Phlpp1 alters the murine chondrocyte phospho-proteome during endochondral bone formation

IF 3.5 2区医学 Q2 ENDOCRINOLOGY & METABOLISM

Bone Pub Date : 2024-09-29 DOI:10.1016/j.bone.2024.117265

Samantha R. Weaver , Eduardo Peralta-Herrera , Haydee M. Torres , Erik Jessen , Elizabeth W. Bradley , Jennifer J. Westendorf

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引用次数: 0

Abstract

Appendicular skeletal growth and bone mass acquisition are controlled by a variety of growth factors, hormones, and mechanical forces in a dynamic process called endochondral ossification. In long bones, chondrocytes in the growth plate proliferate and undergo hypertrophy to drive bone lengthening and mineralization. Pleckstrin homology (PH) domain and leucine rich repeat phosphatase 1 and 2 (Phlpp1 and Phlpp2) are serine/threonine protein phosphatases that regulate cell proliferation, survival, and maturation via Akt, PKC, Raf1, S6k, and other intracellular signaling cascades. Germline deletion of Phlpp1 suppresses bone lengthening in growth plate chondrocytes. Here, we demonstrate that Phlpp2 does not regulate endochondral ossification, and we define the molecular differences between Phlpp1 and Phlpp2 in chondrocytes. Phlpp2^−/− mice were phenotypically indistinguishable from their wildtype (WT) littermates, with similar bone length, bone mass, and growth plate dynamics. Deletion of Phlpp2 had moderate effects on the chondrocyte transcriptome and proteome compared to WT cells. By contrast, Phlpp1/2^−/− (double knockout) mice resembled Phlpp1^−/− mice phenotypically and molecularly, as the chondrocyte phospho-proteomes of Phlpp1^−/− and Phlpp1/2^−/− chondrocytes had similarities and were significantly different from WT and Phlpp2^−/− chondrocyte phospho-proteomes. Data integration via multiparametric analysis showed that the transcriptome explained less variation in the data as a result of Phlpp1 or Phlpp2 deletion than proteome or phospho-proteome. Alterations in cell proliferation, collagen fibril organization, and Pdpk1 and Pak1/2 signaling pathways were identified in chondrocytes lacking Phlpp1, while cell cycle processes and Akt1 and Aurka signaling pathways were altered in chondrocytes lacking Phlpp2. These data demonstrate that Phlpp1, and to a lesser extent Phlpp2, regulate multiple and complex signaling cascades across the chondrocyte transcriptome, proteome, and phospho-proteome and that multi-omic data integration can reveal novel putative kinase targets that regulate endochondral ossification.

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Phlpp1 在软骨内骨形成过程中改变了小鼠软骨细胞磷蛋白组。

在一个称为软骨内骨化的动态过程中，各种生长因子、激素和机械力控制着骨骼的生长和骨量的获得。在长骨中，生长板中的软骨细胞增殖并发生肥大，从而推动骨骼的延长和矿化。Pleckstrin homology（PH）结构域和富亮氨酸重复磷酸酶 1 和 2（Phlpp1 和 Phlpp2）是丝氨酸/苏氨酸蛋白磷酸酶，可通过 Akt、PKC、Raf1、S6k 和其他细胞内信号级联调节细胞增殖、存活和成熟。基因缺失 Phlpp1 会抑制生长板软骨细胞的骨延长。在这里，我们证明了 Phlpp2 不调控软骨内骨化，并明确了 Phlpp1 和 Phlpp2 在软骨细胞中的分子差异。Phlpp2-/-小鼠在表型上与野生型（WT）小鼠无异，具有相似的骨长、骨量和生长板动力学。与 WT 细胞相比，Phlpp2 的缺失对软骨细胞转录组和蛋白质组的影响不大。相比之下，Phlpp1/2-/-（双基因敲除）小鼠在表型和分子上与Phlpp1-/-小鼠相似，因为Phlpp1-/-和Phlpp1/2-/-软骨细胞的软骨细胞磷酸蛋白组与WT和Phlpp2-/-软骨细胞磷酸蛋白组有相似之处和显著差异。通过多参数分析进行的数据整合显示，转录组对Phlpp1或Phlpp2缺失导致的数据变化的解释程度低于蛋白质组或磷酸化蛋白质组。在缺乏 Phlpp1 的软骨细胞中发现了细胞增殖、胶原纤维组织以及 Pdpk1 和 Pak1/2 信号通路的改变，而在缺乏 Phlpp2 的软骨细胞中发现了细胞周期过程以及 Akt1 和 Aurka 信号通路的改变。这些数据表明，Phlpp1（其次是 Phlpp2）可调控软骨细胞转录组、蛋白质组和磷酸化蛋白质组中多种复杂的信号级联，多组学数据整合可揭示调控软骨内骨化的新型推定激酶靶标。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Bone 医学-内分泌学与代谢

CiteScore

8.90

自引率

4.90%

发文量

264

审稿时长

30 days

期刊介绍： BONE is an interdisciplinary forum for the rapid publication of original articles and reviews on basic, translational, and clinical aspects of bone and mineral metabolism. The Journal also encourages submissions related to interactions of bone with other organ systems, including cartilage, endocrine, muscle, fat, neural, vascular, gastrointestinal, hematopoietic, and immune systems. Particular attention is placed on the application of experimental studies to clinical practice.