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鉴定内质网/肌浆网驻留蛋白作为骨骼肌细胞内质网/肌浆网钙耗竭的生物标志物。

Identification of ER/SR resident proteins as biomarkers for ER/SR calcium depletion in skeletal muscle cells.

机构信息

National Institute On Drug Abuse, 251 Bayview Blvd, Baltimore, MD, 21224, USA.

National Institute of Nursing Research, Bethesda, MD, USA.

出版信息

Orphanet J Rare Dis. 2022 Jun 13;17(1):225. doi: 10.1186/s13023-022-02368-9.

Abstract

BACKGROUND

Aberrations to endoplasmic/sarcoplasmic reticulum (ER/SR) calcium concentration can result in the departure of endogenous proteins in a phenomenon termed exodosis. Redistribution of the ER/SR proteome can have deleterious effects to cell function and cell viability, often contributing to disease pathogenesis. Many proteins prone to exodosis reside in the ER/SR via an ER retention/retrieval sequence (ERS) and are involved in protein folding, protein modification, and protein trafficking. While the consequences of their extracellular presence have yet to be fully delineated, the proteins that have undergone exodosis may be useful for biomarker development. Skeletal muscle cells rely upon tightly coordinated ER/SR calcium release for muscle contractions, and perturbations to calcium homeostasis can result in myopathies. Ryanodine receptor type-1 (RYR1) is a calcium release channel located in the SR. Mutations to the RYR1 gene can compromise calcium homeostasis leading to a vast range of clinical phenotypes encompassing hypotonia, myalgia, respiratory insufficiency, ophthalmoplegia, fatigue and malignant hyperthermia (MH). There are currently no FDA approved treatments for RYR1-related myopathies (RYR1-RM).

RESULTS

Here we examine the exodosis profile of skeletal muscle cells following ER/SR calcium depletion. Proteomic analysis identified 4,465 extracellular proteins following ER/SR calcium depletion with 1,280 proteins significantly different than vehicle. A total of 54 ERS proteins were identified and 33 ERS proteins significantly increased following ER/SR calcium depletion. Specifically, ERS protein, mesencephalic astrocyte-derived neurotrophic factor (MANF), was elevated following calcium depletion, making it a potential biomarker candidate for human samples. Despite no significant elevation of MANF in plasma levels among healthy volunteers and RYR1-RM individuals, MANF plasma levels positively correlated with age in RYR1-RM individuals, presenting a potential biomarker of disease progression. Selenoprotein N (SEPN1) was also detected only in extracellular samples following ER/SR calcium depletion. This protein is integral to calcium handling and SEPN1 variants have a causal role in SEPN1-related myopathies (SEPN1-RM). Extracellular presence of ER/SR membrane proteins may provide new insight into proteomic alterations extending beyond ERS proteins. Pre-treatment of skeletal muscle cells with bromocriptine, an FDA approved drug recently found to have anti-exodosis effects, curbed exodosis of ER/SR resident proteins.

CONCLUSION

Changes to the extracellular content caused by intracellular calcium dysregulation presents an opportunity for biomarker development and drug discovery.

摘要

背景

内质网/肌浆网(ER/SR)钙离子浓度的改变会导致内源性蛋白的排出,这一现象被称为外吐。ER/SR 蛋白质组的再分布会对细胞功能和细胞活力产生有害影响,通常导致疾病的发病机制。许多容易发生外吐的蛋白质通过内质网保留/检索序列(ERS)存在于 ER/SR 中,参与蛋白质折叠、蛋白质修饰和蛋白质运输。虽然它们在细胞外的存在的后果尚未完全阐明,但已经发生外吐的蛋白质可能对生物标志物的开发有用。骨骼肌细胞依赖于紧密协调的 ER/SR 钙离子释放来进行肌肉收缩,而钙稳态的改变会导致肌病。兰尼碱受体 1(RYR1)是一种位于 SR 的钙离子释放通道。RYR1 基因突变会破坏钙稳态,导致广泛的临床表型,包括低张力、肌痛、呼吸功能不全、眼肌麻痹、疲劳和恶性高热(MH)。目前,尚无 FDA 批准的 RYR1 相关肌病(RYR1-RM)治疗方法。

结果

在这里,我们研究了 ER/SR 钙离子耗竭后骨骼肌细胞的外吐谱。蛋白质组学分析显示,ER/SR 钙离子耗竭后有 4465 种细胞外蛋白,其中 1280 种蛋白与载体明显不同。共鉴定出 54 种 ERS 蛋白,其中 33 种 ERS 蛋白在 ER/SR 钙离子耗竭后显著增加。特别是,内质网应激蛋白,脑源性神经营养因子(MANF),在钙耗竭后升高,使其成为人类样本的潜在生物标志物候选物。尽管在健康志愿者和 RYR1-RM 个体的血浆水平中,MANF 没有明显升高,但 RYR1-RM 个体的 MANF 血浆水平与年龄呈正相关,提示其可能是疾病进展的生物标志物。SEPN1 也仅在 ER/SR 钙离子耗竭后细胞外样本中检测到。这种蛋白质是钙处理的重要组成部分,SEPN1 变体在 SEPN1 相关肌病(SEPN1-RM)中起因果作用。内质网/肌浆网膜蛋白的细胞外存在可能为超出 ERS 蛋白的蛋白质组改变提供新的见解。用溴隐亭预处理骨骼肌细胞,溴隐亭是一种最近被发现具有抗外吐作用的 FDA 批准药物,可以抑制 ER/SR 驻留蛋白的外吐。

结论

细胞内钙稳态失调引起的细胞外内容物的改变为生物标志物的开发和药物发现提供了机会。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1498/9195201/0b3d54703121/13023_2022_2368_Fig1_HTML.jpg

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