalog #:
31037
, - 31037-XView allHide

PMA-Lite™ 2.0 LED Photolysis Device

From: $2,429 Sizes: EachCatalog #: E90006