The impact of PCR duplication on RNAseq data generated using NovaSeq 6000, NovaSeq X, AVITI, and G4 sequencers

Natalia Zajac; Ioannis S Vlachos; Sija Sajibu; Lennart Opitz; Shuoshuo Wang; Sridar V Chittur; Christopher E Mason; Kevin L Knudtson; John M Ashton; Hubert Rehrauer; Catharine Aquino

doi:10.1186/s13059-025-03613-7

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The impact of PCR duplication on RNAseq data generated using NovaSeq 6000, NovaSeq X, AVITI, and G4 sequencers

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The impact of PCR duplication on RNAseq data generated using NovaSeq 6000, NovaSeq X, AVITI, and G4 sequencers

Natalia Zajac, Ioannis S Vlachos, Sija Sajibu, Lennart Opitz, Shuoshuo Wang, Sridar V Chittur, Christopher E Mason, Kevin L Knudtson, John M Ashton, Hubert Rehrauer, …

Genome biology, Vol.26(1), 145

05/28/2025

DOI: 10.1186/s13059-025-03613-7

PMCID: PMC12117910

PMID: 40437619

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Abstract

Transcriptome sequencing (RNA-seq) is a powerful technology for gene expression profiling. Selection of optimal parameters for cDNA library generation is crucial for acquisition of high-quality data. In this study, we investigate the impact of the amount of RNA and the number of PCR cycles used for sample amplification on the rate of PCR duplication and, in consequence, on the RNA-seq data quality. For broader applicability, we sequenced the data on four short-read sequencing platforms: Illumina NovaSeq 6000, Illumina NovaSeq X, Element Biosciences AVITI, and Singular Genomics G4. The native Illumina libraries were converted for sequencing on AVITI and G4 to assess the effect of library conversion, containing additional PCR cycles. We find that the rate of PCR duplicates depends on the combined effect of RNA input material and the number of PCR cycles used for amplification. For input amounts lower than 125 ng, 34-96% of reads were discarded via deduplication with the percentage increasing with lower input amount and decreasing with increasing PCR cycles. The reduced read diversity for low input amounts leads to fewer genes detected and increased noise in expression counts. Data generated with each of the four sequencing platforms presents similar associations between starting material amount and the number of PCR cycles on PCR duplicates, a similar number of detected genes, and comparable gene expression profiles.

Gene Expression Profiling - methods

Gene Library

High-Throughput Nucleotide Sequencing - methods

Humans

Polymerase Chain Reaction - methods

RNA-Seq - methods

Sequence Analysis, RNA - instrumentation

Sequence Analysis, RNA - methods

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Title: Subtitle: The impact of PCR duplication on RNAseq data generated using NovaSeq 6000, NovaSeq X, AVITI, and G4 sequencers
Creators: Natalia Zajac - University of Zurich
Ioannis S Vlachos - Beth Israel Deaconess Medical Center
Sija Sajibu - University of Zurich
Lennart Opitz - University of Zurich
Shuoshuo Wang - Broad Institute
Sridar V Chittur - Albany State University
Christopher E Mason - Cornell University
Kevin L Knudtson - University of Iowa
John M Ashton - University of Rochester
Hubert Rehrauer - University of Zurich
Catharine Aquino - University of Zurich
Resource Type: Journal article
Publication Details: Genome biology, Vol.26(1), 145
DOI: 10.1186/s13059-025-03613-7
PMID: 40437619
PMCID: PMC12117910
NLM abbreviation: Genome Biol
ISSN: 1474-760X
eISSN: 1474-760X
Publisher: BioMed Central Ltd; LONDON
Grant note: Swiss Federal Institute of Technology Zurich
center dot Lutz Froenicke, DNA Technologies and Expression Analysis Core UC Davis Genome Center Element AVITI sequencing.
Language: English
Date published: 05/28/2025
Academic Unit: Iowa Institute of Human Genetics
Record Identifier: 9984825530002771

The impact of PCR duplication on RNAseq data generated using NovaSeq 6000, NovaSeq X, AVITI, and G4 sequencers

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