RNA analysis tools

EQ SARS COV2 One Step RT qPCR kit for wastewater, 200 rxns

Category: RNA analysis tools

EQ SARS COV2 One Step RT qPCR kit for wastewater contains a 5x reaction buffer optimized for sensitive and specific detection of SARS COV2 RNA from various sources and purity backgrounds.

(SKU: RN016S)

10.00

For detailed product information please refer to the IFU

Product Details

Description:

EQ SARS COV2 One Step RT qPCR kit for wastewater contains a 5x reaction buffer optimized for sensitive and specific detection of SARS COV2 RNA from various sources and purity backgrounds. Enzymes come separately in 20x and 200x formulations to provide flexibility and allow user to optimize depending on the purity of the substrate of interest (mainly on the presence of PCR inhibitors). The 10x SARS COV2 Oligos mix contains a combination of primers and probe for SARS COV2 N gene (modified USA CDC N2 primer/probe set), that allows for the qPCR detection of SARS COV2 transcripts at HEX/VIC channel. Optimizations on wastewater extracts samples guarantee the reproducible and efficient qPCR reactions close to the expected limit of detection (<10 copies per reaction). It can reliably detect and quantify as low as 10 copies per reaction, based on a standard curve produced by analyzing EURM019 dilutions, with efficiency ~ 90-110 %.

 

Reagents supplied:

EQ SARS COV2 One Step RT qPCR kit for wastewater, 200 rxns (Cat No: RN016S)
Cat No Description  Tubes No. 
BR030-1 5x One Step RT-qPCR buffer, 1 ml 
PD015-0.225 20x Hot Start Taq DNA polymerase, 0.225ml 
RN015-0.025 200x Reverse Transcriptase, 0.025ml 
BR060-0.425 10x SARS COV2 Oligos mix, 0.425 ml 
BR033- 1 Nuclease Free Water, 1 ml 
Table 1. RN016S kit components

Standard 20 μl reaction:

ComponentStock solutions1 reaction of 20 μlFinal Concentration/Quantity (20 μl assay) 
15x One Step RT-PCR buffer5x4 ㎕1x
210x SARS COV2 Oligos mix10x2 ㎕1x
320x Hot Start Taq DNA polymerase20x1 ㎕1x
4200x Reverse Transcriptase200x0.1 ㎕ *1x
5Template RNA**5-105 copies of target sequence/μl2-4 ㎕N/A
6Nuclease Free WaterN/ATill 20 ㎕N/A 
Table 2. Standard reaction setup.
*0.08-0.12 μl may be added depending on the substrate used. For Reference Labs wastewater extracts analysis, 0.1 μl has been used extensively used. Do not add more than needed, because of PCR inhibition effect caused by the excess of Reverse transcriptase enzyme in the reaction.
** 2 μl of RNA extracts is recommended. In case of high concentration of PCR inhibitors, perform 1:10 dilution of the original wastewater extract sample and add 2-4 μL per reaction. 2 μL of wastewater extracts from Reference Labs have been extensively used in our analysis.
 
Optional: Depending on the wastewater quality, the region or the season collected, treatment of wastewater extracts with PCR inhibitors removal kits like the ones provided by ZYMO Research (https://zymoresearch.eu/collections/onestep-pcr-inhibitor-removal-kits), may be important to obtain accurate, quantifiable results. In order to verify the necessity of this type of treatment, test 4 independently extracted samples, collected over 2-4 weeks, and compare the quantification of the 1:10 dilution of either treated or untreated sample. If the difference obtained is lower than 30 % then that treatment may be omitted from the analysis.

Proposed assays

There are two assays proposed for the analysis.

The initial assay

The initial standard assay is very important to be able:

  1. To establish the quantification equivalence between the current kit and the standard lab method used so far (if applicable)
  2. To check the necessity of PCR inhibitor removal kits.

To that end, the reactions that needed to be set are the following:

  1. Standard curves 105-101 in triplicates -> 15 reactions
  2. 1:10 dilution of wastewater extracts in triplicates -> 3 x number of samples
  3. (Optional) if PCR inhibitor test needs to be performed, then incubate half the amount of the extracted wastewater samples with PCR inhibitor removal kit, then dilute 1:10 and analyze in triplicates -> 3 x number of samples with PCR inhibitor removal treatment (same samples included in ii)
  4. Two negative control reactions that contain Nuclease free Water (provided in the kit) instead of template.

After the reactions have been completed, produce equation, estimate efficiency and R2. If efficiency is between 90-110% and R2 value is above 0.98 then proceed to quantification. One may exclude reactions that do not conform with the expected values.

