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==2. Diagnostic testing of COVID-19 and other coronaviruses==
==Sandbox begins below==
 
===2.1 Testing terminology===
As you read through this chapter, you may discover terms like "[[polymerase chain reaction]]" (PCR) and "[[Lateral flow test|lateral flow assay]]" (LFA). If you're a laboratorian or have a clinical background, you may already be familiar with these terms. However, it seems prudent to at least briefly discuss a few of them before delving into coronavirus testing itself.
 
====2.1.1. Introduction====
Living organisms store information in their genetic material, using DNA or RNA as the information carrier. That information, or genetic code, essentially provides instructions for organism development, function, growth, and reproduction. In the late twentieth century, researchers were laying the groundwork for molecular diagnostics, the concept of examining an organism's genetic code and its associated biological markers to diagnose and treat disease on a more personalized basis. This requires assays, an investigative procedure for assessing the presence of, or measuring the amount or fuctional activity of, a target analyte. In the case of molecular diagnostics, and more broadly molecular biology, the target is biological in nature, and thus biological assays are used. These biological assays are designed to accurately detect the presence of or enable counts of a biological molecule, including DNA, RNA, proteins, cells, bacteria, and virus particles (e.g., viral plaque assays).<ref name="ADXIntro13">{{cite web |url=https://dx.advamed.org/research/resource-center/introduction-molecular-diagnostics-essentials-diagnostics-series-pdf |title=Introduction to Molecular Diagnostics: The Essentials of Diagnostics Series |author=AdvaMedDx |pages=19 |date=2013 |accessdate=08 April 2020}}</ref>
 
====2.1.2 Polymerase chain reaction (PCR)====
Polymerase chain reaction or PCR is a molecular biology method that takes small amounts of DNA sequences and makes copies of (amplifies) it to the point of having enough material to sufficiently study or work with. The base technique can yield results in several hours and has a high level of sensitivity, with its ability to amplify the DNA to counts of millions or billions. PCR has been used in molecular diagnostics for testing prospective parents for being genetic carriers of particular diseases (i.e., expanded carrier screening)<ref name="GreggExpanded18">{{cite journal |title=Expanded Carrier Screening |journal=Obstetrics and Gynecology Clinics of North America |author=Gregg, A.R. |volume=45 |issue=1 |pages=103–112 |year=2018 |doi=10.1016/j.ogc.2017.10.005 |pmid=29428278}}</ref><ref name="ChokoschviliRepro18">{{cite journal |title=Reproductive autonomy in expanded carrier screening: More than meets the eye? |journal=Expert Review of Molecular Diagnostics |author=Chokoshvili, D.; Vears, D.F.; Borry, P. |volume=18 |issue=12 |pages=993–94 |year=2018 |doi=10.1080/14737159.2018.1544496 |pmid=30394810}}</ref>, tissue typing to ensure more effective organ transplants<ref name="EdgerlyThePast18">{{cite journal |title=The Past, Present, and Future of HLA Typing in Transplantation |journal=Methods in Molecular Biology |author=Edgerly, C.H.; Weimer, E.T. |volume=1802 |pages=1–10 |year=2018 |doi=10.1007/978-1-4939-8546-3_1 |pmid=29858798}}</ref>, and analyzing mutations in oncogenes to customize cancer treatments.<ref name="LodaPoly94">{{cite journal |title=Polymerase chain reaction-based methods for the detection of mutations in oncogenes and tumor suppressor genes |journal=Human Pathology |author=Loda, M. |volume=25 |issue=6 |pages=564–71 |year=1994 |doi=10.1016/0046-8177(94)90220-8 |pmid=7912220}}</ref> However, the method has also been applied to [[forensic science]]<ref name="NinfaFund09">{{Cite book |url=https://books.google.com/books?id=k6_XQwAACAAJ&pg=PA408 |title=Fundamental Laboratory Approaches for Biochemistry and Biotechnology |author=Ninfa, A.J.; Ballou, D.P.; Benore, M. |publisher=Wiley |year=2009 |pages=408–410 |isbn=9780470087664 |accessdate=08 April 2020}}</ref> and [[epidemiology]].<ref name="HamborskyEpidem15">{{cite book |title=Epidemiology and Prevention of Vaccine-Preventable Diseases |editor=Hamborsky, J.; Kroger, A.; Wolfe, C. |edition=13th |publisher=Centers for Disease Control and Prevention |year=2015 |url=https://www.cdc.gov/vaccines/pubs/pinkbook/index.html |accessdate=08 April 2020}}</ref>
 
PCR and its variations have been used to characterize and detect infectious disease organisms such as human immunodeficiency virus (HIV), pathogenic tuberculosis bacteria, and ''Bordetella pertussis'', which causes whooping cough.<ref name="BuckinghamMolec19">{{cite book |url=https://books.google.com/books?hl=en&lr=&id=dJWNDwAAQBAJ&pg=301 |chapter=Chapter 11: Detection and Identification of Microorganisms |title=Molecular Diagnostics: Fundamentals, Methods and Clinical Applications |author=Buckingham, L. |edition=3rd |pages=301–343 |year=2019 |publisher=F.A. Davis Company |isbn=9780803699540}}</ref> Additionally, a selection of viruses can have their RNA detected using PCR, though the primers (short single-strand DNA fragments) used in the process must by sympathetic to the virus' genetic structure to ensure that only target virus material is amplified.<ref name="KimMRPrimer17">{{cite journal |title=MRPrimerV: A database of PCR primers for RNA virus detection |journal=Nucleic Acids Research |author=Kim, H.; Kang, N.; An, K. et al. |volume=45 |issue=D1 |pages=D475–81 |year=2017 |doi=10.1093/nar/gkw1095 |pmid=27899620 |pmc=PMC5210568}}</ref> As it turns out, coronaviruses are RNA viruses, having some of the longest genomes of any RNA virus, and, detrimentally, the highest known frequency of recombination (the exchange of genetic material with another organism); this broadly means high rates of virus mutation, which interferes with maintaining consistent diagnostic detection and therapy.<ref name="MakinHowCorona20">{{cite web |url=https://www.scientificamerican.com/article/how-coronaviruses-cause-infection-from-colds-to-deadly-pneumonia1/ |title=How Coronaviruses Cause Infection—from Colds to Deadly Pneumonia |author=Makin, S. |work=Scientific American |date=05 February 2020 |accessdate=08 April 2020}}</ref><ref name="Rohde2019_20">{{cite web |url=https://asm.org/Articles/2020/January/2019-Novel-Coronavirus-2019-nCoV-Update-Uncoating |title=2019 Novel Coronavirus (2019-nCoV) Update: Uncoating the Virus |author=Rohde, R. |publisher=American Society for Microbiology |date=31 January 2020 |accessdate=08 April 2020}}</ref>
 
PCR comes in several variant methods. For example, while PCR monitors the amplification portion at the end of the overall process, real-time or "quantitative" PCR (qPCR) allows for the generation rate of the amplified product to be monitored at particular point during each PCR cycle. Reverse transcription PCR (RT-PCR) is a combinatory process, applying reverse transcription (creating complementary double-stranded DNA &#91;cDNA&#93; from an RNA template) with PCR. If RT-PCR incorporates qPCR, you end up with "real-time RT-PCR" (rRT-PCR), sometimes referred to as "quantitative RT-PCR" (qRT-PCR). In the case of using PCR for detecting coronaviruses, more often than not we see some variation of RT-PCR, with or without real-time amplification monitoring. (It's important to not asume all RT-PCR processes incorporate qPCR.)
 
How does PCR work in practice? The simplified version (see this [https://doi.org/10.1001/jama.2020.5388 JAMA Patient Page] for a useful graphical explanation, using COVID-19 as an example) has a clinician obtaining a biological specimen from the appropriate location or source material, followed by special techniques to isolate viral (or in some cases, bacterial) genetic material from the specimen. (If RT-PCR is performed, the next step of reverse transcription of the isolated viral RNA into cDNA is also performed.) Once the viral genetic material is isolated, suitable primers that are sympathetic to the structure of the isolated genetic material are introduced. Those primers bind to the virus' genetic material and begins making copies of it. Fluorescent or other biomarkers that were attached to the copies during the PCR process eventually release from the copies, and an attempt is made to detect the presence of those biomarkers. The presence or absence of these markers drives the determination of a positive or negative detection for the sought-after virus.<ref name="HadayaTesting20">{{cite journal |title=Testing Individuals for Coronavirus Disease 2019 (COVID-19) |journal=JAMA |author=Hadaya, J.; Schumm, M.; Livingston, E.H. |year=2020 |doi=10.1001/jama.2020.5388 |pmid=32236503}}</ref>
[[File:Fig2 Foysal Sensors2019 19-21.png|right|thumb|430px|('''a''') Sample LFA strip and ('''b''') region of interest of an LFA strip with an analyte. The intensity and density of red color in the test line region determine the amount of analyte in the sample. ([https://doi.org/10.3390/s19214812 From Foysal ''et al.'' 2019])]]
====2.1.3 Lateral flow assay (LFA)====
The lateral flow assay or LFA is another molecular biology method for detecting the presence of a target analyte in specimen material. In comparison to PCR has the advantages of being more rapid, low-cost, easy-to-use, and applicable at the point of care, though the average LFA is at best semi-quantitative in its results and has slightly lower sensitivity.<ref name="KoczulaLateral16">{{cite journal |title=Lateral flow assays |journal=Essays in Biochemistry |author=Koczula, K.M.; Gallotta, A. |volume=60 |issue=1 |pages=111–20 |year=2016 |doi=10.1042/EBC20150012 |pmid=27365041 |pmc=PMC4986465}}</ref><ref name="LiuPaper18">{{cite book |url=https://books.google.com/books?id=jSk0DwAAQBAJ&pg=PA183 |chapter=Chapter 8: Paper-Based Immunoassays |title=Handbook of Immunoassay Technologies: Approaches, Performances, and Applications |author=Liu, Z.; Hu, J.; Qu, Z.; Xu, F. |editor=Vashist, S.K.; Luong, J.H.T. |publisher=Academic Press |pages=183–202 |year=2018 |isbn=9780128117620 |accessdate=08 April 2020}}</ref> The method involves a celullose-based strip with an ordered collection of specific "pads" and reagents that are reactive to a target analyte in a liquid, which is placed on the strip and moves across the various reagents using capillary and electrostatic interactions.<ref name="KoczulaLateral16" /><ref name="Jauset-RubioUltra16">{{cite journal |title=Ultrasensitive, rapid and inexpensive detection of DNA using paper based lateral flow assay |journal=Scientific Reports |author=Jauset-Rubio, M.; Svobodová, M.; Mairal, T. et al. |volume=6 |at=37732 |year=2016 |doi=10.1038/srep37732 |pmid=27886248 |pmc=PMC5123575}}</ref><ref name="FoysalAnalyte19">{{cite journal |title=Analyte Quantity Detection from Lateral Flow Assay Using a Smartphone |journal=Sensors |author=Foysal, K.H.; Seo, S.E.; Kim, M.J. et al. |volume=19 |issue=21 |at=4812 |year=2019 |doi=10.3390/s19214812 |pmid=31694281 |pmc=PMC6864604}}</ref> LFA has been used in molecular diagonstics for testing urine, saliva, sweat, serum, plasma, and other biological fluids for the presence of specific antigens and antibodies, as well as signs of gene amplification. The method has also been effectively applied to other industries outside healthcare, including the food and beverage, chemical, and environmental industries.<ref name="KoczulaLateral16" />
 
