{"id":293,"date":"2020-03-27T16:07:09","date_gmt":"2020-03-27T13:07:09","guid":{"rendered":"http:\/\/labormed.biz\/?page_id=183"},"modified":"2020-08-31T11:04:08","modified_gmt":"2020-08-31T08:04:08","slug":"covid-pcr-kit","status":"publish","type":"page","link":"http:\/\/www.labormed.biz\/en\/covid-pcr-kit\/","title":{"rendered":"Covid Pcr Kit"},"content":{"rendered":"
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SARS-CoV-2 Real-Time PCR Kit<\/strong><\/center><\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n
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Intended Use<\/h3>\n

This document describes the use of real-time RT-PCR assays for the in vitro qualitative detection of 2019-Novel Coronavirus (SARS-CoV-2) in respiratory specimens. The SARS-CoV-2 primer and probe sets are designed for the specific detection of SARS-CoV-2.<\/p>\n

DIAGNOVITAL\u00ae SARS-CoV-2<\/strong>\u00a0Real-Time PCR Kit is an in vitro nucleic acid amplification assay for qualitative detection of 2019-Novel Coronavirus (SARS-CoV-2) in respiratory specimens using RTA Viral Nucleic Acid Isolation Kit and BIO-RAD CFX96-IVD or Rotor-Gene 3000\/6000 or Applied Biosystems 7500 or HIMEDIA Insta Q96 Plus Real-Time PCR Detection System for amplification, detection and analysis.<\/p>\n

The kits follow CDC\u2019s and WHO\u2019s latest detection guidelines.<\/p>\n

Product Description<\/h3>\n

DIAGNOVITAL\u00ae SARS-CoV-2<\/strong>\u00a0is a real-time RT-PCR-based detection system for the 2019 Wuhan coronavirus (SARS-CoV-2). SARS-CoV-2 is considered a novel human coronavirus that is genetically distinct from the common human coronaviruses (229E, NL63, OC43, HKU1), which cause seasonal acute respiratory illness. It is also genetically distinct from the two newer human coronaviruses, MERS-CoV and SARS-CoV.<\/p>\n

DIAGNOVITAL\u00ae SARS-CoV-2<\/strong>\u00a0detects the presence of 2 different and highly specific gene sequences of SARS-CoV-2: E gene and RdRP gene. All 2 assays must be tested positive to confirm the sample as SARS-CoV-2-positive.<\/p>\n

Additionally, a non-infectious positive control and a negative human extraction control are included. The positive control is used to confirm functionality of the assays and overall PCR performance, the negative human extraction control is included to evaluate the quality of the RNA isolation independently from the SARS-CoV-2 assays.<\/p>\n

QPCR-BASED DETECTION OF SARS-CoV-2<\/h3>\n

The first step in the detection of SARS-CoV-2 is the conversion of viral RNA into cDNA. Afterwards, the target sequences unique for SARS-CoV-2 are specifically amplified with amplification monitored in real time through the use of fluorescently labelled probes: upon incorporation into the newly amplified DNA strands, the fluorophore (FAMTM) is released and an increase in fluorescence signal can be observed.<\/p>\n

Due to the intrinsic mutation rate of coronaviruses, it is possible that mutations in the target sequence occur and accumulate over time. This can lead to false-negative results with a PCR-based detection approach.\u00a0DIAGNOVITAL\u00ae SARS-CoV-2<\/strong>\u00a0addresses this issue by using 3 detection assays on 3 different target sequences to minimize the chance of false-negative results caused by an altered target sequence.
\nIf samples are tested negative in one or more assays, additional complementary testing may be required. The original target sequences for SARS-CoV-2 are included as a non-infectious target positive control (TPC) to check the integrity of the detection assays.<\/p>\n

Samples tested positive should always be confirmed through complementary methods and additional analysis in an independent laboratory.<\/p>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n

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Materials Provided<\/h3>\n

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Additional Materials Required<\/h3>\n

\u2022^Suitable means & equipment for nucleic acid extraction (see chapter 3.4)<\/p>\n

\u2022 Real-time PCR detection system equipped for FAMTM detection<\/p>\n

\u2022 Adjustable pipettes & fitting filtered pipette tips<\/p>\n

\u2022 Appropriate PSA & workspaces for working with potentially infectious samples<\/p>\n

