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- 详细信息
- 文献和实验
- 技术资料
- 库存:
100
- 细胞类型:
科研
- 品系:
详情请咨询我司客服
- 组织来源:
详情请咨询我司客服
- 物种来源:
鼠/人/其它
- 细胞形态:
上皮样/成纤维样/其它
- 器官来源:
详情请咨询我司客服
- 运输方式:
常温运输/干冰运输
- 年限:
详情请咨询我司客服
- 生长状态:
贴壁/悬浮
- 英文名:
H125
产品简介:
[品系] ……………………Human
[组织来源]………………详情请咨询
[生长状态]………………贴壁/悬浮
[细胞类型]………………详情请咨询
[疾病] ……………………正常
[应用] ……………………科研
生物安全:
不含有 HIV-1、 HBV、HCV、支原体、细菌、酵母和真菌等。
产品包装:
提供新鲜或者冻存的细胞
使用方法:
如是新鲜细胞,客户收到细胞后应立即将其放入CO2细胞培养箱内静置3-4个小时,再进行后续的实验操作;如是冻存细胞, 客户收到细胞后应立即将其放入液氮、-80℃冰箱或立即进行复苏。
细胞培养 :
(1)Getting Started with an ATCC Cell Line:
ATCC cell lines and hybridomas are shipped frozen on dry ice in cryopreservation vials or as growing
cultures in flasks at ambient temperature. Upon receipt of frozen cells, it is important to immediately revive
them by thawing and removing the DMSO and placing them into culture. If this is not possible, store the
cells in liquid nitrogen vapor (below −130°C). Do not store frozen cells at temperatures above −130°C as
their viability will decline rapidly.
(2)细胞图片:
(3)Initiating Frozen Cultures:
1. Prepare a culture vessel so that it contains the recommended volume
of the appropriate culture medium as listed on the Product Sheet,
equilibrated for temperature and pH (CO₂).
2. Thaw the vial by gentle agitation in a water bath at 37°C or the normal growth temperature for that cell
line. Thawing should be rapid, approximately 2 minutes or until ice crystals have melted.
3. Remove the vial from the water bath and decontaminate it by dipping in or spraying with 70% ethanol.
Follow strict aseptic conditions in a laminar flow tissue culture hood for all further manipulations.
4. Unscrew the top of the vial and transfer the contents to a sterile
centrifuge tube containing 9 mL of the recommended medium.
Remove the cryoprotectant agent (DMSO) by gentle centrifugation (10
minutes at 125 × g). Discard the supernatant, and resuspend the cells
in 1 or 2 mL of complete growth medium. Transfer the cell suspension
into the culture vessel containing the complete growth medium and
mix thoroughly by gentle rocking.
Some ATCC cell, are shipped as growing cultures in culture vessels. These vessels are seeded with cells,
incubated to ensure cell growth and then filled completely with medium for shipping.
Upon receiving a flask culture, visually examine the medium for macroscopic evidence of microbial contamination. This includes
unusual pH shifts (yellow or purple color from the phenol red),
turbidity, or particles. With an inverted microscope at low power
(100×) check the medium for evidence of microbial contamination
as well as the morphology of the cells. See page 6 for more details
on examining cell cultures.
烜雅生物发布
质量可靠,售后有保障
如运输过程中导致细胞污染或者死亡,我们将无条件补发收货后十个工作日内有其他问题提供照片可半价重发
人肺癌细胞_H125相关产品:
| CHL | 中国仓鼠肺细胞 |
| BRL | 肝细胞 |
| NRK | 鼠肾细胞 |
| L-6TG | 肌母细胞 |
| V79 | 中国仓鼠肺细胞 |
| BHK | 幼仓鼠肾细胞 |
| CHO | 中国仓鼠卵巢细胞 |
| R1610 | 中国仓鼠体细胞 |
| CHO/dhFr- | 二氢叶酸还原酶缺陷型CHO细胞 |
| 2BS | 胚肺细胞 |
| HLF | 胚肺细胞 |
| WI-38 | 胚肺细胞 |
| SL-7 | 胚肺细胞 |
| XJH | B淋巴细胞 |
| L-02 | 肝细胞 |
| Chang Liver | 张氏肝细胞 |
| QSG-7701 | 小肝细胞 |
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文献和实验littleyan0418 我现在的任务是要构建人肺癌细胞的cDNA文库,但我不是这个方面科班出身,好多地方还不是很明白,想请教师兄师姐的经验,应该注意些什么。现在对总RNA的提取我有点找不出头绪。麻烦师兄师姐们可以给我分享些这方面的资料和网址吗?非常感谢!! neuronboy http://www.takara.com.cn/ 价格、试剂盒和说明书都有。呵呵 littleyan0418
我培养过不少肺癌细胞(人类),其中绝大部分都是贴壁细胞,具体如: (1) A549(肺腺癌) (2) NCIH446(小肺细胞癌) (3) 801(非小肺细胞癌) (4) NCIH460 (大细胞肺癌) 在消化传代过程中,步骤基本一致: 吸去旧的培养液->用Hanks'(1X)清洗一两次->加入一定量的消化液(Trpsin-EDTA)->置显微镜下观察,待细胞大部分变圆时,回到超静台->吸去消化液->加入一定量的新培养液->反复吹打细胞->再置显微镜下观察,直到细胞全部悬浮起来->
所需的D-HANK'S液和胰酶和用1640配置的适当浓度小牛血清最好都放在37度预热十分钟左右,让它们和细胞生长环境的温度是一样的。这样能达到既对细胞没有外来刺激的作用又能达到反应的最佳条件。我用的是小培养瓶,方法是:先把旧的培养液倒掉,用D-HANK'S大约3ml洗一次,加浓度为0.1%的胰酶进行消化,添加量只要能均匀的覆盖培养瓶底,大约要1.5ml,最好把瓶盖旋紧放到37度培养箱里培养3-5分钟,在显微镜下观察细胞收缩,变圆,加入3ml的10%的血清终止消化。小心仔细的吹打培养瓶底使细胞
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