CCK试剂盒简介
CCK试剂盒(Cell Counting Kit),为MTT 法的替代方法,是一种基于WST(水溶性四唑盐,化学名:2-(2-甲氧基-4-硝苯基)-3-(4-硝苯基)-5-(2,4-二磺基苯)-2H-四唑单钠盐)的广泛应用于细胞增殖和细胞毒性的快速高灵敏度检测试剂盒。
WST检测原理图
CCK法与其它检测方法之间的比较
CCK用途:药物筛选、细胞增殖测定、细胞毒性测定、肿瘤药敏试验。
CCK试剂盒的优点及应用
CCK试剂盒使用方便,省去了洗涤细胞,不需要同位素和有机溶剂
CCK法的检测灵敏度很高,甚至可以测定较低细胞密度
CCK试剂盒为1瓶溶液,毋需预制,即开即用
CCK法的重复性优于MTT法
CCK试剂毒性
CCK和其他检测方法对比可以得出——CCK对细胞几乎无毒性,不伤害细胞,细胞可重复利用。
资料下载
CCK-8试剂盒使用说明书
客户产品验证及相关生物数据
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数据来源 |
J Hazard Mater (2020 Apr). Figure 6. Cell Counting Kit-8 (AbMole BioScience, Houston, TX, USA) |
| 方法 |
Cell viability assay |
| 细胞系 |
LO2 and HEK 293 cells |
| 浓度 |
- |
| 处理时间 |
- |
| 实验结果 |
As shown in Fig. 6, PAT-J significantly reduced the viability of the two cells compared with the JUICE group, while the cell viability of the PAT-JP and LS-J2 treated groups did not change significantly. |
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数据来源 |
Med Sci Monit (2018 Oct). Figure 2. Cell Counting Kit-8 (Abmole Bioscience, USA) |
| 方法 |
Cell viability assay |
| 细胞系 |
colon cancer cells |
| 浓度 |
10 nmol/L |
| 处理时间 |
1 h |
| 实验结果 |
Then, CCK8 assay was performed to measure the effect of MON1B on cell viability of colon cancer cells, which was inhibited time-dependently (12, 24, and 48 h) in the si-MON1B group, with significant differ�ences at 24 and 48 h (P<0.05, Figure 2C). |
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数据来源 |
Sci Rep (2018;8:3891). Figure 4. CCK-8 (AbMole BioScience) |
| 方法 |
Cell viability assay |
| 细胞系 |
PLC5 cells |
| 浓度 |
10 nmol/L |
| 处理时间 |
48 h |
| 实验结果 |
In accordance with functional analysis, western blot confirmed that CCRK overexpression promoted cell proliferation by activating β-catenin/TCF signaling, which however significantly abrogated by bufalin |
| 评级 |
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数据来源 |
Sci Rep (2018;8:3891). Figure 1. CCK-8 (AbMole BioScience) |
| 方法 |
Cell viability assay |
| 细胞系 |
PLC5 cells |
| 浓度 |
10 nmol/L |
| 处理时间 |
48 h |
| 实验结果 |
After 48 hours incubation, cell viability was measured by CCK-8 assay. In contrast with less influence on the growth of LO2 cells, bufalin exhibited strong ability to suppress the number of PLC5 cells in a dose-dependent manner. |
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数据来源 |
Cancer Biol Ther (2018 Jun 3;19(6):507-517). Figure 7. CCK-8 (Abmole Bioscience, Shanghai, China) |
| 方法 |
CCK-8 assay |
| 细胞系 |
C33A, Hcc94, HeLa, and SiHa cell lines |
| 浓度 |
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| 处理时间 |
72 h |
| 实验结果 |
As the results of the CCK-8 assay shown, the 72-hour treatment with buformin exhibited significant suppressive effects on cellular growth in C33A, Hcc94, and SiHa cells, but only exerted moderate effects in HeLa cells. |
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数据来源 |
Future Oncology (2018 Feb;14(3):241-253) . Figure 3. CCK-8 (AbMole BioScience, Shanghai, China) |
| 方法 |
Cell counting kit-8 assay |
| 细胞系 |
HeLa, SiHa, C33A and CasKi cells |
| 浓度 |
10 μl |
| 处理时间 |
2 h |
| 实验结果 |
Compared with its counterparts, knockdown of PXN suppressed cellular proliferation and induced cellular apoptosis |
| 评级 |
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数据来源 |
PLoS One (2013). Figure 3. Cell counting kit-8 |
| 方法 |
Cell proliferation assay |
| 细胞系 |
Human colon cancer cell lines HT-29, LOVO, and Caco-2 |
| 浓度 |
10 μL/well |
| 处理时间 |
2 h |
| 实验结果 |
The effect of cPA on cell proliferation was determined using a colorimetric assay. We found that cPA inhibited the proliferation of HT-29 and LOVO cells but not of DLD-1 and Caco-2 cells, which have lower endogenous levels of PDE3B than HT-29 and LOVO cells. |
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数据来源 |
PLoS One (2013). Figure 4. Cell counting kit-8 |
| 方法 |
Cell viability |
| 细胞系 |
Human mesenchymal stem cells |
| 浓度 |
20 µL/well |
| 处理时间 |
3 h |
| 实验结果 |
In group A, the cell number remained stable during the first 3 days, followed by a continuous increase till day 14. In group B, the cell number was stable during the first 2 days, then started to increase, and attained a plateau on day 12. In group C (control group), the cell number (Fig. 4A) remained stable during the first 4 days in culture, then started to increase, and plateaued on day 8. |
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