In the realm of infectious disease, the LFA has played an important role in disease diagnosis and control, particularly in resource-constrained settings where resources are limited and point-of-care testing is critical to filling the gap.<ref name="HanafiahDevelop17">{{cite journal |title=Development of Multiplexed Infectious Disease Lateral Flow Assays: Challenges and Opportunities |journal=Diagnostics |author=Hanafiah, K.M.; Arifin, N.; Bustami, T. et al. |volume=7 |issue=3 |at=51 |year=2017 |doi=10.3390/diagnostics7030051 |pmid=28880218 |pmc=PMC5617951}}</ref> Testing for the presence of an infectious agent in body fluids using LFA can be one of two ways: lateral flow immunoassay (LFI) or lateral flow nucleic acid (LFNA). The immunoassay variant looks for antibodies created as a result of the presence of an infectious agent, whereas the nucleic acid variant is built to detect an amplified nucleic acid sequence specific to a target infectious agent.<ref name="NgomDevelop10">{{cite journal |title=Development and application of lateral flow test strip technology for detection of infectious agents and chemical contaminants: A review |journal=Analytical and Bioanalytical Chemistry |author=Ngom, B.; Guo, Y.; Wang, X.; Bi, D. |volume=397 |pages=1113–1135 |year=2010 |doi=10.1007/s00216-010-3661-4 |pmid=20422164}}</ref> Speaking specifically to the SARS-CoV-2 coronavirus, the antibody-based immunoassay method of lateral flow is predominanately used, targeting one of either a monoclonal antibody directed at a viral antigen, or a viral antigen that is recognizable by a patient's developed antibodies.<ref name="SheridanFast20">{{cite web |url=https://www.nature.com/articles/d41587-020-00010-2 |title=Fast, portable tests come online to curb coronavirus pandemic |author=Sheridan, C. |work=Nature Biotechnology - News |date=23 March 2020 |accessdate=08 April 2020 |doi=10.1038/d41587-020-00010-2}}</ref><ref name="RBCoronavirus20">{{cite web |url=https://www.raybiotech.com/index.php?dispatch=attachments.getfile&attachment_id=3095 |format=PDF |title=Novel Coronavirus (SARS-CoV-2) IgM Antibody Detection Kit (Colloidal Gold Method) |publisher=RayBiotech |date=03 April 2020 |accessdate=08 April 2020}}</ref>
 
Testing using LFI is generally as follows. A specialized adsorbant sample pad at one of the LFI strip receives the specimen material. That material then migrates to the next conjugate release pad, where the specimen material is exposed to "antibodies that are specific to the target analyte and are conjugated to coloured or fluorescent particles."<ref name="KoczulaLateral16" /> The material then progresses to a detection zone containing antibodies or antigens that are fixed in the zone and intended to react to a specific analyte. If the analyte is present, a test line produces a visual, qualitative response, and a control line ensures proper liquid flow across the strip. A wicking pad at the other end properly keeps the flow of liquids across the strip.<ref name="KoczulaLateral16" />
 
 
===2.2 Testing conducted on previous coronaviruses===
 
====2.2.1 Severe acute respiratory syndrome (SARS)====
[[Severe acute respiratory syndrome]], otherwise known as SARS, arose in South China in late 2002. Caused by the SARS caronavirus (SARS-CoV) and believed to have originated from horseshoe bats<ref name="McKieScientists17">{{cite web |url=https://www.theguardian.com/world/2017/dec/10/sars-virus-bats-china-severe-acute-respiratory-syndrome |title=Scientists trace 2002 Sars virus to colony of cave-dwelling bats in China |author=McKie, R. |work=The Guardian |date=09 December 2017 |accessdate=03 April 2020}}</ref>, SARS eventually was contained in the summer of 2003. The last known infection was in April 2004, due to a laboratory accident.<ref name="NormileMounting04">{{cite journal |title=Mounting Lab Accidents Raise SARS Fears |journal=Science |author=Normile, D. |volume304 |issue=5671 |pages=659–61 |year=2004 |doi=10.1126/science.304.5671.659 |pmid=15118129}}</ref> During that time, the following sample collection and test procedures evolved from the related outbreaks (note that this is only a summary; consult the cited literature directly for full details)<ref name="NYSDHLab04">{{cite web |url=https://www.health.ny.gov/diseases/communicable/sars/sars_reporting/attachment_6_dear_doctor_lab.htm |title=Laboratory Testing for SARS |author=New York State Department of Health |publisher=State of New York |date=February 2004 |accessdate=03 April 2020}}</ref><ref name="CDCSevere04">{{cite web |url=https://www.cdc.gov/sars/guidance/f-lab/downloads/F-lab-full.pdf |format=PDF |title=Public Health Guidance for Community-Level Preparedness and Response to Severe Acute Respiratory Syndrome (SARS), Version 2 - Supplement F: Laboratory Guidance |author=Centers for Disease Control and Prevention |publisher=Centers for Disease Control and Prevention |date=21 May 2004 |accessdate=03 April 2020}}</ref><ref name="KnoblerLearning04">{{cite book |chapter=Appendix C: In the absence of SARS-CoV transmission worldwide: Guidance for surveillance, clinical and laboratory evaluation, and reporting |title=Learning from SARS: Preparing for the Next Disease Outbreak |editor=Knobler, S.; Mahmoud, A.; Lemon, S. et al. |publisher=National Academies Press |pages=292–302 |year=2004 |isbn=9780309182157 |doi=10.17226/10915}}</ref><ref name="WHO_SARSInt04">{{cite web |url=http://www.who.int/csr/resources/publications/en/SARSReferenceLab.pdf |title=WHO SARS International Reference and Verification Laboratory Network: Policy and Procedures in the Inter-Epidemic Period |author=World Health Organization |publisher=World Health Organization |date=23 January 2004 |accessdate=03 April 2020}}</ref><ref name="LiangLab04">{{cite journal |title=Laboratory Diagnosis of Four Recent Sporadic Cases of Community-acquired SARS, Guangdong Province, China |journal=Emerging Infectious Diseases |author=Liang, G.; Chen, Q.; Xu, J. et al. |volume=10 |issue=10 |pages=1774–81 |year=2004 |doi=10.3201/eid1010.040445 |pmid=15504263 |pmc=PMC3323270}}</ref>:
 
* Determine that the patient is indicating clinical and/or epidemiological evidence of SARS (meets case definitions). As Knobler ''et al.'' put it: "SARS-CoV testing should be considered if no alternative diagnosis is identified 72 hours after initiation of the clinical evaluation and the patient is thought to be at high risk for SARS-CoV disease (e.g., is part of a cluster of unexplained pneumonia cases)."<ref name="KnoblerLearning04" />
 
* Collect multiple specimen types at different time points of the patient's illness. Respiratory and plasma or serum specimens should be collected early into the first week of illness. Respiratory samples should be from [[Nasopharyngeal swab|nasopharyngeal aspirates and swabs]] in the upper respiratory tract, or in some cases fluids from the lower respiratory tract using [[bronchoalveolar lavage]], tracheal aspiration, or a pleural tap. (Sputum can also be collected.) Whole blood (5 to 10 ml) is collected into either a serum separator tube for blood serum or EDTA tube for blood plasma. Stool samples are also of import early on for virus isolation or detection and are useful in at least the first and second weeks of the illness. Blood serum is usefull in weeks two and three for detecting a rising titre. Additionally, the literature also makes reference to methods of collecting specimens post-mortum.
 
* Conduct testing. At the time, the two primary test types used were enzyme immunoassay (EIA; today more commonly known as [[ELISA]]<ref name="LequinEnzyme05">{{cite journal |title=Enzyme Immunoassay (EIA)/Enzyme-Linked Immunosorbent Assay (ELISA) |journal=Clinical Chemistry |author=Lequin, R.M. |volume=51 |issue=12 |pages=2415–18 |year=2005 |doi=10.1373/clinchem.2005.051532 |pmid=16179424}}</ref>) for detection of serum antibody and reverse transcription polymerase chain reaction (RT-PCR) for detection of the virus' RNA. The U.S. Centers for Disease Control and Preventions had this to say about these tests in May 2004<ref name="CDCSevere04" />:
 
<blockquote>Both the EIA and the RT-PCR tests are sensitive and highly specific for SARS-CoV. The ability to diagnose SARS-CoV infection in a patient is often limited, however, by either the low concentration of virus in most clinical specimens (RT-PCR assays) or the time it takes a person to mount a measurable antibody response to SARS-CoV (serologic assays). The likelihood of detecting infection is increased if multiple specimens (e.g., stool, serum, respiratory tract specimens) are collected at several times during the course of illness.</blockquote>
 
:The literature also makes reference to an [[Immunofluorescence|immunofluorescence assay]] (IFA) for detecting antibody, with the CDC calling its results "essentially identical to those for the EIA for SARS antibody."<ref name="CDCSevere04" /> Tangentially, isolation of SARS-CoV in cell culture from a clinical specimen is also referenced, though such activity is reserved for [[Biosafety level|Biosafety Level 3]] (BSL-3) laboratories.
 
* Confirm the results. Laboratory confirmation is based on one of 1. initial local lab detection and subsequent national reference lab confirmation of a validated serology-based test detection; 2. isolation of SARS-CoV in cell culture with subsequent confirmation from a validated test; or 3. initial local lab detection and subsequent national reference lab confirmation of SARS-CoV RNA from a validated RT-PCR test which used either two clinical specimens from different sources or two same-source clinical specimens from two different days.
 
:Additionally, in the case of serology, one of the following must be true:
# SARS-CoV serum antibodies are detected in a single serum specimen; or,
# a "four-fold or greater increase in SARS-CoV antibody titer between acute- and convalescent-phase serum specimens tested in parallel"<ref name="CDCSevere04" /> is detected; or,
# a "negative SARS-CoV antibody test result on acute-phase serum and positive SARS-CoV antibody test result on convalescent-phase serum tested in parallel"<ref name="CDCSevere04" /> is detected.
 
