Design of a targeted blood transcriptional panel for monitoring immunological changes accompanying pregnancy

Simple item page
dc.contributor.authorBrummaier T.
dc.contributor.authorRinchai D.
dc.contributor.authorToufiq M.
dc.contributor.authorKarim M.Y.
dc.contributor.authorHabib T.
dc.contributor.authorUtzinger J.
dc.contributor.authorParis D.H.
dc.contributor.authorMcGready R.
dc.contributor.authorMarr A.K.
dc.contributor.authorKino T.
dc.contributor.authorTerranegra A.
dc.contributor.authorAl Khodor S.
dc.contributor.authorChaussabel D.
dc.contributor.authorSyed Ahamed Kabeer B.
dc.contributor.correspondenceBrummaier T.
dc.contributor.otherMahidol University
dc.date.accessioned2024-02-19T18:04:57Z
dc.date.available2024-02-19T18:04:57Z
dc.date.issued2024-01-01
dc.description.abstractBackground: Immunomodulatory processes exert steering functions throughout pregnancy. Detecting diversions from this physiologic immune clock may help identify pregnant women at risk for pregnancy-associated complications. We present results from a data-driven selection process to develop a targeted panel of mRNAs that may prove effective in detecting pregnancies diverting from the norm. Methods: Based on a de novo dataset from a resource-constrained setting and a dataset from a resource-rich area readily available in the public domain, whole blood gene expression profiles of uneventful pregnancies were captured at multiple time points during pregnancy. BloodGen3, a fixed blood transcriptional module repertoire, was employed to analyze and visualize gene expression patterns in the two datasets. Differentially expressed genes were identified by comparing their abundance to non-pregnant postpartum controls. The selection process for a targeted gene panel considered (i) transcript abundance in whole blood; (ii) degree of correlation with the BloodGen3 module; and (iii) pregnancy biology. Results: We identified 176 transcripts that were complemented with eight housekeeping genes. Changes in transcript abundance were seen in the early stages of pregnancy and similar patterns were observed in both datasets. Functional gene annotation suggested significant changes in the lymphoid, prostaglandin and inflammation-associated compartments, when compared to the postpartum controls. Conclusion: The gene panel presented here holds promise for the development of predictive, targeted, transcriptional profiling assays. Such assays might become useful for monitoring of pregnant women, specifically to detect potential adverse events early. Prospective validation of this targeted assay, in-depth investigation of functional annotations of differentially expressed genes, and assessment of common pregnancy-associated complications with the aim to identify these early in pregnancy to improve pregnancy outcomes are the next steps.
dc.identifier.citationFrontiers in Immunology Vol.15 (2024)
dc.identifier.doi10.3389/fimmu.2024.1319949
dc.identifier.eissn16643224
dc.identifier.scopus2-s2.0-85184703613
dc.identifier.urihttps://repository.li.mahidol.ac.th/handle/20.500.14594/97242
dc.rights.holderSCOPUS
dc.subjectMedicine
dc.subjectImmunology and Microbiology
dc.titleDesign of a targeted blood transcriptional panel for monitoring immunological changes accompanying pregnancy
dc.typeArticle
mu.datasource.scopushttps://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=85184703613&origin=inward
oaire.citation.titleFrontiers in Immunology
oaire.citation.volume15
oairecerif.author.affiliationMahidol Oxford Tropical Medicine Research Unit
oairecerif.author.affiliationSidra Medicine
oairecerif.author.affiliationWeill Cornell Medicine-Qatar
oairecerif.author.affiliationUniversitat Basel
oairecerif.author.affiliationSwiss Tropical and Public Health Institute Swiss TPH
oairecerif.author.affiliationSt. Jude Children's Research Hospital
oairecerif.author.affiliationThe Jackson Laboratory
oairecerif.author.affiliationNuffield Department of Medicine

Files

Collections

Scopus 2024