# P-1844. Performance Characteristics of a Validated Pan-Genotypic Real-Time RT-PCR Assay for the Quantification of Hepatitis Delta Virus from Human Serum and Plasma

**Authors:** Lydia Sweet, Arsalan Khan, Gerald Wallweber, Christos J Petropoulos

PMC · DOI: 10.1093/ofid/ofaf695.2013 · Open Forum Infectious Diseases · 2026-01-11

## TL;DR

A new real-time RT-PCR assay was developed and validated to accurately quantify Hepatitis Delta Virus RNA in human serum and plasma across all genotypes.

## Contribution

A validated pan-genotypic real-time RT-PCR assay for HDV RNA quantification with high inclusivity and analytical performance is introduced.

## Key findings

- The assay demonstrated linearity across a 5–7 log10 range with R squared > 0.99 for all HDV genotypes.
- The limit of detection was 8.81 IU/mL for serum and 9.50 IU/mL for plasma.
- PCR efficiencies were >90% for 21 out of 22 HDV genotypes tested.

## Abstract

Hepatitis Delta Virus (HDV) is a 1.7 kb single-stranded, circular RNA virus that relies on Hepatitis B Virus (HBV) surface antigens (HBsAg) for encapsulation, and therefore is dependent on co-infection with HBV for replication and transmission. Globally, it is estimated that 12-60 million individuals are infected with HDV. There are eight HDV genotypes with distinct and overlapping geographical distributions. Bulevirtide (Hepcludex) is the only approved treatment for HDV infection and currently only in Europe. Testing for HDV is expected to increase once bulevirtide and additional therapies are available. We describe the performance characteristics of a new laboratory-developed test for the quantification of HDV RNA

Total nucleic acid is isolated from human serum and EDTA-plasma with an improved semi-automated extraction protocol on the KingFisher Flex. Samples are spiked with bacteriophage MS2 to monitor performance of the entire procedure. HDV and MS2 RNA are detected using a 2-step RT-PCR assay optimized for the QuantStudio 7 Flex Real-Time PCR System and results report in IU/mL. Assay performance has been validated for accuracy, precision, linearity, sensitivity, specificity and genotype inclusivity.

Matched sample types resulted in similar viral loads; average bias 0.04 log10 IU/mL. The LOD was 8.81 and 9.50 IU/mL for serum and plasma respectively, with an ULOQ of > 2x106 IU/mL for both. Results from a comparator laboratory were similar, slope 1.103 log10 IU/mL and average bias 0.6 log10 IU/mL Results from spike-recovery, precision, cross-reactivity and interfering substances were also similar between sample types. Transcripts from 22 HDV reference plasmids representing all HDV genotypes and subtypes were linear over a 5 – 7 log10 range, R squared > 0.99. PCR efficiencies from 21/22 transcripts were > 90%, genotype 4b had a PCR efficiency of 86%.

The quantitative HDV RNA assay demonstrated acceptable analytical performance as well as inclusivity for all HDV genotypes. The assay has been validated to CLIA/CAP specifications and is suitable for quantification of HDV RNA from human serum and EDTA-plasma.

Lydia Sweet, PhD, Labcorp-Monogram Biosciences: Employee Arsalan Khan, BSc, Labcorp-Monogram Biosciences: Employee Gerald Wallweber, PhD, Labcorp-Monogram Biosciences: employee Christos J. Petropoulos, Ph.D., Labcorp-Monogram Biosciences: employee

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Source: https://tomesphere.com/paper/PMC12791446