Bolnick Alan D, Bolnick Jay M, Kohan-Ghadr Hamid-Reza, Kilburn Brian A, Pasalodos Omar J, Singhal Pankaj K, Dai Jing, Diamond Michael P, Armant D Randall, Drewlo Sascha
Department of Obstetrics and Gynecology, Wayne State University, Detroit, MI, USA.
Department of Obstetrics and Gynecology, Good Samaritan Hospital Medical Center, West Islip, NY, USA.
Hum Reprod. 2017 Jun 1;32(6):1218-1229. doi: 10.1093/humrep/dex069.
Does low molecular weight heparin (LMWH) require heparin-binding epidermal growth factor (EGF)-like growth factor (HBEGF) signaling to induce extravillous trophoblast differentiation and decrease apoptosis during oxidative stress?
LMWH increased HBEGF expression and secretion, and HBEGF signaling was required to stimulate trophoblast extravillous differentiation, increase invasion in vitro and reduce trophoblast apoptosis during oxidative stress.
Abnormal trophoblast differentiation and survival contribute to placental insufficiency syndromes, including preeclampsia and intrauterine growth restriction. Preeclampsia often manifests as a pro-thrombotic state, with unsuccessful transformation of the spiral arteries that reduces oxygen supply and can produce placental infarction. LMWH improves placental function by increasing blood flow. Recent data suggest that the actions of LMWH transcend its anti-coagulative properties, but the molecular mechanism is unknown. There is evidence that LMWH alters the expression of human HBEGF in trophoblast cells, which regulates human trophoblast pathophysiology. HBEGF, itself, is capable of increasing trophoblast survival and invasiveness.
STUDY DESIGN, SIZE, DURATION: First-trimester placental explants and the HTR-8/SVneo cell line, established using extravillous trophoblast outgrowths from first-trimester villous explants, were treated in vitro with LMWH to examine the effects on HBEGF signaling and trophoblast function under normal physiological and pathological conditions. A highly specific antagonist of HBEGF and other inhibitors of HBEGF downstream signaling were used to determine the relationship between LMWH treatment and HBEGF.
PARTICIPANTS/MATERIALS, SETTING, METHODS: Placental tissues (n = 5) were obtained with IRB approval and patient consent from first-trimester terminations. Placental explants and HTR-8/SVneo cells were cultured on plastic or Matrigel™ and treated with a therapeutic dose of LMWH (Enoxaparin; 10 IU/ml), with or without CRM197, pan Erb-B2 Receptor Tyrosine Kinase (ERBB) inhibitor, anti-ERBB1 or ERBB4 blocking antibodies, or pretreatment of cells with heparitinase I. Extravillous differentiation was assessed by immunocytochemistry to determine the relative levels of integrins α6β4 and α1β1. Trophoblast invasiveness was assessed in villous explants by measuring outgrowth from villous tips cultured on Matrigel, and by invasion assays with HTR-8/SVneo cells cultured on Matrigel-coated transwell insert. Placental explants and HTR-8/SVneo cells were exposed to oxidative stress in a hypoxia-reoxygenation (H-R) model, measuring cell death by TUNEL assay, caspase 3 cleavage, and BCL-2α expression.
LMWH induced extravillous differentiation, according to trophoblast invasion assays and integrin (α6β4-α1β1) switching. Treatment with LMWH rescued cytotrophoblasts and HTR-8/SVneo cells from apoptosis during exposure to reoxygenation injury, based on TUNEL, caspase 3 cleavage and BCL-2α expression. Experiments using CRM197, ERBB1 and ERBB4 blocking antibodies, pan-ERBB inhibitor and removal of cell surface heparin demonstrated that the effects of LMWH on trophoblast invasion and survival were dependent upon HBEGF signaling.
N/A.
LIMITATIONS, REASONS FOR CAUTION: The primary limitation of this study was the use of only in vitro experiments. Patient demographics from elective terminations were not available.