:Of note is the WHO's January 2004 cautionary message about serological diagnostics in not only SARS-CoV but other types of coronaviruses. At that time, they showed a level of unsureness in regards to how coronaviruses elicited serological cross-reactions and generated antigenic recall. They also preached caution in interpreting serological results in non-epidemic periods and when no viral sequence data are available. Finally, they also mentioned the added difficulties of rate cases when coinfection with a related human coronavirus occurs, "although the use of expressed proteins in Western blots may help to sort this out."<ref name="WHO_SARSInt04" /> More than 15 years later, Loeffelholz and Tang put this concept into clearer terms, indicating that while "serological assays are not routinely used for diagnosis of &#91;human coronavirus&#93; infections due to the lack of commercial reagents," they still have important value "for understanding the epidemiology of emerging &#91;human cornaviruses&#93;, including the burden and role of asymptomatic infections," as well as for antibody detection of novel and emerging coronaviruses.<ref name="LoeffelholzLab20">{{cite journal |title=Laboratory diagnosis of emerging human coronavirus infections – The state of the art |journal=Emerging Microbes & Infections |author=Loeffelholz, M.J.; Tang, T.-W. |volume=9 |issue=1 |pages=747–56 |year=2020 |doi=10.1080/22221751.2020.1745095 |pmid=32196430}}</ref>
 
* Arrange for confirmatory testing to be performed by an appropriate test site in the case of a positive RT-PCR test.
 
* Report to state or local health departments details of patients radiographically confirmed with pneumonia with at least one SARS-CoV risk factor for exposure, clusters of healthcare workers with unexplained pneumonia, and any positive SARS-CoV test results. Additional international reporting of SARS by WHO Member States in regards to probable and laboratory-confirmed cases is also requested.
 
* Send off for an additional verification by an external member of the WHO's SARS Reference and Verification Laboratory Network before internationally announcing results as a laboratory-confirmed case.
 
====2.2.2 Middle East respiratory syndrome (MERS)====
[[File:MERS-CoV Particles (8414774264).jpg|left|thumb|Colorized transmission electron micrograph showing particles of the Middle East respiratory syndrome coronavirus that emerged in 2012]]Unlike SARS, Middle East respiratory syndrome, or MERS, continues to appear in the human population. Since its appearance in 2012, several thousand laboratory-confirmed cases of MERS have been reported to the WHO.<ref name="Bernard-StoecklinCompar19">{{cite journal |title=Comparative Analysis of Eleven Healthcare-Associated Outbreaks of Middle East Respiratory Syndrome Coronavirus (Mers-Cov) from 2015 to 2017 |journal=Scientific Reports |author=Bernard-Stoecklin, S.; Nikolay, B.; Assiri, A. et al. |volume=9 |at=7385 |year=2019 |doi=10.1038/s41598-019-43586-9 |pmid=31089148 |pmc=PMC6517387}}</ref> The virus MERS-CoV is believed to have originated from bats, which at some unknown point spread to Dromedary camels. Approximately 55 percent of MERS-CoV infections have come from direct contact with such camels, thought it's not entirely clear how the rest of known cases have been caused<ref name="BanerjeeBats19">{{cite journal |title=Bats and Coronaviruses |journal=Viruses |author=Banerjee, A.; Kulcsar, K.; Misra, V. et al. |volume=11 |issue=1 |at=E41 |year=2019 |doi=10.3390/v11010041 |pmid=30634396 |pmc=PMC6356540}}</ref> (Alshukairi ''et al.'' suggest asymptomatic or mildly symptomatic camel workers may serve as a possible transmission source<ref name="AlshukairiHigh18">{{cite journal |title=High Prevalence of MERS-CoV Infection in Camel Workers in Saudi Arabia |journal=mBio |author=Alshukairi, A.N.; Zheng, J.; Zhao, J. et al. |volume=9 |issue=5 |pages=e01985-18 |year=2018 |doi=10.1128/mBio.01985-18 |pmid=30377284 |pmc=PMC6212820}}</ref>). The following sample collection and test procedures have evolved from working with the MERS-CoV virus (note that this is only a summary; consult the cited literature directly for full details)<ref name="CDCLabTestMERS19">{{cite web |url=https://www.cdc.gov/coronavirus/mers/lab/lab-testing.html |title=CDC Laboratory Testing for Middle East Respiratory Syndrome Coronavirus (MERS-CoV) |author=Centers for Disease Control and Prevention |publisher=Centers for Disease Control and Prevention |date=02 August 2019 |accessdate=04 April 2020}}</ref><ref name="CDCInterimMERS19">{{cite web |url=https://www.cdc.gov/coronavirus/mers/guidelines-clinical-specimens.html |title=Interim Guidelines for Collecting, Handling, and Testing Clinical Specimens from Persons Under Investigation (PUIs) for Middle East Respiratory Syndrome Coronavirus (MERS-CoV) – Version 2.1 |author=Centers for Disease Control and Prevention |publisher=Centers for Disease Control and Prevention |date=02 August 2019 |accessdate=04 April 2020}}</ref><ref name="WHOLabMERS18">{{cite web |url=https://www.who.int/csr/disease/coronavirus_infections/mers-laboratory-testing/en/ |title=Laboratory testing for Middle East Respiratory Syndrome Coronavirus: Interim guidance |work=WHO/MERS/LAB/15.1/Rev1/2018 |author=World Health Organization |publisher=World Health Organization |date=January 2018 |accessdate=04 April 2020}}</ref><ref name="Al-AbdelyMiddle19">{{cite journal |title=Middle East Respiratory Syndrome Coronavirus Infection Dynamics and Antibody Responses among Clinically Diverse Patients, Saudi Arabia |journal=Emerging Infectious Diseases |author=Al-Abdely, H.M.; Midgley, C.M.; Alkhamis, A.M. et al. |volume=25 |issue=4 |pages=753-766 |year=2019 |doi=10.3201/eid2504.181595}}</ref><ref name="Kelly-CirinoAnUpdated19">{{cite journal |title=An updated roadmap for MERS-CoV research and product development: focus on diagnostics |journal=BMJ Global Health |author=Kelly-Cirino, C.; Mazzola, L.T.; Chua, A. et al. |volume=4 |issue=Suppl. 2 |at=e001105 |year=2019 |doi=10.1136/bmjgh-2018-001105 |pmid=30815285 |pmc=PMC6361340}}</ref>:
 
* Determine that the patient is indicating clinical and/or epidemiological evidence of MERS (meets case definitions). "Testing for other respiratory pathogens using routinely available laboratory procedures, as recommended in local management guidelines for community-acquired pneumonia, should also be performed but should not delay testing for MERS-CoV."<ref name="WHOLabMERS18" />
 
* Collect at a minumum both lower respiratory and upper respiratory tract samples. Lower respiratory tract specimens are typically the most revealing, as they have been shown to contain the highest viral load (due to the expression of the virus's cellular receptor DPP4 in the lower respiratory system). Bronchoalveolar lavage, tracheal aspiration, or a pleural tap can be used to collect specimens from the lower respiratory tract. (Sputum can also be collected.) Upper respiratory tract specimens (in this case, both a nasopharyngeal and an oropharyngeal swab are recommended) are also valuable in diagnosis, though extra care should be taken to ensure nasopharyngeal swabs gather secretions from the [[Pharynx#Nasopharynx|nasopharynx]] and not just the nostril. Nasopharyngeal aspiration is also an acceptable sample collection method for the upper respiratory tract.
 
:Regarding serum specimens, slight differences in guidance appear between WHO guidance and CDC guidance. The WHO appears to differentiate between symptomatic and asymptomatic patient testing, wheras the U.S. CDC seems to only indirectly differentiate the two. The WHO suggests if testing symptomatic patients, stick with lower and upper respiratory tract specimens, which will be tested using nucleic acid amplification (molecular) testing (NAAT). Serological testing of serum specimens should be used for symptomatic patients "only if NAAT is not available."<ref name="WHOLabMERS18" /> If this is the case, the WHO recommends paired samples, one collected within the first week of illness and the second about three to four weeks later. For asymptomatic patients in high-contact outbreak scenarios, the WHO recommends all three sample types (with respiratory samples taken preferably within 14 days of last documented contact).
 
:The current CDC guidance differentiates between molecular testing for active infections and serology for previous infections. The CDC adds that "MERS-CoV serology tests are for surveillance or investigational purposes and not for diagnostic purposes."<ref name="CDCLabTestMERS19" /> Whether or not to collect a serum specimen in MERS diagnostics may depend on the assay used, however. For example, the CDC, in its Version 2.1 guidance, indicates that testing using the CDC MERS rRT-PCR assay requires collection of serum in addition to upper and lower respiratory tract specimens. For that specific assay, the CDC differentiates between patients who've had symptom onset less than 14 days prior and those who've had it 14 days or later: if prior, serology is for the rRT-PCR test, and if later, serology is for antibody testing. In either case, 200 µL of serum is required.
 
* Conduct testing. NAAT methods like real-time reverse-transcription polymerase chain reaction (rRT-PCR) assays have been the most common tool for diagnosing MERS-CoV infection due to their high sensitivity. According to late 2018 research by Kelly-Cirino ''et al.'', at least 11 commercial single assay and five commercial multiplex assay kits are available (see [https://gh.bmj.com/content/bmjgh/4/Suppl_2/e001105/DC1/embed/inline-supplementary-material-1.pdf Table S1], a PDF file, from their highly relevant paper), perhaps more as of April 2020. Serological antibody detection is performed using ELISA, [[Immunofluorescence#Secondary (indirect)|indirect immunofluorescence]] (IIF), and [[Neutralisation (immunology)|microneutralization]].
 
* Confirm the results. Laboratory confirmation of MERS-CoV infection is the same for both the WHO and the CDC: one of either a validated NAAT test providing a positive result for at least two different genomic targets, or a validated NAAT test providing a positive result for a specific genomic target along with sequencing confirmation of a separate genomic target. Persons under investigation who receive one negative NAAT result on a recommended specimen is considered to be negative for active MERS-CoV infection. The laboratory should consider testing additional specimens after the first negative. The CDC considers known MERS patients to be negative for active MERS-CoV infection after two consecutive negative NAAT tests on all specimens. The WHO adds: "A patient with a positive NAAT result for a single specific target without further testing but with a history of potential exposure and consistent clinical signs is considered a probable case."<ref name="WHOLabMERS18" /> The WHO also has additional guidance on using serology for confirming MERS-CoV infection for purposes of reporting under the International Health Regulations.
 
* Report using national reporting requirements. More broadly, state or local health departments should receive details about received specimens to be tested for MERS-CoV, even before testing begins. Regardless of result, the final positive or negative laboratory confirmation should also be reported to national authorities. If the infection becomes widespread, updates for each new confirmed case or suspected positive should also be made.
 
