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1.
胚泡着床窗口的分子调控 总被引:5,自引:0,他引:5
着床窗口是指当胚胎发育到胚泡阶段时,子宫也增殖和分化到可接受状态,二者相互作用使胚泡着床的短暂时间.雌激素和孕酮是该过程的综合调控分子,它们通过多种局部信号分子的介导,使子宫中的各种细胞类型增殖、分化,为着床窗口的开放做出相互协调的反应.子宫与胚胎在着床窗口通过前列腺素、组织胺、降钙素、多种细胞因子和生长因子的旁分泌作用进行分子对话,使胚泡滋养层与子宫内膜上皮发生附着反应.着床窗口一旦开放,即自动向非接受态转化. 相似文献
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PTEN在早孕小鼠子宫内膜的表达及其对胚泡着床的影响 总被引:1,自引:0,他引:1
本研究旨存检测肿瘤抑制基因PTEN(phosphatase andtensinhomologdeletedonchromosometen)在早孕小鼠子宫内膜中的表达规律,探讨PTEN在小鼠胚胎着床过程中的作用.采用实时荧光定量聚合酶联反应(real.time fluorescent quantitative PCR.FQ.PCR)和免疫组织化学方法分别检测未孕及孕1、3、4、5、7 d小鼠子宫内膜PTEN mRNA和蛋白的表达;子宫角注射PTEN反义寡核苷酸观察胚泡着床数.FQ-PCR结果显示,妊娠小鼠子宫内膜组织PTENmRNA的表达高于未妊娠小鼠,且随着妊娠天数的增加表达逐渐增强,到妊娠第5天达最高.免疫组织化学分析显示,PTEN蛋白在子宫内膜的表达规律与mRNA结果一致.子宫角注射PTEN反义寡核苷酸后胚泡着床数明显减少.结果提示,PTEN在妊娠早期子宫内膜持续表达,可能参与了胚泡着床. 相似文献
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gp130介导的信号转导通路在哺乳动物着床中的作用 总被引:1,自引:0,他引:1
IL—6相关细胞因子家族成员包括LIF、IL-6、IL-11以及它们的共同受体gp130,在哺乳动物的着床过程中起着重要的作用。LIF敲除的小鼠不能着床。IL—11Rα敲除的小鼠不能完全发生蜕膜化,从而导致妊娠的失败。IL—6敲除的小鼠着床数和着床胚胎的存活率均降低。这些细胞因子通过与受体结合,激活下游信号分子STAT,从而形成了gp130/Jak/STAT信号转导通路,并且STAT3基因敲除的小鼠也不能着床。这些细胞因子通过gp130/Jak/STAT信号转导通路在着床过程中起着重要的作用。了解此信号通路在看床中的作用对解决一些不明原因的不孕症,以及开发着床相关的避孕药物等具有重要意义。 相似文献
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白血病抑制因子对胚泡金属蛋白酶表达的影响 总被引:1,自引:0,他引:1
为了探讨白血病抑制因子 (LIF) 对胚泡着床作用的机理,胚泡经与LIF及其特异性抗体培养后,通过RT-PCR及免疫印迹技术,分析了LIF与着床前小鼠胚泡的基质金属蛋白酶9(MMP9)表达和分泌之间的关系.结果显示:LIF可明显诱导胚泡MMP9的分泌和基因表达; 经LIF特异性抗体封闭后,胚泡MMP9的分泌及基因表达下降,且下降趋势随着LIF被封闭时间延长而减弱,对MMPs组织抑制因子1(TIMP1)的影响则不明显.说明LIF可能通过诱导MMP9的分泌及基因表达来影响胚泡对子宫内膜细胞外基质的水解,促进着床. 相似文献
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本研究旨在检测肿瘤抑制基因p16INK4a(inhibitor of cyclin-dependent kinase 4a)在早孕小鼠子宫内膜中的表达规律,探讨p16INK4a在小鼠胚胎着床过程中的作用.采用荧光定量PCR(FQ-PCR)和免疫组织化学方法分别检测未孕小鼠及孕小鼠第2、3、4、5、7天子宫内膜p16INK4a mRNA和蛋白的表达;子宫角注射p16INK4a抗体观察胚泡着床数.FQ-PCR结果显示孕小鼠子宫内膜组织p16INK4amRNA的表达高于未孕小鼠,且随着妊娠天数的增加呈现表达逐渐增强的趋势,到妊娠第5天达到最高,后渐降.免疫组织化学分析显示p16INK4a蛋白在子宫内膜的表达规律与mRNA结果一致.子宫角注射p16INK4a抗体后胚泡着床数明显减少.以上结果提示,P161INK4a在妊娠早期子宫内膜持续表达,可能参与胚泡着床. 相似文献
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羟泰米酚的抗着床作用及其对小鼠子宫雌二醇… 总被引:1,自引:1,他引:0
经雌激素拮抗剂-羟仄米酚处理后的怀孕小鼠,胚泡着床受到明显抑制;同时,着床前子宫细胞质雌二醇受体和孕酮受体和孕酮受体明显减少,细胞核受体明显增加;拮抗剂还使血清雌激素和孕酮含量显著降低。结果表明:羟泰米酚的抗着床作用效应与子宫雌二醇受体和孕酮受体的正常功能受到干扰可能有密切关系的。 相似文献
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为探讨表皮生长因子(epidermal growth factor,EGF)在胚泡着床过程中的作用。本文应用原位杂交和免疫组织化学方法,检测了EGE及其受体在胚泡着床前后小鼠子宫内膜中的转录和表达。结果显示:未孕和受精后第4-5天,子宫内膜表面上皮和腺上皮细胞仍呈EGF,EGFR原位杂交和免疫组化阴性着色,受精后第4-5天子宫内膜基质细胞EGF及其受体转录和表达较未孕期增强,受精后第6天,EGF及其受体免疫组化和原位杂交阳性着色主要分布于初级蜕膜带(primary decidual zone,PDZ);随着胚泡植入的进行,PDZ区蜕膜细胞EGF及其受体的转录和表达明显减少,而PDZ周围蜕膜细胞EGF及其受体的转录和表达增强,结果提示,EGF是小鼠胚泡着床过程中的一个重要调节因子。 相似文献
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利用免疫组织化学及RT—PCR的方法,研究了细胞周期蛋白D3(Cyclin D3)在兔早期妊娠子宫和着床前胚胎中的表达情况,以揭示CyclinD3在兔胚胎着床过程中的可能作用。结果显示:(1)在兔妊娠第3~8天的子宫近肌层的腺上皮中有CyclinD3免疫染色,并且其表达强度在第7天以后呈现下降的趋势,着床的胚胎中未见CyclinD3免疫染色;(2)在第2~5天的假孕兔子宫的腺上皮中有较强的CyclinD3免疫染色;(3)在发情周期的兔子宫中未见其有表达;(4)在切除卵巢的兔中,注射雌激素后子宫中未见CyclinD3免疫染色,注射孕酮后在子宫腺上皮中有CyclinD3免疫染色,在孕酮和雌激素共同处理后的子宫腺上皮中有较强的CyclinD3免疫染色;(5)利用RT—PCR的方法在早期胚胎中均能检测到CyclinD3,但从胚泡期开始表达上升,到扩展胚泡时其表达最强。上述结果表明,CyclinD3的表达可能对兔胚泡的着床具有一定的调节作用。 相似文献
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Leukemia inhibitory factor and interleukin-11: Critical regulators in the establishment of pregnancy
