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RACK1 interaction with c-Src is essential for osteoclast function

机译:RACK1与c-Src的相互作用对于破骨细胞功能至关重要

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摘要

The scaffolding protein receptor for activated C-kinase 1 (RACK1) mediates receptor activator of nuclear factor κΒ ligand (RANKL)-dependent activation of p38 MAPK in osteoclast precursors; however, the role of RACK1 in mature osteoclasts is unclear. The aim of our study was to identify the interaction between RACK1 and c-Src that is critical for osteoclast function. A RACK1 mutant protein (mutations of tyrosine 228 and 246 residues to phenylalanine; RACK1 Y228F/Y246F) did not interact with c-Src. The mutant retained its ability to differentiate into osteoclasts; however, the integrity of the RANKL-mediated cytoskeleton, bone resorption activity, and phosphorylation of c-Src was significantly decreased. Importantly, lysine 152 (K152) within the Src homology 2 (SH2) domain of c-Src is involved in RACK1 binding. The c-Src K152R mutant (mutation of lysine 152 into arginine) impaired the resorption of bone by osteoclasts. These findings not only clarify the role of the RACK1-c-Src axis as a key regulator of osteoclast function but will also help to develop new antiresorption therapies to prevent bone loss-related diseases.
机译:活化的C激酶1(RACK1)的支架蛋白受体介导破骨细胞前体中核因子κΒ配体(RANKL)依赖的p38 MAPK活化的受体激活剂;然而,RACK1在成熟破骨细胞中的作用尚不清楚。我们研究的目的是确定RACK1和c-Src之间的相互作用对破骨细胞功能至关重要。 RACK1突变蛋白(酪氨酸228和246个残基突变为苯丙氨酸; RACK1 Y228F / Y246F)不与c-Src相互作用。该突变体保留了分化成破骨细胞的能力。但是,RANKL介导的细胞骨架的完整性,骨吸收活性和c-Src的磷酸化显着降低。重要的是,c-Src的Src同源2(SH2)域中的赖氨酸152(K152)与RACK1结合有关。 c-Src K152R突变体(赖氨酸152突变为精氨酸)损害了破骨细胞对骨的吸收。这些发现不仅阐明了RACK1-c-Src轴作为破骨细胞功能的关键调节因子的作用,而且还将有助于开发新的抗吸收疗法,以预防与骨丢失相关的疾病。

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