====2.2.3 The common cold====
Approximately 10 to 15 percent of cases of what we call the "common cold" are associated with an endemic coronavirus, of which are two distinct groups: HCoV-229E and HCoV-OC43.<ref name="WatTheCommon04">{{cite journal |title=The common cold: A review of the literature |journal=European Journal of Internal Medicine |author=Wat, D. |volume=15 |issue=2 |pages=79–88 |year=2004 |doi=10.1016/j.ejim.2004.01.006 |pmid=15172021}}</ref> Disease symptoms associated with these coronaviruses—typically in the form of respiratory infection and the symptoms that come with it—by themselves are typically mild<ref name="LoeffelholzLab20" />, and laboratory testing isn't necessarily indicated for those immunocompetent individuals capable of self-limiting.<ref name="BabadyMulti18">{{cite journal |title=Multicenter Evaluation of the ePlex Respiratory Pathogen Panel for the Detection of Viral and Bacterial Respiratory Tract Pathogens in Nasopharyngeal Swabs |journal=Journal of Clinical Microbiology |author=Babady, N.E.; England, M.R.; Jurcic Smith, K.L. et al. |volume=56 |issue=2 |at=e01658-17 |year=2018 |doi=10.1128/JCM.01658-17 |pmid=29212701 |pmc=PMC5786739}}</ref> However, symptom overlap with pharyngitis and bronchitis, as well as the complication of pharyngitis and sinusitis also potentially having bacterial origin, can complicate clinical diagnosis. Additionally, as more antivirals that target a specific virus are created, and as concerns of unnecessarily using antibiotics to treat viral diseases grows<ref name="JenisonRapid16">{{cite web |url=https://www.statnews.com/2016/11/30/antibiotic-resistance-molecular-diagnostics/ |title=Rapid lab tests can help reduce antibiotic resistance |author=Jenison, R. |work=STAT |date=30 November 2016 |accessdate=03 April 2020}}</ref><ref name="RoyRapid18">{{cite web |url=https://www.healio.com/infectious-disease/antimicrobials/news/online/%7B226c31f3-1d8e-4ffe-82b1-654cb37303c4%7D/rapid-test-for-viral-infections-reduces-unnecessary-antibiotic-prescribing |title=Rapid test for viral infections reduces unnecessary antibiotic prescribing |author=Roy, K. |work=Healio |date=26 September 2018 |accessdate=03 April 2020}}</ref>, laboratory methods of respiratory virus diagnosis—particularly for those who are immunocompromised—have value.<ref name="WatTheCommon04" /><ref name="BabadyMulti18" />
 
RT-PCR, a molecular method, have been used for well over a decade for detecting coronaviruses.<ref name="WatTheCommon04" /><ref name="MahonyDetect08">{{cite journal |title=Detection of Respiratory Viruses by Molecular Methods |journal=Clinical Microbiology Reviews |author=Mahoney, J.B. |volume=21 |issue=4 |pages=716–47 |year=2008 |doi=10.1128/CMR.00037-07 |pmid=18854489 |pmc=PMC2570148}}</ref> However, as molecular methods of analysis have expanded over the years, more rapid solutions for testing have been developed. For example, the GenMark ePlex rapid multiplex molecular diagnostics instrument and the ePlex Respiratory Pathogen Panel were evaluated in a multicenter trial by Babady ''et al.'' in 2017.<ref name="BabadyMulti18" /> The panel is capable of testing for the presence of 15 viral types—including the -229E, -OC43, and two other coronaviruses—and two bacterial types in nasopharyngeal swab specimens, with results in typically less than two hours.<ref name="BabadyMulti18" /> The costs associated with these sorts of tests, compared to their benefits, likely limits ubiquitous use at the first sign of a cold<ref name="BabadyMulti18" />, but as molecular diagnostic technologies become more compact and easy-to-use, testing for infection by endemic human coronaviruses may become slightly more commonplace. However, as the authors point out, with no treatment for these endemic coronaviruses, any additional utility beyond diagnosing an illness as viral rather than bacterial would primarily be found in epidemiological studies of the associated genotyping data.<ref name="BabadyMulti18" />
 
 
===2.3 Organizational and agency guidance on COVID-19 testing===
''NOTE: Information shown here may rapidly become outdated given how quickly response to pandemic testing can change. A full attempt to keep the content relavent will be made.''
 
[[File:CDC COVID-19 test kit.jpg|right|thumb|430px|CDC 2019-nCoV Real-time RT-PCR Panel (Research Use Only)]]Laboratory guidance for testing for SARS-CoV-2 has been relatively quick to evolve. The timely development and organized use of accurate assays and meaningful screening protocols, however, has been inconsistent worldwide, with some countries more urgently and agilely responding than others.<ref name="SubbaramanCorona20">{{cite web |url=https://www.nature.com/articles/d41586-020-00827-6 |title=Coronavirus tests: Researchers chase new diagnostics to fight the pandemic |author=Subbaraman, N.; Callaway, E. |work=Nature - News Explainer |date=23 March 2020 |accessdate=05 April 2020 |doi=10.1038/d41586-020-00827-6}}</ref><ref name="ApuzzoCant20">{{cite web |url=https://www.nytimes.com/2020/03/20/world/europe/coronavirus-testing-world-countries-cities-states.html |title=Can’t Get Tested? Maybe You’re in the Wrong Country |author=Apuzzo, M.; Gebrekidan, S. |work=The New York Times |date=20 March 2020 |accessdate=05 April 2020}}</ref><ref name="HindsleyTheLost20">{{cite web |url=https://www.nytimes.com/2020/03/28/us/testing-coronavirus-pandemic.html |title=The Lost Month: How a Failure to Test Blinded the U.S. to COVID-19 |author=Hindsley, G. |work=The New York Times |date=28 March 2020 |accessdate=05 April 2020}}</ref> Of course with any novel virus, clinicians and public health experts are dealing with unknown factors. However, public health organizations and agencies have had a base to work from when creating laboratory testing guidance for a novel coronavirus, with more than 40 years of experience with coronavirus biology, pathogenesis, and diagnosis.<ref name="DenisonCorona04">{{cite book |chapter=Coronavirus Research: Keys to Diagnosis, Treatment, and Prevention of SARS |title=Learning from SARS: Preparing for the Next Disease Outbreak |author=Denison, M.R. |publisher=Institute of Medicine |pages=137–72 |year=2004 |isbn=9780309182157 |doi=10.17226/10915 |url=https://www.nap.edu/read/10915/chapter/5}}</ref> And while there are fundamental differences between SARS-CoV-2 and its predecessor SARS-CoV, they still share approximately 70 to 80 percent of their genetic code.<ref name=CeccarelliDiff20">{{cite journal |title=Differences and similarities between Severe Acute Respiratory Syndrome (SARS)-CoronaVirus (CoV) and SARS-CoV-2. Would a rose by another name smell as sweet? |journal=European Review for Medical and Pharmacological Sciences |author=Ceccarelli, M.; Berretta, M.; Venanzi Rullo, E. et al. |volume=24 |issue=5 |pages=2781-2783 |year=2020 |doi=10.26355/eurrev_202003_20551 |pmid=32196628}}</ref><ref name=Wilder=SmithCanWe20">{{cite journal |title=Can we contain the COVID-19 outbreak with the same measures as for SARS? |journal=The Lancet Infectious Diseases |author=Wilder-Smith, A.; Chiew, C.J.; Lee, V.J. |year=2020 |doi=10.1016/S1473-3099(20)30129-8 |pmid=32145768 |pmc=PMC7102636}}</ref> In fact, the WHO had draft guidance for laboratory testing out as early as January 10, 2020, before gene sequencing was even completed.<ref name="WHOLabJan20">{{cite web |url=https://apps.who.int/iris/bitstream/handle/10665/330374/WHO-2019-nCoV-laboratory-2020.1-eng.pdf |title=Laboratory testing of human suspected cases of novel coronavirus (nCoV) infection: Interim guidance 10 January 2020 |work=WHO/2019-nCoV/laboratory/2020.1 |author=World Health Organization |publisher=World Health Organization |date=10 January 2020 |accessdate=05 April 2020}}</ref> This guidance and similar draft guidance from national public health organizations and agencies has received steady revisions since as understanding of the virus has grown.
 
Similar to its predecessors SARS-CoV and MERS-CoV, RT-PCR is being recommended in guidance for detecting SARS-CoV-2's RNA in specimens and thus laboratory confirmation of COVID-19 cases. Serology has its place in testing as well, though with similar lessons from SARS and MERS that it's best used to test for past infection (typically after 14 days of suspected contact with a carrier, or mild symptoms) and thus potential short-term immunity due to the presence of antibodies in blood. In its March 19 guidance, the WHO said: "In cases where NAAT assays are negative and there is a strong epidemiological link to COVID-19 infection, paired serum samples (in the acute and convalescent phase) could support diagnosis once validated serology tests are available."<ref name="WHOLabMar20">{{cite web |url=https://apps.who.int/iris/handle/10665/331501 |title=Laboratory testing for coronavirus disease (COVID-19) in suspected human cases: Interim guidance, 19 March 2020 |work=WHO/COVID-19/laboratory/2020.5 |author=World Health Organization, et al. |publisher=World Health Organization |date=19 March 2020 |accessdate=05 April 2020}}</ref> On April 3, the U.S. Food and Drug Administration approved the countries first COVID-19 serology test created by Cellex, though Mayo Clinic was also on the verge of rolling out its own in-house serology test as well<ref name="TerryCellex20">{{cite web |url=https://www.biospace.com/article/fda-approves-1st-covid-19-antibody-test/ |title=Cellex and Mayo Clinic Launch Tests to Determine COVID-19 Immunity from Previous Exposure |author=Terry, M. |work=BioSpace |date=03 April 2020 |accessdate=05 April 2020}}</ref> (Note: Johns Hopkins appears to be maintaining [http://www.centerforhealthsecurity.org/resources/COVID-19/Serology-based-tests-for-COVID-19.html a page] tracking approved serology tests around the world.)
 
