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兔脂肪间充质干细胞系、兔脂肪干细胞系、兔脂肪干细胞、兔脂肪间

充质干细胞、永生化兔脂肪间充质干细胞、永生化兔脂肪干细胞
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  • ¥3500 - 4500
  • 欣润生物
  • 江苏无锡
  • IR9002-1
  • 2025年12月13日
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    • 详细信息
    • 文献和实验
    • 技术资料
    • 英文名

      Rabbit adipose derived mesenchymal stem cells

    • 库存

      10

    • 供应商

      欣润生物

    • 肿瘤类型

      NO

    • 细胞类型

      永生化

    • ATCC Number

      11222

    • 品系

      新西兰兔

    • 组织来源

      兔脂肪间充质干

    • 相关疾病

    • 物种来源

    • 免疫类型

      不详

    • 细胞形态

      成纤维细胞样

    • 是否是肿瘤细胞

    • 器官来源

      脂肪

    • 运输方式

      常温

    • 年限

      成年

    • 生长状态

      贴壁生长

    • 规格

      T25方瓶

    永生化兔脂肪间充质干细胞简介:

    产品描述:兔脂肪干细胞分离自成年兔皮下脂肪组织,体外培养的脂肪干细胞呈成纤维细胞样生长,为短梭形、小三角形以及多角形等。来源于中胚层的脂肪组织的干细胞具有向成脂肪、成软骨、成骨、心肌细胞和神经源细胞分化的多分化潜能。因此脂肪组织可以作为兔干细胞库的重要来源,并可作为多种组织工程的种子细胞,有非常重要的研究和应用价值
    产品货号:
    IR9002
    产品类型:
    永生化细胞
    传代能力:
    30代左右
    产品形态:
    成纤维细胞样
    培养基:
    永生化兔脂肪间充质干细胞完全培养基
    支原体质控:
    呈阴性
    产品培养条件:
    37℃,5%CO2
    发货方式:
    T25瓶子常温发货
    货期:
    1周左右货期
      

     产品细节图片1 产品细节图片2 产品细节图片3 产品细节图片4

    产品细节图片5          产品细节图片6         
    产品细节图片7 产品细节图片8
     

    Effects of Astragalus Injection on Cell Cycle and in Vitro Proliferation of Rabbit Adipose-derived Mesenchymal Stem Cells

    Objective:To investigate the effects of astragalus injection on cell cycle and in vitro proliferation of rabbit adipose-derived mesenchymal stem cells(ASCs).Method:ASCs were obtained from an experimental rabbit and cultured.Multi experimental and a control group were designed.Different concentrations of astragalus injection were added to the culture fluid in the experimental group,while a conventional culture method was employed in the control group.The distribution of the cell cycle was measured by flow cytometry and the proliferation rates of ASCs by MTT,and compared between the experimental and the control group.Result:After 24 hours of culture,the number of the cells during the proliferative phase was increased significantly from(65.3±4.8)% for the control group to(72.6±5.7)% for the experimental group,and the differences between each experimental and the control groups were not significant.After 48 hours,the optical density was(2.273±0.100)-(1.983±0.125) in each experimental group at 0.390 6-200 g·L-1 of astragalus,while(1.341±0.424) in the control group,and the 

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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
    • 组织工程概要

      工程的基本要素,细胞主要来源于自体、同种异体、异种组织细胞等。自体组织细胞应为首选。由于组织工程细胞培养多需要高浓度的细胞接种,自体组织细胞存在着数量上的局限性及长期传代后细胞功能老化的问题。现在的研究多集中于以下的几个方面:   1.载体等技术用于细胞的快速增殖。   2.干细胞工程 干细胞工程是利用现代生物医学和组织工程技术,通过对间充质干细胞、胚胎干细胞、血管-造血干细胞、神经干细胞和皮肤、肌肉等前体细胞,进行体外分离纯化、定向诱导分化、转基因及核移植、大量扩增和整合

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    兔脂肪间充质干细胞系、兔脂肪干细胞系、兔脂肪干细胞、兔脂肪间充质干细胞、永生化兔脂肪间充质干细胞、永生化兔脂肪干细胞
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