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Suveillance of antibiotic resistance in urban wastewater treatment plants Blog: surveying antibiotic resistance in wastewater
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Suveillance of antibiotic resistance in urban wastewater treatment plants Blog: surveying antibiotic resistance in wastewater
Tech Note

An effective method to track disease outbreaks and spread of antibiotic resistance in wastewater

  • Routine wastewater surveillance for microbial DNA/RNA can be an efficient, non-invasive tool to provide a near real-time, cost-effective monitoring for viral or bacterial outbreaks and to survey distribution of antibiotic resistance genes.
  • Microbial particles are extremely diluted in wastewater; consequently, extracting DNA/RNA from wastewater is challenging.
  • Concentrating microbial particles is essential for nucleic acid extraction for downstream applications.
  • NucleoMag DNA/RNA Water or NucleoSpin RNA Virus extraction kits can purify inhibitor-free nucleic acids from concentrated microbial particles. The purified nucleic acids can be directly used in downstream applications, such as qPCR, RT-qPCR, or Next Generation Sequencing (NGS).
  • High-throughput surveillance for wastewater monitoring can be efficiently managed by performing highly parallel qPCR using the SmartChip Real-Time PCR System.
Introduction Microbial concentration DNA/RNA isolation Application data Conclusion

Introduction  

Large-scale application of diagnostic testing at the individual level has been the main approach in epidemics. However, testing individuals is a slow process requiring extensive resources. Fast surveys of large populations can be better accomplished by wastewater-based surveillance to provide a near real-time, cost-effective monitoring of community-level transmission. Routine wastewater surveillance can be the efficient, noninvasive tool to not only monitor current and future viral or bacterial outbreaks, but also survey the spread or emergence of antibiotic resistance (AR) genes.

In this technical note, we discuss efficient and inhibitor-free nucleic acid purification from pathogens in wastewater using microbial concentration methods in combination with NucleoMag DNA/RNA Water and NucleoSpin RNA Virus extraction kits, with the DNA/RNA used directly for downstream applications (Figure 1). We show that the purified nucleic acids enabled identification of pathogens like MS2 bacteriophage and SARS-COV-2 using qPCR and RT-qPCR. Finally, we discuss how a multi-city surveillance of wastewater for antibiotic resistance prevalence was tackled using the SmartChip Real-Time PCR System, an automation system that enables highly parallel qPCR.

Figure 1. Steps for microbial detection from wastewater.

Microbial concentration  

Viruses and bacteria are typically found at low concentrations in wastewater. Consequently, extracting microbial DNA/RNA from wastewater is challenging, as the microbial particles are extremely diluted, with large volumes of wastewater needed for detecting their presence. Commonly used wastewater concentration methods, besides being labor intensive and costly, tend to concentrate PCR inhibitors present in the wastewater. Concentrating microbial particles but not PCR inhibitors is essential for downstream applications. Methods to concentrate microbial particles from wastewater samples for these downstream applications include:

Filtration, ultrafiltration, or PEG precipitation (Figure 2).

Figure 2. Microbial concentration by filtration, ultrafiltration, or PEG.

Nanotrap Magnetic Virus Particles from Ceres Nanosciences (Figure 3 and Table 1).

Figure 3. Nanotrap Magnetic particles for capturing virus.

Nanotrap concentration procedure
Capture and concentrate virus Add 150 μl of Nanotrap Magnetic Virus Particles to 10 ml sample. Invert sample 5 times to mix and incubate for 10 minutes at room temperature.
Collect Nanotrap particles Place samples on magnetic rack and allow the Nanotrap particles to come out of solution.
Wash Remove the supernatant and wash particles with 1 ml of 0.05% Tween‑20 in PCR‑grade water. Transfer sample to fresh 1.5 ml tube.
Lysis Pellet Nanotrap particles. Remove the supernatant. Resuspend pellet in 500 μl MWA 1. Incubate at room temperature for 10 minutes.
Extraction Pull Nanotrap particles out of solution with a magnetic rack. Proceed with Step 3 of the NucleoMag DNA/RNA Water protocol using 450 μl of lysate.