(Optional/ When applicable) Quantify samples with or without PCR inhibitor removal treatment and see whether there is a difference greater than 30 %. If there is, then the PCR inhibitor removal kit may be necessary before the RT-qPCR analysis for the accurate quantification of the viral load in the wastewater sample. If in both cases, treatment or not, a similar quantity is estimated for the same sample, then the PCR inhibitor removal step may be omitted.

If the quantification of this kit needs to be compared with a different method, then the same sample needs to be analyzed again with the different method at the same freeze-thaw cycle, meaning that previous quantity record of the sample, may deviate greatly due to RNA degradation and not the difference in kits’/methods’ quantification efficiency.

The Routine assay

 After the initial run, the routine run for wastewater analysis may contain:

  1. A standard Curve of 4 logs in duplicates of 102-105 copies/reaction ->  8 reactions
  2. 1:10 dilutions of wastewater extracts in triplicates -> 3 x number of wastewater samples
  3. 2 negative control reactions 2 reactions

Optimized component addition order for master mix preparation

First add water and then continue by adding the buffer, the oligos, 20x Hot Start Taq DNA polymerase and finally the 200x Reverse Transcriptase. While adding each enzyme to the master mix, pipette up and down for 5-10 times (to dissolve glycerol) and then add the next one. Perform one final mix by mild vortex (1000-1200 rpm) until glycerol is completely dissolved. Aliquot the appropriate volume and add water to the negative control reactions and close the caps. Then proceed to the samples addition and close the caps and finally add template to the standard curves’ reactions and close the caps.

One Step-RT recommended condition

IFU with more details is available!

Additives that improve robustness

In cases of samples with low viral content near the limit of detection (~5-10 copies/μl of wastewater sample) and/or high concentration of inhibitors one may also add extra DTT or T4gp32 protein to improve reactions’ efficiency. Final concentrations in qPCR reactions should be 1mM for DTT and 0.05 μg/μl for T4gp32. An example of the reaction setup including both additives may be found below:

ComponentConcentration of Stock solutions1 reaction of 20 μlFinal Concentration/Quantity (20 μl assay) 
15x One Step RT-PCR buffer5x4 ㎕1x
210x SARS COV2 Oligos mix10x2 ㎕1x
3DTT (Customer provided)100 mM0.2 ㎕1 mM
4Gp32 (Customer provided)10 μg/μl0.1 ㎕0.05 μg/μl
520x Hot Start Taq DNA polymerase20x1 ㎕1x
6200x Reverse Transcriptase200x0.1 ㎕1x
7Template RNA*5-105 copies of target sequence/μl2-4 ㎕N/A
8Nuclease Free WaterN/ATill 20 ㎕N/A 

Recommended suppliers:

  • For DTT, any product that is compatible with molecular biology applications (example A2948/Applichem, DTT Molecular biology grade or equivalent)
  • For Gp32, use any provider that is compatible with molecular biology applications. The inhouse assays have been performed with cat number M300S or L from New England Biolabs (T4 Gene 32 Protein)

DTT may reverse mildly the inhibition potential of the sample whereas both should be used when high inhibition is suspected

Other Quality Controls: 

Certified as DNase-RNase free using fluorescently labeled RNase and DNase probes. Efficiency between 90-110%, with R2 value >0.99 of each lot is estimated by a standard curve assay produced over 5 logs of EURM019 substrate (https://crm.jrc.ec.europa.eu/p/EURM-019)

Shipping 

Shipped on blue ice or dry ice. 

Storage conditions 

Store at -20οC ± 5ο

Shelf life:

1 year upon production

Example: SARS COV 2 standard EURM019

 A. Initial standard curve assay

Figure 1. SARS COV2 standard curves produced by EQ SARS COV2 One Step RT qPCR kit for wastewater (Cat No: RN016S). The standard curves were produced by analyzing the EURM019 SARS COV 2 standard over 5 logs (example of initial assay). Standard dilutions were prepared, having as a given that the EURM-019 stock solution contains 108 copies of SARS COV2 chimeric transcripts/μl (detailed info for EURM019 used may be found at https://crm.jrc.ec.europa.eu/p/EURM-019). Since the quantification of the EURM-019 standard, performed by digital droplet PCR by manufacturer, produced results between 6 – 7.6 x 107 copies/μl depending on the primer set used, the actual number of copies that were introduced in each reaction may be 24-40 % less than indicated in the figure. The results were automatically produced by CFX Maestro software. The reactions were incubated to either CFX96 or OPUS96 qPCR machines with very similar results.

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