Isolation and characterization of bone mesenchymal cell small extracellular vesicles using a novel mouse model.

IF 5.1 1区医学 Q1 ENDOCRINOLOGY & METABOLISM

Journal of Bone and Mineral Research Pub Date : 2024-08-22 DOI:10.1093/jbmr/zjae135

David G Monroe, Naureen Javeed, Jennifer L Rowsey, Ming Ruan, Chantal E McCabe, Bryan T Piatkowski, Abhishek Roy, Madhusudhan R Bobbili, Johannes Grillari, Sundeep Khosla

{"title":"Isolation and characterization of bone mesenchymal cell small extracellular vesicles using a novel mouse model.","authors":"David G Monroe, Naureen Javeed, Jennifer L Rowsey, Ming Ruan, Chantal E McCabe, Bryan T Piatkowski, Abhishek Roy, Madhusudhan R Bobbili, Johannes Grillari, Sundeep Khosla","doi":"10.1093/jbmr/zjae135","DOIUrl":null,"url":null,"abstract":"<p><p>Extracellular vesicles (EVs) are key mediators of cell-cell communication and are involved in transferring specific biomolecular cargo to recipient cells to regulate their physiological functions. A major challenge in the understanding of EV function in vivo is the difficulty ascertaining the origin of the EV particles. The recent development of the \"Snorkel-tag\", which includes EV-membrane-targeted CD81 fused to a series of extra-vesicular protein tags, can be used to mark EVs originating from a specific source for subsequent isolation and characterization. We developed an in vivo mouse model, termed \"CAGS-Snorkel\", which expresses the Snorkel-tag under the control of the Cre-lox system, and crossed this mouse with either Prx1-Cre (mesenchymal progenitors) or Ocn-Cre (osteoblasts/osteocytes) and isolated Snorkel-tagged EVs from the mouse bone marrow plasma using a magnetic bead affinity column. miRNA-sequencing was performed on the isolated EVs, and although similar profiles were observed, a few key miRNAs involved in bone metabolism (miR-106b-5p, miRs-19b-3p and miRs-219a-5p) were enriched in the Ocn-derived relative to the Prx1-derived EV subpopulations. To characterize the effects of these small EVs on a bone cell target, cultured mouse bone marrow stromal cells (mBMSCs) were treated with Prx1 or Ocn EVs, and mRNA-sequencing was performed. Pathways involved in ossification, bone development and extracellular matrix interactions were regulated by both EV subpopulations, whereas a few pathways including advanced glycation end-products (AGE) signaling, were uniquely regulated in the Ocn EV subpopulation, underlying important biological effects of specific EV subpopulations within the bone marrow microenvironment. These data demonstrate that EV isolation in vivo using the CAGS-Snorkel mouse model is a useful tool in characterizing the cargo and understanding the biology of tissue-specific EVs. Moreover, while bone mesenchymal cell populations share a common EV secretory profile, we uncover key differences based on the stage of osteoblastic differentiation that may have important biological consequences.</p>","PeriodicalId":185,"journal":{"name":"Journal of Bone and Mineral Research","volume":null,"pages":null},"PeriodicalIF":5.1000,"publicationDate":"2024-08-22","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Journal of Bone and Mineral Research","FirstCategoryId":"3","ListUrlMain":"https://doi.org/10.1093/jbmr/zjae135","RegionNum":1,"RegionCategory":"医学","ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q1","JCRName":"ENDOCRINOLOGY & METABOLISM","Score":null,"Total":0}

