Vector copy number (VCN) and viral titer are two different parameters that are measured in cell and gene therapy to determine the quality and quantity of viral vectors used for gene delivery. Although both parameters are related to the amount of virus present in the sample, they have different meanings and methods of quantification.

Vector copy number (VCN) refers to the number of vector genomes integrated into the genome of the target cells. To date, three viral vector platforms are the predominant players across gene therapy development: Adenovirus, Adeno-associated virus, and lentivirus1. The efficiency of viral transduction is influenced by several factors including the viral dose, the target cell type, and the expression cassette design. This makes accurate VCN an important parameter for monitoring the long-term expression of the transgene and for determining the optimal viral dose in cell and gene therapy applications.

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Digital PCR (dPCR) is a powerful technique for precise, accurate and reproducible measurement of nucleic targets as it does not require a standard curve or reference to interpret overall quantity. dPCR therefore allows for accurate and sensitive quantification of the number of copies of a transgene or vector in a sample, providing valuable information about the stability and expression of the transgene. In biopharmaceutical production, it is essential to maintain consistent vector copy numbers to help ensure consistent protein expression and product quality. In gene therapy research, VCN analysis can help to optimize the dose and efficacy of the therapy.

The use of dPCR for VCN analysis offers several advantages over traditional methods. These advantages include:

  • Increased sensitivity: dPCR can detect low levels of target molecules with high sensitivity, making it ideal for quantifying vector copy number in samples with low transgene expression.
  • Improved precision and accuracy: dPCR distribute the sample across many small microreactions, which helps reduce the variability in amplification efficiency and improves the precision and accuracy of quantification.
  • Ability to distinguish between integrated and episomal vectors: dPCR can differentiate between integrated and episomal vectors, allowing researchers to assess the stability and expression of the transgene over time.

Overall, vector copy number analysis by digital PCR is a powerful technique. It offers several advantages over traditional methods, including increased sensitivity, improved precision and accuracy, and the ability to differentiate between integrated and episomal vectors. This approach has applications in a wide range of fields, including research for biopharmaceutical production and gene therapy research.

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Viral titer, on the other hand, refers to the concentration of infectious viral particles in the sample. The viral titer is determined by infecting a susceptible cell line with serial dilutions of the viral sample and calculating the concentration of infectious virus particles that cause cytopathic effects (CPE) or produce visible plaques. Viral titer is a measure of the number of infectious viral particles that are present in the sample and is an important parameter for determining the optimal viral dose and assessing the potency of the viral vector.

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Quantifying viral titer is an essential step in the production and testing of viral vectors for cell and gene therapy applications. Digital PCR (dPCR) is an extremely sensitive and precise method that is becoming an increasingly popular tool for viral titer quantification in cell and gene therapy research.

Measuring viral titer quantification by dPCR can help to determine the concentration of infectious viral particles in a sample. This is critical information used to determine the optimal viral dose to potentially deliver in cell and gene therapy research applications. Because of this, the accuracy and precision of dPCR make it an ideal method for determining viral titer.

Overall, digital PCR is a powerful and accurate method for viral titer quantification in cell and gene therapy research applications. It offers several advantages over traditional methods, including improved sensitivity and precision, and can be used for quality control during the production process. As cell and gene therapy continues to advance, the use of dPCR for viral titer quantification is expected to become increasingly prevalent in the industry.

In summary, VCN and viral titer are two different parameters that are used to measure the quantity and quality of viral vectors used for gene delivery in cell and gene therapy. VCN is a measure of the number of vector genomes integrated into the genome of the target cells, while viral titer is a measure of the concentration of infectious viral particles in the sample. Both parameters are essential for optimizing the viral dose and viral vectors.

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References

1. https://www.nature.com/articles/s41392-021-00487-6