Table 1. Procedure for capture and concentration of virus particles.

INNOVAPREP CP‑Select sample concentration device (Figure 4 and Table 2).

Figure 4. INNOVAPREP CP‑Select sample concentration device

INNOVAPREP CP‑Select sample concentration device
Technology Single‑use Concentrating Pipette Tips
Sample volume up to 5 L
Rate up to 150 ml/min
Elution volume 150–1,000 μl (Wet Foam Elution)
Size/weight 13 x 11 x 7/8 lbs

Table 2: Specifications of INNOVAPREP CP‑Select sample concentration device.

DNA/RNA isolation  

Efficiently isolating inhibitor-free nucleic acid from wastewater is the key to conducting reliable monitoring. NucleoMag DNA/RNA Water and NucleoSpin RNA Virus kits isolate microbial RNA/DNA, with the volume of starting material and the technology preferred influencing the choice (Table 3).

NucleoMag DNA/RNA Water kit isolates microbial DNA/RNA by reversible adsorption of nucleic acids to paramagnetic beads under appropriate buffer conditions. DNA and RNA from bacteria, fungi, virus, and algae are isolated simultaneously for subsequent downstream applications. NucleoMag DNA/RNA Water allows easy automation on common liquid handling instruments or automated magnetic separators.

NucleoSpin RNA Virus kit features a special type of silica membrane with a high binding capacity for viral nucleic acids, enabling the simultaneous purification of viral RNA and DNA. The silica membrane improves the binding and recovery of low-concentration viral nucleic acids. Potential PCR inhibitors like salts, soluble macromolecular cellular components, and other contaminants are easily removed by washing with supplied buffers. The isolated nucleic acid is ready-for-use in subsequent downstream applications.

Nucleic acid isolation and purification
NucleoMag DNA/RNA Water NucleoSpin RNA Virus
Technology Magnetic bead technology Silica membrane technology
Sample material 10–1,000 ml <150 μl cell-free fluid
Preparation time 40–120 min/96 preps (excluding lysis and sample concentration) 30 min/4–6 preps (excluding lysis and sample concentration)
Fragment size 300 bp–approx. 50 kb 100 bp–approx. 50 kb
Elution volume 50–250 μl 50 μl

Table 3. Technology specifications for NucleoMag DNA/RNA Water and NucleoSpin RNA Virus.

Application data  

The success of a reliable wastewater surveillance effort is dependent on identifying pathogens and AR genes, even when present in low abundance. We present data to show that the processes outlined above can be used for routine wastewater surveillance.

RT-qPCR analysis for MS2 bacteriophage and SARS-CoV-2

Microbial particles were concentrated from wastewater samples by PEG precipitation or ultrafiltration for subsequent nucleic acid extraction with NucleoMag DNA/RNA Water kit. MS2 bacteriophage was detected consistently and reliably over a range of dilution series with excellent linearity in wastewater precipitate using PEG/NaCl (Figure 5, Panel A) and ultrafiltration (Figure 5, Panel B).

Figure 5. Detection of MS2 bacteriophage by RT-qPCR in wastewater precipitates using PEG/NaCl (Panel A) and wastewater concentrates by ultrafiltration (Panel B)

Pairing NucleoMag DNA/RNA Water kit with the Nanotrap Magnetic Virus Particles from Ceres Nanosciences for wastewater concentration was an efficient, cost-effective method to extract SARS-CoV-2 viral RNA from wastewater samples in four geographic regions of the United States (Figure 6, Panels A and B).

