the effect of incubation time and freeze-thaw process
earlier than 3 days and later than 9 days of incubation.
Another study on the freeze-thaw aspect of RNA
detection by PCR method was carried out on the
dengue virus. The results showed that the freeze-thaw
process did not affect RNA detection (Anwar et al.
2009). Therefore, this method is promising for
continuous development to obtain optimal Ct. It is
necessary to carry out a further study with a longer
incubation time to determine the best conditions for
producing a balanced Ct number between viral genes
and rnp.
4 CONCLUSIONS
The process of harvesting the SARS-CoV-2 virus
culture by the freeze-thaw process is sufficient for an
incubation period of 3 days and can be used for
producing EQA panel material. However, the
detected Ct rnp value was still higher than the viral
Ct. Thus, it is necessary to carry out further
optimization in the process of harvesting the SARS-
CoV-2 virus as a panel material for proficiency
testing that resembles clinical specimens.
ACKNOWLEDGEMENTS
The authors would like to thank the Director of
CDRBBHT and all the team members of SARS-CoV-
2 virus testing at the National Reference Laboratory
for COVID-19.
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