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永生化鸡骨骼肌细胞、鸡骨骼肌细胞系、鸡骨骼肌卫星细胞系、永生

化鸡骨骼肌卫星细胞
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  • ¥4000
  • 欣润生物
  • 江苏
  • IK6001
  • 2026年04月23日
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    • 详细信息
    • 文献和实验
    • 技术资料
    • 英文名

      Immortalized chicken skeletal muscle cells

    • 库存

      10

    • 供应商

      欣润生物

    • 肿瘤类型

      不是

    • 细胞类型

      永生化细胞

    • ATCC Number

      111

    • 品系

    • 组织来源

      骨骼肌

    • 相关疾病

    • 物种来源

    • 免疫类型

      正常

    • 细胞形态

      梭形

    • 是否是肿瘤细胞

    • 器官来源

      肌肉

    • 运输方式

      常温

    • 年限

      成年

    • 生长状态

      贴壁生长

    • 规格

      T25方瓶

    永生化鸡骨骼肌细胞简介:

    产品描述:鸡骨骼肌卫星细胞指骨骼肌中除骨骼肌纤维(肌细胞)外的一种扁平、有突起的细胞。其附着于肌纤维(肌细胞)表面;当肌纤维(肌细胞)受损后,肌卫星细胞可增殖分化,参与肌纤维(肌细胞)的修复,因此具有干细胞性质。
    产品货号:
    IK6001
    产品类型:
    原代细胞建立的永生化
    传代能力:
    30代左右
    产品形态:
    成纤维细胞样
    培养基:
    永生化鸡骨骼肌细胞专用完全培养基,产品编号:IK6001-5
    支原体:
    呈阴性
    产品培养条件:
    37℃,5%CO2
    发货方式:
    常温T25方瓶运输
    货期:
    1周左右货期
     

    222.jpg 22.jpg 图像_00.jpg 1.jpg 图像_02.jpg Composite.jpg      

    Pax7抗体免疫荧光染色鉴定

    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
     

    Chronic leptin treatment stimulates lipid oxidation in immortalized and primary mouse skeletal muscle cells

    Leptin administration enhances lipid oxidation in skeletal muscle. Nevertheless, direct and chronic effect of leptin has not been well characterized. Here, we measured the effect of leptin on skeletal muscles and their signaling pathways using differentiated C 2C 12 myotubes and primary myotube cultures. Differentiated myotubes expressed both the short and long forms of leptin receptors. Leptin increased lipid oxidation in myotubes in a concentration- and time-dependent manner, with significant induction of lipid oxidation occurring after 6h. Actinomycin D completely blocked leptin-induced lipid oxidation. Leptin significantly increased phosphorylation of JAK2 and STAT3 in myotubes, and leptin-induced lipid oxidation was abolished by treatment with a JAK2 inhibitor or STAT3 siRNA. We then used mouse myotubes to measure these effects under physiological conditions. Leptin increased lipid oxidation, which again was blocked by a JAK2 inhibitor and STAT3 siRNA. These results suggest that the JAK2/STAT3 signaling pathway may underlie the chronic effects of leptin on lipid

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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
    • 细胞生物基本方法:肌组织细胞培养

      肌组织细胞培养 1 )骨骼肌细胞培养 1. 杀死动物,无菌取大腿肌组织,切成 0.3 ~ 0.5 厘米小块。 2. 用不含钙镁离子的 Hanks 液配的 0.25 %胰蛋白酶消化,无菌纱网或纱布滤过,合成培养基加 10 %小牛血清培养,为促进分化可加 1 %的胎汁。 3. 细胞接种量为 2 × 106 / 皿,接种在胶原或明胶的底物上能促进细胞分化。明胶制备比较简单,常用 Hanks 液配的 0.01

    • 光学显微镜的使用与细胞形态观察

      (4)上皮细胞(人口腔上皮、小肠切片) 单层扁平上皮:人口腔上皮细胞,细胞轮廓呈多边形或不规则的波浪形,每个细胞内有一个圆形核; 单层柱状上皮:小肠绒毛,由排列紧密的柱状细胞构成,细胞形状高细,似柱状,其卵圆形核靠近基部。 (5) 骨骼肌(横切和纵切) 骨骼肌骨骼肌纤维构成。骨骼肌纤维是长圆柱状细胞,每一条肌纤维内有大量圆形细胞核(可多达上百个)。其细胞质又称肌浆,含有丰富的肌原纤维、线粒体和脂肪滴等。肌原纤维呈细丝状,沿细胞长轴平行

    • 肌组织细胞培养

      骨骼肌 细胞培养 1.杀死动物,无菌取大腿肌组织,切成0.3~0.5厘米小块。 2.用不含钙镁离子的Hanks液配的0.25%胰蛋白酶消化,无菌纱网或纱布滤过,合成培养基加10%小牛血清培养,为促进分化可加1%的胎汁。 3.细胞接种量为2×106/皿,接种在胶原或明胶的底物上能促进细胞分化。明胶制备比较简单,常用Hanks液配的0.01%明胶。

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