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3
Single molecule force measurements of perlecan/HSPG2: A key component of the osteocyte pericellular matrix.核心蛋白聚糖/HSPG2的单分子力测量:骨细胞周细胞基质的关键成分
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4
Appropriate models for novel osteoporosis drug discovery and future perspectives.新型骨质疏松症药物发现的合适模型及未来展望。
Expert Opin Drug Discov. 2015;10(11):1201-16. doi: 10.1517/17460441.2015.1080685. Epub 2015 Aug 19.
5
In vivo mechanical loading rapidly activates β-catenin signaling in osteocytes through a prostaglandin mediated mechanism.在体内,机械负荷通过前列腺素介导的机制迅速激活骨细胞中的β-连环蛋白信号通路。
Bone. 2015 Jul;76:58-66. doi: 10.1016/j.bone.2015.03.019. Epub 2015 Mar 30.
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Integrative transcriptomic and proteomic analysis of osteocytic cells exposed to fluid flow reveals novel mechano-sensitive signaling pathways.整合转录组学和蛋白质组学分析骨细胞在液流刺激下的反应,揭示新的机械敏感信号通路。
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Feedbacks and adaptive capabilities of the PI3K/Akt/mTOR axis in acute myeloid leukemia revealed by pathway selective inhibition and phosphoproteome analysis.通过通路选择性抑制和磷酸化蛋白质组分析揭示急性髓细胞白血病中 PI3K/Akt/mTOR 轴的反馈和适应能力。
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在机械应力条件下对非洲爪蟾骨细胞进行的表达和功能蛋白质组学分析:关于一种合适的新动物模型的初步观察

Expression and functional proteomic analyses of osteocytes from Xenopus laevis tested under mechanical stress conditions: preliminary observations on an appropriate new animal model.

作者信息

Bertacchini Jessika, Benincasa Marta, Checchi Marta, Cavani Francesco, Smargiassi Alberto, Ferretti Marzia, Palumbo Carla

机构信息

Dipartimento di Scienze Biomediche Metaboliche e Neuroscienze, Sezione di Morfologia umana. Università degli Studi di Modena e Reggio Emilia, Modena, Italy.

出版信息

J Anat. 2017 Dec;231(6):823-834. doi: 10.1111/joa.12685. Epub 2017 Sep 19.

DOI:10.1111/joa.12685
PMID:28925539
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5696140/
Abstract

Hitherto, the role of the osteocyte as transducer of mechanical stimuli into biological signals is far from settled. In this study, we used an appropriate model represented by the cortex of Xenopus laevis long bone diaphysis lacking (unlike the mammalian one) of vascular structures and containing only osteocytes inside the bone matrix. These structural features allow any change of protein profile that might be observed upon different experimental conditions, such as bone adaptation to stress/mechanical loading, to be ascribed specifically to osteocytes. The study was conducted by combining ultrastructural observations and two-dimensional electrophoresis for proteomic analysis. The osteocyte population was extracted from long bones of lower limbs of amphibian skeletons after different protocols (free and forced swimming). The experiments were performed on 210 frogs subdivided into five trials, each including free swimming frogs (controls) and frogs submitted to forced swimming (stressed). The stressed groups were obliged to swim (on movable spheres covering the bottom of a pool on a vibrating plate) continuously for 8 h, and killed 24 h later along with the control groups. Long bones free of soft tissues (periosteum, endosteum and bone marrow), as well as muscles of posterior limbs, were processed and analyzed for proteins differentially expressed or phosphorylated between the two sample groups. The comparative analysis showed that protein phosphorylation profiles differ between control and stressed groups. In particular, we found in long bones of stressed samples that both Erk1/2 and Akt are hyperphosphorylated; moreover, the different phosphorylation of putative Akt substrates (recognized by specific Akt phosphosubstrates-antibody) in stressed vs. control samples clearly demonstrated that Akt signaling is boosted by forced swimming (leading to an increase of mechanical stress) of amphibian long bones. In parallel, we found in posterior limb muscles that the expression of heat shock protein HSP27 and HSP70 stress markers increased upon the forced swimming condition. Because the cortexes of frog long bones are characterized by the presence of only osteocytes, all our results establish the suitability of the X. laevis animal model to study the bone response to stress conditions mediated by this cell type and pave the way for further analysis of the signaling pathways involved in these signal transduction mechanisms.

摘要

迄今为止,骨细胞作为机械刺激转化为生物信号的转导器的作用尚未完全明确。在本研究中,我们使用了一种合适的模型,该模型由非洲爪蟾长骨干骺端皮质代表,其缺乏(与哺乳动物不同)血管结构,且骨基质内仅含有骨细胞。这些结构特征使得在不同实验条件下(如骨骼对应力/机械负荷的适应)可能观察到的蛋白质谱变化能够具体归因于骨细胞。该研究通过结合超微结构观察和二维电泳进行蛋白质组分析。在不同方案(自由游泳和强制游泳)后,从两栖动物骨骼下肢的长骨中提取骨细胞群体。实验在210只青蛙上进行,分为五个试验组,每组包括自由游泳的青蛙(对照组)和接受强制游泳的青蛙(应激组)。应激组被迫(在覆盖振动板上水池底部的可移动球体上)连续游泳8小时,并在24小时后与对照组一起处死。对去除软组织(骨膜、骨内膜和骨髓)的长骨以及后肢肌肉进行处理,分析两个样本组之间差异表达或磷酸化的蛋白质。比较分析表明,对照组和应激组的蛋白质磷酸化谱不同。特别是,我们发现在应激样本的长骨中,Erk1/2和Akt均过度磷酸化;此外,应激样本与对照样本中假定的Akt底物(由特异性Akt磷酸化底物抗体识别)的不同磷酸化清楚地表明,两栖动物长骨的强制游泳(导致机械应力增加)会增强Akt信号传导。同时,我们发现在后肢肌肉中,热休克蛋白HSP27和HSP70应激标记物的表达在强制游泳条件下增加。由于青蛙长骨的皮质仅以骨细胞的存在为特征,我们所有的结果证实了非洲爪蟾动物模型适用于研究这种细胞类型介导的骨骼对应激条件的反应,并为进一步分析这些信号转导机制中涉及的信号通路铺平了道路。