The following sample collection and test procedures have evolved from the COVID-19 pandemic (note that this is only a summary; consult the cited literature directly for full details)<ref name="WHOLabMar20" /><ref name="CDCEvalTest20">{{cite web |url=https://www.cdc.gov/coronavirus/2019-nCoV/hcp/clinical-criteria.html |title=Evaluating and Testing Persons for Coronavirus Disease 2019 (COVID-19) |author=Centers for Disease Control and Prevention |publisher=Centers for Disease Control and Prevention |date=24 March 2020 |accessdate=05 April 2020}}</ref><ref name="CDCInterimGuidC19_20">{{cite web |url=https://www.cdc.gov/coronavirus/2019-nCoV/lab/guidelines-clinical-specimens.html |title=Interim Guidelines for Collecting, Handling, and Testing Clinical Specimens from Persons for Coronavirus Disease 2019 (COVID-19) |author=Centers for Disease Control and Prevention |publisher=Centers for Disease Control and Prevention |date=24 March 2020 |accessdate=05 April 2020}}</ref><ref name="UKGovCOVID20">{{cite web |url=https://www.gov.uk/government/publications/wuhan-novel-coronavirus-guidance-for-clinical-diagnostic-laboratories |title=COVID-19: Guidance for sampling and for diagnostic laboratories |author=Public Health England |publisher=U.K Government |date=03 April 2020 |accessdate=05 April 2020}}</ref><ref name="AusGovPHLN20">{{cite web |url=https://www.health.gov.au/resources/publications/phln-guidance-on-laboratory-testing-for-sars-cov-2-the-virus-that-causes-covid-19 |title=PHLN guidance on laboratory testing for SARS-CoV-2 (the virus that causes COVID-19) |author=Public Health Laboratory Network |publisher=Department of Health, Australian Government |date=01 April 2020 |accessdate=05 April 2020}}</ref>:
 
* Determine that the patient is indicating clinical and/or epidemiological evidence of COVID-19 (meets case definitions). Case definitions and testing criteria have initially been strict, but as the CDC notes, as test kit availability ramps up, it "will allow clinicians to consider COVID-19 testing for a wider group of symptomatic patients."<ref name="CDCEvalTest20" /> However, clinicians are still encouraged to consider other causes for respiratory illness. The CDC provides a [https://www.cdc.gov/coronavirus/2019-nCoV/hcp/clinical-criteria.html priority list], making hospitalized patients and symptomatic healthcare workers the top priority, followed by "those who are at highest risk of complication of infection," then "individuals in the surrounding community of rapidly increasing hospital cases." In the future, as more serology options and other resources become available, serological surveys of people who have never been diagnosed (asymptomatic or otherwise) may begin.<ref name="BranswellCDC20">{{cite web |url=https://www.statnews.com/2020/04/04/cdc-launches-studies-to-get-more-precise-count-of-undetected-covid-19-cases/ |title=CDC launches studies to get more precise count of undetected Covid-19 cases |author=Branswell, H. |work=STAT |date=04 April 2020 |accessdate=05 April 2020}}</ref><ref name="JHSerology20">{{cite web |url=http://www.centerforhealthsecurity.org/resources/COVID-19/Serology-based-tests-for-COVID-19.html |title=Serology-based tests for COVID-19 |author=Center for Health Security |publisher=Johns Hopkins University |date=02 April 2020 |accessdate=05 April 2020}}</ref>
 
* Collect at a minumum upper respiratory tract specimens and, whenever possible, lower respiratory tract specimens. Although early to say with certainty, it appears lower respiratory tract specimens such as sputum and bronchoalveolar lavage fluid are typically the most reliable specimen type for RT-PCR applications, as they have been shown to contain the highest viral load, in comparison to upper respirator tract specimens.<ref name="WangDetect20">{{cite journal |title=Detection of SARS-CoV-2 in Different Types of Clinical Specimens |journal=JAMA |author=Wang, W.; Xu, Y.; Gao, R. et al. |year=2020 |doi=10.1001/jama.2020.3786 |pmid=32159775 |pmc=PMC7066521}}</ref><ref name="YuQuant20">{{cite journal |title=Quantitative Detection and Viral Load Analysis of SARS-CoV-2 in Infected Patients |journal=Clinical Infectious Diseases |author=Yu, F.; Yan, L.; Wang, N. et al. |at=ciaa345 |year=2020 |doi=10.1093/cid/ciaa345 |pmid=32221523}}</ref> As Wang ''et al.'' point out, "testing of specimens from multiple sites may improve the sensitivity and reduce false-negative test results,"<ref name="WangDetect20" /> which is largely reflected in WHO, CDC, Public Health England (PHE), and Public Health Laboratory Network (PHLN; Australia) testing guidance.
 
:Slight differences in upper respiratory tract specimen collection procedures can be found between the WHO/CDC and PHE/PHLN. Both the WHO and CDC offer nasopharyngeal and oropharyngeal swabs as options. The WHO doesn't appear to give a preference, wheras the CDC has a preference for nasopharyngeal swabs but maintains oropharyngeal as still remaining "an acceptable specimen type."<ref name="CDCInterimGuidC19_20" /> In comparison, the latest PHE and PHLN guidance prefer the approach of collecting from both pharynx locations—even with the same swab—"to optimise the chances of virus detection."<ref name="AusGovPHLN20" /> Nasopharyngeal aspiration is also an acceptable sample collection method for the upper respiratory tract according to all mentioned entitites, though the PHLN specifies that it is a substitution for only the nasopharyngeal (they now refer to it as "deep nasal") specimen.<ref name="AusGovPHLN20" />
 
:Regarding serum specimens, statements differ slightly. The WHO notes serology to be useful for retrospective case definition, using paired specimens from the acute and convalescent phases of the disease. The CDC doesn't make reference to serum or serology in their clinical specimen guidance. The PHE suggests hospital patients have "a sample for acute serology" taken but say little else.<ref name="UKGovCOVID20" /> The PHLN gives similar advice as the WHO, while emphasizing a need "to facilitate retrospective testing, if this is relevant, once serology tests become available."<ref name="AusGovPHLN20" />
 
* Conduct testing. NAAT methods like rRT-PCR have been the primary tools for diagnosing SARS-CoV-2 infection due to their high sensitivity. The PHLN provides the most background about PCR in their guidance, noting that laboratories in its network are confirmong positive infections "either with RT-PCR assays detecting a different target gene, or broadly reactive PCR tests with sequencing of amplicons."<ref name="AusGovPHLN20" /> The latter option is less common due to long turnaround time. They also note that other zoonotic viruses such as SARS-CoV are capable of being detected from PCR assays, though endemic coronaviruses like -229E won't be. The WHO, CDC, and PHLN underscore the idea that viral cultures for routine diagnoses are not practical and, if attempted, should only be performed in Biosafety Level 3 (BSL-3) laboratories. As of April 5, no specific methods have been suggested for serological antibody detection, though the current set of approved serology tests from around the world appear to use lateral flow immunoassay or [[Neutralisation (immunology)|neutralization]] methods.<ref name="JHSerology20" />
 
* Confirm the results. The strongest public guidance for considering a potential case as being laboratory-confirmed for SARS-CoV-2 infection comes from the WHO. In their guidance, they differentiate between cases by NAAT "in areas with no known COVID-19 virus circulation" and "in areas with established COVID-19 virus circulation." In the first case, one of these conditions must apply: either a validated NAAT test providing a positive result for at least two different genomic targets, or a validated NAAT test providing a positive result for the presences of betacoronavirus along with sequencing confirmation of a separate genomic target, "as long as the sequence target is larger or different from the amplicon probed in the NAAT assay used."<ref name="WHOLabMar20" /> In the latter case of established virus circulation, the WHO notes that "a simpler algorithm might be adopted in which, for example, screening by rRT-PCR of a single discriminatory target is considered sufficient."<ref name="WHOLabMar20" /> However, if testing produces one or more negative results, that doesn't necessarily rule out SARS-CoV-2 infection. If suspicion of infection remains high, particularly if only upper respiratory tract specimens were collected, additional specimens from the lower respiratory tract should be collected and analyzed. They also emphasize that both external and internal controls should be applied to NAAT runs.
 
* Report using national reporting requirements. Regardless of result, the final positive or negative laboratory confirmation should also be reported to state and national authorities. In the U.S., for example, this means reporting to the state health department using the [https://www.cdc.gov/coronavirus/2019-ncov/php/reporting-pui.html CDC's PUI and Case Report Form]. In Canada, reports are sent to the Public Health Agency of Canada (PHAC) via their [https://www.canada.ca/en/public-health/services/diseases/2019-novel-coronavirus-infection/health-professionals/interim-guidance-surveillance-human-infection.html Coronavirus Diseases (COVID-19) Case Report Form].
 
===2.4 Current test methods and their differences===
''NOTE: Information shown here may rapidly become outdated given how quickly response to pandemic testing can change. A full attempt to keep the content relavent will be made.''
 
====2.4.1 Background on the laboratory testing environment====
Before continuing, it should be noted that many elements of the prior-mentioned COVID-19 testing guidance have governmental public health laboratories in mind. However, as the scale of the epidemic has grown, the need for commercial laboratories and assay developers to get involved with increasing analytical testing throughput—through a more rigorous public-private partnership—has become abundantly clear.<ref name="MadrigalPrivate20">{{cite web |url=https://www.theatlantic.com/health/archive/2020/03/next-covid-19-testing-crisis/609193/ |title=Private Labs Are Fueling a New Coronavirus Testing Crisis |author=Madrigal, A.C.; Meyer, R. |work=The Atlantic |date=31 March 2020 |accessdate=07 April 2020}}</ref><ref name="HaleFDAOpens20">{{cite web |url=https://www.fiercebiotech.com/medtech/fda-opens-gates-to-commercial-coronavirus-testing-without-agency-review |title=FDA opens the gates to commercial coronavirus testing without agency review |author=Hale, C. |work=FierceBiotech |date=17 March 2020 |accessdate=07 April 2020}}</ref><ref name="ApplebyWhyIt20">{{cite web |url=https://www.npr.org/sections/health-shots/2020/03/28/822869504/why-it-takes-so-long-to-get-most-covid-19-test-results |title=Why It Takes So Long To Get Most COVID-19 Test Results |author=Appleby, J. |work=NPR - Health Shots |date=28 March 2020 |accessdate=07 April 2020}}</ref><ref name="Ryan-MosleyWhySome20">{{cite web |url=https://www.technologyreview.com/s/615444/covid-19-test-results-faster-commercial-labs-delays-coronavirus/ |title=Why some covid-19 tests in the US take more than a week |author=Ryan-Mosley, T. |work=MIT Technology Review |date=05 April 2020 |accessdate=07 April 2020}}</ref> Even so, at least in the United States, turnaround times have been slow due to a variety of factors, from lack of in-house laboratory resources to handle high test volumes and a slower-than-expected ramping up of test kit production<ref name="MadrigalPrivate20" /><ref name="ApplebyWhyIt20" /><ref name="Ryan-MosleyWhySome20" />, to actually getting diagnostic assays that are more rapid (yet still accurate) in their diagnosis, simpler to use, and useable at the point of care.<ref name="Nguyen2019_20">{{cite journal |title=2019 novel coronavirus disease (COVID-19): Paving the road for rapid detection and point-of-care diagnostics |journal=Micromachines |author=Nguyen, T.; Bang, D.D.; Wolff, A. |volume=11 |issue=3 |at=306 |year=2020 |doi=10.3390/mi11030306 |pmid=32183357}}</ref><ref name="YangPoint20">{{cite journal |title=Point-of-care RNA-based diagnostic device for COVID-19 |journal=Diagnostics |author=Yang, T.; Wang, Y.-C.; Shen, C.-F.; Cheng, C.-M. |volume=10 |issue=3 |at=165 |year=2020 |doi=10.3390/diagnostics10030165}}</ref> The good news is examples of these rapid point-of-care molecular test kits are now becoming available around the globe, including the United States as part of the U.S. Food and Drug Administration's emergency use authorization (EUA) process.
 
