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精子鞭毛的一种130千道尔顿膜蛋白是海星精子激活肽——糙海星海星皂苷的受体。

A 130-kDa membrane protein of sperm flagella is the receptor for asterosaps, sperm-activating peptides of starfish Asterias amurensis.

作者信息

Nishigaki T, Chiba K, Hoshi M

机构信息

Department of Life Science, Tokyo Institute of Technology, 4259 Nagatsuta, Midori-ku, Yokohama, 226-8501, Japan.

出版信息

Dev Biol. 2000 Mar 1;219(1):154-62. doi: 10.1006/dbio.1999.9598.

Abstract

Spermatozoa of the starfish, Asterias amurensis, have a specific receptor for asterosap, a sperm-activating peptide isolated from the jelly coat of homologous eggs. We characterized the receptor by using several asterosap derivatives. Analysis of equilibrium binding of radioactive di-iodinated Bolton-Hunter reagent-labeled asterosap ((125)I(2)-BHP15) to the spermatozoa indicated that the cell has 1.1 x 10(5) binding sites of high affinity (K(d) = 57 pM), and also the receptor showed positive cooperativity for asterosap binding. When spermatozoa were treated with fluorophore-labeled asterosap, the sperm flagella were labeled, indicating that the receptors are mostly localized in the sperm tail. When spermatozoa were reacted with radioactive asterosap prelabeled with photoaffinity cross-linkers, a single 130-kDa membrane protein of sperm flagella was specifically radiolabeled. This result was reproducible regardless of the length of spacer arm of cross-linkers so far studied. Therefore, the 130-kDa protein is likely to be the receptor for asterosaps. Modification of asterosap at the N-terminal region with bulky molecules such as carboxyfluorescein did not affect the activity of asterosap, suggesting that the N-terminus of asterosap is not involved in the ligand-receptor interaction. On the other hand, S-alkylated asterosaps did not compete with (125)I(2)-BHP15 for binding to the receptor, indicating that disulfide linkage of asterosap is essential for the ligand-receptor interaction. The properties of the receptor, high affinity and high concentration, enabled us to apply the fluorescence polarization technique to study the molecular interaction between asterosap and the receptor. Using this method, we performed binding experiments in almost real time and found that divalent cations are significantly involved in the interaction between asterosap and the receptor.

摘要

海星(Asterias amurensis)的精子具有一种针对海星皂角苷的特异性受体,海星皂角苷是一种从同源卵子的卵胶膜中分离出的精子激活肽。我们使用几种海星皂角苷衍生物对该受体进行了表征。对放射性二碘化博尔顿 - 亨特试剂标记的海星皂角苷((125)I(2)-BHP15)与精子的平衡结合分析表明,细胞具有1.1×10(5)个高亲和力结合位点(K(d)=57 pM),并且该受体对海星皂角苷的结合表现出正协同性。当精子用荧光团标记的海星皂角苷处理时,精子鞭毛被标记,这表明受体主要定位于精子尾部。当精子与用光亲和交联剂预标记的放射性海星皂角苷反应时,精子鞭毛的一种单一的130 kDa膜蛋白被特异性放射性标记。无论到目前为止所研究的交联剂间隔臂的长度如何,该结果都是可重复的。因此,130 kDa蛋白可能是海星皂角苷的受体。用诸如羧基荧光素等大分子对海星皂角苷的N端区域进行修饰并不影响海星皂角苷的活性,这表明海星皂角苷的N端不参与配体 - 受体相互作用。另一方面,S - 烷基化的海星皂角苷不与(125)I(2)-BHP15竞争与受体的结合,这表明海星皂角苷的二硫键对于配体 - 受体相互作用至关重要。该受体的高亲和力和高浓度特性使我们能够应用荧光偏振技术来研究海星皂角苷与受体之间的分子相互作用。使用这种方法,我们几乎实时地进行了结合实验,并发现二价阳离子显著参与海星皂角苷与受体之间的相互作用。

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