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足月和早产胎盘无羊膜腔内感染时 16S 原位杂交对微生物的可视化。

Visualization of microbes by 16S in situ hybridization in term and preterm placentas without intraamniotic infection.

机构信息

Department of Obstetrics & Gynecology, Division of Maternal-Fetal Medicine, Baylor College of Medicine, Houston, Texas.

Department of Pathology & Immunology, Baylor College of Medicine and Texas Children's Hospital, Houston, Texas.

出版信息

Am J Obstet Gynecol. 2019 Aug;221(2):146.e1-146.e23. doi: 10.1016/j.ajog.2019.04.036. Epub 2019 May 2.

Abstract

BACKGROUND

Numerous reports have documented bacteria in the placental membranes and basal plate decidua in the absence of immunopathology using histologic techniques. Similarly, independent metagenomic characterizations have identified an altered taxonomic makeup in association with spontaneous preterm birth. Here we sought to corroborate these findings by localizing presumptive intact bacteria using molecular histology within the placental microanatomy.

OBJECTIVE

Here we examined for microbes in term and preterm gestations using a signal-amplified 16S universal in situ hybridization probe set for bacterial rRNA, alongside traditional histologic methods of Warthin-Starry and Gram stains, as well as clinical culture methodologies. We further sought to differentiate accompanying 16S gene sequencing taxonomic profiles from germ-free (gnotobiotic) mouse and extraction and amplicon contamination controls.

STUDY DESIGN

Placentas were collected from a total of 53 subjects, composed of term labored (n = 4) and unlabored cesarean deliveries (n = 22) and preterm vaginal (n = 18) and cesarean deliveries (n = 8); a placenta from a single subject with clinical and histologic evident choriomanionitis was employed as a positive control (n = 1). The preterm cohort included spontaneous preterm birth with (n = 6) and without (n = 10) preterm premature rupture of membranes, as well as medically indicated preterm births (n = 10). Placental microbes were visualized using an in situ hybridization probe set designed against highly conserved regions of the bacterial 16S ribosome, which produces an amplified stable signal using branched DNA probes. Extracted bacterial nucleic acids from these same samples were subjected to 16S rRNA metagenomic sequencing (Illumina, V4) for course taxonomic analysis, alongside environmental and kit contaminant controls. A subset of unlabored, cesarean-delivered term pregnancies were also assessed with clinical culture for readily cultivatable pathogenic microbes.

RESULTS

Molecular in situ hybridization of bacterial rRNA enabled visualization and localization of low-abundance microbes after systematic high-power scanning. Despite the absence of clinical or histologic chorioamnionitis in 52 of 53 subjects, instances of 16S rRNA signal were confidently observed in 13 of 16 spontaneous preterm birth placentas, which was not significantly different from term unlabored cesarean specimens (18 of 22; P > .05). 16S rRNA signal was largely localized to the villous parenchyma and/or syncytiotrophoblast, and less commonly the chorion and the maternal intervillous space. In all term and unlabored cesarean deliveries, visualization of evident placental microbes by in situ hybridization occurred in the absence of clinical or histologic detection using conventional clinical cultivation, hematoxylin-eosin, and Gram staining. In 1 subject, appreciable villous bacteria localized to an infarction, where 16S microbial detection was confirmed by Warthin-Starry stain. In all instances, parallel sample principle coordinate analysis using Bray-Cutis distances of 16S rRNA gene sequencing data demonstrated consistent taxonomic distinction from all negative or potential contamination controls (P = .024, PERMANOVA). Classification from contaminant filtered data identified a distinct taxonomic makeup among term and preterm cohorts when compared with contaminant controls (false discovery rate <0.05).

CONCLUSION

Presumptively intact placental microbes are visualized as low-abundance, low-biomass and sparse populations within the placenta regardless of gestational age and mode of delivery. Their taxonomic makeup is distinct from contamination controls. These findings further support several previously published findings, including our own, which have used metagenomics to characterize low-abundance and low-biomass microbial communities in the placenta.

摘要

背景

使用组织学技术,大量报道记录了胎盘膜和基底板蜕膜中无免疫病理学的细菌。同样,独立的宏基因组特征鉴定与自发性早产相关的分类组成改变。在这里,我们试图通过在胎盘微解剖学中使用分子组织学来定位推定完整的细菌来证实这些发现。

目的

在这里,我们使用针对细菌 rRNA 的信号放大 16S 通用原位杂交探针组,以及传统的沃辛-斯塔尔里和革兰氏染色组织学方法,以及临床培养方法,检查了足月和早产妊娠中的微生物。我们还进一步试图从无菌(无菌)小鼠和提取及扩增子污染对照中区分伴随的 16S 基因测序分类特征。

研究设计

总共收集了 53 名受试者的胎盘,其中包括足月分娩(n=4)和未分娩剖宫产(n=22)和早产阴道(n=18)和剖宫产(n=8);一名患有临床和组织学明显绒毛膜羊膜炎的患者的胎盘被用作阳性对照(n=1)。早产队列包括自发性早产伴(n=6)和不伴(n=10)胎膜早破、以及医学指征的早产(n=10)。使用针对细菌 16S 核糖体高度保守区域设计的原位杂交探针组来可视化微生物,该探针组使用分支 DNA 探针产生放大的稳定信号。从这些相同的样本中提取的细菌核酸进行 16S rRNA 宏基因组测序(Illumina,V4)进行课程分类分析,以及环境和试剂盒污染物对照。一部分未经处理的、剖宫产的足月妊娠也进行了临床培养,以检测可培养的致病微生物。

结果

细菌 rRNA 的分子原位杂交使我们能够在系统地进行高倍扫描后,对低丰度的微生物进行可视化和定位。尽管在 53 名受试者中的 52 名没有临床或组织学绒毛膜羊膜炎,但在 16 例自发性早产胎盘中有信心地观察到 16S rRNA 信号,这与未分娩的剖宫产标本(18/22;P>.05)没有显著差异。16S rRNA 信号主要定位于绒毛小叶实质和/或合体滋养层,较少见于绒毛膜和母体绒毛间隙。在所有足月和未分娩的剖宫产中,通过原位杂交观察到明显的胎盘微生物,而传统的临床培养、苏木精-伊红和革兰氏染色未能检测到临床或组织学。在 1 例患者中,明显的绒毛细菌定位于梗死灶,其中通过沃辛-斯塔尔里染色证实了 16S 微生物的检测。在所有情况下,使用 Bray-Cutis 距离的 16S rRNA 基因测序数据进行平行样本主坐标分析,从所有阴性或潜在污染对照中都证明了一致的分类学区别(P=0.024,PERMANOVA)。与污染对照相比,经过污染过滤的数据的分类确定了足月和早产队列之间独特的分类组成(错误发现率<0.05)。

结论

无论胎龄和分娩方式如何,胎盘内的推定完整的胎盘微生物均被视为低丰度、低生物量和稀疏的群体。它们的分类组成与污染对照不同。这些发现进一步支持了几项先前发表的研究结果,包括我们自己的研究结果,这些研究结果使用宏基因组学来描述胎盘内低丰度和低生物量微生物群落。

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