As the demand for expanded diagnostic testing grows in the face of a pandemic, it's important to compare the U.S. laboratory testing environments of public health and large commercial testing labs with those of small, in-office clinical labs. In the U.S., all but research-based laboratory testing of human specimens is regulated under the [[Clinical Laboratory Improvement Amendments]] (CLIA), including public health laboratories. CLIA is meant to ensure quality laboratory testing in the country. Seven different criteria are used to gauge and assign one of three complexity levels to laboratory devices and [[assay]]s: high, moderate, and waived.<ref name="CDCTestCom">{{cite web |url=https://www.cdc.gov/clia/test-complexities.html |title=Clinical Laboratory Improvement Amendments (CLIA): Test complexities |author=Centers for Disease Control and Prevention |date=06 August 2018 |accessdate=09 April 2020}}</ref><ref name="FDAIVDReg">{{cite web |url=https://www.fda.gov/medical-devices/ivd-regulatory-assistance/clia-categorizations |title=CLIA Categorizations |publisher=U.S. Food and Drug Administration |date=25 February 2020 |accessdate=09 April 2020}}</ref> Additionally, CLIA mandates clinical laboratories handling specimens originating from the U.S. and its territories to apply for a CLIA certificate that is appropriate for the type of testing it performs. Labs using complex devices and assays would have to apply for a high complexity certificate, and so on. Waived tests are recognized as simple to perform with a low risk of erroneous results and include among others urinalysis for pregnancy and drugs of abuse, blood glucose and cholesterol tests, and fertility analysis.
 
Of the more than 256,000 non-exempt CLIA-registered labs in the U.S., only 33,212 or 13 percent of them are certified to perform moderate- and high-complexity testing.<ref name="CMSEnroll19">{{cite web |url=https://www.cms.gov/Regulations-and-Guidance/Legislation/CLIA/Downloads/statupda.pdf |format=PDF |title=CLIA Update - October 2019 |author=Centers for Medicare and Medicaid Services, Division of Clinical Laboratory and Quality |date=October 2019 |accessdate=09 April 2020}}</ref> Your public health labs and commercial diagnostic labs fall into this category, with investments in the personnel, training, certifications, and equipment to conduct those sorts of tests. Contrast this with the small yet numerous [[Physican office laboratory|physician office laboratories]] (POLs) and how they operate. As of October 2019, nearly 46 percent of [[CLIA]]-certified laboratories in the United States are POLs.<ref name="CMSEnroll19" /> Located in an ambulatory or outpatient care setting, these labs test specimens from human patients to assist with the diagnosis, treatment, or monitoring of a patient condition. Testing in the clinical lab generally depends on three common methodologies to meet those goals: comparing the current value of a tested substance to a reference value, examining a specimen with microscopy, and detecting the presence of infection-causing pathogens.<ref name="GarrelsOatis">{{cite book |url=https://books.google.com/books?id=LM9sBQAAQBAJ |title=Laboratory and Diagnostic Testing in Ambulatory Care: A Guide for Healthcare Professionals |author=Garrels, M.; Oatis, C.S. |publisher=Elsevier Health Sciences |edition=3rd |year=2014 |pages=368 |isbn=9780323292368 |accessdate=09 April 2020}}</ref>
 
These POL's operate in a somewhat different environment than your average [[public health laboratory]] or [[Reference lab#Referral and diagnostic|reference lab]] that receives, processes, and reports on specimens ''en masse''. The POL is typically a smaller operation, performing simple laboratory testing that can produce useful diagnostic data cheaply and rapidly. Rather than performing advanced pathology and molecular diagnostic procedures that require specific equipment and expertise, the POL typically focuses on blood chemistry, urinalysis, and other testing domains that don't require significant resources and provide rapid results. This can be seen in [[Centers for Medicare and Medicaid Services]] statistics reported in October 2019 that show nearly 67 percent of POLs in the U.S. are certified to provide CLIA-waived tests<ref name="CMSEnroll19" />, "simple tests with a low risk for an incorrect result."<ref name="CDCTestCom" />
 
As of April 10, with 1. all but a handful of the current EUAed ''in vitro'' diagnostic RT-PCR and lateral flow assay test kits being limited to moderate- and high-complexity CLIA labs<ref name="FDAEmerg20">{{cite web |url=https://www.fda.gov/medical-devices/emergency-situations-medical-devices/emergency-use-authorizations#covid19ivd |title=Emergency Use Authorizations |publisher=U.S. Food and Drug Administration |date=08 April 2020 |accessdate=09 April 2020}}</ref> (the FDA claims that EUAed SARS-CoV-2 tests authorized for "use at the point of care" are considered CLIA-waived tests<ref name="FDA_FAQS20">{{cite web |url=https://www.fda.gov/medical-devices/emergency-situations-medical-devices/faqs-diagnostic-testing-sars-cov-2 |title=FAQs on Diagnostic Testing for SARS-CoV-2 |author=U.S. Food and Drug Administration |publisher=U.S. Food and Drug Administration |date=10 April 2020 |accessdate=10 April 2020}}</ref>), and 2. local government entities such as New York City's Department of Health and Mental Hygiene sending reminders to local laboratories that serology testing (as of April 7) is also still considered high-complexity in nature<ref name="RakemanCOVID20">{{cite web |url=https://www1.nyc.gov/assets/doh/downloads/pdf/imm/covid-19-serology-testing.pdf |format=PDF |title=COVID-19 Serology Testing |author=Rakeman, J.L. |publisher=New York City Department of Health and Mental Hygiene |date=07 April 2020 |accessdate=09 April 2020}}</ref>, a significant majority of clinical laboratories are shut out from assisting with the effort to test the U.S. population for SARS-CoV-2 infection. Given the rapid rate of change at multiple levels of government and society, and wildly varying levels of reliable information being given to the public<ref name="SimoniteTheProf20">{{cite web |url=https://www.wired.com/story/professors-call-bullshit-covid-19-misinformation/ |title=The Professors Who Call ‘Bullshit’ on Covid-19 Misinformation |author=Simonite, T. |work=Wired |date=24 March 2020 |accessdate=09 April 2020}}</ref><ref name="SuciuDuring20">{{cite web |url=https://www.forbes.com/sites/petersuciu/2020/04/08/during-covid-19-pandemic-it-isnt-just-fake-news-but-seriously-bad-misinformation-that-is-spreading-on-social-media/ |title=During COVID-19 Pandemic It Isn't Just Fake News But Seriously Bad Misinformation That Is Spreading On Social Media |author=Suciu, P. |work=Forbes |date=08 April 2020 |accessdate=09 April 2020}}</ref>, it's important to remember these fundamental differences in laboratories when trying to explain to someone why they are, as of yet, unable to go to their primary care physician and get tested for SARS-CoV-2 in the doctor's office. Should researchers develop and the FDA provide EUAs for more CLIA-waived point-of-care assays, these differences may become less noticeable, and more people will able to be tested.
 
====2.4.2 PCR-based====
As of April 10, the U.S. Food and Drug Administration (FDA) has 33 EAUs for ''in vitro'' diagnostic test kits. Thirty-one of those 33 test kits use some form of RT-PCR methods, with most using real-time versions of RT-PCR (rRT-PCR). Twenty of those 31 are only authorized to be used in CLIA-certified high-complexity laboratories, with nine being rated for both moderate- and high-complexity. Two RT-PCR kits—Mesa Biotech's Accula SARS-Cov-2 Test and Cepheid's Xpert Xpress SARS-CoV-2 Test—have an addtional authorization for point-of-care (POC) use (and thus CLIA-waived use), when used with their authorized POC devices.<ref name="FDAEmerg20" />
 
Of course, there are many more test kits than those approved in the United States. The Foundation for Innovative New Diagnostics (FIND) is currently "collating an overview of all SARS-CoV-2 tests commercially available or in development for the diagnosis of COVID-19."<ref name="FINDSARS20">{{cite web |url=https://www.finddx.org/covid-19/pipeline/ |title=SARS-CoV-2 Diagnostic Pipeline |author=Foundation for Innovative New Diagnostics |publisher=Foundation for Innovative New Diagnostics |date=n.d. |accessdate=10 April 2020}}</ref> As of April 10, their site shows more than 150 commercialized manual NAAT tests around the world (most being RT-PCR), with more than 20 in development.
 
====2.4.3 LFA- and LAMP-based====
LFAs are currently rare, but due to their advantages of being quick and useable at the point of care, some have suggested that as a format for antigen and antibody testing, they could positively change the testing landscape.<ref name="SheridanFast20" /><ref name="BistriceanCOVID20">{{cite web |url=https://medium.com/@lablynx/covid-19-testing-for-the-physician-office-laboratory-pol-covidlims-com-bf1615e071ab |title=COVID-19 Testing for the Physician Office Laboratory (POL) - CovidLiMS.com |work=Medium |author=Bistricean, C. |date=01 April 2020 |accessdate=10 April 2020}}</ref><ref name="DickensCorona20">{{cite web |url=https://reaction.life/coronavirus-testing-how-it-works-questions-answered/ |title=Coronavirus testing: How it works – Questions answered |work=Reaction |author=Dickens, J.F. |date=03 April 2020 |accessdate=10 April 2020}}</ref> As of April 10, the only FDA EUA for an LFA is Cellex's qSARS-CoV-2 IgG/IgM Rapid Test, approved for moderate- and high-complexity CLIA-certified labs. An article by Sheridan in ''Nature Biotechnology'' highlights a handful of others developed around the world (see their Table 1).<ref name="SheridanFast20" /> FIND shows more than 120 commercialized rapid diagnostic immunoassay tests around the world, though it's not clear how many of them actually LFAs (from their list, only one is explictly stated as being LFA).<ref name="FINDSARS20" /> At this point, it's safe to say that LFA are still being developed, and it may May before we start seeing more of them, at least in the United States.<ref name="BistriceanCOVID20" />
 
