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小鼠成骨细胞系、永生化小鼠成骨细胞

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  • ¥3500 - 4500
  • 欣润生物(NEWGAINBIO)
  • 江苏无锡
  • IM2022
  • 2025年12月15日
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    • 详细信息
    • 文献和实验
    • 技术资料
    • 英文名

      Immortalized mouse osteoblasts

    • 库存

      100万

    • 供应商

      欣润生物

    • 肿瘤类型

    • 细胞类型

      永生化

    • ATCC Number

    • 品系

      ICR

    • 组织来源

      颅骨

    • 相关疾病

    • 物种来源

      小鼠

    • 免疫类型

      不详

    • 细胞形态

      梭形

    • 是否是肿瘤细胞

    • 器官来源

      颅骨

    • 运输方式

      常温

    • 年限

      /

    • 生长状态

      贴壁生长

    • 规格

      T25方瓶

    产品介绍
    细胞名称:小鼠成骨细胞系、永生化小鼠成骨细胞
    背景描述:小鼠成骨细胞主要由内外骨膜和骨髓中基质内的间充质始祖细胞分化而来,能特异性分泌多种生物活性物质,调节并影响骨的形成和重建过程。小鼠成骨细胞系培养不仅有助于了解骨形成机制、骨骼系统疾病的分子和细胞学基础,也是药物筛选、生物材料开发和生物工程研究的重要手段。
    产品货号:IM2022
    细胞类型:永生化细胞
    传代能力:可传代25代左右
    细胞形态:上皮型
    培养基:小鼠成骨细胞系、永生化小鼠成骨细胞完全培养基
    支原体分析鉴定:阴性
    培养条件:37℃,5%CO2
    发货方式:T25方瓶
    货期:1-2周时间

     
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                                     Collagen II抗体免疫荧光检测呈阳性


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    Immortalized murine osteoblasts derived from BMP 2-T-antigen expressing transgenic mice

    Osteoblast cell lines capable of undergoing bone formation in vitro would provide useful models for understanding gene expression during bone cell differentiation. To that end, transgenic mice were produced using a 2.9-kilobase bone morphogenetic protein 2 (BMP-2) promoter fragment, driving simian virus 40 T antigen as the transgene. The expression of simian virus 40 T antigen driven by the BMP-2 promoter immortalizes the cells. From the calvaria of the transgenic mouse, several osteoblastic cell lines were isolated and cloned. One clonal osteoblast cell line, called 2T3, has been characterized and shown to produce mineralized bone nodules. Recombinant human BMP-2 (rhBMP-2) accelerates the formation of these mineralized bone nodules. 2T3 cells express alkaline phosphatase, collagen type I, osteocalcin, and endogenous BMP-2 messenger RNA (mRNA) in a similar chronological order as normal freshly isolated fetal rat calvarial cells during early nodule formation and subsequent mineralization. The 2T3 cells also exhibit extensive growth and multilayering during 

     

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    图标文献和实验
    该产品被引用文献

    Chicken intestinal epithelial cells were obtained from NEWGAINBIO company. Cells were cultured on 37, with 5% CO2, in the Ham’s F-12 Nutrient (DMEM/12) that contained the following supplementations: fetal bovine serum (5%), in-sulin (5 µg/mL), transferrin (5 µg/mL), selenium (5 ng/mL), epidermal growth factor (5 ng/mL) and penicillin-streptomycin (100–100 U/mL) for cell culturing (full DMEM/12). Experiments were performed with chicken intestinal epithelial cells and working solutions were prepared with plain DMEM/12 without supplementation. For the investigations, cells were seeded onto 96-well, 24-well or 6-well polystyrene cell culture plates.

     

    Primary hVICs (passage 2) were cultured to 50–60% confluence and infected with pGMLV-SV40T-puro lentivirus (NewgainBio, Wuxi, China) at a multiplicity of infection of 80 supplemented with 5 µg/mL polybrene (Sigma-Aldrich, Buchs, Switzerland).

     

    Tissue was cultured until cells became visible around the tissue, and when the fusion reached 90% (FIGURE 1A) §ask ¦lled with the prepared culturing medium was sent to the company for further immortalisation. Cell immortalisation was done for cell stability and longer-term use. Immortalised cells were cultured with 10% FBS and 1% PS in the DMEM medium.  After the cells multiplied and merged, they were routinely passed and grown ( NEWGAINBIO Inc. Wuxi, Jiangsu, China) (FIGURE 1B-C).

    Mouse primary cultured renal vascular ECs and VSMCs were obtained from Newgainbio company, which were tested by Factor VIII and α-smooth muscle actin (α-SMA), the marker of ECs and VSMCs. RNeasy Mini Kit was used for RNA extraction, and the above protocols were repeated.

     

     

    Porcine primary colon epithelial cells (Newgainbio company, Wuxi,China) were cultured in Dulbecco's Modified Eagle's Medium (Solarbio, Beijing, China) containing 10 % fetal bovine serum (BioInd, Kiryat shmona, Lsrael) at 37 C and 5 % CO2 humidity.

    相关实验
    • 小鼠成骨细胞的培养和传代

      原代培养1.取新生3d以内BALB/c小鼠,断颈处死后立即投入75%酒精中消毒5min(虽有头部皮肤保护,但时间不要过长,所以事先要把准备工作做好之后再去杀老鼠)。2.D-Hank’s液漂洗后分离颅盖骨,刮除骨膜和结缔组织,DMEM清洗颅骨骨片并剪碎。(自我感觉碎一点好一些)3.加入0.25%胰蛋白酶(含0.02EDTA),37°恒温消化20min,吸出消化液,之后1mg/1mlI型胶原酶37°恒温消化20min后离心(1000r/min,5min),弃上清液。(消化时间自己摸索,之前我消化

    • 小鼠的R1胚胎干细胞系培养实验步骤

      相关专题   以下是根据NIH老年病研究所 提供的英文的R1胚胎干细胞培养protocol整理而成。根据经验作部分修改。 1、一般培养:保持胚胎干细胞 处于未分化状态 培养基细胞复苏冻存细胞明胶包被细胞传代 2 、体外分化 培养基包被有多聚鸟氨酸/纤维结合蛋白的培养板(使用或不使用盖玻片) 体外分化方法 注:以下培养针对于小鼠的R1胚胎干细胞系,其它胚胎

    • 【求助】表达TLR4,MYD88,TBK1的人和小鼠的肿瘤细胞系

      zcx7792 哪些人和小鼠的肿瘤细胞系表达TLR4,MYD88,TBK1? 哪位高手知道?不甚感激。 zcx7792 自己顶一下 lagopsis SKOV3 livelyding 胰腺癌细胞株 zcx7792 非常感谢二位 本文由丁香园论坛提供,想了解更多有用的、有意思的前沿资讯以及酷炫

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