Abstract
Breakdown of the balance between maternal pro- and anti-inflammatory pathways is thought to allow an anti-fetal maternal immune response that underlies development of chronic placental inflammation. Chronic placental inflammation is manifested by the influx of maternal inflammatory cells, including lymphocytes, histiocytes, and plasma cells, into the placental membranes, villi, and decidua. These infiltrates are recognized pathologically as chronic chorioamnionitis, chronic villitis of unknown etiology, and chronic deciduitis. Each of these histological entities is associated with adverse fetal outcomes including intrauterine growth restriction and preterm birth. Studying the gene expression patterns in chronically inflamed placenta, particularly when overlapping histologies are present, may lead to a better understanding of the underlying mechanism(s). Therefore, this study compared tissue with and without chronic placental inflammation, manifested as overlapping chronic chorioamnionitis, chronic villitis of unknown etiology, and chronic deciduitis. RNA expression profiling was conducted on formalin fixed, paraffin embedded placental tissue using Illumina microarrays. IGJ was the most significant differentially expressed gene identified and had increased expression in the inflamed tissue. In addition, IGLL1, CXCL13, CD27, CXCL9, ICOS, and KLRC1 had increased expression in the inflamed placental samples. These differentially expressed genes are associated with T follicular helper cells, natural killer cells, and B cells. Furthermore, these genes differ from those typically associated with the individual components of chronic placental inflammation, such as chronic villitis, suggesting that the inflammatory infiltrate associated with overlapping chronic chorioamnionitis, chronic villitis of unknown etiology, and chronic deciduitis differs is unique. To further explore and validate gene expression findings, we conducted immunohistochemical assessment of protein level expression and demonstrate that IgJ expression was largely attributable to the presence of plasma cells as part of chronic deciduitis and that IgA positive plasma cells are associated with chronic deciduitis occurring in combination with chronic chorioamnionitis and chronic villitis of unknown etiology but not with isolated chronic deciduitis.
Highlights
During pregnancy the maternal immune system recognizes paternal alloantigens expressed by the fetus but typically does not generate a significant anti-fetal inflammatory response
Loss of maternal tolerance to fetal tissue engenders an inflammatory response comprised primarily of T cells, histiocytes, and plasma cells. This cellular response is evident upon histopathological examination of affected placental and decidual tissue as chronic chorioamnionitis (CC), chronic villitis of unknown etiology (VUE), and chronic deciduitis (CD) [4,5,6]
It is important to recognize that the RNA integrity number (RIN) is a semiquantitative predictor of interexperimental variability for a particular methodology but is not a robust predictor of successful experimental outcomes as this is dependent on the methodology employed [18]
Summary
During pregnancy the maternal immune system recognizes paternal alloantigens expressed by the fetus but typically does not generate a significant anti-fetal inflammatory response. Loss of maternal tolerance to fetal tissue engenders an inflammatory response comprised primarily of T cells, histiocytes, and plasma cells. This cellular response is evident upon histopathological examination of affected placental and decidual tissue as chronic chorioamnionitis (CC), chronic villitis of unknown etiology (VUE), and chronic deciduitis (CD) [4,5,6]. Selection of fresh oCPI tissue for gene expression analysis is problematic as chronic inflammation is spatially and temporally variable and typically is not evident during standard gross placental examination. The use of formalin fixed, paraffin embedded (FFPE) tissue for gene expression study of oCPI is preferable as it allows positive selection of chronically inflamed tissue and incorporation of tissue with similar spatial and temporal distributions of inflammation. We explore the protein-level implication of the most significant gene using immunohistochemical studies
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