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标题:【讨论帖】一种细胞检测MTT法改良试剂测评

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  Michael L. Spencer, Haipeng Shao, and Douglas A. AndresInduction of Neurite Extension and Survival in Pheochromocytoma Cells by the Rit GTPaseJ. Biol. Chem., 277(23), 20160-20168 (2002).
cuturl('http://www.jbc.org/cgi/reprint/277/23/20160?maxtoshow=&HITS=10&hits=10&RESULTFORMAT=&andorexactfulltext=and&searchid=1081494519943_20&stored_search=&FIRSTINDEX=0&sortspec=relevance&volume=277&firstpage=20160&resourcetype=1')
26
  Kazuhiro Yoshihara, Tomohide Okumura, Tomonobu Yoshida and Masatoshi BeppuInhibitory Effect of Peptide-Free Forms of Advanced Glycation Products on the Proliferation and Extracellular Matrix Protein Production of Cultured CellsJ. Health Sci., 47(3), 296-301 (2001).
cuturl('http://jhs.pharm.or.jp/47')(3)/47(3)p296.pdf
27
  Takako Niikura,Yuichi Hashimoto, Takashi Okamoto,Yoichiro Abe, Takashi Yasukawa, Masaoki Kawasumi, Takako Hiraki, Yoshiko Kita, Kenzo Tera***a, Keisuke Kouyama, and Ikuo NishimotoInsulin-Like Growth Factor I (IGF-I) Protects Cells from Apoptosis by Alzheimer's V642I Mutant Amyloid Precursor Protein through IGF-I Receptor in an IGF-Binding Protein-Sensitive MannerThe Journal of Neuroscience, March 15, 2001, 21:1902-1910
cuturl('http://www.jneurosci.org/cgi/reprint/21/6/1902.pdf')
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Tadashi Miyamoto,Wongi Min,and Hyun S. LillehojLymphocyte Proliferation Response During Eimeria tenella Infection Assessed by a New, Reliable, Nonradioactive ColorimetricAssayAvian Diseases: Vol. 46, No. 1, pp. 10–16.cuturl('http://www.bioone.org/bioone/?request=get-abstract&issn=0005-2086&volume=046&issue=01&page=0010')
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Yashusi Adachi, Shigeru Taketani, Junko Toki, Kazuya Ikebukuro, Kikuya Sugiura, Haruki Oyaizu yoji Yasumizu, Minoru Tomita, Hiroyuki Kaneda, Yasuo Amoh, Tomoki Ito Mitsuhiko Okigaki, Muneo Inaba, Susumu IkeharaMarked Increase in Number of Dendritic Cells in Autoimmune-Prone (NZW x BXSF1 Mice with Age Stem Cells 2002;20:61-72cuturl('http://stemcells.alphamedpress.org/cgi/reprint/20/1/61.pdf')
19
Shiro YamashojiMenadione-Catalyzed Luminol Chemiluminescent Assay for Viability of Mycobacterium bovisMicrobiol. Immunol., 46, 571—573, 2002
cuturl('http://www.sanbi.co.jp/capj/46/abs/460807.pdf')
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1、Christopher A. Reilly, Jack L. Taylor, Diane L. Lanza, Brian A. Carr, Dennis J. Crouch, and Garold S. Yost
Capsaicinoids Cause Inflammation and Epithelial Cell Death through Activation of Vanilloid Receptors
Toxicol. Sci., May 2003; 73: 170 - 181.
2、 Edward Chaum and Huaitao Yang
Transgenic Expression of IGF-1 Modifies the Proliferative Potential of Human Retinal Pigment Epithelial Cells
Invest. Ophthalmol. Vis. Sci., Dec 2002; 43: 3758 - 3764
3、Maaria Ikonen, Bingrong Liu, Yuichi Hashimoto, Liqun Ma, Kuk-Wha Lee, Takako Niikura, Ikuo Nishimoto, and Pinchas Cohen
Interaction between the Alzheimer's survival peptide humanin and insulin-like growth factor-binding protein 3 regulates cell survival and apoptosis
PNAS, Oct 2003; 100: 13042 - 13047.
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中华中西医杂志 第五卷 2004年第11期
论文名:重组改构人肿瘤坏死因子(rmhTNF)增强乳腺癌细胞对阿霉素的敏 感性
摘要 目的, 探讨重组改构人肿瘤坏死因子(rmhTNF)在人乳腺癌细胞株MCF-7细胞中对阿霉素(ADM)的增敏作用和逆转多药耐药性细胞株MCF-7/Adr细胞对ADM的耐药性,并初步探讨rmhTNF与ADM联合使用时的用药顺序,为临床用药提供依据。
方法 用CCK-8法测定不同顺序联合使用rmhTNF和ADM后的人乳腺癌细胞MCF-7及其耐药性细胞MCF-7/Adr的细胞存活率(cell survival rate,CSR)。
结果 先用ADM处理24h后再更换使用rmhTNF处理24h后,能够提高MCF-7细胞对ADM的敏感性,同样的处理还能逆转多药耐药性MCF-7/Adr细胞对ADM的耐药性;联合使用ADM及rmhTNF时,能显著提高MCF-7细胞对ADM的敏感性,但MCF-7/Adr细胞对ADM没有明显增敏作用。
结论 rmhTNF与ADM联合使用时,能够提高MCF-7细胞对ADM的敏感性,并可逆转MCF-7/Adr细胞对ADM的耐药性.