Figure 6: Detection of SARS-CoV-2 in wastewater samples from four geographic regions of the US. Viral detection was performed using the SARS-CoV-2 Wastewater RT-qPCR Kit (Promega) for both N1 and N2 primers. Samples were from Seattle, WA (1–9), San Bernardino, CA (10–15), Storrs, CT (16–19), and Los Angeles, CA (20–26). Detection as Ct is seen in Panel A. In Panel B, the amount of virus was quantified and normalized to BCoV spike-in control.

qPCR for MS2 bacteriophage

Combining INNOVAPREP’s CP-Select sample concentration device with Nucleospin RNA Virus and NucleoMag DNA/RNA Water nucleic acid purification procedures gave reliable nucleic acid concentration and purification from wastewater samples (Figure 7, Panels A and B).

Figure 7. Consistent detection of MS2 bacteriophage RNA from wastewater concentrates by qPCR. RNA was purified from synthetic wastewater concentrates spiked with different amounts of MS2 phage RNA. INNOVAPREP’s CP-Select device was used to concentrate the samples, followed by nucleic acid isolation using Nucleospin RNA Virus (Panel A) or Nucleomag DNA/RNA Water (Panel B).

Highly parallel qPCR for detecting antibiotic resistance

High-throughput wastewater surveillance entails processing hundreds of samples for the assay of many potential targets with precision, reproducibility, and speed. Researchers used highly parallel qPCR to target 229 antibiotic resistance genes and 25 mobile genetic elements in wastewater from 12 urban wastewater treatment plants located in seven countries (Figure 8). They used the high-throughput, quantitative SmartChip Real-Time PCR system to successfully survey AR distribution and concluded that AR profiles in urban wastewater treatment plants mirrored the AR gradient observed in clinics. The authors suggest that high-throughput data should be routinely obtained from highly parallel qPCR to improve antibiotic resistance control.

Figure 8. Abundance of resistance genes observed in wastewater samples from countries with HAC (high antibiotic consumption) and LAC (low antibiotic consumption). HAC countries were Portugal (PT), Spain (ES), and Cyprus (CYP). LAC countries were Germany (DE), Finland (FI), and Norway (NO). Samples taken in Spring 2016 (C2) and Autumn 2016 (C3). Resistance gene categories: AMG (aminoglycosides), MDR (multidrug resistance), SUL (sulfonamides), BL (β-lactams), MLSB (macrolide, lincosamide and streptogramin B), TET (tetracycline), QUI (quinolones), AMP (amphenicols), and VAN (vancomycin). Image and caption adapted from Pärnänen et al. 2019 and used under Creative Commons Attribution 4.0 International license.

Conclusion  

Effective surveillance systems are the key to rapid intervention. Real-time analysis of wastewater samples to track circulating and emerging variants can be the basis for monitoring disease outbreaks and tracking spread of antibiotic resistance.

There are two main challenges to wastewater surveillance: purifying high-quality nucleic acids from large volumes of water containing complex matrices and scaling up sample processing while testing for many clinically relevant genes.

Here, we showed that our nucleic acid purification kits, NucleoMag DNA/RNA Water and NucleoSpin RNA, in combination with microbial concentration, provide an efficient method for extracting nucleic acids for downstream applications like qPCR and RT-qPCR. We discussed how the daunting task of processing hundreds of samples to identify numerous potential targets is efficiently tackled by the SmartChip Real-Time PCR System.

The method presented can be used on a routine basis as an affordable, noninvasive tool for wastewater surveillance.

Ordering Information

Cat. # Product Size Price License Quantity Details
744220.1 NucleoMag® DNA/RNA Water 1 x 96 Preps USD $465.00

The NucleoMag DNA/RNA Water kit employs magnetic bead technology to enable efficient isolation of microbial DNA and RNA from diverse air and water samples using manual or automated processing. The kit is compatible with a variety of filters and filtration systems, and can be used to process salt or fresh water samples ranging from turbid to clear. The kit protocol enables efficient removal of inhibitory compounds that might interfere with downstream assays while avoiding the use of reducing agents, and also allows for incorporation of a homogenization step using MN bead tubes for improved sample lysis. Purified DNA and RNA obtained with the kit are suitable for downstream applications such as qPCR and NGS.