\u2022 Surface decontaminants such as DNAZapTM (Life Technologies), DNA AwayTM (Fisher Scientific), RNAse AwayTM (Fisher Scientific), 10% bleach (1:10 dilution of commercial 5.25-6.0% sodium hypochlorite)<\/p>\n

\u2022 Nuclease-free tubes \/ strips \/ plates to prepare dilutions, mastermixes etc.<\/p>\n

\u2022 Nuclease-free tubes \/ strips \/ plates corresponding to the PCR device<\/p>\n

\u2022 Suitable storage options for reagents and specimen (4\u00b0C, -20\u00b0C, -70\u00b0C)<\/p>\n

Storage<\/h3>\n

\u2022 Store all components at -20\u00b0C and avoid repeated freeze and thaw cycles.<\/p>\n

\u2022 Protect the 2X qPCR mastermixes from light as prolonged exposure can diminish the performance of the fluorophores.<\/p>\n

\u2022 If the kit components have been damaged during transport, contact A1 Life Sciences. Do not use as performance may be compromised.<\/p>\n

\u2022 Keep reagents separate from sample material to avoid contamination.<\/p>\n

\u2022 Do not use after the designated expiry date.<\/p>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n

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Performance Characteristics<\/h3>\n

Analytical sensitivity<\/strong><\/p>\n

Analytical sensitivity was analyzed by use of a dilution series of DIAGNOVITAL SARS-CoV-2 Reference samples. A dilution series of a DIAGNOVITAL SARS-CoV-2 Reference samples was prepared to give the final concentrations of 300, 100, 30 and 10 copies\/ml. Each dilution was tested in 24 replicates. Lower limit was calculated by probit analysis done by PASW Statistics 18 program. For each genotype\/subtype, Limit of Detection (LoD) values and 95 % confidence ranges are summarized in Table 1. Table 1: SARS-CoV-2qPCR Kit – Limit of Detection (LoD) values and 95 % confidence ranges summarized in table 1.<\/p>\n

Table 1:<\/strong>\u00a0SARS-CoV-2qPCR Kit – Limit of Detection (LoD) values and 95 % confidence ranges<\/p>\n

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Precision<\/h3>\n

In this study, precision of the kit was evaluated for intra-assay, inter-assay, inter-batch, by using RTA Viral NA Isolation Kit (Cat No: 09029) and different specimen types (oropharyngeal vs. nasopharyngal swabs). For each target gene and different assay, 24 replicates of 103 copies\/ml DIAGNOVITAL SARS-CoV-2 Reference samples were used. Descriptive statistics were analyzed by IBM SPSS Statistics program. Overall precision assays associated with Ct values were summarized in Table 2.<\/p>\n

Table 2:<\/strong>\u00a0Overall descriptive statistics of SARS-CoV-2 precision data.<\/p>\n

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Diagnostic specificity<\/h3>\n

SARS-CoV-2 RNA negative clinical specimens were analyzed to determine the diagnostic specificity of DIAGNOVITAL SARS-CoV-2Real Time PCR Kit. 40 SARS-CoV-2 RNA negative clinical oropharygal swab specimens and 40 SARS-CoV-2 RNA negative clinical oropharygal swab specimens and 30 bronchoalveolar lavage specimens were used. None of the 100 SARS-CoV-2 negative clinical specimens gave positive test result for SARS-CoV-2. Diagnostic specificity of DIAGNOVITAL SARS-CoV-2 Real Time PCR Kit is 100 %. All of the Human Extraxtion Controls (HEC) of tests gave positive result.<\/p>\n

Cross-reactivity<\/h3>\n

To examine the specificity of an assay, cross-reactivity studies should be performed for potential cross-reactive markers. In this study, the specificity of the assay was evaluated by testing. 9 reference organism and 11 clinical specimens which were positive.<\/p>\n

DIAGNOVITAL SARS-CoV-2 Real Time PCR Kit do not show any cross-reactivity with other potential cross-reactive markers given in the table 3 below:<\/p>\n

Table 3:<\/strong>\u00a0Potential cross-reactive markers tested in the study.<\/p>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n

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Considerations Before Starting<\/h3>\n

BIOSAFETY<\/strong><\/p>\n

\u2022 Wear appropriate personal protective equipment (e.g. gowns, powder-free gloves, eye protection) when working with clinical specimen.<\/p>\n

\u2022 Specimen processing should be performed in a certified class II biological safety cabinet following biosafety level 2 or higher guidelines.<\/p>\n

