Маркетинговые исследования
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Nonetheless, handful of modifiable threat aspects for ovarian cancers

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 Nonetheless, handful of modifiable threat aspects for ovarian cancers  Empty Nonetheless, handful of modifiable threat aspects for ovarian cancers

Сообщение  wangqian Пт Май 09, 2014 12:29 pm

The blend index was calculated from the Chou Talalay equation, which requires under consideration the two the potency and the form of your dose impact curve taking benefit with the Compusyn computer software. The blend index is made use of to the quantification of synergism or an tagonism for two medication exactly where CI 1, 1, and 17-AAG 構造 1 indicate synergism, additive result, and antagonism, respectively. Analysis of cell cycle distribution by movement cytometry H 460 cells have been seeded in T 25 tissue culture flasks at a density of 1. 0106mL and incubated overnight at 37 C. Next day the cells had been handled with compounds. On the finish of treatment method time period the cells had been harvested and professional cessed for movement cytometry as described previously.<br><br> Annexin V staining Annexin V staining was performed as described from the producer. Briefly, 1105 cells have been washed twice in PBS and resuspended in binding buffer, 140 mM NaCl, 2. 5 mM CaCl2 at a concentration of 1106 cellsml. 5 ul of FITC Annexin V and 10 ul of PI were added, and also the cells incubated for 15 min from the dark at room temperature. A complete 17-DMAG 分子量 of 400 ul of binding buffer was then added and the cells analyzed by movement cytometry. Planning and examination of cell lysates by immunoblotting Cells had been seeded, handled with or with no P276 00 or doxorubicin or their mixture and have been harvested at sought after time factors and western blotting was carried out as previously described. Antibodies utilized in this examine were Bcl 2, Bax, p53, Cdk 1, cyclin D1, Cox 2, anti rabbitHRP and anti mouse HRP se condary antibodies.<br><br> Clonogenic assay H 460 cells have been seeded at a density of 7501000 cells per 35 mm tissue culture grade plate and incubated overnight at 37 C for your cells to attach. The cells have been treated together with the cytotoxic drug doxorubicin for A66 溶解度 24 h fol lowed by elimination of medium and addition of fresh medium containing P276 00 for 96 h. On the end in the treatment method, the medium was replaced by fresh complete medium and incubated for 714 days for colony forma tion. When visible colonies appeared on the plate the medium was removed and colonies were fixed with methanol acetic acid mixture while in the ratio of 21 for 5 min. The plates had been washed with water plus the fix ation method was repeated.<br><br> The plates were dried plus the colonies have been stained with 0. 1% crystal violet stain for 35 min. The plates were rinsed cautiously with water and dried and the colonies counted. Tumor xenograft model Somewhere around 5106 H 460 cells had been subcutaneously injected into significant combined immunodeficient mice in 0. 2 ml volume to the suitable flank and observed every day for tumor look. When the tumors attained a diameter of 50 mm3, they had been randomized into four groups Group I, handle car. Group II, doxorubicin 2 mpk ip. once every week for 2 weeks. Group III, P276 00 20 mpk ip. each and every day for 5 days every week for 2 weeks. Group IV, blend of doxorubicin and P276 00, doxorubicin was followed by P276 00 right after an interval of 6 h, followed daily with P276 00 for a total of five days which comprised of a single cycle. The treatment com prised of complete of two cycles. Entire body fat was recorded everyday. Tumor measurements i. e. the length and width with the tumors have been measured applying the vernier caliper.

wangqian

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