Cat. # 744220.1 includes sufficient quantities of reagents and materials for processing 1 x 96 samples.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

Documents You May Also Like Image Data

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744220.1: NucleoMag DNA/RNA Water

744220.1: NucleoMag DNA/RNA Water

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Overview of NucleoMag DNA/RNA Water protocol for manual processing of 96 samples using NucleoMag SEP

Overview of NucleoMag DNA/RNA Water protocol for manual processing of 96 samples using NucleoMag SEP

Overview of NucleoMag DNA/RNA Water protocol for manual processing of 96 samples using NucleoMag SEP.

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Efficient detection of microbial DNA from different water and air samples

Efficient detection of microbial DNA from different water and air samples

Efficient detection of microbial DNA from different water and air samples. Various water samples and an air sample were filtered and DNA extracted with the NucleoMag DNA/RNA Water kit was analyzed by PCR. Microbial DNA could be efficiently measured for all of the samples, demonstrating the versatility of the NucleoMag DNA/RNA Water kit.

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Compatibility with different homogenization devices

Compatibility with different homogenization devices

Compatibility with different homogenization devices. Nucleic acids were extracted from spiked or unspiked tapwater samples with the inclusion of a homogenization step on either a Vortex Genie 2 device (using the MN Bead Tube Holder) or a dedicated instrument (Retsch), and resulting yields were measured by qPCR. Both homogenization approaches yielded comparable results for each sample type, indicating the flexibility of the NucleoMag DNA/RNA Water kit in regards to its compatibility with the respective homogenization devices.

Back

Compatibility with different filtration systems

Compatibility with different filtration systems

Compatibility with different filtration systems. qPCR was performed with nucleic acids isolated from either round filters or a cartridge system using the NucleoMag DNA/RNA Water kit. Comparable CT values were obtained for each prep, demonstrating the versatility of the kit in providing efficient sample processing for each filtration system.

Back

Efficient removal of PCR inhibitors

Efficient removal of PCR inhibitors

Efficient removal of PCR inhibitors. Serial dilutions were performed on nucleic acids extracted from three different samples (pondwater, seawater, and lakewater) and the dilutions were analyzed by qPCR. The linearity of the inhibition plots indicates the absence of PCR inhibition for each sample.

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Automated processing on popular platforms

Automated processing on popular platforms

Automated processing on popular platforms. The NucleoMag DNA/RNA Water kit was used to purify nucleic acids from two different water samples using two different automation platforms, KingFisher (magnetic rods) and epMotion (liquid handling), respectively. qPCR analysis of the purfied nucleic acids indicated that comparable yields were obtained from each sample, indicating the adaptability of the kit to both automation approaches.

744220.4 NucleoMag® DNA/RNA Water 4 x 96 Preps USD $1585.00

The NucleoMag DNA/RNA Water kit employs magnetic bead technology to enable efficient isolation of microbial DNA and RNA from diverse air and water samples using manual or automated processing. The kit is compatible with a variety of filters and filtration systems, and can be used to process salt or fresh water samples ranging from turbid to clear. The kit protocol enables efficient removal of inhibitory compounds that might interfere with downstream assays while avoiding the use of reducing agents, and also allows for incorporation of a homogenization step using MN bead tubes for improved sample lysis. Purified DNA and RNA obtained with the kit are suitable for downstream applications such as qPCR and NGS.

Cat. # 744220.4 includes sufficient quantities of reagents and materials for processing 4 x 96 samples.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

Documents You May Also Like Image Data

Back

Overview of NucleoMag DNA/RNA Water protocol for manual processing of 96 samples using NucleoMag SEP

Overview of NucleoMag DNA/RNA Water protocol for manual processing of 96 samples using NucleoMag SEP

Overview of NucleoMag DNA/RNA Water protocol for manual processing of 96 samples using NucleoMag SEP.