These data provide new insights into the non-coagulation-related aspects of perinatal LMWH treatment in the management of placental insufficiency disorders.
STUDY FUNDING/COMPETING INTEREST(S): This research was supported by grants from the National Institutes of Health (HD071408 and HL128628), the March of Dimes, and the W. K. Kellogg Foundation. There were no conflicts or competing interests.
低分子量肝素(LMWH)是否需要肝素结合表皮生长因子(EGF)样生长因子(HBEGF)信号传导来诱导绒毛外滋养层细胞分化并减少氧化应激期间的细胞凋亡?
LMWH增加了HBEGF的表达和分泌,并且HBEGF信号传导是刺激滋养层细胞绒毛外分化、增加体外侵袭以及减少氧化应激期间滋养层细胞凋亡所必需的。
滋养层细胞分化和存活异常会导致胎盘功能不全综合征,包括先兆子痫和胎儿生长受限。先兆子痫通常表现为血栓形成倾向,螺旋动脉转化失败,减少了氧气供应并可导致胎盘梗死。LMWH通过增加血流量来改善胎盘功能。最近的数据表明,LMWH的作用超越了其抗凝特性,但其分子机制尚不清楚。有证据表明,LMWH会改变滋养层细胞中人类HBEGF的表达,而HBEGF可调节人类滋养层细胞的病理生理学。HBEGF本身能够提高滋养层细胞的存活率和侵袭性。
研究设计、规模、持续时间:使用来自孕早期绒毛外植体的绒毛外滋养层细胞建立的孕早期胎盘外植体和HTR-8/SVneo细胞系,在体外使用LMWH进行处理,以研究在正常生理和病理条件下对HBEGF信号传导和滋养层细胞功能的影响。使用HBEGF的高度特异性拮抗剂和其他HBEGF下游信号传导抑制剂来确定LMWH处理与HBEGF之间的关系。
参与者/材料、设置、方法:经机构审查委员会批准并获得患者同意后,从孕早期终止妊娠中获取胎盘组织(n = 5)。胎盘外植体和HTR-8/SVneo细胞在塑料或基质胶上培养,并用治疗剂量的LMWH(依诺肝素;10 IU/ml)处理,同时或不添加CRM197、泛Erb-B2受体酪氨酸激酶(ERBB)抑制剂、抗ERBB1或ERBB4阻断抗体,或先用肝素酶I预处理细胞。通过免疫细胞化学评估绒毛外分化,以确定整合素α6β4和α1β1的相对水平。通过测量在基质胶上培养的绒毛尖端的生长情况以及用在基质胶包被的Transwell小室中培养的HTR-8/SVneo细胞进行侵袭试验,评估绒毛外植体中的滋养层细胞侵袭性。胎盘外植体和HTR-8/SVneo细胞在缺氧复氧(H-R)模型中暴露于氧化应激,通过TUNEL检测、半胱天冬酶3切割和BCL-2α表达来测量细胞死亡。
根据滋养层细胞侵袭试验和整合素(α6β4-α1β1)转换,LMWH诱导了绒毛外分化。基于TUNEL、半胱天冬酶3切割和BCL-2α表达,LMWH处理可使细胞滋养层细胞和HTR-8/SVneo细胞在暴露于复氧损伤期间免于凋亡。使用CRM197、ERBB1和ERBB4阻断抗体、泛ERBB抑制剂以及去除细胞表面肝素的实验表明,LMWH对滋养层细胞侵袭和存活的影响依赖于HBEGF信号传导。
无。
局限性、谨慎理由:本研究的主要局限性在于仅使用了体外实验。无法获得来自选择性终止妊娠的患者人口统计学数据。
这些数据为围产期LMWH治疗在胎盘功能不全疾病管理中与凝血无关的方面提供了新的见解。
研究资金/竞争利益:本研究得到了美国国立卫生研究院(HD071408和HL128628)、美国疾病控制与预防中心出生缺陷基金会以及W.K.凯洛格基金会的资助。不存在冲突或竞争利益。