\u2022 For more information, refer to:<\/p>\n

\u2022 Interim Guidelines for Collecting, Handling, and Testing Clinical Specimens from Patients Under Investigation (PUIs) for 2019 Novel Coronavirus (SARS-CoV-2)\u00a0https:\/\/www.cdc.gov\/coronavirus\/SARS-CoV-2\/guidelines-clinical-specimens.html\u00a0<\/a><\/p>\n

\u2022 Biosafety in Microbiological and Biomedical Laboratories 5th edition available at\u00a0http:\/\/www.cdc.gov\/biosafety\/publications\/<\/a>.<\/p>\n

\u2022 The use of DIAGNOVITAL\u00ae SARS-CoV-2 is restricted to trained laboratory personnel only.<\/p>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n

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SPECIMENS<\/h3>\n

Only use appropriate specimens for testing, such as:<\/p>\n

\u2022 Respiratory specimens including nasopharyngeal \/ oropharyngeal aspirates or washes, nasopharyngeal \/ oropharyngeal swabs, broncheoalveolar lavage, tracheal aspirates and sputum.<\/p>\n

\u2022 Swab specimens should be collected only on swabs with a synthetic tip (such as polyester or Dacron\u00ae) with plastic shafts. Swabs with calcium alginate or cotton tips with wooden shafts are not acceptable<\/p>\n

SPECIMENS – HANDLING AND STORAGE<\/h3>\n

\u2022 Specimens can be stored at 4\u00b0C for up to 72 hours after collection.<\/p>\n

\u2022 If a delay in extraction is expected, store specimens at -70\u00b0C or lower.<\/p>\n

\u2022 Extracted nucleic acids should be stored at -70\u00b0C or lower. Do not use specimens if<\/p>\n

\u2022 they were not kept at 2-4\u00b0C (\u2264 4 days) or frozen at -70\u00b0C or below.<\/p>\n

\u2022 they are insufficiently labelled or lack documentation.<\/p>\n

\u2022 they are not suitable for this purpose (see above for suitable sample material).<\/p>\n

the specimen volume is insufficient.<\/p>\n

Sample Preparation<\/h3>\n

\u2022 The performance of RT-PCR assays strongly depends on the amount and quality of sample template RNA. It is strongly recommended to qualify and validate RNA extraction procedures for recovery and purity before testing specimens.<\/p>\n

\u2022 Suitable nucleic acid extraction systems successfully used in combination with DIAGNOVITAL DETECTION KITS include: RTA Viral NA Isolation Kit from Swabs, bioM\u00e9rieux NucliSens\u00ae systems, QIAamp\u00ae Viral RNA Mini Kit, QIAamp\u00ae MinElute Virus Spin Kit or RNeasy\u00ae Mini Kit (QIAGEN), EZ1 DSP Virus Kit (QIAGEN), Roche MagNA Pure Compact RNA Isolation Kit, Roche MagNA Pure Compact Nucleic Acid Isolation Kit, and Roche MagNA Pure 96 DNA and Viral NA Small Volume Kit, and Invitrogen ChargeSwitch\u00ae Total RNA Cell Kit.<\/p>\n

\u2022 Store and keep residual specimens and extracted nucleic acids at -70\u00b0C.<\/p>\n

\u2022 Only thaw the number of specimen extracts that will be tested in a single day.<\/p>\n

\u2022 Do not freeze\/thaw extracts more than once before testing as each freeze\/thaw cycle will decrease the RNA quality.<\/p>\n

\u2022 It may be possible to use patient samples directly, depending on the sample type. However, this may require a prior lysis step and titration of the amount on sample that can be used without inhibiting the reaction. This procedure has not been validated, use of isolated RNA is recommended.<\/p>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n

