Department of Biomedical Engineering, University of Utah, Salt Lake City, Utah, USA.
Department of Oncological Sciences, and University of Utah, Salt Lake City, Utah, USA.
Tissue Eng Part A. 2020 Nov;26(21-22):1169-1179. doi: 10.1089/ten.TEA.2020.0062. Epub 2020 Jul 9.
Stem cell therapies have shown promise for regenerative treatment for musculoskeletal conditions, but their success is mixed. To enhance regenerative effects, growth factors are utilized to induce differentiation into native cell types, but uncontrollable conditions inhibit differentiation, and precise control of expressed matrix proteins is difficult to achieve. To address these issues, we investigated a novel method of enhancing regenerative phenotype through direct upregulation of major cartilaginous tissue proteins, aggrecan (), and collagen II () using dCas9-VPR CRISPR gene activation systems. We demonstrated increased expression and deposition of targeted proteins independent of exogenous growth factors in pellet culture. Singular upregulation of interestingly indicates that upregulation mediates the highest sulfated glycosaminoglycan (sGAG) deposition, in addition to collagen II deposition. Through RNA-seq analysis, this was shown to occur by upregulation mediating broader chondrogenic gene expression changes. Multiplex upregulation of and together resulted in the highest sGAG, and collagen II deposition, with levels comparable to those in chondrogenic growth factor-differentiated pellets. Overall, this work indicates dCas9-VPR systems can robustly upregulate and deposition without growth factors, to provide a novel, precise method of controlling stem cell phenotype for cartilage and intervertebral disc cell therapies and tissue engineering. Impact statement Stem cell therapies have come about as a potential regenerative treatment for musculoskeletal disease, but clinically, they have mixed results. To improve stem cell therapies, growth factors are used to aid a regenerative cell phenotype, but their effects are inhibited by musculoskeletal disease environments. This article describes CRISPR gene activation-based cell engineering methods that provide a growth factor-free method of inducing chondrogenic extracellular matrix deposition. This method is demonstrated to be as/more potent as growth factors in inducing a chondrogenic phenotype in pellet culture, indicating potential utility as a method of enhancing stem cell therapies for musculoskeletal disease.
干细胞疗法在治疗肌肉骨骼疾病的再生治疗方面显示出了希望,但它们的效果参差不齐。为了增强再生效果,利用生长因子诱导分化为天然细胞类型,但不可控的条件抑制分化,并且难以精确控制表达的基质蛋白。为了解决这些问题,我们研究了一种通过使用 dCas9-VPR CRISPR 基因激活系统直接上调主要软骨组织蛋白聚集蛋白聚糖()和胶原 II()来增强再生表型的新方法。我们在微球培养中证明了在不依赖外源性生长因子的情况下,靶向蛋白的表达和沉积增加。有趣的是,的单一上调表明,除了胶原 II 沉积外,的上调介导了最高的硫酸化糖胺聚糖(sGAG)沉积。通过 RNA-seq 分析,这表明通过的上调介导了更广泛的软骨基因表达变化。和一起的多重上调导致 sGAG 和胶原 II 的沉积最高,与软骨形成生长因子分化的微球相当。总的来说,这项工作表明,dCas9-VPR 系统可以在没有生长因子的情况下强有力地上调和的沉积,为软骨和椎间盘细胞治疗和组织工程提供一种新的、精确的控制干细胞表型的方法。