Also of note is the LAMP (and RT-LAMP) method. Abbott's ID NOW COVID-19 test is described by the FDA as using "isothermal nucleic acid amplification technology for the qualitative detection of SARS-CoV-2 viral nucleic acids."<ref name="HintonIDNOW20">{{cite web |url=https://www.fda.gov/media/136522/download |title=ID NOW COVID-19 |author=Hinton, D.M. |publisher=U.S. Food and Drug Administration |date=27 March 2020 |accessdate=10 April 2020}}</ref> This is presumably loop-mediated isothermal amplification or LAMP test, the only one so far approved by the FDA. Among FIND's list of more than 150 commercialized manual NAAT tests around the world, five of them are explicitly shown to be some form of LAMP test. Multiple preprint papers on ''medRxiv'' and ''bioRxiv'' suggest that RT-LAMP could provide rapid results for SARS-CoV-2 testing<ref name="Schmid-BurgkLAMP20">{{cite journal |title=LAMP-Seq: Population-Scale COVID-19 Diagnostics Using a Compressed Barcode Space |journal=bioRxiv |author=Schmid-Burgk, J.L.; Li, D.; Feldman, D. et al. |year=2020 |doi=10.1101/2020.04.06.025635}}</ref><ref name="LambRapid20">{{cite journal |title=Rapid Detection of Novel Coronavirus (COVID-19) by Reverse Transcription-Loop-Mediated Isothermal Amplification |journal=medRxiv |author=Lamb, L.E.; Barolone, S.N.; Ward, E. et al. |year=2020 |doi=10.1101/2020.02.19.20025155}}</ref><ref name="YuRapid20">{{cite journal |title=Rapid colorimetric detection of COVID-19 coronavirus using a reverse tran-scriptional loop-mediated isothermal amplification (RT-LAMP) diagnostic plat-form: iLACO |journal=medRxiv |author=Yu, L.; Wu, S.; Hao, X. et al. |year=2020 |doi=10.1101/2020.02.20.20025874}}</ref><ref name="ParkDevelop">{{cite journal |title=Development of Reverse Transcription Loop-mediated Isothermal Amplification (RT-LAMP) Assays Targeting SARS-CoV-2 |journal=bioRxiv |author=Park, G.-S.; Ku, K.; Baek, S.-H. et al. |year=2020 |doi=10.1101/2020.03.09.983064}}</ref>, and Abbott is stating its EUAed ID NOW COVID-19 test can be completed as quickly as five minutes<ref name="AbbottDetect20">{{cite web |url=https://www.abbott.com/corpnewsroom/product-and-innovation/detect-covid-19-in-as-little-as-5-minutes.html |title=Detect COVID-19 in as Little as 5 Minutes |publisher=Abbott |date=27 March 2020 |accessdate=10 April 2020}}</ref>, providing further optimism for rapid point-of-care testing in the near future.
 
====2.4.4 Blood serum====
[[File:Blood in tubes (9617266704).jpg|left|250px]]Blood serum or serology assays come in three common varieties: LFA, enzyme-linked immunosorbent assay (ELISA), or neutralization assay.<ref name="JHSerology20" /> As discussed prior, LFAs are intended to be rapid point-of-care tools for qualitatively testing body fluids for patient antibodies or viral antigen. The ELISA is, in contrast, a more lab-bound method which produces results that are qualitative or quantitative. In the context of COVID-19 testing, ELISA tests for the presence of patient antibodies in a given specimen based upon whether or not an interaction is observed with the viral proteins present on the test plate. However, even if antibodies are present, ELISA isn't able to tell a clinician if those antibodies are able to protect against future infection. Neutralization assays are the lengthiest to complete, taking from three upwards to five days.<ref name="JHSerology20" /> This is largely due to the fact the assay depends on culturing cells that encourage growth of the target virus. Afterwards, introduced patient antibodies, if present, will fight to prevent viral infection of cells. This process is performed in decreasing concentrations, giving the clinician an opportunity to "visualize and quantify how many antibodies in the patient serum are able to block virus replication."<ref name="JHSerology20" /> In contrast to ELISA, a neutralization assay is able to determine if a patient's antibodies are actively fighting against the target virus, even after recovering from the infection.
 
Johns Hopkins' Center for Health Security [http://www.centerforhealthsecurity.org/resources/COVID-19/Serology-based-tests-for-COVID-19.html appears to be tracking] serology-based COVID-19 tests that are in development or have been approved in various parts of the globe. As of April 2, they show one assay approved for diagnostic use in the U.S. and seven similarly approved in other parts of the world. They also show 22 approved for research or surveillance purposes, and nine in development around the world.
 
Of the eight assays approved for diagnostic use, six appear to be LFAs. ScanWell Health's kit appears to be proprietary, but given its claims of rapid results, it too is probably LFA. A Singapore-based operation has two tests, one that is advertised as rapid, another as a neutralization test. Of the 22 assays approved for research or surveillance, six appear to be be based on ELISA, one is unknown, and the rest are LFA-based assays. Among those still in development, an LFA stands out for integrating CRISPR detection.<ref name="MBAProto20">{{cite web |url=https://mammoth.bio/wp-content/uploads/2020/03/Mammoth-Biosciences-A-protocol-for-rapid-detection-of-SARS-CoV-2-using-CRISPR-diagnostics-DETECTR.pdf |format=PDF |title=A protocol for rapid detection of the 2019 novel coronavirus SARS-CoV-2 using CRISPR diagnostics: SARS-CoV-2 DETECTR |publisher=Mammoth Biosciences |date=02 March 2020 |accessdate=09 April 2020}}</ref> CRISPR (clustered regularly interspaced short palindromic repeats) represents bacterial and archaeal DNA sequences derived from DNA fragments of previous infection. This genetic material can then be used as an activator of biomarkers when attached RNA "guides" find a match with target viral RNA in patient specimen.<ref name="NatureCRISPR18">{{cite web |url=https://www.nature.com/articles/d41586-018-02200-0 |title=CRISPR’s powers unleashed for disease detection |work=Nature - Research Highlights |date=16 February 2018 |accessdate=09 April 2020}}</ref>
 
====2.4.5 Testing alternatives and challenges====
 
<blockquote>''We’ve never faced this before, where clinical labs needed to very quickly be able to ramp up a test so fast.''<ref name="TerryCRISPR20">{{cite web |url=https://www.biospace.com/article/crispr-discoverer-jennifer-doudna-launches-covid-19-test-lab/ |title=CRISPR Pioneer Jennifer Doudna Expects Automated COVID-19 Test Lab to Begin Testing Next Week |work=BioSpace |author=Terry, M. |date=30 March 2020 |accessdate=10 April 2020}}</ref><br />&nbsp;<br />- Jennifer Doudna, Executive Director of the Innovative Genomics Institute, University of California, Berkeley</blockquote>
 
Though the dismantling and fund-cutting (proposed and real) of government programs designed to protect the populace from pandemics—as well as shortfalls in funding overall<ref name="SandsTheNeglect16">{{cite journal |title=The Neglected Dimension of Global Security — A Framework for Countering Infectious-Disease Crises |journal=The New England Journal of Medicine |author=Sands, P.; Mundaca-Shah, C.; Dzau, V.J. |volume=374 |issue=13 |pages=1281–87 |year=2016 |doi=10.1056/NEJMsr1600236 |pmid=26761419}}</ref>—have likely hobbled local, national, and global response to COVID-19<ref name="MorrisTrump20">{{cite web |url=https://fortune.com/2020/02/26/coronavirus-covid-19-cdc-budget-cuts-us-trump/ |title=Trump administration budget cuts could become a major problem as coronavirus spreads |work=Fortune |author=Morris, C. |date=26 February 2020 |accessdate=10 April 2020}}</ref><ref name="SpecterTheCorona20">{{cite web |url=https://www.newyorker.com/news/daily-comment/coronavirus-and-the-gutting-of-americas-public-health-system |title=The Coronavirus and the Gutting of America’s Public-Health System |work=The New Yorker |author=Specter, M. |date=17 March 2020 |accessdate=10 April 2020}}</ref><ref name="RoosCongress07">{{cite web |url=https://www.cidrap.umn.edu/news-perspective/2007/05/congress-cut-pandemic-funds-passing-spending-bill |title=Congress cut pandemic funds before passing spending bill |work=CIDRAP - News & Perspective |author=Roos, R. |date=25 May 2007 |accessdate=10 April 2020}}</ref><ref name="SchnirringCongress07">{{cite web |url=https://www.cidrap.umn.edu/news-perspective/2007/12/congress-slashes-pandemic-preparedness-funding |title=Congress slashes pandemic preparedness funding |work=CIDRAP - News & Perspective |author=Schnirring, L. |date=20 December 2007 |accessdate=10 April 2020}}</ref>, it should be recognized that this pandemic may arguably represent a once-in-a-century type of event.<ref name="GatesRespond20">{{cite journal |title=Responding to Covid-19 — A Once-in-a-Century Pandemic? |journal=The New England Journal of Medicine |author=Gates, B. |year=2020 |doi=10.1056/NEJMp2003762 |pmid=32109012}}</ref><ref name="ShontellMelinda20">{{cite web |url=https://www.businessinsider.com/melinda-gates-coronavirus-interview-vaccine-timeline-2020-4 |title=Melinda Gates: This is not a once-in-a-century pandemic. 'We will absolutely have more of these.' The billionaire philanthropist predicts a timeline for going back to normal |work=Business Insider |author=Shontell, A. |date=10 April 2020 |accessdate=10 April 2020}}</ref> That said, even the most well-prepared governments would still face challenges in quickly learning about, controlling, and developing therapies for a novel disease agent. Shortages in supplies, workers, funding, and other resources are inevitably caused with a pandemic as people across all types of infrastructure fall ill.<ref name="SandsTheNeglect16" /><ref name="MadhavPandemics17">{{cite book |url=https://www.ncbi.nlm.nih.gov/books/NBK525302/ |chapter=Chapter 17: Pandemics: Risks, Impacts, and Mitigation |title=Disease Control Priorities: Improving Health and Reducing Poverty |edition=3rd |author=Madhav, N.; Oppenheim, B.; Gallivan, M. et al. |editor=Jamison, D.T.; Gelband, H.; Horton, S. et al. |publisher=The World Bank |year=2017 |isbn=9781464805288}}</ref> This requires the additional human elements of adaptability, drive, and shared knowledge to find new and alternative solutions to fighting the challenges inherent to fighting against a novel disease.
 