Blastocyst implantation into a receptive endometrium is critical to the establishment of pregnancy and is tightly regulated by factors within the blastocyst–endometrial micro-environment. Leukemia inhibitory factor (LIF) and interleukin-11 (IL11) have key roles during implantation. Female mice with a null mutation in the LIF or IL11RA gene are infertile due to a complete failure of implantation or a defective differentiation/decidualization response to the implanting blastocyst, respectively. LIF and IL11 deficiency during pregnancy is associated with infertility and miscarriage in women. Numerous cell populations at the maternal–fetal interface are regulated by LIF/IL11 including the endometrial epithelium, decidualizing stroma, placental trophoblasts and leukocytes. This review focuses on the roles of LIF/IL11 during early pregnancy and highlights their potential as contraceptive targets and therapeutic agents for infertility. 相似文献
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Leukemia inhibitory factor (LIF) is essential for embryo implantation in mice. Whether LIF plays a role in termination of embryonic diapause and initiation of implantation in carnivores, especially in species with obligate delayed implantation such as the mink, is not known. The objectives of this study were to clone the LIF coding sequence in the mink and determine its mRNA abundance in the uterus through embryonic diapause, implantation, and early postimplantation. We show that the mink LIF cDNA contains 609 nt encoding a deduced protein of 203 amino acids. The homologies are 80.6, 90, 88.2, 87.6, and 86.8% in coding sequence and 79.2, 90.1, 91, 90.1 and 85.4% in amino acid sequence with mouse, human, pig, cow, and sheep respectively. Glycosylation sites and disulfide bonds present in other species are generally conserved in the mink LIF sequence. Quantitation by polymerase chain reaction amplification indicates that LIF mRNA is expressed in mink uterus just prior to implantation and during the first two days after implantation, but not during diapause or later after implantation pregnancy. The abundance of LIF mRNA was significantly higher in the uterus at the embryo expansion stage (P < 0.05) than at days 1–2 of postimplantation. By immunohistochemical localization it was shown that LIF is expressed in the uterine epithelial glands at time of embryonic expansion and in early postimplantation. The coincidence of LIF expression with implantation in this species suggests that LIF is involved in the implantation process, and may be a maternal signal which terminates obligate embryonic diapause. Mol. Reprod. Dev. 51:13–21, 1998. © 1998 Wiley-Liss, Inc. 相似文献
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Benkhalifa M Demirol A Sari T Balashova E Tsouroupaki M Giakoumakis Y Gurgan T 《Zygote (Cambridge, England)》2012,20(2):173-180
