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New CRISPR-Based Test That Is Much Faster and Easier to Deploy than qRT-PCR Diagnoses COVID-19 in 20 Minutes

By LabMedica International staff writers
Posted on 10 Aug 2021
Illustration
Illustration
In their efforts to develop a diagnostic test that is much faster and easier to deploy than qRT-PCR, scientists have combined two different types of CRISPR enzymes to create an assay that can detect small amounts of viral RNA in less than an hour.

While the new technique developed by researchers at the University of California, Berkeley (Berkeley, CA, USA) is not yet at the stage where it rivals the sensitivity of qRT-PCR, which can detect just a few copies of the virus per microliter of liquid, it is already able to pick up levels of viral RNA - about 30 copies per microliter - sufficient to be used to surveil the population and limit the spread of infections.
Frequent, rapid testing for COVID-19 is critical to controlling the spread of outbreaks, especially as new, more transmissible variants emerge. While today’s gold standard COVID-19 diagnostic test, which uses qRT-PCR - quantitative reverse-transcriptase-polymerase chain reaction (PCR) - is extremely sensitive, detecting down to one copy of RNA per microliter, it requires specialized equipment, a runtime of several hours and a centralized laboratory facility. As a result, testing typically takes at least one to two days.

Several CRISPR-based assays have been authorized for emergency use by the Food and Drug Administration, but all require an initial step in which the viral RNA is amplified so that the detection signal - which involves release of a fluorescent molecule that glows under blue light - is bright enough to see. While this initial amplification increases the test’s sensitivity to a similar level as qRT-PCR, it also introduces steps that make the test more difficult to carry out outside of a laboratory. The UC Berkeley-led team sought to reach a useful sensitivity and speed without sacrificing the simplicity of the assay.

Aside from having an added step, another disadvantage of initial amplification is that, because it makes billions of copies of viral RNA, there is a greater chance of cross-contamination across patient samples. The new technique developed by the team flips this around and instead boosts the fluorescent signal, eliminating a major source of cross-contamination. The amplification-free technique, which they term Fast Integrated Nuclease Detection In Tandem (FIND-IT), could enable quick and inexpensive diagnostic tests for many other infectious diseases. The researchers are currently in the process of building such a diagnostic using FIND-IT, which would include steps to collect and process samples and to run the assay on a compact microfluidic device.

“You don’t need the sensitivity of PCR to basically catch and diagnose COVID-19 in the community, if the test’s convenient enough and fast enough,” said co-author David Savage, professor of molecular and cell biology. “Our hope was to drive the biochemistry as far as possible to the point where you could imagine a very convenient format in a setting where you can get tested every day, say, at the entrance to work.”

“For point of care applications, you want to have a rapid response so that people can quickly know if they’re infected or not, before you get on a flight, for example, or go visit relatives,” said team leader Tina Liu, a research scientist in the lab of Jennifer Doudna at the Innovative Genomics Institute (IGI), a CRISPR-focused center involving UC Berkeley and UC San Francisco scientists.

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