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Reaction Setup<\/h3>\n

1. Make sure that all necessary equipment and devices are suitable, calibrated and functional before starting the experiments.
\n2. Decontaminate equipment and workspace and prepare everything needed for the following experiment to keep the workflow short and repeatable.
\n3. Switch on the PCR detection system and program it to avoid delays after setting up the reactions.
\n4.Thaw all components of DIAGNOVITAL\u00ae SARS-CoV-2 on ice and mix gently but thoroughly to ensure even distribution of components. Collect liquid at the bottom of the tube with a quick spin.
\n5. For first tests, prepare a dilution series of your RNA to determine your ideal concentration window. The recommended sample volume is 5 \u00b5l \/ reaction.
\n6. Set up your Mastermix Plate:
\na. Always prepare control reactions with nuclease-free dH2O instead of sample material (NTC) to detect contamination in your reagents.
\nb. Always include the assay for the negative human extraction control (HEC) to evaluate the quality of your RNA isolate.
\nc. When using the provided target positive control (TPC), use 5 \u03bcl \/ reaction and add nuclease-free dH2O to 20 \u03bcl.
\nd. > 2 replicates \/ sample are strongly recommended.
\ne. Prepare enough mastermix for all planned reactions. It is recommended to prepare mastermix for 2 additional reactions to compensate for pipetting inaccuracies.<\/p>\n

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Figure 1:<\/strong> Example pipetting scheme for the distribution of mastermixes with the individual assay mixes<\/p>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n

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7. Transfer the Mastermix Plate to a separate workspace to add the sample material. Preparing reagents and final reaction setup in separate workspaces helps to avoid contamination of equipment and reagents with sample material.
\na. Prepare negative reactions first and seal them before handling positive samples. It is recommended to only bring potentially positive sample material and the included target positive control to the workspace once the NTC is prepared and sealed.
\nb. Add your samples to the Mastermix Plate. An example setup is given in Fig 2).
\nc. Keep reactions on ice until transferring them to the PCR device.
\n\"\"Figure 2:<\/strong> Example pipetting scheme for the addition of samples. The bottom half of the plate could be used for replicates with an identical setup8. Transfer the reactions to the PCR device, then cycle according to these guidelines:\"\"<\/p>\n

9. Once the run is finished, do not open the reaction tubes to avoid contamination and discard according to local guidelines and regulations. Do not autoclave as this may contaminate laboratory equipment with amplicons.<\/p>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n

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Analysis & Troubleshooting<\/h3>\n

EXEMPLARY RESULT<\/strong><\/p>\n

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\u2022\u00a0dH2O controls (NTC) must not give a positive Ct for any assay<\/strong>. If they do, the reaction was contaminated with sample RNA \/ DNA. Decontaminate equipment and workspace and repeat the reactions.<\/p>\n

\u2022\u00a0For a sample to be considered<\/strong>\u00a0positive for SARS-CoV-2,<\/strong><\/span>\u00a0all 2 assays (E \/ RdRP) must give positive Ct values.<\/strong>\u00a0If the HEC fails to amplify, the sample must still be considered positive.<\/p>\n

\u2022\u00a0For a sample to be considered<\/strong>\u00a0negative for SARS-CoV-2,<\/strong><\/span>\u00a0none of the 2 assays (E \/ RdRP) must give positive Ct values.<\/strong>\u00a0The HEC must give a positive Ct value (< 35 cycles) for these samples to ensure that sample material of suitable quality was present.<\/p>\n

\u2022\u00a0All reactions containing RNA isolate must give positive Ct values for the HEC assay. The Ct values should be < 35 cycles.<\/strong>\u00a0Failure to amplify the negative human extraction control indicates a flawed RNA extraction or loss of RNA isolate due to RNAse contamination. The sample is not sufficient, results cannot be interpreted.<\/p>\n

\u2022\u00a0When using the TPC for SARS-CoV-2, a positive Ct for all 2 assays must be observed. The Ct value for the TPC should be < 35 cycles.<\/strong>\u00a0If the Ct value does not correspond to the expected value or not all assays are tested positive, PCR was compromised. Check the reaction setup and PCR device settings and repeat the reactions. Repeated freeze and thaw cycles of the TPC can compromise its quality resulting in late Ct values.<\/p>\n

\u2022\u00a0If no amplification signal is observed for any assay, PCR was inhibited<\/strong>. Check reaction setup and device settings and repeat the RNA extraction if necessary. Results are invalid and cannot be interpreted. Doc. Nr. : A1-15259EN_v3.3<\/p>\n

\u2022\u00a0If < 3 of the target assays are positive (e.g. only E gene, only RdRP gene etc.), results are inconclusive.<\/strong> Check reaction setup and device settings and repeat the RNA extraction if necessary. Results are invalid and cannot be interpreted<\/p>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n

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Limitations<\/h3>\n

\u2022 For reliable results, it is essential to adhere to the guidelines given in this manual. Changes in reaction setup or cycling protocol may lead to failed experiments.<\/p>\n