In repeated implantation failure, the co-culture of human embryos with somatic cells has been reported to promote the improvement of embryos quality, implantation and pregnancy rate. It was reported that feeder cells can be more beneficial to the oocyte and embryo by detoxifying the culture medium and supporting embryo development via different pathways. In this study, 432 patients, each with a minimum of three repeated implantation failures, were accepted for a prospective randomized study with or without autologous cumulus cell embryo co-culture and transfer at day 3 or day 5-6. We also investigated the expression of leukaemia inhibitor factor (LIF) and platelet activating factor receptor (PAF-R) on day 3 confluent cumulus cells. The statistic analysis of the data showed significant difference of implantation and clinical pregnancy rates between classical culture and day 3 compared with co-culture and day 5-6 transfer. The molecular analysis showed that cumulus cells express the LIF and the PAF-R genes and confirmed the possible positive role of growth factors and cytokines in early embryo development. Embryo co-culture systems with autologous cells can be beneficial in routine in vitro fertilization for embryo selection and implantation improvement. More molecular investigations need to be done to improve elucidation of the complex dialogue between the embryo and feeder cells prior to implantation and to understand the involved biological function and molecular process during embryo development. 相似文献
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Leukaemia inhibitory factor (LIF) is a pleiotrophic cytokine. Recent reports indicate that LIF is relevant to murine embryo implantation. In this work, results of indirect immunofluorescence under a confocal microscope illustrated that LIF was mainly located in the uterine lumen and uterine epithelial cells in pregnant mice on day 4. The number of embryos implanted in pregnant mice on day 8 decreased significantly after injection of 3 microg LIF antibodies into a uterine horn (P<0.001), which demonstrated again that LIF is a critical factor for embryo implantation. In a co-culture system, LIF (0.1 ng/ml, 1 ng/ml, 10 ng/ml and 100 ng/ml) significantly enhanced the blastocyst outgrowth after 24, 48 or 72 h of co-culture, and outgrowth areas after 72 h of co-culture. Conversely, 5 microg/ml and 10 microg/ml, but not 1 microg/ml, LIF antibodies decreased the percentage of blastocysts with outgrowth; only 10 microg/ml LIF antibody inhibited blastocyst outgrowth area significantly (P<0.001). However, neither LIF nor its antibodies changed embryo attachment. Analysis of correlation showed that the effects of LIF or its antibodies on the blastocyst outgrowth were dose-dependent. In summary, different pathways may exist to regulate the blastocyst attachment and outgrowth on a monolayer of uterine epithelial cells. LIF protein from the maternal uterus exerts an essential role in embryo implantation in the mouse, which is mediated by stimulating trophoblast outgrowth, but not by promoting the attachment. 相似文献
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Colin L. Stewart 《Molecular reproduction and development》1994,39(2):233-238