引用次数: 0

Abstract

Extracellular vesicles (EVs) are key mediators of cell-cell communication and are involved in transferring specific biomolecular cargo to recipient cells to regulate their physiological functions. A major challenge in the understanding of EV function in vivo is the difficulty ascertaining the origin of the EV particles. The recent development of the "Snorkel-tag", which includes EV-membrane-targeted CD81 fused to a series of extra-vesicular protein tags, can be used to mark EVs originating from a specific source for subsequent isolation and characterization. We developed an in vivo mouse model, termed "CAGS-Snorkel", which expresses the Snorkel-tag under the control of the Cre-lox system, and crossed this mouse with either Prx1-Cre (mesenchymal progenitors) or Ocn-Cre (osteoblasts/osteocytes) and isolated Snorkel-tagged EVs from the mouse bone marrow plasma using a magnetic bead affinity column. miRNA-sequencing was performed on the isolated EVs, and although similar profiles were observed, a few key miRNAs involved in bone metabolism (miR-106b-5p, miRs-19b-3p and miRs-219a-5p) were enriched in the Ocn-derived relative to the Prx1-derived EV subpopulations. To characterize the effects of these small EVs on a bone cell target, cultured mouse bone marrow stromal cells (mBMSCs) were treated with Prx1 or Ocn EVs, and mRNA-sequencing was performed. Pathways involved in ossification, bone development and extracellular matrix interactions were regulated by both EV subpopulations, whereas a few pathways including advanced glycation end-products (AGE) signaling, were uniquely regulated in the Ocn EV subpopulation, underlying important biological effects of specific EV subpopulations within the bone marrow microenvironment. These data demonstrate that EV isolation in vivo using the CAGS-Snorkel mouse model is a useful tool in characterizing the cargo and understanding the biology of tissue-specific EVs. Moreover, while bone mesenchymal cell populations share a common EV secretory profile, we uncover key differences based on the stage of osteoblastic differentiation that may have important biological consequences.

查看原文本刊更多论文

利用新型小鼠模型分离骨间充质细胞小细胞外囊泡并确定其特征。

细胞外囊泡（EV）是细胞-细胞通讯的关键媒介，参与将特定的生物分子货物转移到受体细胞，以调节其生理功能。要了解EV在体内的功能，一个主要挑战是难以确定EV颗粒的来源。最近开发的 "Snorkel-tag"（包括EV膜靶向CD81与一系列囊外蛋白标签融合）可用于标记来自特定来源的EV，以便随后进行分离和表征。我们开发了一种体内小鼠模型，称为 "CAGS-Snorkel"，它在 Cre-lox 系统控制下表达 Snorkel 标记，并将这种小鼠与 Prx1-Cre （间充质祖细胞）或 Ocn-Cre （成骨细胞/骨细胞）杂交，使用磁珠亲和柱从小鼠骨髓血浆中分离出 Snorkel 标记的 EVs。对分离出的EVs进行了miRNA测序，虽然观察到了相似的图谱，但与Prx1衍生的EV亚群相比，Ocn衍生的EV亚群中富集了一些参与骨代谢的关键miRNA（miR-106b-5p、miR-19b-3p和miR-219a-5p）。为了描述这些小EV对骨细胞靶标的影响，用Prx1或Ocn EV处理培养的小鼠骨髓基质细胞（mBMSCs），并进行mRNA测序。参与骨化、骨骼发育和细胞外基质相互作用的途径受到两种EV亚群的调控，而包括高级糖化终产物（AGE）信号转导在内的一些途径则受到Ocn EV亚群的独特调控，这说明特定EV亚群在骨髓微环境中具有重要的生物学效应。这些数据表明，利用 CAGS-Snorkel 小鼠模型进行体内 EV 分离是鉴定货物特征和了解组织特异性 EV 生物学特性的有用工具。此外，虽然骨间充质细胞群具有共同的 EV 分泌特征，但我们发现了基于成骨细胞分化阶段的关键差异，这些差异可能会产生重要的生物学后果。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

求助全文

约1分钟内获得全文求助全文

来源期刊

Journal of Bone and Mineral Research 医学-内分泌学与代谢

CiteScore

11.30

自引率

6.50%

发文量

257

审稿时长

2 months

期刊介绍： The Journal of Bone and Mineral Research (JBMR) publishes highly impactful original manuscripts, reviews, and special articles on basic, translational and clinical investigations relevant to the musculoskeletal system and mineral metabolism. Specifically, the journal is interested in original research on the biology and physiology of skeletal tissues, interdisciplinary research spanning the musculoskeletal and other systems, including but not limited to immunology, hematology, energy metabolism, cancer biology, and neurology, and systems biology topics using large scale “-omics” approaches. The journal welcomes clinical research on the pathophysiology, treatment and prevention of osteoporosis and fractures, as well as sarcopenia, disorders of bone and mineral metabolism, and rare or genetically determined bone diseases.