Molt-inhibiting hormone stimulates vitellogenesis at advanced ovarian developmental stages in the female blue crab, Callinectes sapidus 2: novel specific binding sites in hepatopancreas and cAMP as a second messenger.

Nilli Zmora, Amir Sagi, Yonathan Zohar, J Sook Chung
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引用次数: 47

Abstract

The finding that molt-inhibiting hormone (MIH) regulates vitellogenesis in the hepatopancreas of mature Callinectes sapidus females, raised the need for the characterization of its mode of action. Using classical radioligand binding assays, we located specific, saturable, and non-cooperative binding sites for MIH in the Y-organs of juveniles (J-YO) and in the hepatopancreas of vitellogenic adult females. MIH binding to the hepatopancreas membranes had an affinity 77 times lower than that of juvenile YO membranes (KD values: 3.22 x 10(-8) and 4.19 x 10(-10) M/mg protein, respectively). The number of maximum binding sites (B(MAX)) was approximately two times higher in the hepatopancreas than in the YO (B(MAX) values: 9.24 x 10(-9) and 4.8 x 10(-9) M/mg protein, respectively). Furthermore, MIH binding site number in the hepatopancreas was dependent on ovarian stage and was twice as high at stage 3 than at stages 2 and 1. SDS-PAGE separation of [125I] MIH or [125I] crustacean hyperglycemic hormone (CHH) crosslinked to the specific binding sites in the membranes of the J-YO and hepatopancreas suggests a molecular weight of approximately 51 kDa for a MIH receptor in both tissues and a molecular weight of approximately 61 kDa for a CHH receptor in the hepatopancreas. The use of an in vitro incubation of hepatopancreas fragments suggests that MIH probably utilizes cAMP as a second messenger in this tissue, as cAMP levels increased in response to MIH. Additionally, 8-Bromo-cAMP mimicked the effects of MIH on vitellogenin (VtG) mRNA and heterogeneous nuclear (hn) VtG RNA levels. The results imply that the functions of MIH in the regulation of molt and vitellogenesis are mediated through tissue specific receptors with different kinetics and signal transduction. MIH ability to regulate vitellogenesis is associated with the appearance of MIH specific membrane binding sites in the hepatopancreas upon pubertal/final molt.

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在雌性蓝蟹(Callinectes sapidus)卵巢发育晚期,脱毛抑制激素刺激卵黄发生:肝胰腺中新的特异性结合位点和cAMP作为第二信使。
研究发现,蜕皮抑制激素(MIH)调节成熟雌性糙皮Callinectes sapidus的肝胰腺卵黄形成,这一发现提出了对其作用方式进行表征的必要性。使用经典的放射配体结合试验,我们在幼鱼的y器官(J-YO)和卵黄变性成年雌性的肝胰腺中找到了MIH的特异性、饱和和非合作结合位点。MIH结合肝胰脏膜的亲和力比幼鱼YO膜低77倍(KD值分别为3.22 × 10(-8)和4.19 × 10(-10) M/mg蛋白)。肝胰脏的最大结合位点(B(MAX))数量约为YO的两倍(B(MAX)值分别为9.24 × 10(-9) M/mg蛋白和4.8 × 10(-9) M/mg蛋白)。此外,肝胰脏中的MIH结合位点数与卵巢分期有关,3期的MIH结合位点数是2期和1期的两倍。SDS-PAGE分离[125I] MIH或[125I]甲壳类高血糖激素(CHH)交联到J-YO和肝胰腺膜上的特定结合位点,表明两种组织中MIH受体的分子量约为51 kDa,肝胰腺中CHH受体的分子量约为61 kDa。肝胰脏碎片体外培养的使用表明,MIH可能利用cAMP作为该组织中的第二信使,因为cAMP水平在MIH反应中增加。此外,8-溴- camp模拟了MIH对卵黄蛋白原(VtG) mRNA和异质核(hn) VtG RNA水平的影响。结果表明,MIH在脱毛和卵黄发生中的调节作用是通过具有不同动力学和信号转导的组织特异性受体介导的。MIH调节卵黄形成的能力与肝胰腺中MIH特异性膜结合位点的出现有关。
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