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本文引用的文献

1
A Unique Egg Cortical Granule Localization Motif Is Required for Ovastacin Sequestration to Prevent Premature ZP2 Cleavage and Ensure Female Fertility in Mice.一种独特的卵皮质颗粒定位基序是将卵母细胞溶素隔离以防止过早的ZP2裂解并确保小鼠雌性生育能力所必需的。
PLoS Genet. 2017 Jan 23;13(1):e1006580. doi: 10.1371/journal.pgen.1006580. eCollection 2017 Jan.
2
Zinc sparks induce physiochemical changes in the egg zona pellucida that prevent polyspermy.锌离子火花会引起卵透明带的理化变化,从而防止多精受精。
Integr Biol (Camb). 2017 Feb 20;9(2):135-144. doi: 10.1039/c6ib00212a.
3
Recombinant fetuin-B protein maintains high fertilization rate in cumulus cell-free mouse oocytes.重组胎球蛋白-B蛋白维持无卵丘细胞小鼠卵母细胞的高受精率。
Mol Hum Reprod. 2017 Jan;23(1):25-33. doi: 10.1093/molehr/gaw067. Epub 2016 Oct 12.
4
Down-regulation of the liver-derived plasma protein fetuin-B mediates reversible female infertility.肝脏来源的血浆蛋白胎球蛋白-B的下调介导可逆性女性不孕。
Mol Hum Reprod. 2017 Jan;23(1):34-44. doi: 10.1093/molehr/gaw068. Epub 2016 Oct 12.
5
Molecular architecture of the human sperm IZUMO1 and egg JUNO fertilization complex.人类精子IZUMO1与卵子JUNO受精复合体的分子结构
Nature. 2016 Jun 23;534(7608):562-5. doi: 10.1038/nature18595. Epub 2016 Jun 15.
6
Structure of IZUMO1-JUNO reveals sperm-oocyte recognition during mammalian fertilization.IZUMO1-JUNO 结构揭示了哺乳动物受精过程中精子-卵子的识别。
Nature. 2016 Jun 23;534(7608):566-9. doi: 10.1038/nature18596. Epub 2016 Jun 15.
7
Divergent evolution of vitamin B9 binding underlies Juno-mediated adhesion of mammalian gametes.维生素B9结合的趋异进化是Juno介导的哺乳动物配子黏附的基础。
Curr Biol. 2016 Feb 8;26(3):R100-1. doi: 10.1016/j.cub.2015.12.034.
8
Membrane associated cancer-oocyte neoantigen SAS1B/ovastacin is a candidate immunotherapeutic target for uterine tumors.膜相关癌症-卵母细胞新抗原SAS1B/卵母细胞抑素是子宫肿瘤的候选免疫治疗靶点。
Oncotarget. 2015 Oct 6;6(30):30194-211. doi: 10.18632/oncotarget.4734.
9
Quantitative mapping of zinc fluxes in the mammalian egg reveals the origin of fertilization-induced zinc sparks.定量绘制哺乳动物卵中的锌流图谱揭示了受精诱导锌火花的起源。
Nat Chem. 2015 Feb;7(2):130-9. doi: 10.1038/nchem.2133. Epub 2014 Dec 15.
10
Mammalian gamete fusion depends on the inhibition of ovastacin by fetuin-B.哺乳动物配子融合依赖于胎球蛋白-B对卵母细胞溶素的抑制作用。
Biol Chem. 2014 Oct;395(10):1195-9. doi: 10.1515/hsz-2014-0189.

卵朊酶的细胞内激活介导了透明带的预受精硬化。

Intracellular activation of ovastacin mediates pre-fertilization hardening of the zona pellucida.

机构信息

Institute of Molecular Physiology, Department of Biology, Johannes Gutenberg-University Mainz, 55099 Mainz, Germany.

Max-Planck Research Group Molecular Physiology, Center of Advanced European Studies And Research (CAESAR), 53175 Bonn, Germany.

出版信息

Mol Hum Reprod. 2017 Sep 1;23(9):607-616. doi: 10.1093/molehr/gax040.

DOI:10.1093/molehr/gax040
PMID:28911209
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5909858/
Abstract

STUDY QUESTION

How and where is pro-ovastacin activated and how does active ovastacin regulate zona pellucida hardening (ZPH) and successful fertilization?

STUDY FINDING

Ovastacin is partially active before exocytosis and pre-hardens the zona pellucida (ZP) before fertilization.

WHAT IS KNOWN ALREADY

The metalloproteinase ovastacin is stored in cortical granules, it cleaves zona pellucida protein 2 (ZP2) upon fertilization and thereby destroys the ZP sperm ligand and triggers ZPH. Female mice deficient in the extracellular circulating ovastacin-inhibitor fetuin-B are infertile due to pre-mature ZPH.

