Publication:
Investigation of Different Library Preparation and Tissue of Origin Deconvolution Methods for Urine and Plasma cfDNA Methylome Analysis.

cris.virtual.author-orcid0000-0002-8244-665X
cris.virtualsource.author-orcid96c694d9-a9e1-4bd4-a71e-0aee7ace559a
cris.virtualsource.author-orcid2cbd9e6a-4be4-44fa-89ad-067f82762d16
cris.virtualsource.author-orcid5cf54cef-0b9b-48ee-a517-51eafd1fb458
cris.virtualsource.author-orcidf34c7371-748b-4478-8d2e-40dddd291954
cris.virtualsource.author-orcid89351f1b-c3b3-4ff0-af2f-033f39da3188
cris.virtualsource.author-orcid235f92d3-3899-486c-8fb8-81960d8b7d58
datacite.rightsopen.access
dc.contributor.authorKüng, Nicholas Fabian
dc.contributor.authorSidler, Daniel
dc.contributor.authorBanz Wüthrich, Vanessa
dc.contributor.authorLargiadèr, Carlo Rodolfo
dc.contributor.authorNg, Kiu Yan Charlotte
dc.contributor.authorAmstutz, Ursula
dc.date.accessioned2024-10-25T17:05:52Z
dc.date.available2024-10-25T17:05:52Z
dc.date.issued2023-07-27
dc.description.abstractMethylation sequencing is a promising approach to infer the tissue of origin of cell-free DNA (cfDNA). In this study, a single- and a double-stranded library preparation approach were evaluated with respect to their technical biases when applied on cfDNA from plasma and urine. Additionally, tissue of origin (TOO) proportions were evaluated using two deconvolution methods. Sequencing cfDNA from urine using the double-stranded method resulted in a substantial within-read methylation bias and a lower global methylation (56.0% vs. 75.8%, p ≤ 0.0001) compared to plasma cfDNA, both of which were not observed with the single-stranded approach. Individual CpG site-based TOO deconvolution resulted in a significantly increased proportion of undetermined TOO with the double-stranded method (urine: 32.3% vs. 1.9%; plasma: 5.9% vs. 0.04%; p ≤ 0.0001), but no major differences in proportions of individual cell types. In contrast, fragment-level deconvolution led to multiple cell types, with significantly different TOO proportions between the two methods. This study thus outlines potential limitations of double-stranded library preparation for methylation analysis of cfDNA especially for urinary cfDNA. While the double-stranded method allows jagged end analysis in addition to TOO analysis, it leads to significant methylation bias in urinary cfDNA, which single-stranded methods can overcome.
dc.description.sponsorshipDepartment for BioMedical Research, Gruppe Ng
dc.description.sponsorshipUniversitätsinstitut für Klinische Chemie (UKC)
dc.description.sponsorshipUniversitätsklinik für Nephrologie und Hypertonie
dc.description.sponsorshipUniversitätsklinik für Viszerale Chirurgie und Medizin - Viszeral- und Transplantationschirurgie
dc.identifier.doi10.48350/185421
dc.identifier.pmid37568867
dc.identifier.publisherDOI10.3390/diagnostics13152505
dc.identifier.urihttps://boris-portal.unibe.ch/handle/20.500.12422/169244
dc.language.isoen
dc.publisherMDPI
dc.relation.ispartofDiagnostics
dc.relation.issn2075-4418
dc.relation.organizationDCD5A442BA49E17DE0405C82790C4DE2
dc.relation.organizationDCD5A442BB17E17DE0405C82790C4DE2
dc.relation.organizationDCD5A442BD11E17DE0405C82790C4DE2
dc.relation.organizationDCD5A442C059E17DE0405C82790C4DE2
dc.relation.schoolDCD5A442C27BE17DE0405C82790C4DE2
dc.subjectcfDNA enzymatic conversion methylation sequencing plasma single-stranded library preparation tissue of origin transplant urine
dc.subject.ddc600 - Technology::610 - Medicine & health
dc.titleInvestigation of Different Library Preparation and Tissue of Origin Deconvolution Methods for Urine and Plasma cfDNA Methylome Analysis.
dc.typearticle
dspace.entity.typePublication
dspace.file.typetext
oaire.citation.issue15
oaire.citation.volume13
oairecerif.author.affiliationUniversitätsinstitut für Klinische Chemie (UKC)
oairecerif.author.affiliationUniversitätsklinik für Nephrologie und Hypertonie
oairecerif.author.affiliationUniversitätsklinik für Viszerale Chirurgie und Medizin - Viszeral- und Transplantationschirurgie
oairecerif.author.affiliationUniversitätsinstitut für Klinische Chemie (UKC)
oairecerif.author.affiliationDepartment for BioMedical Research, Gruppe Ng
oairecerif.author.affiliationUniversitätsinstitut für Klinische Chemie (UKC)
unibe.contributor.rolecreator
unibe.contributor.rolecreator
unibe.contributor.rolecreator
unibe.contributor.rolecreator
unibe.contributor.rolecreator
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unibe.date.licenseChanged2023-08-16 13:31:34
unibe.description.ispublishedpub
unibe.eprints.legacyId185421
unibe.refereedtrue
unibe.subtype.articlejournal

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