IInstituto de Biología y Medicina Experimental (IByME-CONICET), Vuelta de Obligado 2490, C1428ADN, Buenos Aires, Argentina.
Instituto de Investigaciones Farmacológicas (ININFA-UBA-CONICET), Facultad de Farmacia y Bioquímica, Universidad de Buenos Aires, Buenos Aires, Argentina.
Hum Reprod. 2018 May 1;33(5):844-859. doi: 10.1093/humrep/dey045.
Is ceramide-1-phosphate (C1P) an ovarian protective agent during alkylating chemotherapy?
Local administration of C1P drastically reduces ovarian damage induced by cyclophosphamide (Cy) via protection of follicular reserve, restoration of hormone levels, inhibition of apoptosis and improvement of stromal vasculature, while protecting fertility, oocyte quality and uterine morphology.
Cancer-directed therapies cause accelerated loss of ovarian reserve and lead to premature ovarian failure (POF). Previous studies have demonstrated that C1P regulates different cellular processes including cell proliferation, cell migration, angiogenesis and apoptosis. This sphingolipid may be capable of modulating vascular development and apoptosis in ovaries affected by chemotherapy.
STUDY DESIGN, SIZE, DURATION: The 6-8-week-old mice were weighed and administered either a single intraperitoneal injection of Cy (75 mg/kg) or an equal volume of saline solution only for control mice. Control and Cy mice underwent sham surgery and received an intrabursal injection of saline solution, while Cy + C1P animal groups received 5 μl C1P, either 0.5 or 1 mM, under the bursa of both ovaries 1 h prior to Cy administration.
PARTICIPANTS/MATERIALS, SETTING, METHODS: Animals were euthanized by cervical dislocation or cardiac puncture 2 weeks after surgery for collection of blood orovary and uterus samples, which were cleaned of adhering tissue in culture medium and used for subsequent assays. Ovaries were used for Western blotting or immunohistochemical and/or histological analyses or steroid extraction, as required (n = 5-8 per group). A set of mice (n = 3/group) was destined for oocyte recovery and IVF. Finally, another set (n = 5-6/group) was separated to study fertility parameters.
The number of primordial (P < 0.01), primary (P < 0.05) and preantral follicles (P < 0.05) were decreased in Cy-treated mice compared to control animals, while atretic follicles were increased (P < 0.001). In Cy + C1P mice, the ovaries recovered control numbers of these follicular structures, in both C1P doses studied. Cy affected AMH expression, while it was at least partially recovered when C1P is administered as well. Cy caused an increase in serum FSH concentration (P < 0.01), which was prevented by C1P coadministration (P < 0.01). E2 levels in Cy-treated ovaries decreased significantly compared to control ovaries (P < 0.01), whilst C1P restored E2 levels to those of control ovaries (P < 0.01). Cy increased the expression of BAX (P < 0.01) and decreased the expression of BCLX-L compared to control ovaries (P < 0.01). The ovarian BCLX-L:BAX ratio was also lower in Cy-treated mice (P < 0.05). In the Cy + C1P group, the expression levels of BAX, BCLX-L and BCLX-L:BAX ratio were no different than those in control ovaries. In addition, acid sphingomyelinase (A-SMase) expression was higher in Cy-treated ovaries, whilst remaining similar to the control in the Cy + C1P group. Cy increased the apoptotic index (TUNEL-positive follicles/total follicles) in preantral and early antral stages, compared to control ovaries (P < 0.001 and P < 0.01, respectively). C1P protected follicles from this increase. No primordial or primary follicular cells stained for either cleaved caspase-3 or TUNEL when exposed to Cy, therefore, we have found no evidence for follicular reserve depletion in response to Cy being due to apoptosis. Cy caused evident vascular injury, especially in large cortical stromal vessels, and some neovascularization. In the Cy + C1P group, the disruptions in vascular wall continuity were less evident and the number of healthy stromal blood vessels seemed to be restored. In Cy-treated ovaries α-SMA-positive cells showed a less uniform distribution around blood vessels. C1P coadministration partially prevented this Cy-induced effect, with a higher presence of α-SMA-positive cells surrounding vessels. By H&E staining, Cy-treated mice showed endometrial alterations compared to controls, affecting both epithelial and stromal compartments. However, C1P allowed that the stromal tissue to maintain its loose quality and its glandular branches. Cy-treated animals had significantly lower pregnancy rates and smaller litter sizes compared with control mice (P = 0.013 and P < 0.05, respectively), whereas cotreatment with C1P preserved normal fertility. Furthermore, a higher (P < 0.05) proportion of abnormal oocytes was recovered from Cy-treated mice compared to the control, which was prevented by C1P administration.
N/A.
The results of this study were generated from an in-vivo animal experimental model, already used by several authors. Further studies on C1P functions in female reproduction in pathological conditions such as chemotherapy-induced ovarian failure and on the safety of use of this sphingolipid are required.
The present findings showed that C1P administration prior to Cy might be a promising fertility preservation strategy in female patients who undergo chemotherapy.