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感谢l楼主寄来试剂和资料。我已用过,测定药物对肝癌细胞的毒性。有几个问题请教。
1、加入CCK-8后,不到1小时颜色已有明显变化,而此后逐渐加深。如何确定测定的时间点?对结果有无影响?
2、阴性对照组细胞增殖快,未加CCK-8前pH和培养基颜色已变化明显,是否应将所有孔中培养液吸去重新加入培养基,再加CCK-8?
3、使用单波长450 nm测定和双波长450、630nm测定,哪个结果更敏感?
谢谢
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1、CCK-8试剂灵敏度较高,相对而言培养时间较短,一般在目测发现颜色有明显变化时,即可确定为测定时间。以后每次测定都按照同样的条件。
2、若pH和培养基颜色已变化明显,应将所有孔中培养液吸去重新加入培养基,再加CCK-8。
3、关于单波长和双波长,国内喜欢用单波长,国外喜欢用双波长。双波长可以去除细胞碎片和其他非特异因素造成的干扰。
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由于CCK-8有一定粘性,故在用移液枪加试剂时,速度要快,尽量避免试剂沾在移液枪的管壁上,可以减少实验误差。
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Seongwoo Hwang, Natarajan Tamilarasu, Karen Kibler, Hong Cao, Akbar Ali, Yueh-Hsin Ping, Kuan-Teh Jeang, and Tariq M. Rana
Discovery of a Small Molecule Tat-trans-Activation-responsive RNA Antagonist That Potently Inhibits Human Immunodeficiency Virus-1 Replication
THE JOURNAL OF BIOLOGICAL CHEMISTRYOF BIOLOGICAL CHEMISTRY Vol. 278, No. 40, Issue of October 3, pp. 39092–39103, 2003
Antiretroviral therapy to treat AIDS uses molecules that target the reverse transcriptase and protease enzymes of human immunodeficiency virus, type 1 (HIV-1). A major problem associated with these treatments, however, is the emergence of drug-resistant strains. Thus, there is a compelling need to find drugs against other viral targets. One such target is the interaction between Tat, an HIV-1 regulatory protein essential for viral replication, and trans-activation-responsive (TAR) RNA. Here we describe the design and synthesis of an encoded combinatorial library containing 39,304 unnatural small molecules. Using a rapid high through-put screening technology, we identified 59 compounds. Structure-activity relationship studies led to the synthesis of 19 compounds that bind TAR RNA with high affinities. In the presence of a representative Tat-TAR inhibitor (5 microM TR87), we observed potent and sustained suppression of HIV replication in cultured cells over 24 days. The same concentration of this inhibitor did not exhibit any toxicity in cell cultures or in mice. TR87 was also shown to specifically disrupt Tat-TAR binding in vitro and inhibit Tat-mediated transcriptional activation in vitro and in vivo, providing a strong correlation between its activities and inhibition of HIV-1 replication. These results provide a structural scaffold for further development of new drugs, alone or in combination with other drugs, for treatment of HIV-1-infected individuals. Our results also suggest a general strategy for discovering pharmacophores targeting RNA structures that are essential in progression of other infectious, inflammatory, and genetic diseases.
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Negative regulation of hepatocellular carcinoma cell growth by signal regulatory protein 1
HEPATOLOGY 2004;40:618–628.
Abstract
Signal regulatory protein (SIRP) 1 is a member of the SIRP family that undergoes tyrosine phosphorylation and binds SHP-2 tyrosine phosphatase in response to various mitogens. The expression levels of SIRP1 were decreased in HCC tissues, compared with the matched normal tissues. Exogenous expression of wild type SIRP1, but not of a mutant SIRP1 lacking the tyrosine phosphorylation sites, in SIRP1-negative Huh7 human HCC cells resulted in suppression of tumor cell growth both in vitro and in vivo. Treatment of Huh7 transfectants with EGF or HGF induced tyrosine phosphorylation of SIRP1 and its association with SHP-2, which were accompanied by reduced ERK1 activation. Expression of SIRP1 significantly suppressed activation of NF-B and also sensitized Huh7 cells to TNF or cisplatin-induced cell death. In addition, SIRP1-transfected Huh7 cells displayed reduced cell migration and cell spreading in a fashion that was dependent on SIRP1/SHP-2 complex formation. In conclusion, a negative regulatory effect of SIRP1 on hepatocarcinogenesis is exerted, at least in part, through inhibition of ERK and NF-B pathways.
cuturl('http://www3.interscience.wiley.com/cgi-bin/abstract/109606299/ABSTRACT')
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 旧的MTT用于悬浮细胞和贴壁不紧的细胞检测不太准确,因为离心后去掉上清总会有一部分细胞被倒出来,我是先从24孔培养板吸到EP管离心后再吸弃上清,然后溶解的方法,比较麻烦,如果是48孔那岂不烦死?不知CCK-8是怎么处理这一点的,是否不用去除上清就可以检测MTT?
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