See for example a non-peer-reviewed paper published on bioRxiv in early April 2020, where Schmid-Burgk ''et al.'' point out that though RT-PCR methods are the most common for currently testing for SARS-CoV-2, "global capacity for testing using these approaches, however, has been limited by a combination of access and supply issues for reagents and instruments." They propose "a novel protocol that would allow for population-scale testing using massively parallel RT-LAMP by employing sample-specific barcodes." They claim that a single heating step, pooled processing, and parallel sequencing with computational analysis would allow for the testing and tacking of "tens of millions of samples." Though the protocol has not been validated with clinical samples, and concerns about sensitivity levels of RT-LAMP (an isothermal nucleic acid amplification technique that allows for RNA amplification) have been raised, the authors' work exemplifies the immediacy and inginuity going into finding workable solutions to a once-a-century problem.<ref name="Schmid-BurgkLAMP20" />
 
Another example of ingenuity in the face of difficult circumstances can be found at the University of California, Berkeley. Its Innovative Genomics Institute (IGI) has rapidly repurposed a 2,500-square-foot scientific lab into an automated diagnostic laboratory that can initially process more than 1,000 patient samples per day, with the ability to ramp up to 3,000 per day thanks to robotics and a streamlined workflow. Partnering with dozens of people from Thermo Fisher Scientific, Salesforce, Third Wave Analytics, and Hamilton Corp., the lab is focused on not only turnaround time but also accuracy of results through automation. Their continued success, of course, relies on a steady supply of reagents and related supplies from Thermo Fisher.<ref name="TerryCRISPR20" /><ref name="SandersUCBerk20">{{cite web |url=https://news.berkeley.edu/2020/03/30/uc-berkeley-scientists-spin-up-a-robotic-covid-19-testing-lab/ |title=UC Berkeley scientists spin up a robotic COVID-19 testing lab |work=Berkeley News |author=Sanders, R. |date=30 March 2020 |accessdate=10 April 2020}}</ref>
 
Others have also expressed concerned about the global supply of reagents necessary to test for SARS-CoV-2. Successful testing using RT-PCR requires two different enzymes: reverse transcriptase, for converting RNA to DNA, and polymerase, for amplifying the converted DNA. These enzymes and other reagent components may be instrument-specific, and at least one component has to be sympathetic to detection of the target virus' RNA. Little of this can be prepared without a proper sequence of the virus in question. Dr. Ronald Leonard, president and medical director of Cytocheck Laboratory and medical director of the Labette Health hospital, has expressed the difficulties associated with reagents manufacting thusly<ref name="NoltingLocal20">{{cite web |url=https://www.parsonssun.com/news/coronavirus/article_99193646-7aec-11ea-a7c5-b700f82332db.html |title=Local testing delayed by lack of reagents |work=Parsons Sun |author=Nolting, R. |date=10 April 2020 |accessdate=10 April 2020}}</ref>:
 
<blockquote>With the instant demand for SARS-CoV-2 testing, the manufacturing process had to start from scratch for the SARS-CoV-2 specific components, and this did cause a lag time before reagents were available. The increased demand coupled with the decision to only allocate reagents to two national laboratories, some state health departments, and to "hot spots" has compounded the difficulty for laboratories like ours to obtain the necessary reagents to perform the testing.</blockquote>
 
Reports of reagent shortages appeared in March and April from various sources<ref name="HerperShortage20">{{cite web |url=https://www.statnews.com/2020/03/10/shortage-crucial-chemicals-us-coronavirus-testing/ |title=Shortage of crucial chemicals creates new obstacle to U.S. coronavirus testing |work=STAT |author=Herper, M.; Branswell, H. |date=10 March 2020 |accessdate=10 April 2020}}</ref><ref name="HaleQiagen20">{{cite web |url=https://www.fiercebiotech.com/medtech/qiagen-aims-to-more-than-quadruple-its-covid-19-reagent-production-6-weeks |title=Qiagen aims to more than quadruple its COVID-19 reagent production in 6 weeks |work=Fierce Biotech |author=Hale, C. |date=18 March 2020 |accessdate=10 April 2020}}</ref><ref name="MehtaMystery20">{{cite web |url=https://www.chemistryworld.com/mystery-surrounds-uk-claim-of-covid-19-test-reagent-shortage/4011457.article |title=Mystery surrounds UK claim of Covid-19 test reagent ‘shortage’ |work=Chemistry World |author=Mehta, A. |date=03 April 2020 |accessdate=10 April 2020}}</ref><ref name="RocheIrish20">{{cite web |url=https://www.irishtimes.com/news/science/irish-scientists-develop-reagent-in-effort-to-ease-covid-19-testing-delays-1.4223897 |title=Irish scientists develop reagent in effort to ease Covid-19 testing delays |work=The Irish Times |author=Roche, B. |date=08 April 2020 |accessdate=10 April 2020}}</ref>, though whether the shortage is a real supply issue or "a consequence of restrictive policies on where and how testing could be completed" is argued by some.<ref name="NoltingLocal20" /><ref name="MehtaMystery20" /> Others have taken matters into their own hands in regards to reagent component shortages. Noting Irish laboratories' difficulties sourcing lysis buffer (for isolating molecules of interest and keeping them stable), Cork Institute of Technology's Dr. Brigid Lucey worked with several other virologists and microbiologists, as well as pharmaceutical company Eli Lilly, to produce a custom-formulated yet high-quality lysis buffer for not only Irish laboratories but also other countries can take advantage of. "We are happy to share what we found with other countries and it’s important our scientists retain their skills to make this kind of formulation because we may need to do this again in the future if we get other pandemics," she said.<ref name="RocheIrish20" />
 
 
===2.5 Regulatory and recommended requirements for reporting test results===
Epidemiology can broadly be split into two categories: descriptive epidemiology and analytical epidemiology. Descriptive epidemiology involves studies and other activites that deal with geographical comparisons and temporal trend descriptions of disease. As such, the collection and use of quality incidence data is vital to developing hypotheses.<ref name="NaitoUtil14">{{cite journal |title=Utilization and application of public health data in descriptive epidemiology |journal=Journal of Epidemiology |author=Naito, M. |volume=24 |issue=6 |pages=435–6 |year=2014 |doi=10.2188/jea.je20140182 |pmid=25327184 |pmc=PMC4213216}}</ref> Analytical epidemiology allows for the testing of those hypotheses using both experimental and obsevational studies, as well as control groups. Similarly, the collection and use of quality experimental and observational data is vital for providing or disproving hypotheses.<ref name="CDCPrinc12">{{cite book |url=https://www.cdc.gov/csels/dsepd/ss1978/SS1978.pdf |format=PDF |title=Principles of Epidemiology in Public Health Practice |author=Centers for Disease Control and Prevention |edition=3rd |publisher=Centers for Disease Control and Prevention |year=2012 |accessdate=11 April 2020}}</ref> In both cases, proper reporting of data is critical to the success of epidemiologists' response to outbreaks and pandemics, as well as the credibility of their research.<ref name="HamiltonUsing19">{{cite book |chapter=Chapter 5: Using Technologies for Data Collection and Management |title=The CDC Field Epidemiology Manual |author=Hamilton, J.J.; Hopkins, R.S. |editor=Rasmussen, S.A.; Goodman, R.A. |publisher=Oxford University Press |edition=4th |pages=71–104 |year=2019 |isbn=9780190933692}}</ref><ref name="vonElmTheStren07">{{cite journal |title=The Strengthening the Reporting of Observational Studies in Epidemiology (STROBE) statement: Guidelines for reporting observational studies |journal=PLoS Medicine |author=von Elm, E.; Altman, D.G.; Egger, M. et al. |volume=4 |issue=10 |at=e296 |year=2007 |doi=10.1371/journal.pmed.0040296 |pmid=17941714 |pmc=PMC2020495}}</ref>
 
The proper reporting of COVID-19 case data is no exception. In the United States, the CDC has taken a standardized approach to collecting reports on "individuals with at least one respiratory specimen that tested positive for the virus that causes COVID-19."<ref name="CDCInformRepo20">{{cite web |url=https://www.cdc.gov/coronavirus/2019-ncov/php/reporting-pui.html |title=Information for Health Departments on Reporting Cases of COVID-19 |author=Centers for Disease Control and Prevention |work=Coronavirus Disease 2019 (COVID-19) |publisher=Centers for Disease Control and Prevention |date=21 March 2020 |accessdate=21 March 2020}}</ref> Their COVID-19 Case Report Form is designed to collect a wide variety of information about a COVID-19 case, including patient demographics, epidemiological characteristics, exposure and contact history, and clinical diagnosis and treatment procedures. Currently, the CDC is asking local and state health departments to submit case reports, and asking healthcare providers to contact those health departments when "concerned that a patient may have COVID-19." The CDC has also slimmed its reporting requirements, limiting reporting of "persons under investigation" to areas where testing must be forwarded to the CDC due to insufficient capacity to test locally.<ref name="CDCInformRepo20" /> Electronic reporting using the CDC's system is preferred, but they have a protocol for those areas unable to submit electronically. Canada has similar reporting expectations, with their own case report form and electronic data submission process through the Public Health Agency of Canada.<ref name="CanadaInterim20">{{cite web |url=https://www.canada.ca/en/public-health/services/diseases/2019-novel-coronavirus-infection/health-professionals/interim-guidance-surveillance-human-infection.html |title=Interim national surveillance guidelines for human infection with Coronavirus disease (COVID-19) |author=Government of Canada |publisher=Government of Canada |date=10 February 2020 |accessdate=11 April 2020}}</ref> And in the European Union, member countries and the U.K. are asked to report through the Early Warning and Response System.<ref name="ECDCCaseDef20">{{cite web |url=https://www.ecdc.europa.eu/en/case-definition-and-european-surveillance-human-infection-novel-coronavirus-2019-ncov |title=Case definition and European surveillance for COVID-19, as of 2 March 2020 |author=European Centre for Disease Prevention and Control |publisher=European Centre for Disease Prevention and Control |work=COVID-19 Portal |date=02 March 2020 |accessdate=11 April 2020}}</ref>
 
Somewhat related are any internal reporting requirements, particularly for test reporting in labs and medical facilities. The [[International Statistical Classification of Diseases and Related Health Problems]] (ICD) is a system of diagnostic codes for classifying diseases, including nuanced classifications of a wide variety of signs, symptoms, abnormal findings, complaints, social circumstances, and external causes of injury or disease. Their ICD-10-CM code set has been modified to include lab testing codes for COVID-19, as has the [[Current Procedural Terminology]] (CPT) code set. [https://www.mgma.com/data/data-stories/coding-guidance-for-new-icd-10-cm-and-lab-testing Green and Bradley] provide insight into these additions<ref name="GreenCoding20">{{cite web |url=https://www.mgma.com/data/data-stories/coding-guidance-for-new-icd-10-cm-and-lab-testing |title=Coding guidance for new ICD-10-CM and lab testing codes for COVID-19 |work=MGMA Stat |author=Green, C.; Bradley, V. |date=01 April 2020 |accessdate=11 April 2020}}</ref>, as does the [https://www.aappublications.org/news/2020/03/12/coding031220 American Academy of Pediatrics].<ref name="AAPHowTo20">{{cite web |url=https://www.aappublications.org/news/2020/03/12/coding031220 |title=How to use ICD-10-CM, new lab testing codes for COVID-19 |author=AAP Division of Health Care Finance |publisher=American Academy of Pediatrics |date=12 March 2020 |accessdate=11 April 2020}}</ref>
 
 
==References==
{{Reflist|colwidth=30em}}

Latest revision as of 20:37, 16 August 2023

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