硅和钙单独及联合作用均靶向增强MC3T3-E1亚克隆4早期成骨标志物的表达。
Si and Ca individually and combinatorially target enhanced MC3T3-E1 subclone 4 early osteogenic marker expression.
作者信息
Varanasi Venu G, Leong Kelly K, Dominia Lisa M, Jue Stephanie M, Loomer Peter M, Marshall Grayson W
机构信息
Department of Biomedical Sciences, Texas A&M Health Science Center, Baylor College of Dentistry, Dallas, TX, USA.
出版信息
J Oral Implantol. 2012 Aug;38(4):325-36. doi: 10.1563/AAID-JOI-D-11-00108.
This study tests the hypothesis that silicon and calcium ions combinatorially target gene expression during osteoblast differentiation. MC3T3-E1 subclone 4 osteoblast progenitors (transformed mouse calvarial osteoblasts) were exposed to Si(4+) (from Na(2)SiO(3)) and Ca(2+) (from CaCl(2):H(2)O) ion treatments both individually (0.4 mM each + control treatment) and combinatorially (0.4 mM Si(4+) + 0.4 mM Ca(2+) + control treatment) and compared to control treated (α-minimum essential medium, 10% fetal bovine serum, and 1% penicillin-streptomycin) cells. Cell proliferation studies showed no significant increase in cell density between treatments over 5 days of culture. Cellular differentiation studies involved addition of ascorbic acid (50 mg/L) for all treatments. Relative gene expression was determined for collagen type 1 (Col(I)α1/Col(I)α2), core-binding factor a (cbfa1/Runx2), and osteocalcin (OCN), which indicated osteoblast progenitor differentiation into a mineralizing phenotype. Increased Si(4+) or Ca(2+) ion treatments enhanced Col(I)α1, Col(I)α2, Runx2, and OCN expression, while increased Si(4+) + Ca(2+) ion treatments enhanced OCN expression. Moreover, it was found that a Si(4+)/Ca(2+) ratio of unity was optimal for maximal expression of OCN. Collagen fiber bundles were dense, elongated, and thick within extracellular matrices (ECM) exposed to Si(4+) and Si(4+) + Ca(2+) treatments, while collagen fiber bundles were sparse, short, and thin within Ca(2+) and control treated ECM. These results indicated that individual ions enhance multiple osteogenic gene expression, while combined ion treatments enhance individual gene expression. In addition, these results indicated that Si(4+) enhanced osteoblast gene expression and ECM formation at higher levels than Ca(2+). These results support the larger concept that ions (possibly released from bioactive glasses) could control bone formation by targeting osteoblast marker expression.
本研究检验了以下假设
硅离子和钙离子在成骨细胞分化过程中以组合方式靶向基因表达。将MC3T3-E1亚克隆4成骨祖细胞(转化的小鼠颅盖成骨细胞)分别单独(每种离子0.4 mM + 对照处理)和组合(0.4 mM Si(4+) + 0.4 mM Ca(2+) + 对照处理)暴露于Si(4+)(来自Na(2)SiO(3))和Ca(2+)(来自CaCl(2):H(2)O)离子处理,并与对照处理的细胞(α-最低必需培养基、10%胎牛血清和1%青霉素-链霉素)进行比较。细胞增殖研究表明,在5天的培养过程中,各处理组之间的细胞密度没有显著增加。细胞分化研究涉及对所有处理添加抗坏血酸(50 mg/L)。测定了1型胶原(Col(I)α1/Col(I)α2)、核心结合因子a(cbfa1/Runx2)和骨钙素(OCN)的相对基因表达,这些指标表明成骨祖细胞分化为矿化表型。增加Si(4+)或Ca(2+)离子处理可增强Col(I)α1、Col(I)α2、Runx2和OCN的表达,而增加Si(4+) + Ca(2+)离子处理可增强OCN的表达。此外,发现Si(4+)/Ca(2+)比值为1时最有利于OCN的最大表达。在暴露于Si(4+)和Si(4+) + Ca(2+)处理的细胞外基质(ECM)中,胶原纤维束密集、细长且粗大,而在Ca(2+)和对照处理的ECM中,胶原纤维束稀疏、短小且细小。这些结果表明,单个离子可增强多种成骨基因的表达,而离子组合处理可增强单个基因的表达。此外,这些结果表明,Si(4+)比Ca(2+)在更高水平上增强成骨细胞基因表达和ECM形成。这些结果支持了一个更大的概念,即离子(可能从生物活性玻璃中释放)可以通过靶向成骨细胞标志物表达来控制骨形成。
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