Department of Obstetrics and Gynecology, Sun Yat-Sen Memorial Hospital, Sun Yat-Sen University, Guangzhou, China.
Guangdong Provincial Key Laboratory of Malignant Tumor Epigenetics and Gene Regulation, Guangdong-Hong Kong Joint Laboratory for RNA Medicine, Sun Yat-Sen Memorial Hospital, Sun Yat-Sen University, Guangzhou, China.
Front Immunol. 2021 Aug 13;12:717785. doi: 10.3389/fimmu.2021.717785. eCollection 2021.
Unexplained recurrent spontaneous abortion (URSA) is a common pregnancy complication and the etiology is unknown. URSA-associated lncRNAs are expected to be potential biomarkers for diagnosis, and might be related to the disease pathogenesis.
To investigate differential lncRNAs in peripheral blood of non-pregnant URSA patients and matched healthy control women and to explore the possible mechanism of differential lncRNAs leading to URSA.
We profiled lncRNAs expression in peripheral blood from 5 non-pregnant URSA patients and 5 matched healthy control women by lncRNA microarray analysis. Functions of URSA-associated lncRNAs were further investigated .
RP11-115N4.1 was identified as the most differentially expressed lncRNA which was highly upregulated in peripheral blood of non-pregnant URSA patients ( = 3.63E-07, Fold change = 2.96), and this dysregulation was further validated in approximately 26.67% additional patients (4/15). RP11-115N4.1 expression was detected in both lymphocytes and monocytes of human peripheral blood, and overexpression of RP11-115N4.1 decreased cell proliferation in K562 cells significantly. Furthermore, heat-shock HSP70 genes ( and ) were found to be significantly upregulated upon RP11-115N4.1 overexpression by transcriptome analysis ( ( = 4.39E-08, Fold change = 4.17), ( = 2.26E-06, Fold change = 2.99)). RNA pull down and RNA immunoprecipitation assay (RIP) analysis demonstrated that RP11-115N4.1 bound to HNRNPH3 protein directly, which in turn activate heat-shock proteins (HSP70) analyzed by protein-protein interaction and knockdown assays. Most importantly, the high expression of HSP70 was also verified in the serum of URSA patients and the supernatant of K562 cells with RP11-115N4.1 activation, and HSP70 in supernatant can exacerbate inflammatory responses in monocytes by inducing IL-6, IL-1β, and TNF-α and inhibit the migration of trophoblast cells, which might associate with URSA.
Our results demonstrated that the activation of RP11-115N4.1 can significantly increase the protein level of HSP70 binding to HNRNPH3, which may modulate the immune responses and related to URSA. Moreover, RP11-115N4.1 may be a novel etiological biomarker and a new therapeutic target for URSA.
不明原因的复发性自然流产(URSA)是一种常见的妊娠并发症,其病因尚不清楚。与 URSA 相关的长非编码 RNA(lncRNA)有望成为诊断的潜在生物标志物,可能与疾病发病机制有关。
探讨非妊娠 URSA 患者与匹配健康对照组女性外周血中差异表达的 lncRNA,并探讨差异表达的 lncRNA 导致 URSA 的可能机制。
我们通过 lncRNA 微阵列分析检测了 5 例非妊娠 URSA 患者和 5 例匹配健康对照组女性外周血中的 lncRNA 表达。进一步研究了与 URSA 相关的 lncRNA 的功能。
RP11-115N4.1 被鉴定为差异表达最显著的 lncRNA,在非妊娠 URSA 患者外周血中高度上调( = 3.63E-07,倍数变化 = 2.96),在约 26.67%的额外患者(4/15)中进一步验证了这种失调。RP11-115N4.1 的表达在人外周血的淋巴细胞和单核细胞中均被检测到,并且 RP11-115N4.1 的过表达显著降低了 K562 细胞的细胞增殖。此外,通过转录组分析发现,热休克 HSP70 基因( 和 )在 RP11-115N4.1 过表达时显著上调(( = 4.39E-08,倍数变化 = 4.17), ( = 2.26E-06,倍数变化 = 2.99))。RNA 下拉和 RNA 免疫沉淀分析(RIP)实验表明,RP11-115N4.1 直接与 HNRNPH3 蛋白结合,进而通过蛋白质-蛋白质相互作用和 knockdown 实验分析激活热休克蛋白(HSP70)。最重要的是,在 URSA 患者的血清和具有 RP11-115N4.1 激活的 K562 细胞上清液中也验证了 HSP70 的高表达,并且上清液中的 HSP70 可以通过诱导 IL-6、IL-1β 和 TNF-α 来加重单核细胞的炎症反应,并抑制滋养层细胞的迁移,这可能与 URSA 有关。
我们的结果表明,RP11-115N4.1 的激活可以显著增加与 HNRNPH3 结合的 HSP70 蛋白水平,这可能调节免疫反应,并与 URSA 相关。此外,RP11-115N4.1 可能是一种新的病因生物标志物和 URSA 的新治疗靶点。
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