STUDY FUNDING/COMPETING INTEREST(S): This work was supported by grants from ANPCyT (PICT 2015-1117), CONICET (PIP 380), Cancer National Institute (INC) and Roemmers Foundation, Argentina. The authors declare no conflicts of interest.
神经酰胺-1-磷酸(C1P)是否是烷化化疗过程中卵巢的保护剂?
局部给予 C1P 可通过保护卵泡储备、恢复激素水平、抑制细胞凋亡和改善基质血管来显著减少环磷酰胺(Cy)诱导的卵巢损伤,同时保护生育能力、卵母细胞质量和子宫形态。
癌症靶向治疗会导致卵巢储备迅速丧失,并导致卵巢早衰(POF)。先前的研究表明,C1P 调节包括细胞增殖、细胞迁移、血管生成和细胞凋亡在内的不同细胞过程。这种鞘脂可能能够调节受化疗影响的卵巢中的血管发育和细胞凋亡。
研究设计、规模、持续时间:6-8 周龄的小鼠称重后,单次腹腔内注射 Cy(75mg/kg)或仅生理盐水作为对照小鼠。对照和 Cy 小鼠接受假手术,并接受囊内生理盐水注射,而 Cy+C1P 动物组在给予 Cy 前 1 小时在囊下给予 5μl C1P,浓度为 0.5 或 1mM。
参与者/材料、设置、方法:手术后 2 周,通过颈椎脱位或心脏穿刺处死动物,收集血液、卵巢和子宫样本,在培养基中清除附着的组织,然后用于随后的检测。卵巢用于 Western blot 或免疫组织化学和/或组织学分析或类固醇提取(每组 5-8 只)。一组(每组 3 只)用于卵母细胞回收和体外受精。最后,另一组(每组 5-6 只)用于研究生育能力参数。
与对照组动物相比,Cy 处理小鼠的原始卵泡(P<0.01)、初级卵泡(P<0.05)和初级卵泡(P<0.05)数量减少,而闭锁卵泡增加(P<0.001)。在 Cy+C1P 小鼠中,卵巢恢复了这些卵泡结构的对照数量,在研究的两种 C1P 剂量中都是如此。Cy 影响 AMH 表达,而当给予 C1P 时至少部分恢复。Cy 导致血清 FSH 浓度升高(P<0.01),这一作用被 C1P 共同给药所阻止(P<0.01)。与对照卵巢相比,Cy 处理的卵巢中 E2 水平显著降低(P<0.01),而 C1P 则将 E2 水平恢复至对照卵巢的水平(P<0.01)。Cy 增加了 BAX 的表达(P<0.01),并降低了 BCLX-L 的表达与对照组卵巢相比(P<0.01)。Cy 处理的小鼠卵巢中 BCLX-L:BAX 比值也较低(P<0.05)。在 Cy+C1P 组中,BAX、BCLX-L 和 BCLX-L:BAX 比值的表达水平与对照卵巢无差异。此外,Cy 处理的卵巢中酸性鞘磷脂酶(A-SMase)的表达较高,而在 Cy+C1P 组中与对照卵巢相似。Cy 增加了 preantral 和早期 antral 阶段的凋亡指数(TUNEL 阳性卵泡/总卵泡),与对照组相比(P<0.001 和 P<0.01)。C1P 保护卵泡免受这种增加。在 Cy 处理的卵巢中,没有原始卵泡或初级卵泡细胞对 cleaved caspase-3 或 TUNEL 染色,因此,我们没有发现 Cy 导致的卵泡储备耗竭是由于细胞凋亡所致的证据。Cy 引起明显的血管损伤,特别是在大皮质基质血管中,并且存在一些新血管生成。在 Cy+C1P 组中,血管壁连续性的中断不那么明显,并且似乎恢复了健康的基质血管数量。在 Cy 处理的卵巢中,α-SMA 阳性细胞在血管周围的分布不均匀。C1P 共同给药部分阻止了 Cy 诱导的这种作用,使更多的α-SMA 阳性细胞围绕血管。通过 H&E 染色,与对照组相比,Cy 处理的小鼠子宫内膜发生改变,影响上皮和基质细胞。然而,C1P 允许基质组织保持其疏松的质量及其腺支。与对照组相比,Cy 处理的动物妊娠率显著降低,产仔数减少(P=0.013 和 P<0.05),而 C1P 共同给药可保留正常生育能力。此外,与对照组相比,从 Cy 处理的小鼠中回收的异常卵母细胞比例更高(P<0.05),而给予 C1P 可防止这种情况。
无。
本研究结果来自于已被多位作者使用的体内动物实验模型。需要进一步研究 C1P 在化疗诱导的卵巢衰竭等病理情况下在女性生殖中的功能以及使用这种鞘脂的安全性。
本研究结果表明,在接受化疗的女性患者中,在给予 Cy 之前给予 C1P 可能是一种有前途的生育力保存策略。
研究资金/利益冲突:本工作得到了 ANPCyT(PICT 2015-1117)、CONICET(PIP 380)、癌症国家研究所(INC)和 Roemmers 基金会的支持。作者没有利益冲突。
