heavy metals then coat the surface of the virus particles to reveal their internal and
external structures [6]. The stained samples are then deposited and dried on dedicated
grids. The quantitative evaluation of viral particles is feasible but with high variability
as the analysis is performed by visual counting on NSTEM grids.
Such tools also permit to qualify the viral suspension quality as it will be pos-
sible to observe other nanoparticles like exosomes or micro-vesicles. However,
such assays are very complex to implement as a quantification assay. NSTEM is
very long and costly. Consequently it can not be used for screening. It is most of
the time applied on highly purified samples as protein and cell debris will also have
a strong response to electron-dense stain.
For process optimization and development, electron microscopy is not the
appropriate tool as it will be necessary to screen production conditions with impure
material. Thus, other types of assays allowing the quantification of parts of the virus
(genome, viral protein) are preferred for high-throughput analyses. In such a case,
the evaluation of the number of total viral particles is performed by calculating the
theoretical amount of genome or protein within a viral particle. Such indirect
quantification methods imply that an external standard is used to calibrate the
amount of total viral particles. Thus, biochemical or molecular biology assays are
qualified with electron microscopy viral particle counting.
Viral genome quantification by quantitative qPCR and RT-qPCR was in the
last 10 years the method of choice to determine total viral particles amount. Indeed,
the assumption is here that each viral particle carries a single copy of its genome.
Thus, quantifying the number of viral genomes within a sample gives access to the
number of particles. Such tools based on molecular biology techniques allow for the
design of probes that could have nucleotide sequences highly specific to a virus or a
viral strain. It was particularly exploited for the presence of viral adventitious agents
within pharmaceutical products as it could allow screening for several viruses at the
same time. As preliminary steps, this assay necessitates extracting the viral genome
from the particles and eventually convert RNA in cDNA if the virus strain is an RNA
virus. These two steps include purification and sample handling steps, which might
affect again the variability of the assay. The second step consists of the incubation of
the viral genomes with a specific probe carrying both a fluorophore and its quencher to
allow for fixation of the probes on the nucleic acid sequences. Release of the fluor-
ophore then happens while the DNA polymerase degrades the specific probe.
Correlation between the number of fluorophores released and the number of viral
particles then must be established upfront. This means that a reference material with
its associate reference qualification assay is then necessary. In the last decade,
high‐throughput droplet‐based digital PCR (ddPCR) has been developed as an im-
provement of the conventional polymerase chain reaction (PCR) methods. In ddPCR,
DNA/RNA is encapsulated inside reaction chambers formed of microdroplets. This
was render possible thanks to the improvement reached in microfluidic science
working on mixture between immiscible fluid (i.e., the so-called dispersed fluid) and a
continuous fluid to generate submicroliter droplets at kilohertz rates [7]. Thus, the
reaction chamber contains one or fewer copies of the DNA or RNA. Some of the main
features of ddPCR include high sensitivity and specificity, absolute quantification
without a standard curve, high reproducibility, good tolerance to PCR inhibitor, and
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