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Rheb,雷帕霉素的靶点激活剂,在黑蟹(Gecarcinus lateralis)中:克隆及蜕皮和失重对骨骼肌表达的影响。

Rheb, an activator of target of rapamycin, in the blackback land crab, Gecarcinus lateralis: cloning and effects of molting and unweighting on expression in skeletal muscle.

机构信息

Department of Biology, Colorado State University, Fort Collins, CO 80523, USA.

出版信息

J Exp Biol. 2012 Feb 15;215(Pt 4):590-604. doi: 10.1242/jeb.062869.

DOI:10.1242/jeb.062869
PMID:22279066
Abstract

Molt-induced claw muscle atrophy in decapod crustaceans facilitates exuviation and is coordinated by ecdysteroid hormones. There is a 4-fold reduction in mass accompanied by remodeling of the contractile apparatus, which is associated with an 11-fold increase in myofibrillar protein synthesis by the end of the premolt period. Loss of a walking limb or claw causes a loss of mass in the associated thoracic musculature; this unweighting atrophy occurs in intermolt and is ecdysteroid independent. Myostatin (Mstn) is a negative regulator of muscle growth in mammals; it suppresses protein synthesis, in part, by inhibiting the insulin/metazoan target of rapamycin (mTOR) signaling pathway. Signaling via mTOR activates translation by phosphorylating ribosomal S6 kinase (s6k) and 4E-binding protein 1. Rheb (Ras homolog enriched in brain), a GTP-binding protein, is a key activator of mTOR and is inhibited by Rheb-GTPase-activating protein (GAP). Akt protein kinase inactivates Rheb-GAP, thus slowing Rheb-GTPase activity and maintaining mTOR in the active state. We hypothesized that the large increase in global protein synthesis in claw muscle was due to regulation of mTOR activity by ecdysteroids, caused either directly or indirectly via Mstn. In the blackback land crab, Gecarcinus lateralis, a Mstn-like gene (Gl-Mstn) is downregulated as much as 17-fold in claw muscle during premolt and upregulated 3-fold in unweighted thoracic muscle during intermolt. Gl-Mstn expression in claw muscle is negatively correlated with hemolymph ecdysteroid level. Full-length cDNAs encoding Rheb orthologs from three crustacean species (G. lateralis, Carcinus maenas and Homarus americanus), as well as partial cDNAs encoding Akt (Gl-Akt), mTOR (Gl-mTOR) and s6k (Gl-s6k) from G. lateralis, were cloned. The effects of molting on insulin/mTOR signaling components were quantified in claw closer, weighted thoracic and unweighted thoracic muscles using quantitative polymerase chain reaction. Gl-Rheb mRNA levels increased 3.4-fold and 3.9-fold during premolt in claw muscles from animals induced to molt by eyestalk ablation (ESA) and multiple leg autotomy (MLA), respectively, and mRNA levels were positively correlated with hemolymph ecdysteroids. There was little or no effect of molting on Gl-Rheb expression in weighted thoracic muscle and no correlation of Gl-Rheb mRNA with ecdysteroid titer. There were significant changes in Gl-Akt, Gl-mTOR and Gl-s6k expression with molt stage. These changes were transient and were not correlated with hemolymph ecdysteroids. The two muscles differed in terms of the relationship between Gl-Rheb and Gl-Mstn expression. In thoracic muscle, Gl-Rheb mRNA was positively correlated with Gl-Mstn mRNA in both ESA and MLA animals. By contrast, Gl-Rheb mRNA in claw muscle was negatively correlated with Gl-Mstn mRNA in ESA animals, and no correlation was observed in MLA animals. Unweighting increased Gl-Rheb expression in thoracic muscle at all molt stages; the greatest difference (2.2-fold) was observed in intermolt animals. There was also a 1.3-fold increase in Gl-s6k mRNA level in unweighted thoracic muscle. These data indicate that the mTOR pathway is upregulated in atrophic muscles. Gl-Rheb, in particular, appears to play a role in the molt-induced increase in protein synthesis in the claw muscle.

摘要

蜕皮诱导的十足目甲壳动物爪肌肉萎缩有助于蜕皮,并受蜕皮激素的协调。质量减少了 4 倍,伴随着收缩装置的重塑,这与肌原纤维蛋白合成在蜕皮前期间期增加了 11 倍有关。失去一条行走的肢体或爪子会导致相关胸肌质量下降;这种失重性萎缩发生在间蜕期,与蜕皮激素无关。肌肉生长抑制素 (Mstn) 是哺乳动物肌肉生长的负调节剂;它通过抑制胰岛素/后生动物雷帕霉素靶蛋白 (mTOR) 信号通路部分抑制蛋白质合成。mTOR 通过磷酸化核糖体 S6 激酶 (s6k) 和 4E 结合蛋白 1 来激活翻译。Rheb(富含大脑的 Ras 同源物)是 mTOR 的关键激活剂,它被 Rheb-GTPase-activating protein (GAP) 抑制。Akt 蛋白激酶使 Rheb-GAP 失活,从而减缓 Rheb-GTPase 活性并使 mTOR 保持活跃状态。我们假设爪肌肉中整体蛋白质合成的大量增加是由于蜕皮激素对 mTOR 活性的调节,这种调节要么是直接的,要么是通过 Mstn 间接的。在黑背地蟹(Gecarcinus lateralis)中,一种类似于 Mstn 的基因(Gl-Mstn)在蜕皮前期间歇期间在爪肌肉中的表达下调了 17 倍,在失重的胸肌中上调了 3 倍。爪肌肉中的 Gl-Mstn 表达与血淋巴蜕皮激素水平呈负相关。从三种甲壳动物(G. lateralis、Carcinus maenas 和 Homarus americanus)克隆了全长 cDNA 编码 Rheb 同源物,以及从 G. lateralis 克隆了部分 cDNA 编码 Akt(Gl-Akt)、mTOR(Gl-mTOR)和 s6k(Gl-s6k)。使用定量聚合酶链反应在诱导蜕皮的眼柄切除(ESA)和多次腿自截(MLA)动物的爪夹、称重胸肌和未称重胸肌中定量了蜕皮对胰岛素/mTOR 信号成分的影响。Gl-Rheb mRNA 水平在 ESA 和 MLA 诱导的蜕皮前期间歇期间分别增加了 3.4 倍和 3.9 倍,mRNA 水平与血淋巴蜕皮激素呈正相关。蜕皮对 Gl-Rheb 在称重胸肌中的表达几乎没有影响,也没有 Gl-Rheb mRNA 与蜕皮激素滴度的相关性。Gl-Akt、Gl-mTOR 和 Gl-s6k 的表达随着蜕皮阶段而发生显著变化。这些变化是短暂的,与血淋巴蜕皮激素无关。Gl-Rheb 和 Gl-Mstn 表达之间的关系在两种肌肉中有所不同。在胸肌中,Gl-Rheb mRNA 在 ESA 和 MLA 动物中均与 Gl-Mstn mRNA 呈正相关。相比之下,在 ESA 动物的爪肌肉中,Gl-Rheb mRNA 与 Gl-Mstn mRNA 呈负相关,而在 MLA 动物中则没有相关性。失重增加了所有蜕皮阶段胸肌中的 Gl-Rheb 表达;在间蜕期动物中观察到最大差异(2.2 倍)。未称重胸肌中的 Gl-s6k mRNA 水平也增加了 1.3 倍。这些数据表明 mTOR 途径在萎缩肌肉中上调。特别是 Gl-Rheb 似乎在蜕皮诱导的爪肌肉蛋白质合成增加中起作用。

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