This paper reviews the evidence that certain growth factors, particularily leukaemia inhibitory factor (LIF), play a crucial role in regulating the development of the pre-implantation mammalian embryo. LIF was originally implicated in regulating the early development of the mouse embryo because it inhibited the differentiation of embryonic stem (ES) cells, pluripotential cells derived from the inner cell mass of the blastocyst. Subsequent studies on its role in vivo revealed, surprisingly, that it is essential for the growth rather than the differentiation of the blastocyst. In vivo, overtly normal blastocysts can be produced in a LIF-deficient environment that are capable of forming viable fertile adults. However, in the absence of LIF, they fail to implant and enter into a state resembling that exhibited by blastocysts undergoing delayed implantation, which is characterized by a cessation of cell proliferation. This failure to implant occurs because the principle sites of LIF production are the endometrial glands of the uterus. These synthesize and secrete LIF at implantation, with LIF synthesis essential for implantation. Preliminary evidence indicates that LIF synthesis is required both by the uterus for it to undergo decidualization and by the blastocyst for implantation. These data indicate that the maternal environment plays a crucial role in the development and growth of the pre-implantation embryo, by supplying factors that regulate these processes in the embryo. © 1994 Wiley-Liss, Inc. 相似文献
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小鼠早期胚胎发育期间LIF基因表达的研究(简报) 总被引:1,自引:0,他引:1
白血病抑制因子(Leukemia inhibitory fac-tor,LIF)是近年来研究较为广泛的细胞生长调节因子之一。最初发现LIF能够在体外诱导小鼠髓样白血病细胞株M1细胞向正常细胞分化,进一步分离纯化蛋白以及克隆基因后发现LIF在体外还具有多种功能,作用于不同的靶细胞时引起的生理效应也各不相同。目前已知的功能有:刺激肝脏细胞急性期反应蛋白的 相似文献
19.
Oshima K Watanabe H Yoshihara K Kojima T Dochi O Takenouchi N Fukushima M Komatsu M 《Theriogenology》2003,60(7):1217-1226
Leukemia inhibitory factor (LIF) and macrophage colony stimulating factor (M-CSF), members of the group of hemopoietic cytokines, play a primary role in the control of embryo development and implantation and in the growth of the placenta in humans and mice. Gene expressions of LIF and M-CSF were investigated using quantitative RT-PCR in bovine endometrial tissues during early and mid-pregnancy (Days 16-17, 20-21, 30-36, 48-49 and 74-140) and during the estrous cycle (Days 13-14). Leukemia inhibitory factor and M-CSF genes were expressed in all samples examined. Significant differences were found between the gene expression patterns of LIF and M-CSF. Leukemia inhibitory factor expression level at Days 48-49 was the highest in caruncular endometrium, however, the large variability negated any significant differences. Leukemia inhibitory factor expression levels in intercaruncular endometrium at Days 48-49 and 74-140 of pregnancy were greater than at Days 13-14 of the estrous cycle and at other days of pregnancy. No significant change was recognized in M-CSF expression levels in caruncular endometrium. Macrophage colony stimulating factor expression level in intercaruncular endometrium at Days 74-140 was greater than those of the other samples. These results suggest that LIF and M-CSF are produced in the endometrium and may play different roles in early and mid-pregnancy. 相似文献
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Evdokia Dimitriadis Andrew M Sharkey Yee Lee Tan Lois A Salamonsen J Robert A Sherwin 《Reproductive biology and endocrinology : RB&E》2007,5(1):44-8