\u2022 Depending on the sample matrix, inhibitors may be present in the isolated RNA and disable reverse transcription and \/ or PCR amplification. If this is the case, another sample type or isolation method may be beneficial.<\/p>\n

\u2022 Spontaneous mutations within the target sequence may result in failure to detect the target sequence.<\/p>\n

\u2022 Results must always be interpreted in consideration of all other data gathered from a sample. Interpretation must be performed by personnel trained and experienced with this kind of experiment.<\/p>\n

Trademarks<\/h3>\n

DIAGNOVITAL\u00ae, NucliSens\u00ae (bioM\u00e9rieux), QIAamp\u00ae, RNeasy\u00ae (QIAGEN), ChargeSwitch\u00ae (Invitrogen), ROXTM, FAMTM (Life Technologies), DNAZapTM , DNA AwayTM, RNAse AwayTM
\nRegistered names, trademarks, etc. used in this document, even if not specifically marked as such, are not to be considered unprotected by law.<\/p>\n

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Address :<\/strong>\u00a0Izzetpasa Mahallesi Gurun Caddesi No:1 D:1 Sisli \/ Istanbul \/ Turkey<\/p>\n

Phone:<\/strong>\u00a0+90 212 343 72 05<\/a><\/p>\n

E-mail<\/strong>: labor@labormed.biz<\/p>\n

Web:<\/strong>\u00a0http:\/\/labormed.biz\/<\/a><\/p>\n<\/div>\n<\/div>\n<\/div>\n<\/div>\n

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\n\t\t\t\n\t\t\n\t\t\t<\/span>\n\t\t\tSARS-Cov-2 Real-Time PCR Kiti\t\t<\/span>\n\t\t\t<\/a>\n\t<\/div>\n<\/div><\/div>\n
\n\t\t\t\n\t\t\n\t\t\t<\/span>\n\t\t\tAB - UYGUNLUK BEYANI\t\t<\/span>\n\t\t\t<\/a>\n\t<\/div>\n<\/div><\/div>\n
\n\t\t\t\n\t\t\n\t\t\t<\/span>\n\t\t\tSERT\u0130F\u0130KA\t\t<\/span>\n\t\t\t<\/a>\n\t<\/div>\n<\/div><\/div>\n<\/div>\n<\/div>\n<\/div>\n","protected":false},"excerpt":{"rendered":"

SARS-CoV-2 Real-Time PCR Kit Intended Use This document describes the use of real-time RT-PCR assays for the in vitro qualitative detection of 2019-Novel Coronavirus (SARS-CoV-2) in respiratory specimens. The SARS-CoV-2 primer and probe sets are designed for the specific detection of SARS-CoV-2. DIAGNOVITAL\u00ae SARS-CoV-2\u00a0Real-Time PCR Kit is an in vitro nucleic acid amplification assay for […]<\/p>\n","protected":false},"author":1,"featured_media":0,"parent":0,"menu_order":0,"comment_status":"closed","ping_status":"closed","template":"no-sidebar.php","meta":{"footnotes":""},"class_list":["post-293","page","type-page","status-publish","hentry"],"_links":{"self":[{"href":"http:\/\/www.labormed.biz\/en\/wp-json\/wp\/v2\/pages\/293","targetHints":{"allow":["GET"]}}],"collection":[{"href":"http:\/\/www.labormed.biz\/en\/wp-json\/wp\/v2\/pages"}],"about":[{"href":"http:\/\/www.labormed.biz\/en\/wp-json\/wp\/v2\/types\/page"}],"author":[{"embeddable":true,"href":"http:\/\/www.labormed.biz\/en\/wp-json\/wp\/v2\/users\/1"}],"replies":[{"embeddable":true,"href":"http:\/\/www.labormed.biz\/en\/wp-json\/wp\/v2\/comments?post=293"}],"version-history":[{"count":13,"href":"http:\/\/www.labormed.biz\/en\/wp-json\/wp\/v2\/pages\/293\/revisions"}],"predecessor-version":[{"id":317,"href":"http:\/\/www.labormed.biz\/en\/wp-json\/wp\/v2\/pages\/293\/revisions\/317"}],"wp:attachment":[{"href":"http:\/\/www.labormed.biz\/en\/wp-json\/wp\/v2\/media?parent=293"}],"curies":[{"name":"wp","href":"https:\/\/api.w.org\/{rel}","templated":true}]}}