STUDY DESIGN, SAMPLES/MATERIALS, METHODS: We isolated oocytes from wild-type and ovastacin-deficient (Astlnull) FVB mice before and after fertilization (in vitro and in vivo) and quantified ovastacin activity and cleavage of ZP2 by immunoblot. We assessed ZPH by measuring ZP digestion time using α-chymotrypsin and by determining ZP2 cleavage. We determined cellular distribution of ovastacin by immunofluorescence using domain-specific ovastacin antibodies. Experiments were performed at least in triplicate with a minimum of 20 oocytes. Data were pre-analyzed using Shapiro-Wilk test. In case of normal distribution, significance was determined via two-sided Student's t-test, whereas in case of non-normal distribution via Mann-Whitney U-test.

MAIN RESULTS AND THE ROLE OF CHANCE

Metaphase II (MII) oocytes contained both inactive pro-ovastacin and activated ovastacin. Immunoblot and ZP digestion assays revealed a partial cleavage of ZP2 even before fertilization in wild-type mice. Partial cleavage coincided with germinal-vesicle breakdown and MII, despite the presence of fetuin-B protein, an endogenous ovastacin inhibitor, in the follicular and oviductal fluid. Upon exocytosis, part of the C-terminal domain of ovastacin remained attached to the plasmalemma, while the N-terminal active ovastacin domain was secreted. This finding may resolve previously conflicting data showing that ovastacin acts both as an oolemmal receptor termed SAS1B (sperm acrosomal SLLP1 binding protein; SLLP, sperm lysozyme like protein) and a secreted protease mediating ZP2 cleavage.

LIMITATIONS, REASONS FOR CAUTION: For this study, only oocytes isolated from wild-type and ovastacin-deficient FVB mice were investigated. Some experiments involved oocyte activation by the Ca2+ ionophore A23187 to trigger ZPH.

WIDER IMPLICATIONS OF THE FINDINGS

This study provides a detailed spatial and temporal view of pre-mature cleavage of ZP2 by ovastacin, which is known to adversely affect IVF rate in mice and humans.

LARGE SCALE DATA

None.

STUDY FUNDING AND COMPETING INTEREST(S): This work was supported by the Center of Natural Sciences and Medicine and by a start-up grant of the Johannes Gutenberg University Mainz to W.S., and by a grant from Deutsche Forschungsgemeinschaft and by the START program of the Medical Faculty of RWTH Aachen University to J.F. and W.J.D. There are no competing interests to declare.

摘要

研究问题

前ovastacin 如何激活以及如何调节透明带硬化(ZPH)和成功受精?

研究发现

ovastacin 在胞吐作用之前部分激活,并在受精前预硬化透明带(ZP)。

已知事实

金属蛋白酶 ovastacin 储存在皮质颗粒中,在受精时它会切割透明带蛋白 2(ZP2),从而破坏 ZP 精子配体并触发 ZPH。由于过早的 ZPH,缺乏细胞外循环 ovastacin 抑制剂 fetuin-B 的雌性小鼠不育。

研究设计、样本/材料、方法:我们在体外和体内从野生型和 ovastacin 缺陷(Astlnull)FVB 小鼠中分离出受精前和受精后的卵母细胞,并通过免疫印迹定量 ovastacin 活性和 ZP2 的切割。我们通过使用α-糜蛋白酶测量 ZP 消化时间和确定 ZP2 切割来评估 ZPH。我们通过使用针对特定结构域的 ovastacin 抗体的免疫荧光来确定 ovastacin 的细胞分布。至少进行了三次重复实验,每个实验至少有 20 个卵母细胞。使用 Shapiro-Wilk 检验对数据进行了预分析。在正态分布的情况下,通过双侧学生 t 检验确定显著性,而在非正态分布的情况下通过曼-惠特尼 U 检验确定显著性。

主要结果和机会作用

中期 II(MII)卵母细胞既含有无活性的 pro-ovastacin,也含有有活性的 ovastacin。免疫印迹和 ZP 消化分析显示,即使在野生型小鼠中,ZP2 也存在部分切割,甚至在受精前。部分切割与生发泡破裂和 MII 同时发生,尽管卵泡液和输卵管液中存在内源性 ovastacin 抑制剂 fetuin-B 蛋白。胞吐作用后,ovastacin 的 C 端结构域的一部分仍然附着在质膜上,而 N 端活性 ovastacin 结构域被分泌出来。这一发现可能解决了先前相互矛盾的数据,表明 ovastacin 既作为一种称为 SAS1B(精子顶体 SLLP1 结合蛋白;SLLP,精子溶菌酶样蛋白)的卵母细胞膜受体,又作为一种介导 ZP2 切割的分泌蛋白酶发挥作用。

局限性、谨慎的原因:对于这项研究,只研究了从野生型和 ovastacin 缺陷型 FVB 小鼠中分离出来的卵母细胞。一些实验涉及卵母细胞通过钙离子载体 A23187 激活以触发 ZPH。

研究结果的更广泛意义

本研究提供了 ovastacin 对 ZP2 进行预成熟切割的详细时空视图,已知这会对小鼠和人类的体外受精率产生不利影响。

大规模数据

无。

研究资金和利益冲突

这项工作得到了自然科学和医学中心以及美因茨约翰内斯古腾堡大学启动资金的支持,由德国研究基金会和 RWTH 亚琛大学医学系的 START 计划支持。没有利益冲突。