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脑型大麻素受体的激活会干扰植入前小鼠胚胎的发育。

Activation of brain-type cannabinoid receptors interferes with preimplantation mouse embryo development.

作者信息

Yang Z M, Paria B C, Dey S K

机构信息

Department of Physiology, Ralph L. Smith Research Center, University of Kansas Medical Center, Kansas City 66160-7338, USA.

出版信息

Biol Reprod. 1996 Oct;55(4):756-61. doi: 10.1095/biolreprod55.4.756.

DOI:10.1095/biolreprod55.4.756
PMID:8879486
Abstract

The recent identification and cloning of guanine nucleotide regulatory protein-coupled brain-type and spleen-type cannabinoid receptors (CB1-R and CB2-R, respectively) provide evidence that many of the effects of cannabinoids are mediated via these receptors. Our recent observation of expression of both CB1-R and CB2-R genes in the preimplantation mouse embryo suggests that it could also be a target for cannabinoids. Indeed, cannabinoid agonists interfered with preimplantation embryo development in vitro. To examine whether cannabinoid effects on preimplantation embryos are mediated via CB1-R, we developed rabbit antipeptide antibodies against the N-terminal region of CB1-R and examined the receptor protein in the blastocyst by Western blotting and its spatiotemporal distribution in preimplantation mouse embryos by immunohistochemistry. Cannabinoid binding sites in the blastocyst were examined by Scatchard analysis, while the reversibility of cannabinoid-induced embryonic arrest in vitro was monitored using a specific antagonist to CB1-R, SR141716A. Western blot analysis detected a major band of approximately 59 kDa and a minor band of approximately 54 kDa in the blastocyst. Immunocytochemistry detected this receptor protein from the 2-cell through the blastocyst stages. Scatchard analysis using 3H-anandamide (an endogenous ligand) showed a single class of binding sites in Day 4 blastocysts with an apparent Kd of 1.0 nM and Bmax of 0.09 fmol/blastocyst. Considering the total number of cells (approximately 50) and total protein content (approximately 20 ng) of a blastocyst, it is apparent that the mouse blastocyst has many more high-affinity receptors than those in the mouse brain (Kd: 1.8 nM and Bmax: 18.8 pmol/mg membrane protein). Cannabinoid agonists and the CB1-R antagonist SR141716A effectively competed for anandamide binding in the blastocyst. To determine whether cannabinoid inhibition of embryonic development could be reversed by SR141716A, 2-cell embryos were cultured in the presence of cannabinoid agonists with or without SR141716A for 72 h. Most of the 2-cell embryos cultured in the absence of the agonists developed into blastocysts (approximately 90%). In contrast, the addition of cannabinoid agonists anandamide, Win 55212-2, or CP 55,940 in the culture medium severely compromised embryonic development: more than 60% of the 2-cell embryos failed to develop to blastocysts. A reduction in trophectoderm cell numbers was noted in those blastocysts that escaped the developmental arrest in the presence of cannabinoid agonists. However, this reduction was corrected when embryos were cultured simultaneously with an agonist and SR141716A. Furthermore, embryonic arrest was reversed when embryos were cultured simultaneously in the presence of an agonist and SR141716A. The addition of SR141716A alone in the culture medium apparently had no effects on embryonic development: more than 90% of the embryos developed into blastocysts. The results suggest that the CB1 receptors in preimplantation mouse embryos are biologically active and cannabinoid effects on them are primarily mediated by these receptors.

摘要

最近对鸟嘌呤核苷酸调节蛋白偶联的脑型和脾型大麻素受体(分别为CB1-R和CB2-R)的鉴定和克隆表明,大麻素的许多作用是通过这些受体介导的。我们最近观察到CB1-R和CB2-R基因在植入前小鼠胚胎中均有表达,这表明它也可能是大麻素的作用靶点。事实上,大麻素激动剂在体外干扰了植入前胚胎的发育。为了研究大麻素对植入前胚胎的作用是否通过CB1-R介导,我们制备了针对CB1-R N端区域的兔抗肽抗体,并通过蛋白质印迹法检测囊胚中的受体蛋白,通过免疫组织化学法检测其在植入前小鼠胚胎中的时空分布。通过Scatchard分析检测囊胚中的大麻素结合位点,同时使用CB1-R特异性拮抗剂SR141716A监测大麻素诱导的体外胚胎发育停滞的可逆性。蛋白质印迹分析在囊胚中检测到一条约59 kDa的主要条带和一条约54 kDa的次要条带。免疫细胞化学检测到从2细胞期到囊胚期均有这种受体蛋白。使用3H-花生四烯酸乙醇胺(一种内源性配体)进行的Scatchard分析显示,在第4天的囊胚中有一类单一的结合位点,其表观解离常数(Kd)为1.0 nM,最大结合容量(Bmax)为0.09 fmol/囊胚。考虑到一个囊胚的细胞总数(约50个)和总蛋白含量(约20 ng),显然小鼠囊胚的高亲和力受体比小鼠脑中的多得多(小鼠脑的Kd:1.8 nM,Bmax:18.8 pmol/mg膜蛋白)。大麻素激动剂和CB1-R拮抗剂SR141716A在囊胚中有效竞争花生四烯酸乙醇胺的结合。为了确定SR141716A是否能逆转大麻素对胚胎发育的抑制作用,将2细胞胚胎在有或无SR141716A的情况下与大麻素激动剂一起培养72小时。在无激动剂的情况下培养的大多数2细胞胚胎发育成了囊胚(约90%)。相反,在培养基中添加大麻素激动剂花生四烯酸乙醇胺、Win 55212-2或CP 55940严重损害了胚胎发育:超过60%的2细胞胚胎未能发育成囊胚。在存在大麻素激动剂时逃脱发育停滞的那些囊胚中,滋养外胚层细胞数量减少。然而,当胚胎与激动剂和SR141716A同时培养时,这种减少得到了纠正。此外,当胚胎在激动剂和SR141716A同时存在的情况下培养时,胚胎发育停滞得到了逆转。在培养基中单独添加SR141716A显然对胚胎发育没有影响:超过90%的胚胎发育成了囊胚。结果表明,植入前小鼠胚胎中的CB1受体具有生物学活性,大麻素对它们的作用主要由这些受体介导。

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