Back

Efficient detection of microbial DNA from different water and air samples

Efficient detection of microbial DNA from different water and air samples

Efficient detection of microbial DNA from different water and air samples. Various water samples and an air sample were filtered and DNA extracted with the NucleoMag DNA/RNA Water kit was analyzed by PCR. Microbial DNA could be efficiently measured for all of the samples, demonstrating the versatility of the NucleoMag DNA/RNA Water kit.

Back

Compatibility with different homogenization devices

Compatibility with different homogenization devices

Compatibility with different homogenization devices. Nucleic acids were extracted from spiked or unspiked tapwater samples with the inclusion of a homogenization step on either a Vortex Genie 2 device (using the MN Bead Tube Holder) or a dedicated instrument (Retsch), and resulting yields were measured by qPCR. Both homogenization approaches yielded comparable results for each sample type, indicating the flexibility of the NucleoMag DNA/RNA Water kit in regards to its compatibility with the respective homogenization devices.

Back

Compatibility with different filtration systems

Compatibility with different filtration systems

Compatibility with different filtration systems. qPCR was performed with nucleic acids isolated from either round filters or a cartridge system using the NucleoMag DNA/RNA Water kit. Comparable CT values were obtained for each prep, demonstrating the versatility of the kit in providing efficient sample processing for each filtration system.

Back

Efficient removal of PCR inhibitors

Efficient removal of PCR inhibitors

Efficient removal of PCR inhibitors. Serial dilutions were performed on nucleic acids extracted from three different samples (pondwater, seawater, and lakewater) and the dilutions were analyzed by qPCR. The linearity of the inhibition plots indicates the absence of PCR inhibition for each sample.

Back

Automated processing on popular platforms

Automated processing on popular platforms

Automated processing on popular platforms. The NucleoMag DNA/RNA Water kit was used to purify nucleic acids from two different water samples using two different automation platforms, KingFisher (magnetic rods) and epMotion (liquid handling), respectively. qPCR analysis of the purfied nucleic acids indicated that comparable yields were obtained from each sample, indicating the adaptability of the kit to both automation approaches.

Back

744220.4: NucleoMag DNA/RNA Water

744220.4: NucleoMag DNA/RNA Water
740956.50 NucleoSpin® RNA Virus 50 Preps USD $236.00

NucleoSpin RNA Virus is designed for the isolation of viral nucleic acids from serum, plasma, or any cell-free biological fluid.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

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740956.50: NucleoSpin RNA Virus

740956.50: NucleoSpin RNA Virus

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NucleoSpin RNA Virus procedure

NucleoSpin RNA Virus procedure
NucleoSpin RNA Virus procedure.
740956.250 NucleoSpin® RNA Virus 250 Preps USD $1020.00

NucleoSpin RNA Virus is designed for the isolation of viral nucleic acids from serum, plasma, or any cell-free biological fluid.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

Documents Image Data

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740956.250: NucleoSpin RNA Virus

740956.250: NucleoSpin RNA Virus

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NucleoSpin RNA Virus procedure

NucleoSpin RNA Virus procedure
NucleoSpin RNA Virus procedure.

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That's GOOD Science!

What does it take to generate good science? Careful planning, dedicated researchers, and the right tools. At Takara Bio, we thoughtfully develop exceptional products to tackle your most challenging research problems, and have an expert team of technical support professionals to help you along the way, all at superior value.

Explore what makes good science possible

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Takara Bio USA, Inc. provides kits, reagents, instruments, and services that help researchers explore questions about gene discovery, regulation, and function. As a member of the Takara Bio Group, Takara Bio USA is part of a company that holds a leadership position in the global market and is committed to improving the human condition through biotechnology. Our mission is to develop high-quality innovative tools and services to accelerate discovery.

FOR RESEARCH USE ONLY. NOT FOR USE IN DIAGNOSTIC PROCEDURES (EXCEPT AS SPECIFICALLY NOTED).

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